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| <?xml version="1.0" encoding="UTF-8"?><!DOCTYPE article PUBLIC "-//NLM//DTD JATS (Z39.96) Journal Archiving and Interchange DTD v1.1d1 20130915//EN" "JATS-archivearticle1.dtd"><article article-type="research-article" dtd-version="1.1d1" xmlns:xlink="http://www.w3.org/1999/xlink"><front><journal-meta><journal-id journal-id-type="nlm-ta">elife</journal-id><journal-id journal-id-type="hwp">eLife</journal-id><journal-id journal-id-type="publisher-id">eLife</journal-id><journal-title-group><journal-title>eLife</journal-title></journal-title-group><issn publication-format="electronic">2050-084X</issn><publisher><publisher-name>eLife Sciences Publications, Ltd</publisher-name></publisher></journal-meta><article-meta><article-id pub-id-type="publisher-id">02949</article-id><article-id pub-id-type="doi">10.7554/eLife.02949</article-id><article-categories><subj-group subj-group-type="display-channel"><subject>Research article</subject></subj-group><subj-group subj-group-type="heading"><subject>Microbiology and infectious disease</subject></subj-group></article-categories><title-group><article-title>Prion propagation can occur in a prokaryote and requires the ClpB chaperone</article-title></title-group><contrib-group><contrib contrib-type="author" id="author-12717"><name><surname>Yuan</surname><given-names>Andy H</given-names></name><xref ref-type="aff" rid="aff1"/><xref ref-type="aff" rid="aff2"/><xref ref-type="other" rid="par-2"/><xref ref-type="fn" rid="con1"/><xref ref-type="fn" rid="conf1"/></contrib><contrib contrib-type="author" id="author-12718"><name><surname>Garrity</surname><given-names>Sean J</given-names></name><xref ref-type="aff" rid="aff1"/><xref ref-type="fn" rid="con2"/><xref ref-type="fn" rid="conf1"/></contrib><contrib contrib-type="author" id="author-12719"><name><surname>Nako</surname><given-names>Entela</given-names></name><xref ref-type="aff" rid="aff1"/><xref ref-type="fn" rid="con3"/><xref ref-type="fn" rid="conf1"/></contrib><contrib contrib-type="author" corresp="yes" id="author-12664"><name><surname>Hochschild</surname><given-names>Ann</given-names></name><xref ref-type="aff" rid="aff1"/><xref ref-type="corresp" rid="cor1">*</xref><xref ref-type="other" rid="par-1"/><xref ref-type="fn" rid="con4"/><xref ref-type="fn" rid="conf1"/></contrib><aff id="aff1"><institution content-type="dept">Department of Microbiology and Immunobiology</institution>, <institution>Harvard Medical School</institution>, <addr-line><named-content content-type="city">Boston</named-content></addr-line>, <country>United States</country></aff><aff id="aff2"><institution>Whitehead Institute for Biomedical Research</institution>, <addr-line><named-content content-type="city">Cambridge</named-content></addr-line>, <country>United States</country></aff></contrib-group><contrib-group content-type="section"><contrib contrib-type="editor"><name><surname>Greenberg</surname><given-names>Peter</given-names></name><role>Reviewing editor</role><aff><institution>University of Washington</institution>, <country>United States</country></aff></contrib></contrib-group><author-notes><corresp id="cor1"><label>*</label>For correspondence: <email>ahochschild@hms.harvard.edu</email></corresp></author-notes><pub-date date-type="pub" publication-format="electronic"><day>13</day><month>08</month><year>2014</year></pub-date><pub-date pub-type="collection"><year>2014</year></pub-date><volume>3</volume><elocation-id>e02949</elocation-id><history><date date-type="received"><day>29</day><month>03</month><year>2014</year></date><date date-type="accepted"><day>12</day><month>08</month><year>2014</year></date></history><permissions><copyright-statement>© 2014, Yuan et al</copyright-statement><copyright-year>2014</copyright-year><copyright-holder>Yuan et al</copyright-holder><license xlink:href="http://creativecommons.org/licenses/by/4.0/"><license-p>This article is distributed under the terms of the <ext-link ext-link-type="uri" xlink:href="http://creativecommons.org/licenses/by/4.0/">Creative Commons Attribution License</ext-link>, which permits unrestricted use and redistribution provided that the original author and source are credited.</license-p></license></permissions><self-uri content-type="pdf" xlink:href="elife02949.pdf"/><abstract><object-id pub-id-type="doi">10.7554/eLife.02949.001</object-id><p>Prions are self-propagating protein aggregates that are characteristically transmissible. In mammals, the PrP protein can form a prion that causes the fatal transmissible spongiform encephalopathies. Prions have also been uncovered in fungi, where they act as heritable, protein-based genetic elements. We previously showed that the yeast prion protein Sup35 can access the prion conformation in <italic>Escherichia coli</italic>. Here, we demonstrate that <italic>E. coli</italic> can propagate the Sup35 prion under conditions that do not permit its de novo formation. Furthermore, we show that propagation requires the disaggregase activity of the ClpB chaperone. Prion propagation in yeast requires Hsp104 (a ClpB ortholog), and prior studies have come to conflicting conclusions about ClpB's ability to participate in this process. Our demonstration of ClpB-dependent prion propagation in <italic>E. coli</italic> suggests that the cytoplasmic milieu in general and a molecular machine in particular are poised to support protein-based heredity in the bacterial domain of life.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.001">http://dx.doi.org/10.7554/eLife.02949.001</ext-link></p></abstract><abstract abstract-type="executive-summary"><object-id pub-id-type="doi">10.7554/eLife.02949.002</object-id><title>eLife digest</title><p>Unlike most infectious agents—such as viruses or bacteria—that contain genetic material in the form of DNA or RNA, a prion is simply an aggregate of misfolded proteins. Although they are not living organisms, these prion aggregates can self-propagate; when they enter a healthy organism, they cause existing, correctly folded proteins to adopt the prion fold. Within the aggregate, the prion proteins have a corrugated structure that allows them to stack together tightly, which in turn makes the aggregates very stable. As more prions are formed, they then trigger other protein molecules to misfold and join the aggregates, and the aggregates continue to grow and spread within the infected organism causing tissue damage and cell death.</p><p>Prion diseases are well known in mammals, where the prion aggregates typically destroy tissue within the brain or nervous system. Bovine spongiform encephalopathy (also commonly known as BSE or ‘mad cow disease’) is an example of a prion disease that affects cattle and can be transmitted to humans by eating infected meat. Prions also form in yeast and other fungi. These prions, however, do not cause disease or cell death; instead, yeast prions act as protein-based elements that can be inherited over multiple generations and which provide the yeast with new traits or characteristics. Although prions can form spontaneously in yeast cells, their stable propagation depends on so-called chaperone proteins that help to remodel the prion aggregates. Previous work has shown that bacterial cells can also support the formation of prion-like aggregates. The bacteria were engineered to produce two yeast prion proteins—one of which spontaneously formed aggregates that were needed to trigger the conversion of the other to its prion form. However, it was not known if bacterial cells could support the stable propagation of prions if the initial trigger for prion conversion was removed.</p><p>Yuan et al. now reveal that the bacterium <italic>Escherichia coli</italic> can propagate a yeast prion for over a hundred generations, even when the cells can no longer make the protein that serves as the trigger for the initial conversion. This propagation depends on a bacterial chaperone protein called ClpB, which is related to another chaperone protein that is required for stable prion propagation in yeast. As such, the findings of Yuan et al. raise the possibility that, even though a prion specific to bacteria has yet to be identified, prions or prion-like proteins might also contribute to the diversity of traits found in bacteria. Furthermore, since both yeast and bacteria form and propagate prions in similar ways, such protein-based inheritance might have evolved in these organisms' common ancestor over two billion years ago.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.002">http://dx.doi.org/10.7554/eLife.02949.002</ext-link></p></abstract><kwd-group kwd-group-type="author-keywords"><title>Author keywords</title><kwd>prions</kwd><kwd>chaperones</kwd><kwd>Sup35</kwd><kwd>ClpB</kwd><kwd>protein-based heredity</kwd></kwd-group><kwd-group kwd-group-type="research-organism"><title>Research organism</title><kwd><italic>E. coli</italic></kwd><kwd><italic>S. cerevisiae</italic></kwd></kwd-group><funding-group><award-group id="par-1"><funding-source><institution-wrap><institution-id institution-id-type="FundRef">http://dx.doi.org/10.13039/100000002</institution-id><institution>National Institutes of Health</institution></institution-wrap></funding-source><award-id>Pioneer award, OD003806</award-id><principal-award-recipient><name><surname>Hochschild</surname><given-names>Ann</given-names></name></principal-award-recipient></award-group><award-group id="par-2"><funding-source><institution-wrap><institution-id institution-id-type="FundRef">http://dx.doi.org/10.13039/100000001</institution-id><institution>National Science Foundation</institution></institution-wrap></funding-source><award-id>Graduate research fellowship</award-id><principal-award-recipient><name><surname>Yuan</surname><given-names>Andy H</given-names></name></principal-award-recipient></award-group><funding-statement>The funders had no role in study design, data collection and interpretation, or the decision to submit the work for publication.</funding-statement></funding-group><custom-meta-group><custom-meta><meta-name>elife-xml-version</meta-name><meta-value>2</meta-value></custom-meta><custom-meta specific-use="meta-only"><meta-name>Author impact statement</meta-name><meta-value>The bacterium <italic>Escherichia coli</italic> possesses a permissive cytoplasmic environment and the requisite molecular machinery to support the propagation of prions.</meta-value></custom-meta></custom-meta-group></article-meta></front><body><sec id="s1" sec-type="intro"><title>Introduction</title><p>Prions are infectious, self-propagating protein aggregates first described in the context of scrapie (<xref ref-type="bibr" rid="bib44">Prusiner, 1982</xref>), an example of a class of devastating neurodegenerative diseases known as the transmissible spongiform encephalopathies (TSEs). Specifically, the prion form of a protein known as PrP is the causative agent of the TSEs, which afflicts humans and other mammals. Native PrP (PrP<sup>C</sup>) undergoes a dramatic change in conformation upon conversion to its prion form (PrP<sup>Sc</sup>), forming distinctive cross-β aggregates termed as amyloid (<xref ref-type="bibr" rid="bib14">Diaz-Espinoza and Soto, 2012</xref>). Highly resistant to denaturation and proteolysis, PrP<sup>Sc</sup> is infectious and templates the conformational conversion of PrP<sup>C</sup> molecules (<xref ref-type="bibr" rid="bib4">Caughey et al., 2009</xref>).</p><p>Prion-like phenomena have also been described in budding yeast and other fungi. Since Wickner first invoked prions to account for two examples of non-Mendelian genetic elements in <italic>Saccharomyces cerevisiae</italic> (<xref ref-type="bibr" rid="bib8">Cox, 1965</xref>; <xref ref-type="bibr" rid="bib1">Aigle and Lacroute, 1975</xref>; <xref ref-type="bibr" rid="bib66">Wickner, 1994</xref>), the study of fungal prion proteins has resulted in profound advances in the understanding of prion biology, including the first demonstration that purified prion protein aggregates are infectious (<xref ref-type="bibr" rid="bib36">Maddelein et al., 2002</xref>; <xref ref-type="bibr" rid="bib28">King and Diaz-Avalos, 2004</xref>; <xref ref-type="bibr" rid="bib55">Tanaka et al., 2004</xref>). In general, such prion proteins exist in either a native, soluble form or a self-perpetuating, amyloid form with spontaneous conversion between forms representing a rare event (<xref ref-type="bibr" rid="bib3">Allen et al., 2007</xref>; <xref ref-type="bibr" rid="bib30">Lancaster et al., 2010</xref>). However, unlike PrP<sup>Sc</sup>, yeast prions do not normally cause cell death. Instead, they can act as protein-based genetic elements that confer new phenotypes on those cells that harbor them (<xref ref-type="bibr" rid="bib62">True and Lindquist, 2000</xref>; <xref ref-type="bibr" rid="bib63">Tuite and Serio, 2010</xref>; <xref ref-type="bibr" rid="bib39">Newby and Lindquist, 2013</xref>). Fungal prion proteins have been found to participate in diverse cellular processes (<xref ref-type="bibr" rid="bib7">Coustou et al., 1997</xref>; <xref ref-type="bibr" rid="bib61">True et al., 2004</xref>; <xref ref-type="bibr" rid="bib54">Suzuki et al., 2012</xref>; <xref ref-type="bibr" rid="bib27">Holmes et al., 2013</xref>). The conversion of these proteins to their prion forms typically results in a dominant loss-of-function phenotype (<xref ref-type="bibr" rid="bib8">Cox, 1965</xref>; <xref ref-type="bibr" rid="bib1">Aigle and Lacroute, 1975</xref>). A particularly well-characterized example involves the essential translation release factor Sup35, which confers on cells a heritable nonsense suppression phenotype upon conversion to the prion form (<xref ref-type="bibr" rid="bib8">Cox, 1965</xref>; <xref ref-type="bibr" rid="bib58">Ter-Avanesyan et al., 1994</xref>; <xref ref-type="bibr" rid="bib42">Patino et al., 1996</xref>; <xref ref-type="bibr" rid="bib43">Paushkin et al., 1996</xref>).</p><p>Like other yeast prion proteins, Sup35 has a modular structure with a distinct prion domain (PrD) that mediates conversion to the prion form, [<italic>PSI</italic><sup>+</sup>]. In the case of Sup35, the essential prion determinants, which include a glutamine- and asparagine-rich segment and five complete copies of an imperfect oligopeptide repeat sequence, lie in the N-terminal domain (N), whereas translation release activity resides in the C-terminal domain (C) (<xref ref-type="bibr" rid="bib59">Ter-Avanesyan et al., 1993</xref>). A highly charged middle region (M) increases the solubility of native Sup35 and enhances the mitotic stability of [<italic>PSI</italic><sup>+</sup>] (<xref ref-type="bibr" rid="bib34">Liu et al., 2002</xref>). Together, Sup35 N and M function as a transferable prion-forming module (NM) that maintains its prionogenic potential when fused to heterologous proteins (<xref ref-type="bibr" rid="bib32">Li and Lindquist, 2000</xref>). A distinctive property of the Sup35 conversion process in yeast is its dependence on the presence of a pre-existing prion, designated [<italic>PIN</italic><sup>+</sup>] for [<italic>PSI</italic><sup>+</sup>] inducibility factor (<xref ref-type="bibr" rid="bib12">Derkatch et al., 1997</xref>). Thus, yeast strains containing Sup35 in the non-prion form, [<italic>psi</italic><sup>–</sup>], support the spontaneous conversion to [<italic>PSI</italic><sup>+</sup>] only if they contain [<italic>PIN</italic><sup>+</sup>], typically the prion form of the Rnq1 protein (<xref ref-type="bibr" rid="bib11">Derkatch et al., 2000</xref>). However, several other yeast prion proteins, including the New1 protein, have the capacity to function as [<italic>PIN</italic><sup>+</sup>] in their prion forms (<xref ref-type="bibr" rid="bib10">Derkatch et al., 2001</xref>; <xref ref-type="bibr" rid="bib41">Osherovich and Weissman, 2001</xref>).</p><p>Importantly, the stable propagation of yeast prions—and thus, the heritability of their associated phenotypes—depends on the function of chaperone proteins (<xref ref-type="bibr" rid="bib6">Chernoff et al., 1995</xref>). Specifically, the AAA+ disaggregase Hsp104 is strictly required for the propagation of virtually all yeast prions characterized thus far, and several other chaperone proteins have been implicated in this process as well (<xref ref-type="bibr" rid="bib33">Liebman and Chernoff, 2012</xref>; <xref ref-type="bibr" rid="bib67">Winkler et al., 2012</xref>). Various lines of evidence support the view that the essential role of Hsp104 with respect to prion propagation stems from its ability to fragment prion aggregates and thereby to generate smaller seed particles known as propagons that can be efficiently partitioned to daughter cells during cell division (<xref ref-type="bibr" rid="bib43">Paushkin et al., 1996</xref>; <xref ref-type="bibr" rid="bib38">Ness et al., 2002</xref>; <xref ref-type="bibr" rid="bib9">Cox et al., 2003</xref>; <xref ref-type="bibr" rid="bib29">Kryndushkin et al., 2003</xref>; <xref ref-type="bibr" rid="bib48">Satpute-Krishnan et al., 2007</xref>; <xref ref-type="bibr" rid="bib26">Higurashi et al., 2008</xref>). Accordingly, depletion or inhibition of Hsp104 in a prion-containing cell leads to prion loss in progeny cells.</p><p>The molecular processes underlying prion biology constitute at least two distinct phases, namely, (i) the de novo conversion of a protein from its native to prion form, and (ii) the subsequent propagation of the self-perpetuating prion form over multiple generations. While studies have demonstrated that the bacterial cytoplasm can support the de novo formation of prion-like aggregates (<xref ref-type="bibr" rid="bib47">Sabaté et al., 2009</xref>; <xref ref-type="bibr" rid="bib19">Fernándes-Tresguerres et al., 2010</xref>; <xref ref-type="bibr" rid="bib21">Garrity et al., 2010</xref>; <xref ref-type="bibr" rid="bib17">Espargaró et al., 2012</xref>; <xref ref-type="bibr" rid="bib22">Gasset-Rosa et al., 2014</xref>), evidence for prion propagation—and thus, protein conformation-dependent heredity—in bacteria has remained elusive. We previously demonstrated that conversion of Sup35 NM to its prion form in <italic>Escherichia coli</italic>, as in <italic>S. cerevisiae</italic>, depends on [<italic>PIN</italic><sup>+</sup>], which is formed by providing the bacterial cells with the yeast New1 protein (<xref ref-type="bibr" rid="bib21">Garrity et al., 2010</xref>). This [<italic>PIN</italic><sup>+</sup>] dependence provides an experimental framework for distinguishing between the initial conversion and subsequent propagation phases of the prion cycle. In particular, the formation of prion-like Sup35 NM aggregates can be induced in bacterial cells containing the New1 protein; subsequent depletion of the New1 protein from these cells reveals whether or not the bacterial cytoplasm can support the propagation of the Sup35 NM prion in the absence of [<italic>PIN</italic><sup>+</sup>].</p><p>Here we show that bacteria can propagate the Sup35 prion in an infectious conformation over at least ∼100 generations under conditions that do not permit de novo prion formation. More specifically, we demonstrate maintenance of the Sup35 NM prion over multiple rounds of restreaking in <italic>E. coli</italic> cells no longer capable of synthesizing the New1 protein. Furthermore, we establish that propagation of the Sup35 NM prion in <italic>E. coli</italic> requires the disaggregase activity of ClpB, the bacterial ortholog of Hsp104. The striking parallel between the requirements for both prion formation and prion propagation in yeast and bacteria, which are thought to have diverged more than 2.2 billion years ago, suggests that the paradigm of protein-based heredity may be more ancient than previously inferred (<xref ref-type="bibr" rid="bib13">DeSantis et al., 2012</xref>).</p></sec><sec id="s2" sec-type="results"><title>Results</title><sec id="s2-1"><title><italic>E. coli</italic> cells can propagate SDS-stable Sup35 NM aggregates</title><p>Having previously shown that Sup35 NM can adopt an infectious amyloid conformation in the <italic>E. coli</italic> cytoplasm (<xref ref-type="bibr" rid="bib21">Garrity et al., 2010</xref>), we wished to determine whether or not <italic>E. coli</italic> cells could stably propagate Sup35 NM in its prion form. To address this question, we took advantage of the fact that conversion of Sup35 NM to its prion conformation in <italic>E. coli</italic> depends on the presence of New1, mirroring features of the [<italic>PIN</italic><sup>+</sup>] dependence of Sup35 prion formation in <italic>S. cerevisiae</italic> (<xref ref-type="fig" rid="fig1">Figure 1A</xref>). Thus, our plan was to induce the formation of infectious Sup35 NM aggregates in <italic>E. coli</italic> cells containing the prionogenic module of New1 and then to monitor the fate of Sup35 NM over multiple generations after curing the cells of New1-encoding DNA.<fig-group><fig id="fig1" position="float"><object-id pub-id-type="doi">10.7554/eLife.02949.003</object-id><label>Figure 1.</label><caption><title>Conversion of Sup35 NM to its prion form in <italic>E. coli</italic> requires New1.</title><p>(<bold>A</bold>) Cartoon representation of how conversion of soluble Sup35 NM (Sup35<sub>soluble</sub>) to its amyloid conformation (Sup35<sub>amyloid</sub>) depends on the presence of New1 in its amyloid conformation (New1<sub>amyloid</sub>). Sup35 NM and New1 (black) are depicted as fusions to mCherry (red) and mGFP (green), respectively. (<bold>B</bold>) SDS-stable Sup35 NM aggregates are detected only in cells producing SDS-stable New1 aggregates as assessed by filter retention analysis. For each sample, undiluted lysate and three twofold dilutions are shown (see ‘Materials and methods’). Sup35 NM and New1 aggregates are no longer detected once boiled. The α-Sup35 antibody recognizes the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein, and the α-GFP antibody detects the New1-mGFP fusion protein. (<bold>C</bold>) Intracellular full-length (FL) Sup35 NM fusion protein levels are comparable in the presence and absence of New1 as assessed by Western blot analysis. The α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase. (<bold>D</bold>) Fluorescence images of representative cells containing Sup35 NM and New1 or Sup35 NM alone. For cells containing both fusion proteins, the mCherry channel, GFP channel, and merged images are shown.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.003">http://dx.doi.org/10.7554/eLife.02949.003</ext-link></p></caption><graphic xlink:href="elife02949f001"/></fig><fig id="fig1s1" position="float" specific-use="child-fig"><object-id pub-id-type="doi">10.7554/eLife.02949.004</object-id><label>Figure 1—figure supplement 1.</label><caption><title>α-Sup35 and α-His<sub>6X</sub> antibodies are interchangeable for detecting the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein.</title><p>(<bold>A</bold>) Probing nitrocellulose membranes with either α-Sup35 antibody (<xref ref-type="fig" rid="fig1">Figure 1C</xref>) or α-His<sub>6X</sub> antibody results in the detection of similar intracellular Sup35 NM fusion protein products in the presence or absence of New1 as assessed by Western blot analysis. Full-length (FL) Sup35 NM fusion proteins are indicated by arrows. (<bold>B</bold>) Probing cellulose acetate membranes with either α-His<sub>6X</sub> antibody (<xref ref-type="fig" rid="fig3">Figure 3B</xref>) or α-Sup35 antibody results in the detection of similar aggregate-positive and aggregate-negative samples in starter cultures (ST) and Round 1 (R1) experimental clones as assessed by filter retention analysis. For each sample, undiluted lysate and three twofold dilutions are shown. Starter cultures of cells containing Sup35 NM and New1 and cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. (<bold>C</bold>) Probing cellulose acetate membranes with either α-His<sub>6X</sub> antibody (<xref ref-type="fig" rid="fig3">Figure 3D</xref>) or α-Sup35 antibody results in the detection of similar aggregate-positive and aggregate-negative samples in starter cultures (ST) and R1 control clones as assessed by filter retention analysis.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.004">http://dx.doi.org/10.7554/eLife.02949.004</ext-link></p></caption><graphic xlink:href="elife02949fs001"/></fig></fig-group></p><p>To facilitate these experiments, we fused Sup35 NM and New1 to two monomeric fluorescent proteins (mCherry bearing a C-terminal hexahistidine tag and mGFP, respectively). The two fusion proteins were produced from compatible plasmids under the control of IPTG-inducible promoters. The plasmid encoding New1-mGFP (pSC101<sup>TS</sup>-<italic>NEW1</italic>) bore a temperature-sensitive origin of replication, enabling us to cure cells of New1-encoding DNA and thereby deplete cells of the New1 fusion protein. As an initial test of our experimental system, we introduced the plasmid encoding Sup35 NM-mCherry-His<sub>6x</sub> (pBR322-<italic>SUP35 NM</italic>) together with either pSC101<sup>TS</sup>-<italic>NEW1</italic> or an empty vector control (pSC101<sup>TS</sup>) into <italic>E. coli</italic> cells and induced the synthesis of the fusion proteins at the permissive temperature. After overnight growth, we detected SDS-stable Sup35 NM aggregates (‘Materials and methods’) only in cells producing the New1 fusion protein (<xref ref-type="fig" rid="fig1">Figure 1B</xref>). As New1 can independently adopt an amyloid conformation in <italic>E. coli</italic> (<xref ref-type="bibr" rid="bib21">Garrity et al., 2010</xref>), we also detected SDS-stable New1 aggregates in cells containing both fusion proteins (<xref ref-type="fig" rid="fig1">Figure 1B</xref>). Western blot analysis revealed that the intracellular levels of the Sup35 NM fusion protein were comparable in the presence and absence of the New1 fusion protein (<xref ref-type="fig" rid="fig1">Figure 1C</xref>, <xref ref-type="fig" rid="fig1s1">Figure 1—figure supplement 1A</xref>). We also examined cells by fluorescence microscopy. In cells containing both fusion proteins, Sup35 NM formed twisted ring structures (<xref ref-type="bibr" rid="bib21">Garrity et al., 2010</xref>) or large polar foci in 22.5% of cells (<italic>N</italic> = 258), whereas New1 formed punctate foci in 89.8% of cells (<italic>N</italic> = 258). (<xref ref-type="fig" rid="fig1">Figure 1D</xref>). In contrast, Sup35 NM exhibited diffuse fluorescence in 100% of cells lacking New1 (<italic>N</italic> = 532) (<xref ref-type="fig" rid="fig1">Figure 1D</xref>).</p><p>We then sought to determine whether or not <italic>E. coli</italic> cells could propagate SDS-stable Sup35 NM aggregates over multiple generations under conditions that do not permit the de novo formation of aggregates (that is, in the absence of New1). Our experimental protocol is illustrated in <xref ref-type="fig" rid="fig2">Figure 2</xref> (see also <xref ref-type="fig" rid="fig3">Figure 3A</xref>). We first induced fusion protein synthesis in cells transformed with pBR322-<italic>SUP35 NM</italic> and either pSC101<sup>TS</sup>-<italic>NEW1</italic> (experimental sample) or pSC101<sup>TS</sup> (control sample). These ‘starter cultures’ were grown overnight to allow for the formation of SDS-stable Sup35 NM aggregates in the experimental sample. The cells were then plated and grown at the non-permissive temperature to cure the cells of pSC101<sup>TS</sup>-<italic>NEW1</italic> or pSC101<sup>TS</sup>, thereby generating a set of Round 1 (R1) colonies. 20 R1 experimental colonies and 20 R1 control colonies were subsequently examined; each was (a) patched onto selective medium to test for loss of pSC101<sup>TS</sup>-<italic>NEW1</italic> or pSC101<sup>TS</sup>, (b) restreaked to generate Round 2 (R2) colonies, and (c) inoculated into liquid medium for overnight growth to test for the presence of SDS-stable Sup35 NM aggregates. Four separate experimental lineages (L1<sub>E</sub>–L4<sub>E</sub>) originating from ancestral R1 experimental colonies containing detectable Sup35 NM aggregates along with four separate control lineages (L1<sub>C</sub>–L4<sub>C</sub>) originating from ancestral R1 control colonies were then followed through Round 3 (R3) and Round 4 (R4). For R2 and each subsequent round, 10 experimental colonies and 10 control colonies were analyzed.<fig id="fig2" position="float"><object-id pub-id-type="doi">10.7554/eLife.02949.005</object-id><label>Figure 2.</label><caption><title>Experimental protocol for assessing the ability of <italic>E. coli</italic> cells to propagate SDS-stable Sup35 NM aggregates.</title><p>Experiments are initiated with either a starter culture (ST) of cells containing Sup35 NM and New1 (shown) or a starter culture of cells containing Sup35 NM alone (not shown). For each of the 4 lineages (L1–L4), the total number of generations over which Sup35 NM prion propagation is monitored corresponds to the number of cell divisions that occur in the absence of New1 during 4 rounds (R1–R4) of growth on solid medium and an additional round of growth in liquid medium. Growth in the absence of New1 begins at the time the starter culture cells are plated at 37°C (R1). Single R1 colonies were found to contain ∼950,000 colony forming units (CFUs), and the liquid cultures contain ∼10<sup>8</sup> CFUs per μl. Thus, prion propagation is monitored over 98.7 or ∼100 generations. We note that the presence of SDS-stable Sup35 NM aggregates in experimental starter culture cells does not represent prion propagation because the presence of New1 (i.e., [<italic>PIN</italic><sup>+</sup>]) enables the continuing de novo conversion of newly synthesized Sup35 NM to the prion form.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.005">http://dx.doi.org/10.7554/eLife.02949.005</ext-link></p></caption><graphic xlink:href="elife02949f002"/></fig><fig id="fig3" position="float"><object-id pub-id-type="doi">10.7554/eLife.02949.006</object-id><label>Figure 3.</label><caption><title>Converted Sup35 NM can remain in its prion conformation in <italic>E. coli</italic> cells lacking New1.</title><p>(<bold>A</bold>) Cartoon representation of how Sup35 NM can convert to its prion form in the presence of New1 and remain in the prion conformation after cells have been cured of New1-encoding DNA. Sup35 NM and New1 (black) are depicted as fusions to mCherry (red) and mGFP (green), respectively. (<bold>B</bold>) SDS-stable Sup35 NM aggregates are detected in 8 of 20 Round 1 (R1) experimental clones derived from a starter culture (ST) of cells containing Sup35 NM and New1 as assessed by filter retention analysis. Starter cultures of cells containing Sup35 NM and New1 and cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. The four aggregate-positive clones selected to establish the four experimental lineages are indicated by asterisks. In all 20 R1 experimental samples, intracellular Sup35 NM fusion protein levels are comparable, and New1 fusion protein is not detectable as assessed by Western blot analysis. The α-His<sub>6X</sub> and α-Sup35 antibodies recognize the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein (see <xref ref-type="fig" rid="fig1s1">Figure 1—figure supplement 1B,C</xref>), the α-GFP antibody detects the New1-mGFP fusion protein, and the α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase. (<bold>C</bold>) In all 20 R1 experimental samples, DNA encoding Sup35 NM is detectable whereas DNA encoding the prionogenic module of New1 is not detectable by PCR. (<bold>D</bold>) SDS-stable Sup35 NM aggregates are not detected in any of the 20 R1 control clones derived from a starter culture of cells containing Sup35 NM alone as assessed by filter retention analysis. The four aggregate-negative clones selected to establish the four control lineages are indicated by asterisks. Intracellular Sup35 NM fusion protein levels are comparable in all 20 R1 control samples.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.006">http://dx.doi.org/10.7554/eLife.02949.006</ext-link></p></caption><graphic xlink:href="elife02949f003"/></fig></p><p>All R1 experimental and control colonies (20 of each) had lost pSC101<sup>TS</sup>-<italic>NEW1</italic> or pSC101<sup>TS</sup>, respectively, as assessed by patching on selective medium (data not shown). Moreover, the absence of <italic>NEW1</italic> DNA was confirmed by PCR (<xref ref-type="fig" rid="fig3">Figure 3C</xref>) and the absence of New1 protein was confirmed by Western blot analysis (<xref ref-type="fig" rid="fig3">Figure 3B</xref>). We detected SDS-stable Sup35 NM aggregates in 8 of 20 experimental samples (<xref ref-type="fig" rid="fig3">Figure 3B</xref>) and none of the control samples (<xref ref-type="fig" rid="fig3">Figure 3D</xref>). We selected 4 of the 8 aggregate-positive clones (<xref ref-type="fig" rid="fig3">Figure 3B</xref>, asterisks) to establish the four experimental lineages and arbitrarily selected four aggregate-negative control clones (<xref ref-type="fig" rid="fig3">Figure 3D</xref>, asterisks) to establish the four control lineages. 2 of the 4 experimental lineages (L1<sub>E</sub> and L3<sub>E</sub>) retained SDS-stable Sup35 NM aggregates throughout the course of the experiment (<xref ref-type="fig" rid="fig4">Figure 4A</xref>, <xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1B</xref>). Of these two lineages, one maintained aggregates in 9 of 10 R4 clones (<xref ref-type="fig" rid="fig4">Figure 4A</xref>) and the other maintained aggregates in 7 of 10 R4 clones (<xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1B</xref>). We conclude that SDS-stable Sup35 NM aggregates can be propagated in <italic>E. coli</italic> for at least ∼100 generations in the absence of New1 (<xref ref-type="fig" rid="fig5">Figure 5A</xref>).<fig-group><fig id="fig4" position="float"><object-id pub-id-type="doi">10.7554/eLife.02949.007</object-id><label>Figure 4.</label><caption><title><italic>E. coli</italic> can propagate the Sup35 NM prion over ∼100 generations.</title><p>(<bold>A</bold>) Experimental Lineage 1 (L1<sub>E</sub>). An aggregate-positive Round 1 (R1) experimental clone (gray box) derived from a starter culture (ST) of cells containing Sup35 NM and New1 is identified and restreaked to yield progeny Round 2 (R2) clones (gray bracket). All 10 R2 clones analyzed contain detectable SDS-stable Sup35 NM aggregates. An aggregate-positive R2 clone (blue box) is identified and restreaked to yield progeny Round 3 (R3) clones (blue bracket). Again, all 10 R3 clones analyzed contain SDS-stable Sup35 NM aggregates. An aggregate-positive R3 clone (green box) is identified and restreaked to yield progeny Round 4 (R4) clones (green bracket). 9 of 10 R4 clones analyzed contain SDS-stable Sup35 NM aggregates. The filter retention assay is used to detect SDS-stable Sup35 NM aggregates. Intracellular Sup35 NM fusion protein levels are comparable in all 40 samples as assessed by Western blot analysis. Starter cultures of cells containing Sup35 NM and New1 and cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. The α-His<sub>6X</sub> and α-Sup35 antibodies recognize the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein, and the α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase. (<bold>B</bold>) Control Lineage 1 (L1<sub>C</sub>). An aggregate-negative R1 control clone (gray box) derived from a starter culture of cells containing Sup35 NM alone is identified and restreaked to yield progeny R2 clones (gray bracket), an aggregate-negative R2 clone (blue box) is identified and restreaked to yield progeny R3 clones (blue bracket), and an aggregate-negative R3 clone (green box) is identified and restreaked to yield progeny R4 clones (green bracket). No SDS-stable Sup35 NM aggregates are detectable in any sample. Intracellular Sup35 NM fusion protein levels are comparable in all 40 samples as assessed by Western blot analysis.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.007">http://dx.doi.org/10.7554/eLife.02949.007</ext-link></p></caption><graphic xlink:href="elife02949f004"/></fig><fig id="fig4s1" position="float" specific-use="child-fig"><object-id pub-id-type="doi">10.7554/eLife.02949.008</object-id><label>Figure 4—figure supplement 1.</label><caption><title>The fate of Sup35 NM in experimental Lineages 2-4.</title><p>(<bold>A</bold>) Experimental Lineage 2 (L2<sub>E</sub>). An aggregate-positive Round 1 (R1) clone (gray box) derived from a starter culture (ST) of cells containing Sup35 NM and New1 is identified and restreaked to yield progeny Round 2 (R2) clones (gray bracket). 8 of 10 R2 clones analyzed contain detectable SDS-stable Sup35 NM aggregates as assessed by filter retention analysis. An aggregate-positive R2 clone (blue box) is restreaked to yield progeny Round 3 (R3) clones (blue bracket). 0 of 10 R3 clones analyzed contain detectable SDS-stable Sup35 NM aggregates. The apparent loss of aggregates coincides with the loss of detectable Sup35 NM fusion protein as assessed by Western blot analysis. Assaying the 10 Round 4 (R4) progeny clones derived from an aggregate-negative R3 clone (green box) reveals that fusion protein levels can be restored without the recovery of SDS-stable Sup35 NM aggregates (green bracket). Starter cultures of cells containing Sup35 NM and New1 and cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. The α-His<sub>6X</sub> and α-Sup35 antibodies recognize the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein, and the α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase. (<bold>B</bold>) Experimental Lineage 3 (L3<sub>E</sub>). 9 of 10 R2 clones analyzed contain detectable SDS-stable Sup35 NM aggregates, which are retained in 8 of 10 R3 progeny clones and 7 of 10 R4 progeny clones. (<bold>C</bold>) Experimental Lineage 4 (L4<sub>E</sub>). 8 of 10 R2 clones analyzed contain detectable SDS-stable Sup35 NM aggregates, which are retained in 9 of 10 R3 progeny clones. 0 of 10 R4 clones analyzed contain detectable SDS-stable Sup35 NM aggregates. As in R3 of L2<sub>E</sub> (<bold>A</bold>), the apparent loss of aggregates coincides with a dramatic drop in Sup35 NM fusion protein levels.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.008">http://dx.doi.org/10.7554/eLife.02949.008</ext-link></p></caption><graphic xlink:href="elife02949fs002"/></fig><fig id="fig4s2" position="float" specific-use="child-fig"><object-id pub-id-type="doi">10.7554/eLife.02949.009</object-id><label>Figure 4—figure supplement 2.</label><caption><title>The fate of Sup35 NM in control Lineages 2–4.</title><p>(<bold>A</bold>) Control Lineage 2 (L2<sub>C</sub>). An aggregate-negative Round 1 (R1) clone (gray box) derived from a starter culture (ST) of cells containing Sup35 NM alone is identified and restreaked to yield progeny Round 2 (R2) clones (gray bracket). 0 of 10 R2 clones analyzed contain detectable SDS-stable Sup35 NM aggregates as assessed by filter retention analysis. An aggregate-negative R2 clone (blue box) is restreaked to yield progeny R3 clones (blue bracket). 0 of 10 R3 clones analyzed contain detectable SDS-stable Sup35 NM aggregates. An aggregate-negative R3 clone (green box) is restreaked to yield progeny R4 clones (green bracket). 0 of 10 R4 clones analyzed contain detectable SDS-stable Sup35 NM aggregates. Starter cultures of cells containing Sup35 NM and New1 and cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. The α-His<sub>6X</sub> and α-Sup35 antibodies recognize the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein, and the α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase. (<bold>B</bold>) Control Lineage 3 (L3<sub>C</sub>). As in L2<sub>C</sub> (<bold>A</bold>), no SDS-stable Sup35 NM aggregates are detectable in progeny R2, R3, or R4 clones. (<bold>C</bold>) Control Lineage 4 (L4<sub>C</sub>). As in L2<sub>C</sub> (<bold>A</bold>) and L3<sub>C</sub> (<bold>B</bold>), no SDS-stable Sup35 NM aggregates are detectable in progeny R2, R3, or R4 clones.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.009">http://dx.doi.org/10.7554/eLife.02949.009</ext-link></p></caption><graphic xlink:href="elife02949fs003"/></fig></fig-group><fig-group><fig id="fig5" position="float"><object-id pub-id-type="doi">10.7554/eLife.02949.010</object-id><label>Figure 5.</label><caption><title>Genealogy of <italic>E. coli</italic> cell lineages propagating Sup35 NM in an infectious prion conformation.</title><p>(<bold>A</bold>) The fate of Sup35 NM in four experimental lineages (L1<sub>E</sub>-L4<sub>E</sub>) established from a starter culture of cells containing Sup35 NM and New1 is shown. Clones that maintain or lose the Sup35 NM prion are indicated by black or pink lines, respectively. Rounds 1–4 (R1–R4) are depicted as gray arcs, with R1 situated at the center of the tree. Clones are designated as aggregate-positive if they contain SDS-stable Sup35 NM aggregates that are detectable in the undiluted sample and at least 1 of the 3 two-fold serial dilutions, as analyzed by filter retention. L1<sub>E</sub> and L3<sub>E</sub> retain SDS-stable Sup35 NM aggregates for the duration of the experiment (<xref ref-type="fig" rid="fig4">Figure 4A</xref>, <xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1B</xref>). L2<sub>E</sub> and L4<sub>E</sub> lose detectable SDS-stable Sup35 NM aggregates at R3 and R4, respectively. In both cases, the loss of SDS-stable aggregates coincides with a dramatic yet apparently reversible drop in fusion protein levels (<xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1A,C</xref>; see ‘Discussion’). Cells from four aggregate-positive L1<sub>E</sub>-R4 clones visualized by fluorescence microscopy are indicated by asterisks. (<bold>B</bold>) The fate of Sup35 NM in four control lineages (L1<sub>C</sub>–L4<sub>C</sub>) established from a starter culture of cells containing Sup35 NM alone is shown. None of the 120 clones analyzed contain SDS-stable Sup35 NM aggregates (<xref ref-type="fig" rid="fig4">Figure 4B</xref>, <xref ref-type="fig" rid="fig4s2">Figure 4—figure supplement 2</xref>). Cells from four aggregate-negative L1<sub>C</sub>-R4 clones visualized by fluorescence microscopy are indicated by asterisks. (<bold>C</bold>) Fluorescence images of representative cells corresponding to the four aggregate-positive R4 clones indicated by asterisks in (<bold>A</bold>). (<bold>D</bold>) Fluorescence images of representative cells corresponding to the four aggregate-negative R4 clones indicated by asterisks in (<bold>B</bold>). (<bold>E</bold>) <italic>E. coli</italic> cell extracts containing propagated, SDS-stable Sup35 NM aggregates are infectious when transformed into <italic>S. cerevisiae</italic> [<italic>psi</italic><sup>−</sup>] cells. A starter culture (ST) of cells containing Sup35 NM and New1 contain infectious SDS-stable Sup35 NM aggregates capable of converting [<italic>psi</italic><sup>−</sup>] yeast cells to [<italic>PSI</italic><sup>+</sup>]. In contrast, a starter culture of cells containing Sup35 NM alone lacks detectable infectivity. Progeny cell extracts transformed into yeast are identified as R<italic>X</italic>-<italic>Y</italic>, where <italic>X</italic> corresponds to a round number and <italic>Y</italic> corresponds to a clone number assigned sequentially and clockwise according to (<bold>A</bold>) and (<bold>B</bold>). Clones that gave rise to aggregate-negative progeny in the subsequent round are indicated by asterisks. Analysis of these data by Fisher's exact test indicates that the differences in the frequency of [<italic>PSI</italic><sup>+</sup>] transformants observed with samples containing SDS-stable Sup35 NM aggregates compared with the sample containing soluble Sup35 NM are statistically significant (p < 0.0001). The percentages given refer to strong [<italic>PSI</italic><sup>+</sup>] transformants; samples containing SDS-stable Sup35 NM aggregates (but not samples containing soluble Sup35 NM) also gave rise to weak [<italic>PSI</italic><sup>+</sup>] transformants (<xref ref-type="fig" rid="fig5s1">Figure 5—figure supplement 1</xref>), but these were not quantified (‘Results’).</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.010">http://dx.doi.org/10.7554/eLife.02949.010</ext-link></p></caption><graphic xlink:href="elife02949f005"/></fig><fig id="fig5s1" position="float" specific-use="child-fig"><object-id pub-id-type="doi">10.7554/eLife.02949.011</object-id><label>Figure 5—figure supplement 1.</label><caption><title>Bacterial cell extracts containing propagated, infectious Sup35 NM aggregates yield both strong and weak [<italic>PSI</italic><sup>+</sup>] yeast transformants.</title><p>The phenotypes of five representative strong [<italic>PSI</italic><sup>+</sup>] (<bold>A</bold>) and weak [<italic>PSI</italic><sup>+</sup>] (<bold>B</bold>) strains obtained by transforming <italic>S. cerevisiae</italic> [<italic>psi</italic><sup>−</sup>] cells with <italic>E. coli</italic> cell extracts containing propagated, SDS-stable Sup35 NM-aggregates on 1/4 YPD agar before (left) and after (right) passage on YPD agar supplemented with 3 mM GuHCl. For the purposes of comparison, untransformed [<italic>psi</italic><sup>−</sup>], weak [<italic>PSI</italic><sup>+</sup>], and strong [<italic>PSI</italic><sup>+</sup>] yeast strains are shown.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.011">http://dx.doi.org/10.7554/eLife.02949.011</ext-link></p></caption><graphic xlink:href="elife02949fs004"/></fig></fig-group></p><p>The remaining two experimental lineages (L2<sub>E</sub> and L4<sub>E</sub>) lost detectable SDS-stable Sup35 NM aggregates at R3 and R4, respectively (<xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1A,C</xref>, <xref ref-type="fig" rid="fig5">Figure 5A</xref>). Moreover, the loss of aggregates manifested itself in all ten of the selected colonies at either R3 or R4 (<xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1A,C</xref>, <xref ref-type="fig" rid="fig5">Figure 5A</xref>). Curiously, the loss of SDS-stable Sup35 NM aggregates from a particular lineage coincided with a loss of detectable fusion protein, as assessed by Western blot analysis (<xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1A,C</xref>), suggesting that the loss of aggregates represented an indirect consequence of a radical drop in protein levels (see ‘Discussion’). We note that the observed drop in Sup35 NM-mCherry-His<sub>6x</sub> fusion protein levels is not irreversible, as exemplified by L2<sub>E</sub>, which exhibited a loss of detectable Sup35 NM aggregates coincident with an R3 drop in fusion protein levels and an apparent restoration of fusion protein levels by R4 in all 10 samples (<xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1A</xref>). Despite the presence of normal levels of fusion protein, SDS-stable Sup35 NM aggregates were not recovered in R4 of L2<sub>E</sub>, consistent with the expectation that prion propagation requires that prion protein synthesis be maintained above some threshold level (<xref ref-type="fig" rid="fig4s1">Figure 4—figure supplement 1A</xref>, <xref ref-type="fig" rid="fig5">Figure 5A</xref>; <xref ref-type="bibr" rid="bib27">Holmes et al., 2013</xref>). Critically, none of the samples (120 in total) from any of the four control lineages contained detectable SDS-stable Sup35 NM aggregates (<xref ref-type="fig" rid="fig4">Figure 4B</xref>, <xref ref-type="fig" rid="fig4s2">Figure 4—figure supplement 2</xref>).</p><p>Fluorescence microscopy revealed that cells containing propagated Sup35 NM aggregates exhibited smaller foci emanating from large aggregates typically localized at cell poles, a phenotype distinguished from experimental starter culture cells by the lack of twisted ring structures (<xref ref-type="fig" rid="fig5">Figure 5C</xref>). However, we observed one instance of aggregate-positive R1 cells exhibiting twisted ring structures (see <xref ref-type="fig" rid="fig6s2">Figure 6—figure supplement 2C</xref>). Whereas we cannot definitively assign the SDS-stable Sup35 NM aggregates detected by filter retention to those structures detected by fluorescence microscopy, we note that fluorescence microscopy of prion-containing yeast cells has also revealed structural diversity (<xref ref-type="bibr" rid="bib10">Derkatch et al<italic>.</italic>, 2001</xref>; <xref ref-type="bibr" rid="bib68">Zhou et al., 2001</xref>). Furthermore, cells from aggregate-negative samples invariably exhibited diffuse fluorescence (<xref ref-type="fig" rid="fig5">Figure 5D</xref>).<fig-group><fig id="fig6" position="float"><object-id pub-id-type="doi">10.7554/eLife.02949.012</object-id><label>Figure 6.</label><caption><title>Sup35 NM prion propagation in <italic>E. coli</italic> requires ClpB.</title><p>(<bold>A</bold>) Cartoon representation of how Sup35 NM can convert to its prion form in the presence of New1 and ClpB but cannot propagate in the prion conformation after cells have been cured of New1- and ClpB-encoding DNA. Sup35 NM and New1 (black) are depicted as fusions to mCherry (red) and mGFP (green), respectively. ClpB is depicted as a purple hexamer. (<bold>B</bold>) SDS-stable Sup35 NM aggregates are detected in 5 of 20 Round 1 (R1) wild-type (WT) clones derived from a starter culture (ST) of wild-type cells containing Sup35 NM and New1 as assessed by filter retention analysis. In total, 17 of 60 R1 wild-type clones are aggregate-positive (<xref ref-type="fig" rid="fig6s2">Figure 6—figure supplement 2A</xref>). Starter cultures of cells containing Sup35 NM and New1 and cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. In all 20 R1 wild-type clones shown, full-length (FL) ClpB is detectable, Sup35 NM fusion protein levels are comparable, and New1 fusion protein is not detectable as assessed by Western blot analysis. The α-His<sub>6X</sub> and α-Sup35 antibodies recognize the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein, the α-GFP antibody recognizes the New1–mGFP fusion protein, the α-ClpB antibody recognizes the <italic>E. coli</italic> ClpB chaperone, and the α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase. Cells from four aggregate-positive R1 wild-type clones visualized by fluorescence microscopy (<xref ref-type="fig" rid="fig6s2">Figure 6—figure supplement 2C</xref>) are indicated by asterisks. (<bold>C</bold>) SDS-stable Sup35 NM aggregates are not detectable in R1 Δ<italic>clpB</italic> clones derived from a starter culture of Δ<italic>clpB</italic> cells containing Sup35 NM, New1, and ectopically produced ClpB as assessed by filter retention analysis. In total, 0 of 60 R1 Δ<italic>clpB</italic> clones are aggregate-positive (<xref ref-type="fig" rid="fig6s2">Figure 6—figure supplement 2B</xref>). Starter cultures of wild-type cells containing Sup35 NM and New1 and wild-type cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. In all 20 R1 Δ<italic>clpB</italic> clones shown, Sup35 NM fusion protein levels are comparable, and neither ClpB nor New1 fusion protein is detectable as assessed by Western blot analysis. Cells from four aggregate-negative R1 wild-type clones visualized by fluorescence microscopy (<xref ref-type="fig" rid="fig6s2">Figure 6—figure supplement 2D</xref>) are indicated by asterisks. (<bold>D</bold>) Extract prepared from cells lacking ClpB is not infectious when transformed into <italic>S. cerevisiae</italic> [<italic>psi</italic><sup>–</sup>] cells. Starter cultures of wild-type cells transformed with pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic> as well as Δ<italic>clpB</italic> cells transformed with pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> contain infectious SDS-stable Sup35 NM aggregates capable of converting [<italic>psi</italic><sup>−</sup>] yeast cells to [<italic>PSI</italic><sup>+</sup>]. Wild-type starter culture cells containing Sup35 NM alone lack detectable infectivity. An aggregate-positive R1 wild-type clone retains infectious Sup35 NM aggregates. In contrast, an aggregate-negative R1 Δ<italic>clpB</italic> clone lacks detectable infectivity, as does an aggregate-negative R1 wild-type clone. Analysis of these data by Fisher's exact test indicates that the differences in the frequency of [<italic>PSI</italic><sup>+</sup>] transformants observed with samples containing SDS-stable Sup35 NM aggregates compared with the samples containing soluble Sup35 NM are statistically significant (p < 0.0001).</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.012">http://dx.doi.org/10.7554/eLife.02949.012</ext-link></p></caption><graphic xlink:href="elife02949f006"/></fig><fig id="fig6s1" position="float" specific-use="child-fig"><object-id pub-id-type="doi">10.7554/eLife.02949.013</object-id><label>Figure 6—figure supplement 1.</label><caption><title>Δ<italic>clpB</italic> cells containing New1 and ectopically produced ClpB support the formation of SDS-stable Sup35 NM aggregates.</title><p>(<bold>A</bold>) SDS-stable Sup35 NM aggregates are detected in wild-type (WT) cells producing SDS-stable New1 aggregates as assessed by filter retention analysis. SDS-stable Sup35 NM aggregates are also detected in Δ<italic>clpB</italic> cells containing SDS-stable New1 aggregates and ectopically produced ClpB. The α-His<sub>6X</sub> antibody detects the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein, and the α-GFP antibody detects the New1-mGFP fusion protein. A lane cropped from the same immunoblot is indicated by a hash mark. Intracellular levels of full-length (FL) ClpB, Sup35 NM fusion protein, and New1 fusion protein are comparable in the presence and absence of New1 and ectopically produced ClpB as assessed by Western blot analysis. The α-ClpB antibody recognizes the <italic>E. coli</italic> ClpB chaperone, the α-Sup35 antibody recognizes the Sup35 NM fusion protein, and the α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase. (<bold>B</bold>) Fluorescence images of representative wild-type cells containing Sup35 NM and New1 and Δ<italic>clpB</italic> cells containing Sup35 NM, New1, and ectopically produced ClpB. The mCherry channel, GFP channel, and merged images are shown.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.013">http://dx.doi.org/10.7554/eLife.02949.013</ext-link></p></caption><graphic xlink:href="elife02949fs005"/></fig><fig id="fig6s2" position="float" specific-use="child-fig"><object-id pub-id-type="doi">10.7554/eLife.02949.014</object-id><label>Figure 6—figure supplement 2.</label><caption><title>The fate of Sup35 NM in 40 wild-type R1 clones and 40 Δ<italic>clpB</italic> R1 clones.</title><p>(<bold>A</bold>) SDS-stable Sup35 NM aggregates are detected in 12 of 40 Round 1 (R1) wild-type (WT) clones derived from a starter culture (ST) of wild-type cells containing Sup35 NM and New1 as assessed by filter retention analysis. In total, 17 of 60 R1 wild-type clones are aggregate-positive (<xref ref-type="fig" rid="fig6">Figure 6B</xref>). Starter cultures of cells containing Sup35 NM and New1 and cells containing Sup35 NM alone serve as positive (P) and negative (N) controls, respectively. The α-His<sub>6X</sub> antibody detects the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein. (<bold>B</bold>) In contrast, 0 of 40 R1 Δ<italic>clpB</italic> clones derived from a starter culture of Δ<italic>clpB</italic> cells transformed with pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> contain detectable SDS-stable Sup35 NM aggregates. In total, 0 of 60 R1 Δ<italic>clpB</italic> clones are aggregate-positive (<xref ref-type="fig" rid="fig6">Figure 6C</xref>). The observed difference in the number of aggregate-positive clones of wild-type vs Δ<italic>clpB</italic> cells is statistically significant (p < 0.0001 as determined by Fisher's Exact Test). (<bold>C</bold>) Fluorescence images of representative cells corresponding to the four aggregate-positive R1 wild-type clones indicated by asterisks in <xref ref-type="fig" rid="fig6">Figure 6B</xref>. Notably, wild-type clone R1-14 exhibits twisted ring structures. (<bold>D</bold>) Fluorescence images of representative cells corresponding to the four aggregate-negative R1 Δ<italic>clpB</italic> clones indicated by asterisks in <xref ref-type="fig" rid="fig6">Figure 6C</xref>.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.014">http://dx.doi.org/10.7554/eLife.02949.014</ext-link></p></caption><graphic xlink:href="elife02949fs006"/></fig></fig-group></p></sec><sec id="s2-2"><title>Propagated SDS-stable Sup35 NM aggregates are infectious when introduced into [<italic>psi</italic><sup>−</sup>] yeast cells</title><p>We next sought to determine whether cells that maintained SDS-stable Sup35 NM aggregates in the absence of New1 contained infectious material capable of converting [<italic>psi</italic><sup>−</sup>] yeast cells to [<italic>PSI</italic><sup>+</sup>]. We prepared bacterial cell extracts from both experimental and control starter cultures, as well as aggregate-positive samples from each of the four experimental lineages. For each experimental lineage, we examined an arbitrarily chosen sample obtained from the last aggregate-positive round. In addition, for L2<sub>E</sub> and L4<sub>E</sub>, we examined, respectively, the R2 and R3 samples (indicated by asterisks in <xref ref-type="fig" rid="fig5">Figure 5E</xref>) that gave rise to aggregate-negative clones in the subsequent round. We used these bacterial extracts to transform <italic>S. cerevisiae</italic> spheroplasts prepared from a [<italic>pin</italic><sup>−</sup>][<italic>psi</italic><sup>−</sup>] strain. The use of a [<italic>pin</italic><sup>−</sup>] recipient strain was critical as transient overproduction of Sup35 (or Sup35 NM) in [<italic>PIN</italic><sup>+</sup>][<italic>psi</italic><sup>−</sup>] strains significantly stimulates the conversion from [<italic>psi</italic><sup>−</sup>] to [<italic>PSI</italic><sup>+</sup>] (<xref ref-type="bibr" rid="bib12">Derkatch et al., 1997</xref>), whereas conversion in a [<italic>pin</italic><sup>−</sup>][<italic>psi</italic><sup>−</sup>] background requires the introduction of infectious seed material (<xref ref-type="bibr" rid="bib56">Tanaka and Weissman, 2006</xref>).</p><p>The experimental starter culture yielded [<italic>PSI</italic><sup>+</sup>] yeast transformants at a frequency of ∼1% (<xref ref-type="fig" rid="fig5">Figure 5E</xref>), consistent with our previous findings (<xref ref-type="bibr" rid="bib21">Garrity et al., 2010</xref>). Similarly, each of the aggregate-positive samples from the four experimental lineages yielded [<italic>PSI</italic><sup>+</sup>] yeast transformants at a frequency of ∼1%; in contrast, the aggregate-negative samples yielded no [<italic>PSI</italic><sup>+</sup>] yeast transformants (<xref ref-type="fig" rid="fig5">Figure 5E</xref>). Among the [<italic>PSI</italic><sup>+</sup>] transformants we obtained with the experimental samples, we observed both ‘strong’ and ‘weak’ strains (<xref ref-type="fig" rid="fig5s1">Figure 5—figure supplement 1</xref>; <xref ref-type="bibr" rid="bib55">Tanaka et al., 2004</xref>; <xref ref-type="bibr" rid="bib20">Frederick et al., 2014</xref>). We note that ∼1% corresponds only to the frequency of strong [<italic>PSI</italic><sup>+</sup>] transformants and therefore represents a conservative estimate of <italic>E. coli</italic> cell extract infectivity; we did not attempt to quantify weak [<italic>PSI</italic><sup>+</sup>] transformants because they are difficult to distinguish from [<italic>psi</italic><sup>−</sup>] transformants on the medium utilized to isolate transformants. We conclude that <italic>E. coli</italic> cells can propagate Sup35 NM in an infectious prion conformation over at least ∼100 generations under conditions that do not permit de novo prion formation.</p></sec><sec id="s2-3"><title>Propagation of infectious Sup35 NM aggregates depends on ClpB</title><p>The propagation of [<italic>PSI</italic><sup>+</sup>] and other prions in yeast requires Hsp104, an Hsp100-family ATP-dependent disaggregase that functions as a ring-shaped hexamer. Specifically, Hsp104 is thought to facilitate prion propagation by fragmenting large aggregates into smaller propagons that are subsequently disseminated during cell division (<xref ref-type="bibr" rid="bib43">Paushkin et al., 1996</xref>; <xref ref-type="bibr" rid="bib38">Ness et al., 2002</xref>; <xref ref-type="bibr" rid="bib9">Cox et al., 2003</xref>; <xref ref-type="bibr" rid="bib29">Kryndushkin et al., 2003</xref>; <xref ref-type="bibr" rid="bib48">Satpute-Krishnan et al., 2007</xref>; <xref ref-type="bibr" rid="bib26">Higurashi et al., 2008</xref>). We therefore investigated whether or not the propagation of Sup35 NM aggregates in <italic>E. coli</italic> requires ClpB, the bacterial ortholog of Hsp104. To address this question, we sought to deplete cells of ClpB specifically during the propagation phase of our experiments. To accomplish this, we modified pSC101<sup>TS</sup>-<italic>NEW1</italic> such that it also directed the expression of <italic>clpB</italic> under the control of its native promoter. When transformed into Δ<italic>clpB</italic> cells, pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> enabled us to grow starter cultures containing ClpB and subsequently to deplete both ClpB and New1 in cells plated at the non-permissive temperature (<xref ref-type="fig" rid="fig6">Figure 6A</xref>).</p><p>As expected, we detected SDS-stable Sup35 NM aggregates in Δ<italic>clpB</italic> starter culture cells transformed with pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> (<xref ref-type="fig" rid="fig6s1">Figure 6—figure supplement 1A</xref>). Furthermore, fluorescence microscopy revealed that these cells contained visible aggregates that were nearly indistinguishable from those in wild-type cells containing pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic> (<xref ref-type="fig" rid="fig6s1">Figure 6—figure supplement 1B</xref>). After plating Δ<italic>clpB</italic> starter culture cells containing pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> at the non-permissive temperature to cure cells of ClpB- and New1-encoding DNA, we examined 60 R1 colonies for the presence of SDS-stable Sup35 NM aggregates. In parallel, we examined 60 R1 colonies derived from wild-type starter culture cells containing pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>. As before, every selected colony was patched onto selective medium to test for the loss of pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> or pSC101<sup>TS</sup>-<italic>NEW1</italic> and inoculated into liquid medium for overnight growth to test for the presence of SDS-stable Sup35 NM aggregates. All selected colonies had lost the appropriate temperature-sensitive vector and the absence of New1 and/or ClpB was confirmed by Western blot analysis (<xref ref-type="fig" rid="fig6">Figure 6B</xref>, <xref ref-type="fig" rid="fig6">Figure 6C</xref>). Whereas 17 of 60 (28%) wild-type R1 samples tested aggregate-positive, all Δ<italic>clpB</italic> R1 samples tested aggregate-negative (<xref ref-type="fig" rid="fig6">Figure 6B</xref>, <xref ref-type="fig" rid="fig6s2">Figure 6—figure supplement 2A</xref>, <xref ref-type="fig" rid="fig6">Figure 6C</xref>, <xref ref-type="fig" rid="fig6s2">Figure 6—figure supplement 2B</xref>). Western blot analysis revealed that the wild-type and Δ<italic>clpB</italic> R1 cells contained comparable amounts of Sup35 NM fusion protein (<xref ref-type="fig" rid="fig6">Figure 6B</xref>, <xref ref-type="fig" rid="fig6">Figure 6C</xref>). Furthermore, yeast transformation assays confirmed the presence of infectious material capable of converting [<italic>psi</italic><sup>−</sup>] yeast cells to [<italic>PSI</italic><sup>+</sup>] in Δ<italic>clpB</italic> starter culture cells transformed with pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> as well as in an aggregate-positive R1 clone derived from wild-type starter culture cells (<xref ref-type="fig" rid="fig6">Figure 6D</xref>). In contrast, a Δ<italic>clpB</italic> R1 clone derived from Δ<italic>clpB</italic> starter culture cells containing pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> as well as an aggregate-negative R1 clone derived from wild-type starter culture cells containing pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup> lacked detectable infectivity (<xref ref-type="fig" rid="fig6">Figure 6D</xref>). We conclude that cells lacking ClpB cannot propagate Sup35 NM in its infectious prion conformation.</p></sec><sec id="s2-4"><title>ClpB disaggregase activity is required for propagation of SDS-stable Sup35 NM aggregates</title><p>To investigate the mechanistic basis for the ClpB dependence of Sup35 NM prion propagation in <italic>E. coli</italic>, we devised a strategy that enabled us to test the abilities of specific ClpB mutants to support the propagation of SDS-stable Sup35 NM aggregates after their formation in the presence of wild-type ClpB. The disaggregase function of ClpB, which assembles as a two-tiered hexameric ring (<xref ref-type="bibr" rid="bib31">Lee et al., 2003</xref>), depends on its abilities to hydrolyze ATP, to translocate polypeptides through its central pore and to collaborate with DnaK (the bacterial Hsp70) and its co-chaperones DnaJ and the nucleotide exchange factor GrpE (reviewed in <xref ref-type="bibr" rid="bib16">Doyle and Wickner, 2009</xref>). Accordingly, we tested previously characterized ClpB mutants specifically defective for (i) ATP hydrolysis (E279A/E678A) (<xref ref-type="bibr" rid="bib64">Weibezahn et al., 2003</xref>) (ii) substrate threading through the ClpB pore (Y653A) (<xref ref-type="bibr" rid="bib65">Weibezahn et al., 2004</xref>), and (iii) collaboration with DnaK (E432A) (<xref ref-type="bibr" rid="bib40">Oguchi et al., 2012</xref>; <xref ref-type="bibr" rid="bib49">Seyffer et al., 2012</xref>; <xref ref-type="bibr" rid="bib3a">Carroni et al., 2014</xref>). We note that each of these ClpB mutants is fully proficient for oligomerization and only ClpB E279A/E678A is deficient in ATPase activity (<xref ref-type="bibr" rid="bib37">Mogk et al., 2003</xref>; <xref ref-type="bibr" rid="bib65">Weibezahn et al., 2004</xref>; <xref ref-type="bibr" rid="bib40">Oguchi et al., 2012</xref>). Our strategy required us to construct strains in which we could induce the production of a ClpB mutant specifically during the propagation phase of the experiment while providing wild-type ClpB during the formation phase of the experiment only. To accomplish this, we placed each of the mutant <italic>clpB</italic> alleles (or the wild-type allele) under the control of the anhydrotetracycline (aTc)-inducible promoter P<sub>LtetO-I</sub> (<xref ref-type="bibr" rid="bib35">Lutz and Bujard, 1997</xref>), integrated these constructs onto the chromosome of our Δ<italic>clpB</italic> strain, and transformed the resulting strains with pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic>.</p><p>As expected, we detected SDS-stable Sup35 NM aggregates in starter culture cells of all strains producing plasmid-encoded Sup35 NM-mCherry-His<sub>6X</sub>, New1-mGFP, and wild-type ClpB (<xref ref-type="fig" rid="fig7">Figure 7A</xref>). To determine whether or not each of the mutants could support the propagation of these aggregates following the depletion of New1 and wild-type ClpB, we plated the starter culture cells at the nonpermissive temperature on solid medium lacking or containing increasing concentrations of aTc, generating sets of R1 colonies. We prepared cell extracts from scraped R1 colonies (‘Materials and methods’) and examined these extracts for the presence or absence of SDS-stable Sup35 NM aggregates. Whereas SDS-stable Sup35 NM aggregates were detected as a function of increasing aTc concentration in cells carrying the wild-type <italic>clpB</italic> allele, no aggregates were detected in cells harboring the <italic>clpB</italic> E279A/E678A, <italic>clpB</italic> Y653A, or <italic>clpB</italic> E432A allele at any concentration of aTc (<xref ref-type="fig" rid="fig7">Figure 7A</xref>). Western blot analysis revealed that levels of chromosomally-encoded wild-type ClpB and each of the three disaggregase mutants were comparable in cell extracts prepared from colonies scraped off of plates containing 50 ng/ml aTc (<xref ref-type="fig" rid="fig7">Figure 7B</xref>). Furthermore, replica plating confirmed that all colonies of R1 cells grown on medium supplemented with 50 ng/ml aTc had been cured of pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> (<xref ref-type="fig" rid="fig7s1">Figure 7—figure supplement 1</xref>). We conclude that ATP hydrolysis coupled to substrate translocation through the ClpB central pore and collaboration with DnaK are required for propagation of SDS-stable Sup35 NM aggregates in the absence of New1.<fig-group><fig id="fig7" position="float"><object-id pub-id-type="doi">10.7554/eLife.02949.015</object-id><label>Figure 7.</label><caption><title>Propagation of SDS-stable Sup35 NM aggregates in <italic>E. coli</italic> requires ClpB disaggregase activity.</title><p>(<bold>A</bold>) SDS-stable Sup35 NM aggregates are detected in starter cultures (ST) of Δ<italic>clpB</italic> cells containing pBR322-<italic>SUP35 NM</italic>, pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic>, and one of four aTc-inducible chromosomal <italic>clpB</italic> alleles. Wild-type (WT) ClpB is depicted as a purple hexamer. ClpB E279A/E678A is unable to hydrolyze ATP, ClpB Y653A is pore-deficient, and ClpB E432A is unable to collaborate with DnaK. Propagated Sup35 NM aggregates are detected in scraped cell suspensions as a function of increasing aTc concentration only for Round 1 (R1) clones producing wild-type ClpB. Sup35 NM aggregates are not detected at any aTc concentration in scraped cell suspensions of R1 clones producing ClpB disaggregase mutants or in R1 clones lacking ClpB. Lanes cropped from the same immunoblot are indicated by hash marks. The α-His<sub>6X</sub> antibody recognizes the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein. (<bold>B</bold>) Wild-type and mutant ClpB levels along with Sup35 NM fusion protein levels are comparable in R1 clones grown on solid medium supplemented with 50 ng/ml aTc as assessed by Western blot analysis. The α-Sup35 antibody recognizes the Sup35 NM-mCherry-His<sub>6X</sub> fusion protein, the α-GFP antibody recognizes the New1-mGFP fusion protein, the α-ClpB antibody recognizes the <italic>E. coli</italic> ClpB chaperone, and the α-RpoA antibody recognizes the α subunit of <italic>E. coli</italic> RNA polymerase.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.015">http://dx.doi.org/10.7554/eLife.02949.015</ext-link></p></caption><graphic xlink:href="elife02949f007"/></fig><fig id="fig7s1" position="float" specific-use="child-fig"><object-id pub-id-type="doi">10.7554/eLife.02949.016</object-id><label>Figure 7—figure supplement 1.</label><caption><title>All Round 1 clones producing wild-type ClpB are cured of pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic>.</title><p>All Round 1 (R1) clones derived from a starter culture of Δ<italic>clpB</italic> cells containing pBR322-<italic>NM SUP35</italic>, pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic>, and chromosomal aTc-inducible wild-type <italic>clpB</italic> lose pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> as assessed by replica plating from solid medium supplemented with carbenicillin (Carb), chloramphenicol (Cam), IPTG, and 50 ng/ml aTc to solid medium containing either Carb or Cam. pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> confers Cam resistance.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.016">http://dx.doi.org/10.7554/eLife.02949.016</ext-link></p></caption><graphic xlink:href="elife02949fs007"/></fig></fig-group></p></sec></sec><sec id="s3" sec-type="discussion"><title>Discussion</title><p>Our findings establish that bacteria can propagate a prion. This is, to our knowledge, the first formal demonstration of prion propagation in a non-eukaryote. More specifically, the [<italic>PIN</italic><sup>+</sup>]-dependent de novo conversion of Sup35 NM to its prion form in our <italic>E. coli</italic> system enabled us to distinguish experimentally between the initial formation phase and subsequent propagation phase of the prion cycle. Under our experimental conditions, two of four cell lineages (L1<sub>E</sub> and L3<sub>E</sub>) maintained the prion for the duration of the experiment (that is, ∼100 generations), one lineage (L4<sub>E</sub>) maintained the prion for ∼80 generations, and one lineage (L2<sub>E</sub>) maintained the prion for ∼60 generations. Furthermore, our work demonstrates that prion propagation in <italic>E. coli</italic> requires the disaggregase activity of ClpB, the bacterial ortholog of Hsp104. We conclude that bacteria can support a chaperone-dependent, protein-based mode of heredity and speculate that the emergence of prion-like phenomena may have predated the evolutionary split between eukaryotes and bacteria.</p><sec id="s3-1"><title>Stability of prion propagation in <italic>E. coli</italic></title><p>As only two of four lineages retained the prion for the full duration of our experiments, propagation of the Sup35 NM prion may be less stable in <italic>E. coli</italic> than in <italic>S. cerevisiae</italic> (<xref ref-type="bibr" rid="bib15">DiSalvo et al., 2011</xref>). However, as noted above, loss of the prion in two lineages was coincident with a dramatic drop in Sup35 NM fusion protein levels. Furthermore, this drop was evidently reversible as Sup35 NM fusion protein levels were restored in R4 of L2<sub>E</sub> without reappearance of the prion. We do not understand the mechanism underlying this reversible change in protein levels; however, we suggest that stochastic fluctuations in plasmid copy number may set the stage for such an event. We note that our experiments were performed in <italic>recA</italic><sup>−</sup> cells, which should prevent plasmid rearrangements that might lead to a permanent loss of fusion protein coding capacity.</p></sec><sec id="s3-2"><title>Bacterial machinery capable of remodeling Sup35 NM aggregates</title><p>The question of whether or not ClpB can substitute for Hsp104 in promoting Sup35 prion propagation has been addressed in a number of studies yielding conflicting indications. On one hand, several in vitro studies have provided evidence that Hsp104 (<xref ref-type="bibr" rid="bib50">Shorter and Lindquist, 2004</xref>, <xref ref-type="bibr" rid="bib51">2006</xref>, <xref ref-type="bibr" rid="bib52">2008</xref>; <xref ref-type="bibr" rid="bib13">DeSantis et al., 2012</xref>), but not ClpB (<xref ref-type="bibr" rid="bib13">DeSantis et al., 2012</xref>), can fragment amyloid aggregates in the absence of auxiliary factors. Furthermore, whereas the presence of various combinations of <italic>S. cerevisiae</italic> Hsp70- and Hsp40-family proteins was found to modulate Hsp104 activity on amyloid substrates (<xref ref-type="bibr" rid="bib52">Shorter and Lindquist, 2008</xref>; <xref ref-type="bibr" rid="bib13">DeSantis et al., 2012</xref>), ClpB appeared to remain inert even in the presence of bacterial Hsp70 (DnaK), Hsp40 (DnaJ), and nucleotide exchange factor GrpE despite exhibiting robust activity on various disordered protein aggregates in vitro (<xref ref-type="bibr" rid="bib13">DeSantis et al., 2012</xref>).</p><p>On the other hand, the results of several in vivo studies suggest that ClpB, in the presence of appropriate co-chaperones, is competent to support Sup35 prion propagation in yeast (<xref ref-type="bibr" rid="bib60">Tipton et al., 2008</xref>; <xref ref-type="bibr" rid="bib45">Reidy et al., 2012</xref>). Based on an analysis of the in vivo activities of Hsp104/ClpB chimeras, Tipton et al. argue that prion replication in yeast requires that Hsp104 collaborate with its cognate Hsp70 chaperone system. A logical inference from their work is that the inability of ClpB to substitute for Hsp104 in supporting Sup35 prion propagation in <italic>S. cerevisiae</italic> is an indirect consequence of the inability of ClpB to cooperate with fungal co-chaperones. More recently, Reidy et al. provided direct support for this inference. In particular, Reidy et al. found that ClpB supported prion propagation in yeast provided that DnaK and GrpE were present. Interestingly, the activity of the bacterial disaggregase machinery in yeast was dependent on the fungal Hsp40-family Sis1 protein, consistent with prior work implicating Sis1 as a necessary component of the chaperone network required for prion propagation in yeast (<xref ref-type="bibr" rid="bib26">Higurashi et al., 2008</xref>; <xref ref-type="bibr" rid="bib60">Tipton et al., 2008</xref>). Our work demonstrates that no exogenous fungal accessory factors are required for prion propagation in bacteria. Taken together, these observations argue that the amyloid remodeling activity of Hsp104 is an evolutionarily conserved feature of the Hsp100-family chaperones, an inference that is strongly supported by our finding that propagation of the Sup35 NM prion in <italic>E. coli</italic> requires ClpB disaggregase activity.</p><p>Despite the apparent prevalence of prions in the fungal kingdom, to date, no bacterial prion has been identified. Notably, the absence of cytoplasmic mixing during conjugation would preclude the discovery of prion-like phenomena by classic genetic approaches, which facilitated the discovery of prions in yeast based on the non-Mendelian inheritance of their associated phenotypes (<xref ref-type="bibr" rid="bib8">Cox, 1965</xref>; <xref ref-type="bibr" rid="bib1">Aigle and Lacroute, 1975</xref>; <xref ref-type="bibr" rid="bib66">Wickner, 1994</xref>). Nevertheless, recent bioinformatic analyses of prokaryotic proteomes have revealed that bacterial and archaeal genomes encode many proteins containing glutamine- and asparagine-rich prion-like domains resembling those found in most confirmed and putative <italic>S. cerevisiae</italic> prions (<xref ref-type="bibr" rid="bib2">Alberti et al., 2009</xref>; <xref ref-type="bibr" rid="bib18">Espinosa Angarica et al., 2013</xref>; Yuan et al., unpublished data). Moreover, it is becoming increasingly clear that Q/N-richness at the level of primary amino acid sequence is neither a prerequisite for prion conversion (<xref ref-type="bibr" rid="bib57">Taneja et al., 2007</xref>; <xref ref-type="bibr" rid="bib54">Suzuki et al., 2012</xref>) nor protein amyloidogenesis (<xref ref-type="bibr" rid="bib23">Goldschmidt et al., 2010</xref>). In fact, several bacteria utilize non-Q/N-rich amyloid-forming proteins to assemble extracellular appendages mediating surface attachment and biofilm formation (<xref ref-type="bibr" rid="bib5">Chapman et al., 2002</xref>; <xref ref-type="bibr" rid="bib46">Romero et al., 2010</xref>). These considerations—in conjunction with the work presented here—suggest that prions or prion-like proteins may exist as epigenetic reservoirs of phenotypic diversity in the bacterial domain of life.</p></sec></sec><sec id="s4" sec-type="materials|methods"><title>Materials and methods</title><sec id="s4-1"><title>Strains, plasmids, and cell growth</title><p>Bacteria experiments were performed with <italic>E. coli</italic> strain DH5αZ1 (<xref ref-type="bibr" rid="bib35">Lutz and Bujard, 1997</xref>) grown in LB (Miller) medium. To construct DH5αZ1 Δ<italic>clpB</italic>, a temperature-sensitive plasmid encoding the RecA protein (pSC101<sup>TS</sup>-<italic>recA</italic>) was constructed and transformed into DH5αZ1 cells. A Δ<italic>clpB</italic>::<italic>kan</italic> allele from strain JW2573 (Keio collection) was transferred to DH5αZ1 cells containing pSC101<sup>TS</sup>-<italic>recA</italic> via P1 transduction. Cells were subsequently cured of pSC101<sup>TS</sup>-<italic>recA</italic> by overnight growth and plating in the absence of antibiotic selection at the non-permissive temperature (37°C).</p><p>To construct strains harboring chromosomal P<sub>LtetO-I</sub>-<italic>clpB</italic> alleles, plasmids pAY152, pAY154, pAY155, pAY156, and pAY157 were cloned in strain AY290 and integrated onto the chromosome of strain AY295 at <italic>attB</italic>(HK022). Single-copy integrants were selected on LB agar supplemented with kanamycin (10 μg/ml) and verified by PCR as described (<xref ref-type="bibr" rid="bib24">Haldimann and Wanner, 2001</xref>).</p><p>Yeast experiments were performed with <italic>S. cerevisiae</italic> strain YJW187 [<italic>pin</italic><sup>−</sup>][<italic>psi</italic><sup>−</sup>] grown in yeast extract peptone dextrose (YPD) medium. For yeast infectivity assays, cell extracts were co-transformed with pRS316 into YJW187 spheroplasts; [<italic>PSI</italic><sup>+</sup>] URA<sup>+</sup> transformants were identified by plating the yeast cells in top agar containing synthetic defined medium lacking uracil and adenine (SD-Ura-Ade) and supplemented with 10 mg/ml adenine hemisulfate (Sunrise Science, San Diego, CA).</p><p>Further details concerning strains and plasmids are provided in <xref ref-type="supplementary-material" rid="SD1-data">Supplementary file 1</xref>.</p></sec><sec id="s4-2"><title>Propagation experiments</title><p>Cells were transformed with pBR322-<italic>SUP35 NM</italic> and pSC101<sup>TS</sup>, pSC101<sup>TS</sup>-<italic>NEW1</italic>, or pSC101<sup>TS</sup>-<italic>NEW1</italic>-<italic>clpB</italic> and grown at 30°C on LB agar supplemented with carbenicillin (Carb, 100 μg/ml) and chloramphenicol (Cam, 12.5 μg/ml). Starter cultures were generated by growing transformants at 30°C in 6 ml of LB broth supplemented with Carb (100 μg/ml), Cam (12.5 μg/ml), and 10 μM IPTG to an OD<sub>600</sub> of 2.0–2.5. To cure cells of pSC101<sup>TS</sup>-derivatives and generate Round 1 (R1) colonies, starter cultures were diluted (10<sup>−5</sup>) in pre-warmed (37°C) LB broth supplemented with Carb (100 μg/ml) and 10 μM IPTG. Diluted cells were grown at 37°C on pre-warmed (37°C) LB agar supplemented with Carb (100 μg/ml) and 10 μM IPTG. R1–R4 colonies were, (a) patched on LB agar supplemented with Cam (12.5 μg/ml), (b) restreaked and grown at 30°C on pre-warmed (30°C) LB agar supplemented with Carb (100 μg/ml) and 10 μM IPTG, and (c) inoculated and grown at 30°C in 6 ml LB broth supplemented with Carb (100 μg/ml) and 10 μM IPTG. For analysis of ClpB disaggregase mutants, ∼1000 R1 colonies were gently scraped off LB agar plates containing Carb (100 μg/ml), 10 μM IPTG, and a range of aTc concentrations (0–500 ng/ml) in 3 ml LB broth supplemented with Carb (100 μg/ml) and 10 μM IPTG.</p><p>Cell cultures and scraped cell suspensions were normalized to 8 ml of an OD<sub>600</sub> of 1.0 and pelleted by centrifugation. Cell pellets were resuspended in 166 ml STC Buffer (1 M sorbitol, 10 mM Tris–HCl [pH 7.5], 10 mM CaCl<sub>2</sub>) supplemented with 10 U of rLysozme (Novagen, Germany) and 0.1 U of OmniCleave endonuclease (Epicentre, Wisconsin, MA), incubated at room-temperature for 30 min, and incubated on ice for an additional 30 min. Omnicleave endonuclease was omitted from samples destined for PCR analysis and yeast infectivity assays. Finally, samples were flash frozen and thawed on ice to yield unclarified lysates (used in filter retention assays). To generate partially clarified lysates (used in Western blot analysis and yeast transformation assays), unclarified lysates were subjected to two rounds of low-speed centrifugation, each at 500 RCF for 15 min at 4°C.</p></sec><sec id="s4-3"><title>Filter retention assays</title><p>25 μl of unclarified lysates was added to 375 μl of BugBuster protein extraction reagent (Novagen) supplemented with 5 U of rLysozyme and 0.1 U of Omnicleave endonuclease and gently rocked at room-temperature for 30 min. Samples were challenged with 100 μl of 10% (wt/vol) SDS (2% SDS final concentration) and gently rocked at room-temperature for an additional 30 min. For each sample, 100 μl of undiluted lysate and three twofold serial dilutions made in PBS containing 2% SDS were filtered through a 0.2-μm cellulose acetate membrane (Advantec, Japan) in a dot-blotting vacuum manifold. Samples on membranes were washed twice with 100 μl of PBS containing 2% SDS and twice with 100 μl of PBS.</p></sec><sec id="s4-4"><title>Immunoblotting</title><p>Cellulose acetate membranes (used in filter retention assays) and Hybond-C Extra nitrocellulose membranes (used in Western blot analysis) were blocked for 30 min in PBS containing 3% (wt/vol) milk. Membranes were probed with one of the following primary antibodies: anti-Sup35 (yS-20, Santa Cruz Biotechnology, Dallas, TX, 1:5000), anti-His<sub>6X</sub> (His-2; Roche, Indianapolis, IN, 1:10,000), anti-GFP (Roche, 1:10,000), anti-RpoA (NeoClone, Madison, WI, 1:10,000), or anti-ClpB (gift from S Wickner, 1:10,000). Membranes were washed and probed with one of the following HRP-conjugated secondary antibodies: anti-goat IgG (Santa Cruz Biotechnology, 1:10,000), anti-mouse IgG (Cell Signaling, Beverly, MA, 1:10,000), or anti-rabbit IgG (Cell Signaling, 1:10,000). Proteins were detected with ECL Plus Western blot detection reagents (GE Healthcare, Pittsburgh, PA) and a ChemiDock XRS+ imaging system (Bio-Rad, Hercules, CA).</p></sec><sec id="s4-5"><title>Yeast infectivity assays</title><p>Protein concentrations of partially clarified <italic>E. coli</italic> cell extracts were determined by the bicinchoninic acid (BCA) assay (ThermoFisher, Waltham, MA) and normalized to ∼1 mg/ml. Protein transformations were performed as previously described (<xref ref-type="bibr" rid="bib56">Tanaka and Weissman, 2006</xref>; <xref ref-type="bibr" rid="bib21">Garrity et al., 2010</xref>). Each and every putative [<italic>PSI</italic><sup>+</sup>] transformant was (a) restreaked on 1/4 YPD agar to assess the [<italic>PSI</italic><sup>+</sup>] phenotype, (b) restreaked on YPD containing 3 mM GuHCl to cure cells of [<italic>PSI</italic><sup>+</sup>], and (c) restreaked on 1/4 YPD to assess the [<italic>psi</italic><sup>−</sup>] phenotype. Only those transformants exhibiting curability were scored as [<italic>PSI</italic><sup>+</sup>].</p></sec><sec id="s4-6"><title>Fluorescence microscopy</title><p>Cells were spotted onto 1% (wt/vol) agarose pads consisting of Seakem LE Agarose (Lonza, Walkersville, MD) in PBS and visualized with an UplanFL N 100x/1.30 phase contrast objective mounted on an Olympus BX61 microscope. Images were captured with a CoolSnapHQ camera (Photometrics, Tucson, AZ) and the Metamorph software package (Molecular Devices, Sunnyvale, CA). All fluorescence images were obtained from 10 ms exposures.</p></sec></sec></body><back><ack id="ack"><title>Acknowledgements</title><p>We thank Simon Dove (Harvard Medical School, Boston, MA) for comments on the manuscript, Sue Wickner (National Cancer Institute, Bethesda, MD) for anti-ClpB serum, and Renate Hellmiss for preparing <xref ref-type="fig" rid="fig2">Figure 2</xref>.</p></ack><sec sec-type="additional-information"><title>Additional information</title><fn-group content-type="competing-interest"><title>Competing interests</title><fn fn-type="conflict" id="conf1"><p>The authors declare that no competing interests exist.</p></fn></fn-group><fn-group content-type="author-contribution"><title>Author contributions</title><fn fn-type="con" id="con1"><p>AHY, Conception and design, Acquisition of data, Analysis and interpretation of data, Drafting or revising the article</p></fn><fn fn-type="con" id="con2"><p>SJG, Conception and design, Contributed unpublished essential data or reagents</p></fn><fn fn-type="con" id="con3"><p>EN, Conception and design, Contributed unpublished essential data or reagents</p></fn><fn fn-type="con" id="con4"><p>AH, Conception and design, Analysis and interpretation of data, Drafting or revising the article</p></fn></fn-group></sec><sec sec-type="supplementary-material"><title>Additional files</title><supplementary-material id="SD1-data"><object-id pub-id-type="doi">10.7554/eLife.02949.017</object-id><label>Supplementary file 1.</label><caption><p>Strains and Plasmids.</p><p><bold>DOI:</bold> <ext-link ext-link-type="doi" xlink:href="10.7554/eLife.02949.017">http://dx.doi.org/10.7554/eLife.02949.017</ext-link></p></caption><media mime-subtype="pdf" mimetype="application" xlink:href="elife02949s001.pdf"/></supplementary-material></sec><ref-list><title>References</title><ref id="bib1"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Aigle</surname><given-names>M</given-names></name><name><surname>Lacroute</surname><given-names>F</given-names></name></person-group><year>1975</year><article-title>Genetical aspects of [URE3], a non-mitochondrial, cytoplasmically inherited mutation in yeast</article-title><source>Molecular & General Genetics</source><volume>136</volume><fpage>327</fpage><lpage>335</lpage><pub-id pub-id-type="doi">10.1007/BF00341717</pub-id></element-citation></ref><ref id="bib2"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Alberti</surname><given-names>S</given-names></name><name><surname>Halfmann</surname><given-names>R</given-names></name><name><surname>King</surname><given-names>O</given-names></name><name><surname>Kapila</surname><given-names>A</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>2009</year><article-title>A systematic survey identifies prions and illuminates sequence features of prionogenic proteins</article-title><source>Cell</source><volume>137</volume><fpage>146</fpage><lpage>158</lpage><pub-id pub-id-type="doi">10.1016/j.cell.2009.02.044</pub-id></element-citation></ref><ref id="bib3"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Allen</surname><given-names>KD</given-names></name><name><surname>Chernova</surname><given-names>TA</given-names></name><name><surname>Tennant</surname><given-names>EP</given-names></name><name><surname>Wilkinson</surname><given-names>KD</given-names></name><name><surname>Chernoff</surname><given-names>YO</given-names></name></person-group><year>2007</year><article-title>Effects of ubiquitin system alterations on the formation and loss of a yeast prion</article-title><source>The Journal of Biological Chemistry</source><volume>282</volume><fpage>3004</fpage><lpage>3013</lpage><pub-id pub-id-type="doi">10.1074/jbc.M609597200</pub-id></element-citation></ref><ref id="bib3a"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Carroni</surname><given-names>M</given-names></name><name><surname>Kummer</surname><given-names>E</given-names></name><name><surname>Oguchi</surname><given-names>Y</given-names></name><name><surname>Wendler</surname><given-names>P</given-names></name><name><surname>Clare</surname><given-names>DK</given-names></name><name><surname>Sinning</surname><given-names>I</given-names></name><name><surname>Kopp</surname><given-names>J</given-names></name><name><surname>Mogk</surname><given-names>A</given-names></name><name><surname>Bukau</surname><given-names>B</given-names></name><name><surname>Saibil</surname><given-names>H</given-names></name></person-group><year>2014</year><article-title>Head-to-tail interactions of the coiled-coil domains regulate ClpB cooperation with Hsp70 in protein disaggregation</article-title><source>eLife</source><pub-id pub-id-type="doi">10.7554/eLife.02481</pub-id></element-citation></ref><ref id="bib4"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Caughey</surname><given-names>B</given-names></name><name><surname>Baron</surname><given-names>GS</given-names></name><name><surname>Chesebro</surname><given-names>B</given-names></name><name><surname>Jeffrey</surname><given-names>M</given-names></name></person-group><year>2009</year><article-title>Getting a grip on prions: oligomers, amyloids, and pathological membrane interactions</article-title><source>Annual Review of Biochemistry</source><volume>78</volume><fpage>177</fpage><lpage>204</lpage><pub-id pub-id-type="doi">10.1146/annurev.biochem.78.082907.145410</pub-id></element-citation></ref><ref id="bib5"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Chapman</surname><given-names>MR</given-names></name><name><surname>Robinson</surname><given-names>LS</given-names></name><name><surname>Pinkner</surname><given-names>JS</given-names></name><name><surname>Roth</surname><given-names>R</given-names></name><name><surname>Heuser</surname><given-names>J</given-names></name><name><surname>Hammar</surname><given-names>M</given-names></name><name><surname>Normark</surname><given-names>S</given-names></name><name><surname>Hultgren</surname><given-names>SJ</given-names></name></person-group><year>2002</year><article-title>Role of <italic>Escherichia coli</italic> curli operons in directing amyloid fiber formation</article-title><source>Science</source><volume>295</volume><fpage>851</fpage><lpage>855</lpage><pub-id pub-id-type="doi">10.1126/science.1067484</pub-id></element-citation></ref><ref id="bib6"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Chernoff</surname><given-names>YO</given-names></name><name><surname>Lindquist</surname><given-names>SL</given-names></name><name><surname>Ono</surname><given-names>B</given-names></name><name><surname>Inge-Vechtomov</surname><given-names>SG</given-names></name><name><surname>Liebman</surname><given-names>SW</given-names></name></person-group><year>1995</year><article-title>Role of the chaperone protein Hsp104 in propagation of the yeast prion-like factor [psi+]</article-title><source>Science</source><volume>268</volume><fpage>880</fpage><lpage>884</lpage><pub-id pub-id-type="doi">10.1126/science.7754373</pub-id></element-citation></ref><ref id="bib7"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Coustou</surname><given-names>V</given-names></name><name><surname>Deleu</surname><given-names>C</given-names></name><name><surname>Saupe</surname><given-names>S</given-names></name><name><surname>Begueret</surname><given-names>J</given-names></name></person-group><year>1997</year><article-title>The protein product of the het-s heterokaryon incompatibility gene of the fungus <italic>Podospora anserina</italic> behaves as a prion analog</article-title><source>Proceedings of the National Academy of Sciences of USA</source><volume>94</volume><fpage>9773</fpage><lpage>9778</lpage><pub-id pub-id-type="doi">10.1073/pnas.94.18.9773</pub-id></element-citation></ref><ref id="bib8"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Cox</surname><given-names>BS</given-names></name></person-group><year>1965</year><article-title>ψ, a cytoplasmic suppressor of super-suppressor in yeast</article-title><source>Heredity</source><volume>20</volume><fpage>505</fpage><lpage>521</lpage><pub-id pub-id-type="doi">10.1038/hdy.1965.65</pub-id></element-citation></ref><ref id="bib9"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Cox</surname><given-names>B</given-names></name><name><surname>Ness</surname><given-names>F</given-names></name><name><surname>Tuite</surname><given-names>M</given-names></name></person-group><year>2003</year><article-title>Analysis of the generation and segregation of propagons: entities that propagate the [PSI<sup>+</sup>] prion in yeast</article-title><source>Genetics</source><volume>165</volume><fpage>23</fpage><lpage>33</lpage></element-citation></ref><ref id="bib10"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Derkatch</surname><given-names>IL</given-names></name><name><surname>Bradley</surname><given-names>ME</given-names></name><name><surname>Hong</surname><given-names>JY</given-names></name><name><surname>Liebman</surname><given-names>SW</given-names></name></person-group><year>2001</year><article-title>Prions affect the appearance of other prions: the story of [PIN<sup>+</sup>]</article-title><source>Cell</source><volume>106</volume><fpage>171</fpage><lpage>182</lpage><pub-id pub-id-type="doi">10.1016/S0092-8674(01)00427-5</pub-id></element-citation></ref><ref id="bib11"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Derkatch</surname><given-names>IL</given-names></name><name><surname>Bradley</surname><given-names>ME</given-names></name><name><surname>Masse</surname><given-names>SV</given-names></name><name><surname>Zadorsky</surname><given-names>SP</given-names></name><name><surname>Polozkov</surname><given-names>GV</given-names></name><name><surname>Inge-Vechtomov</surname><given-names>SG</given-names></name><name><surname>Liebman</surname><given-names>SW</given-names></name></person-group><year>2000</year><article-title>Dependence and independence of [PSI<sup>+</sup>] and [PIN<sup>+</sup>]: a two-prion system in yeast?</article-title><source>The EMBO Journal</source><volume>19</volume><fpage>1942</fpage><lpage>1952</lpage><pub-id pub-id-type="doi">10.1093/emboj/19.9.1942</pub-id></element-citation></ref><ref id="bib12"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Derkatch</surname><given-names>IL</given-names></name><name><surname>Bradley</surname><given-names>ME</given-names></name><name><surname>Zhou</surname><given-names>P</given-names></name><name><surname>Chernoff</surname><given-names>YO</given-names></name><name><surname>Liebman</surname><given-names>SW</given-names></name></person-group><year>1997</year><article-title>Genetic and environmental factors affecting the <italic>de novo</italic> appearance of the [PSI<sup>+</sup>] prion in <italic>Saccharomyces cerevisiae</italic></article-title><source>Genetics</source><volume>147</volume><fpage>507</fpage><lpage>519</lpage></element-citation></ref><ref id="bib13"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>DeSantis</surname><given-names>ME</given-names></name><name><surname>Leung</surname><given-names>EH</given-names></name><name><surname>Sweeny</surname><given-names>EA</given-names></name><name><surname>Jackrel</surname><given-names>ME</given-names></name><name><surname>Cushman-Nick</surname><given-names>M</given-names></name><name><surname>Neuhaus-Follini</surname><given-names>A</given-names></name><name><surname>Vashist</surname><given-names>S</given-names></name><name><surname>Sochor</surname><given-names>MA</given-names></name><name><surname>Knight</surname><given-names>MN</given-names></name><name><surname>Shorter</surname><given-names>J</given-names></name></person-group><year>2012</year><article-title>Operational plasticity enables Hsp104 to disaggregate diverse amyloid and nonamyloid clients</article-title><source>Cell</source><volume>151</volume><fpage>778</fpage><lpage>793</lpage><pub-id pub-id-type="doi">10.1016/j.cell.2012.09.038</pub-id></element-citation></ref><ref id="bib14"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Diaz-Espinoza</surname><given-names>R</given-names></name><name><surname>Soto</surname><given-names>C</given-names></name></person-group><year>2012</year><article-title>High-resolution structure of infectious prion protein: the final frontier</article-title><source>Nature Structural & Molecular Biology</source><volume>19</volume><fpage>370</fpage><lpage>377</lpage><pub-id pub-id-type="doi">10.1038/nsmb.2266</pub-id></element-citation></ref><ref id="bib15"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>DiSalvo</surname><given-names>S</given-names></name><name><surname>Derdowski</surname><given-names>A</given-names></name><name><surname>Pezza</surname><given-names>JA</given-names></name><name><surname>Serio</surname><given-names>TR</given-names></name></person-group><year>2011</year><article-title>Dominant prion mutants induce curing through pathways that promote chaperone-mediated disaggregation</article-title><source>Nature Structural & Molecular Biology</source><volume>18</volume><fpage>486</fpage><lpage>492</lpage><pub-id pub-id-type="doi">10.1038/nsmb.2031</pub-id></element-citation></ref><ref id="bib16"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Doyle</surname><given-names>SM</given-names></name><name><surname>Wickner</surname><given-names>S</given-names></name></person-group><year>2009</year><article-title>Hsp104 and ClpB: protein disaggregating machines</article-title><source>Trends in Biochemical Sciences</source><volume>34</volume><fpage>40</fpage><lpage>48</lpage><pub-id pub-id-type="doi">10.1016/j.tibs.2008.09.010</pub-id></element-citation></ref><ref id="bib17"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Espargaró</surname><given-names>A</given-names></name><name><surname>Villar-Piqué</surname><given-names>A</given-names></name><name><surname>Sabaté</surname><given-names>R</given-names></name><name><surname>Ventura</surname><given-names>S</given-names></name></person-group><year>2012</year><article-title>Yeast prions form infectious amyloid inclusion bodies in bacteria</article-title><source>Microbial Cell Factories</source><volume>11</volume><fpage>89</fpage><pub-id pub-id-type="doi">10.1186/1475-2859-11-89</pub-id></element-citation></ref><ref id="bib18"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Espinosa Angarica</surname><given-names>V</given-names></name><name><surname>Ventura</surname><given-names>S</given-names></name><name><surname>Sancho</surname><given-names>J</given-names></name></person-group><year>2013</year><article-title>Discovering putative prion sequences in complete proteomes using probabilistic representations of Q/N-rich domains</article-title><source>BMC Genomics</source><volume>14</volume><fpage>316</fpage><pub-id pub-id-type="doi">10.1186/1471-2164-14-316</pub-id></element-citation></ref><ref id="bib19"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Fernándes-Tresguerres</surname><given-names>ME</given-names></name><name><surname>Moreno-Díaz de la Espina</surname><given-names>S</given-names></name><name><surname>Gasset-Rosa</surname><given-names>F</given-names></name><name><surname>Giraldo</surname><given-names>R</given-names></name></person-group><year>2010</year><article-title>A DNA-promoted amyloid proteinopathy in <italic>Escherichia coli</italic></article-title><source>Molecular Microbiology</source><volume>77</volume><fpage>1456</fpage><lpage>1469</lpage><pub-id pub-id-type="doi">10.1111/j.1365-2958.2010.07299.x</pub-id></element-citation></ref><ref id="bib20"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Frederick</surname><given-names>KK</given-names></name><name><surname>Debelouchina</surname><given-names>GT</given-names></name><name><surname>Kayatekin</surname><given-names>C</given-names></name><name><surname>Dorminy</surname><given-names>T</given-names></name><name><surname>Jacavone</surname><given-names>AC</given-names></name><name><surname>Griffin</surname><given-names>RG</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>2014</year><article-title>Distinct prion strains are defined by amyloid core structure and chaperone binding site dynamics</article-title><source>Chemistry & Biology</source><volume>21</volume><fpage>295</fpage><lpage>305</lpage><pub-id pub-id-type="doi">10.1016/j.chembiol.2013.12.013</pub-id></element-citation></ref><ref id="bib21"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Garrity</surname><given-names>SJ</given-names></name><name><surname>Sivanathan</surname><given-names>V</given-names></name><name><surname>Dong</surname><given-names>J</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name><name><surname>Hochschild</surname><given-names>A</given-names></name></person-group><year>2010</year><article-title>Conversion of a yeast prion protein to an infectious form in bacteria</article-title><source>Proceedings of the National Academy of Sciences of USA</source><volume>107</volume><fpage>10596</fpage><lpage>10601</lpage><pub-id pub-id-type="doi">10.1073/pnas.0913280107</pub-id></element-citation></ref><ref id="bib22"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Gasset-Rosa</surname><given-names>F</given-names></name><name><surname>Coquel</surname><given-names>AS</given-names></name><name><surname>Moreno-Del Álamo</surname><given-names>M</given-names></name><name><surname>Chen</surname><given-names>P</given-names></name><name><surname>Song</surname><given-names>X</given-names></name><name><surname>Serrano</surname><given-names>AM</given-names></name><name><surname>Fernández-Tresguerres</surname><given-names>ME</given-names></name><name><surname>Moreno-Díaz de la Espina</surname><given-names>S</given-names></name><name><surname>Lindner</surname><given-names>AB</given-names></name><name><surname>Giraldo</surname><given-names>R</given-names></name></person-group><year>2014</year><article-title>Direct assessment in bacteria of prionoid propagation and phenotype selection by Hsp70 chaperone</article-title><source>Molecular Microbiology</source><volume>91</volume><fpage>1070</fpage><lpage>1087</lpage><pub-id pub-id-type="doi">10.1111/mmi.12518</pub-id></element-citation></ref><ref id="bib23"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Goldschmidt</surname><given-names>L</given-names></name><name><surname>Teng</surname><given-names>PK</given-names></name><name><surname>Riek</surname><given-names>R</given-names></name><name><surname>Eisenberg</surname><given-names>D</given-names></name></person-group><year>2010</year><article-title>Identifying the amylome, proteins capable of forming amyloid-like fibrils</article-title><source>Proceedings of the National Academy of Sciences of USA</source><volume>107</volume><fpage>3487</fpage><lpage>3492</lpage><pub-id pub-id-type="doi">10.1073/pnas.0915166107</pub-id></element-citation></ref><ref id="bib24"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Haldimann</surname><given-names>A</given-names></name><name><surname>Wanner</surname><given-names>BL</given-names></name></person-group><year>2001</year><article-title>Conditional-replication, integration, excision, and retrieval plasmid-host systems for gene structure-function studies of bacteria</article-title><source>Journal of Bacteriology</source><volume>183</volume><fpage>6384</fpage><lpage>6393</lpage><pub-id pub-id-type="doi">10.1128/JB.183.21.6384-6393.2001</pub-id></element-citation></ref><ref id="bib26"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Higurashi</surname><given-names>T</given-names></name><name><surname>Hines</surname><given-names>JK</given-names></name><name><surname>Sahi</surname><given-names>C</given-names></name><name><surname>Aron</surname><given-names>R</given-names></name><name><surname>Craig</surname><given-names>EA</given-names></name></person-group><year>2008</year><article-title>Specificity of the J-protein Sis1 in the propagation of 3 yeast prions</article-title><source>Proceedings of the National Academy of Sciences of USA</source><volume>105</volume><fpage>16596</fpage><lpage>16601</lpage><pub-id pub-id-type="doi">10.1073/pnas.0808934105</pub-id></element-citation></ref><ref id="bib27"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Holmes</surname><given-names>DL</given-names></name><name><surname>Lancaster</surname><given-names>AK</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name><name><surname>Halfmann</surname><given-names>R</given-names></name></person-group><year>2013</year><article-title>Heritable remodeling of yeast multicellularity by an environmentally responsive prion</article-title><source>Cell</source><volume>153</volume><fpage>153</fpage><lpage>165</lpage><pub-id pub-id-type="doi">10.1016/j.cell.2013.02.026</pub-id></element-citation></ref><ref id="bib28"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>King</surname><given-names>C</given-names></name><name><surname>Diaz-Avalos</surname><given-names>R</given-names></name></person-group><year>2004</year><article-title>Protein-only transmission of three yeast prion strains</article-title><source>Nature</source><volume>428</volume><fpage>319</fpage><lpage>323</lpage><pub-id pub-id-type="doi">10.1038/nature02391</pub-id></element-citation></ref><ref id="bib29"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Kryndushkin</surname><given-names>DS</given-names></name><name><surname>Alexandrov</surname><given-names>IM</given-names></name><name><surname>Ter-Avanesyan</surname><given-names>MD</given-names></name><name><surname>Kushnirov</surname><given-names>VV</given-names></name></person-group><year>2003</year><article-title>Yeast [PSI<sup>+</sup>] prion aggregates are formed by small Sup35 polymers fragmented by Hsp104</article-title><source>The Journal of Biological Chemistry</source><volume>278</volume><fpage>49636</fpage><lpage>49643</lpage><pub-id pub-id-type="doi">10.1074/jbc.M307996200</pub-id></element-citation></ref><ref id="bib30"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Lancaster</surname><given-names>AK</given-names></name><name><surname>Bardill</surname><given-names>JP</given-names></name><name><surname>True</surname><given-names>HL</given-names></name><name><surname>Masel</surname><given-names>J</given-names></name></person-group><year>2010</year><article-title>The spontaneous appearance rate of the yeast prion [PSI+] and its implications for the evolution of the evolvability properties of the [PSI+] system</article-title><source>Genetics</source><volume>184</volume><fpage>393</fpage><lpage>400</lpage><pub-id pub-id-type="doi">10.1534/genetics.109.110213</pub-id></element-citation></ref><ref id="bib31"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Lee</surname><given-names>S</given-names></name><name><surname>Sowa</surname><given-names>ME</given-names></name><name><surname>Watanabe</surname><given-names>YH</given-names></name><name><surname>Sigler</surname><given-names>PB</given-names></name><name><surname>Chiu</surname><given-names>W</given-names></name><name><surname>Yoshida</surname><given-names>M</given-names></name><name><surname>Tsai</surname><given-names>FT</given-names></name></person-group><year>2003</year><article-title>The structure of ClpB: a molecular chaperone that rescues proteins from an aggregated state</article-title><source>Cell</source><volume>115</volume><fpage>229</fpage><lpage>240</lpage><pub-id pub-id-type="doi">10.1016/S0092-8674(03)00807-9</pub-id></element-citation></ref><ref id="bib32"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Li</surname><given-names>L</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>2000</year><article-title>Creating a protein-based element of inheritance</article-title><source>Science</source><volume>287</volume><fpage>661</fpage><lpage>676</lpage><pub-id pub-id-type="doi">10.1126/science.287.5453.661</pub-id></element-citation></ref><ref id="bib33"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Liebman</surname><given-names>SW</given-names></name><name><surname>Chernoff</surname><given-names>YO</given-names></name></person-group><year>2012</year><article-title>Prions in yeast</article-title><source>Genetics</source><volume>191</volume><fpage>1041</fpage><lpage>1072</lpage><pub-id pub-id-type="doi">10.1534/genetics.111.137760</pub-id></element-citation></ref><ref id="bib34"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Liu</surname><given-names>JJ</given-names></name><name><surname>Sondheimer</surname><given-names>N</given-names></name><name><surname>Lindquist</surname><given-names>SL</given-names></name></person-group><year>2002</year><article-title>Changes in the middle region of Sup35 profoundly alter the nature of epigenetic inheritance for the yeast prion [PSI<sup>+</sup>]</article-title><source>Proceedings of the National Academy of Sciences of USA</source><volume>99</volume><fpage>16446</fpage><lpage>16453</lpage><pub-id pub-id-type="doi">10.1073/pnas.252652099</pub-id></element-citation></ref><ref id="bib35"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Lutz</surname><given-names>R</given-names></name><name><surname>Bujard</surname><given-names>H</given-names></name></person-group><year>1997</year><article-title>Independent and tight regulation of transcriptional units in <italic>Escherichia coli</italic> via the LacR/O, the TetR/O and AraC/I1-I2 regulatory elements</article-title><source>Nucleic Acids Research</source><volume>25</volume><fpage>1203</fpage><lpage>1210</lpage><pub-id pub-id-type="doi">10.1093/nar/25.6.1203</pub-id></element-citation></ref><ref id="bib36"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Maddelein</surname><given-names>ML</given-names></name><name><surname>Reis</surname><given-names>SD</given-names></name><name><surname>Duvezin-Caubet</surname><given-names>S</given-names></name><name><surname>Coulary-Salin</surname><given-names>B</given-names></name><name><surname>Saupe</surname><given-names>SJ</given-names></name></person-group><year>2002</year><article-title>Amyloid aggregates of the HET-s prion protein are infectious</article-title><source>Proceedings of the National Academy of Sciences of USA</source><volume>99</volume><fpage>7402</fpage><lpage>7407</lpage><pub-id pub-id-type="doi">10.1073/pnas.072199199</pub-id></element-citation></ref><ref id="bib37"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Mogk</surname><given-names>A</given-names></name><name><surname>Schlieker</surname><given-names>C</given-names></name><name><surname>Strub</surname><given-names>C</given-names></name><name><surname>Rist</surname><given-names>W</given-names></name><name><surname>Weibezahn</surname><given-names>J</given-names></name><name><surname>Bukau</surname><given-names>B</given-names></name></person-group><year>2003</year><article-title>Roles of individual domains and conserved motifs of the AAA+ chaperone ClpB in oligomerization, ATP hydrolysis, and chaperone activity</article-title><source>The Journal of Biological Chemistry</source><volume>278</volume><fpage>17615</fpage><lpage>17624</lpage><pub-id pub-id-type="doi">10.1074/jbc.M209686200</pub-id></element-citation></ref><ref id="bib38"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Ness</surname><given-names>F</given-names></name><name><surname>Ferreira</surname><given-names>P</given-names></name><name><surname>Cox</surname><given-names>BS</given-names></name><name><surname>Tuite</surname><given-names>MF</given-names></name></person-group><year>2002</year><article-title>Guanidine hydrochloride inhibits the generation of prion “seeds” but not prion protein aggregation in yeast</article-title><source>Molecular and Cellular Biology</source><volume>22</volume><fpage>5593</fpage><lpage>5605</lpage><pub-id pub-id-type="doi">10.1128/MCB.22.15.5593-5605.2002</pub-id></element-citation></ref><ref id="bib39"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Newby</surname><given-names>GA</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>2013</year><article-title>Blessings in disguise: biological benefits of prion-like mechanisms</article-title><source>Trends in Cell Biology</source><volume>23</volume><fpage>251</fpage><lpage>259</lpage><pub-id pub-id-type="doi">10.1016/j.tcb.2013.01.007</pub-id></element-citation></ref><ref id="bib40"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Oguchi</surname><given-names>Y</given-names></name><name><surname>Kummer</surname><given-names>E</given-names></name><name><surname>Seyffer</surname><given-names>F</given-names></name><name><surname>Berynskyy</surname><given-names>M</given-names></name><name><surname>Anstett</surname><given-names>B</given-names></name><name><surname>Zahn</surname><given-names>R</given-names></name><name><surname>Wade</surname><given-names>RC</given-names></name><name><surname>Mogk</surname><given-names>A</given-names></name><name><surname>Bukau</surname><given-names>B</given-names></name></person-group><year>2012</year><article-title>A tightly regulated molecular toggle controls AAA+ disaggregase</article-title><source>Nature Structural & Molecular Biology</source><volume>19</volume><fpage>1338</fpage><lpage>1346</lpage><pub-id pub-id-type="doi">10.1038/nsmb.2441</pub-id></element-citation></ref><ref id="bib41"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Osherovich</surname><given-names>LZ</given-names></name><name><surname>Weissman</surname><given-names>JS</given-names></name></person-group><year>2001</year><article-title>Multiple Gln/Asn-rich prion domains confer susceptibility to induction of the yeast [PSI(+)] prion</article-title><source>Cell</source><volume>106</volume><fpage>183</fpage><lpage>194</lpage><pub-id pub-id-type="doi">10.1016/S0092-8674(01)00440-8</pub-id></element-citation></ref><ref id="bib42"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Patino</surname><given-names>MM</given-names></name><name><surname>Liu</surname><given-names>JJ</given-names></name><name><surname>Glover</surname><given-names>JR</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>1996</year><article-title>Support for the prion hypothesis for inheritance of a phenotypic trait in yeast</article-title><source>Science</source><volume>273</volume><fpage>622</fpage><lpage>626</lpage><pub-id pub-id-type="doi">10.1126/science.273.5275.622</pub-id></element-citation></ref><ref id="bib43"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Paushkin</surname><given-names>SV</given-names></name><name><surname>Kushnirov</surname><given-names>VV</given-names></name><name><surname>Smirnov</surname><given-names>VN</given-names></name><name><surname>Ter-Avanesyan</surname><given-names>MD</given-names></name></person-group><year>1996</year><article-title>Propagation of the yeast prion-like [<italic>psi</italic>+] determinant is mediated by oligomerization of the SUP35-encoded polypeptide chain release factor</article-title><source>The EMBO Journal</source><volume>15</volume><fpage>3127</fpage><lpage>3134</lpage></element-citation></ref><ref id="bib44"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Prusiner</surname><given-names>SB</given-names></name></person-group><year>1982</year><article-title>Novel proteinaceous infectious particles cause scrapie</article-title><source>Science</source><volume>216</volume><fpage>136</fpage><lpage>144</lpage><pub-id pub-id-type="doi">10.1126/science.6801762</pub-id></element-citation></ref><ref id="bib45"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Reidy</surname><given-names>M</given-names></name><name><surname>Miot</surname><given-names>M</given-names></name><name><surname>Masison</surname><given-names>DC</given-names></name></person-group><year>2012</year><article-title>Prokaryotic chaperones support yeast prions and thermotolerance and define disaggregation machinery interactions</article-title><source>Genetics</source><volume>192</volume><fpage>185</fpage><lpage>193</lpage><pub-id pub-id-type="doi">10.1534/genetics.112.142307</pub-id></element-citation></ref><ref id="bib46"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Romero</surname><given-names>D</given-names></name><name><surname>Aguilar</surname><given-names>C</given-names></name><name><surname>Losick</surname><given-names>R</given-names></name><name><surname>Kolter</surname><given-names>R</given-names></name></person-group><year>2010</year><article-title>Amyloid fibers provide structural integrity to <italic>Bacillus subtilis</italic> biofilms</article-title><source>Proceedings of the National Academy of Sciences of USA</source><volume>107</volume><fpage>2230</fpage><lpage>2234</lpage><pub-id pub-id-type="doi">10.1073/pnas.0910560107</pub-id></element-citation></ref><ref id="bib47"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Sabaté</surname><given-names>R</given-names></name><name><surname>Espargaró</surname><given-names>A</given-names></name><name><surname>Saupe</surname><given-names>SJ</given-names></name><name><surname>Ventura</surname><given-names>S</given-names></name></person-group><year>2009</year><article-title>Characterization of the amyloid bacterial inclusion bodies of the HET-s fungal prion</article-title><source>Microbial Cell Factories</source><volume>8</volume><fpage>56</fpage><pub-id pub-id-type="doi">10.1186/1475-2859-8-56</pub-id></element-citation></ref><ref id="bib48"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Satpute-Krishnan</surname><given-names>P</given-names></name><name><surname>Langseth</surname><given-names>SX</given-names></name><name><surname>Serio</surname><given-names>TR</given-names></name></person-group><year>2007</year><article-title>Hsp104-dependent remodeling of prion complexes mediates protein-only inheritance</article-title><source>PLOS Biology</source><volume>5</volume><fpage>e24</fpage><pub-id pub-id-type="doi">10.1371/journal.pbio.0050024</pub-id></element-citation></ref><ref id="bib49"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Seyffer</surname><given-names>F</given-names></name><name><surname>Kummer</surname><given-names>E</given-names></name><name><surname>Oguchi</surname><given-names>Y</given-names></name><name><surname>Winkler</surname><given-names>J</given-names></name><name><surname>Kumar</surname><given-names>M</given-names></name><name><surname>Zahn</surname><given-names>R</given-names></name><name><surname>Sourjik</surname><given-names>V</given-names></name><name><surname>Bukau</surname><given-names>B</given-names></name><name><surname>Mogk</surname><given-names>A</given-names></name></person-group><year>2012</year><article-title>Hsp70 proteins bind Hsp100 regulatory M domains to activate AAA+ disaggregase at aggregate surfaces</article-title><source>Nature Structural & Molecular Biology</source><volume>19</volume><fpage>1347</fpage><lpage>1355</lpage><pub-id pub-id-type="doi">10.1038/nsmb.2442</pub-id></element-citation></ref><ref id="bib50"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Shorter</surname><given-names>J</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>2004</year><article-title>Hsp104 catalyzes formation and elimination of self-replicating Sup35 prion conformers</article-title><source>Science</source><volume>304</volume><fpage>1793</fpage><lpage>1797</lpage><pub-id pub-id-type="doi">10.1126/science.1098007</pub-id></element-citation></ref><ref id="bib51"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Shorter</surname><given-names>J</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>2006</year><article-title>Destruction or potentiation of different prions catalyzed by similar Hsp104 remodeling activities</article-title><source>Molecular Cell</source><volume>23</volume><fpage>425</fpage><lpage>438</lpage><pub-id pub-id-type="doi">10.1016/j.molcel.2006.05.042</pub-id></element-citation></ref><ref id="bib52"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Shorter</surname><given-names>J</given-names></name><name><surname>Lindquist</surname><given-names>S</given-names></name></person-group><year>2008</year><article-title>Hsp104, Hsp70 and Hsp40 interplay regulates formation, growth and elimination of Sup35 prions</article-title><source>The EMBO Journal</source><volume>27</volume><fpage>2712</fpage><lpage>2724</lpage><pub-id pub-id-type="doi">10.1038/emboj.2008.194</pub-id></element-citation></ref><ref id="bib54"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Suzuki</surname><given-names>G</given-names></name><name><surname>Shimazu</surname><given-names>N</given-names></name><name><surname>Tanaka</surname><given-names>M</given-names></name></person-group><year>2012</year><article-title>A yeast prion, Mod5, promotes acquired drug resistance and cell survival under environmental stress</article-title><source>Science</source><volume>336</volume><fpage>355</fpage><lpage>359</lpage><pub-id pub-id-type="doi">10.1126/science.1219491</pub-id></element-citation></ref><ref id="bib55"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Tanaka</surname><given-names>M</given-names></name><name><surname>Chien</surname><given-names>P</given-names></name><name><surname>Naber</surname><given-names>N</given-names></name><name><surname>Cooke</surname><given-names>R</given-names></name><name><surname>Weissman</surname><given-names>JS</given-names></name></person-group><year>2004</year><article-title>Conformational variations in an infectious protein determine prion strain differences</article-title><source>Nature</source><volume>428</volume><fpage>323</fpage><lpage>328</lpage><pub-id pub-id-type="doi">10.1038/nature02392</pub-id></element-citation></ref><ref id="bib56"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Tanaka</surname><given-names>M</given-names></name><name><surname>Weissman</surname><given-names>JS</given-names></name></person-group><year>2006</year><article-title>An efficient protein transformation protocol for introducing prions into yeast</article-title><source>Methods in Enzymology</source><volume>412</volume><fpage>185</fpage><lpage>200</lpage><pub-id pub-id-type="doi">10.1016/S0076-6879(06)12012-1</pub-id></element-citation></ref><ref id="bib57"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Taneja</surname><given-names>V</given-names></name><name><surname>Maddelein</surname><given-names>ML</given-names></name><name><surname>Talarek</surname><given-names>N</given-names></name><name><surname>Saupe</surname><given-names>SJ</given-names></name><name><surname>Liebman</surname><given-names>SW</given-names></name></person-group><year>2007</year><article-title>A non-Q/N-rich prion domain of a foreign prion, [Het-s], can propagate as a prion in yeast</article-title><source>Molecular Cell</source><volume>27</volume><fpage>67</fpage><lpage>77</lpage><pub-id pub-id-type="doi">10.1016/j.molcel.2007.05.027</pub-id></element-citation></ref><ref id="bib58"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Ter-Avanesyan</surname><given-names>MD</given-names></name><name><surname>Dagkesamanskaya</surname><given-names>AR</given-names></name><name><surname>Kushnirov</surname><given-names>VV</given-names></name><name><surname>Smirnov</surname><given-names>VN</given-names></name></person-group><year>1994</year><article-title>The <italic>SUP35</italic> omnipotent suppressor gene is involved in the maintenance of the non-Mendelian determinant [<italic>psi</italic><sup>+</sup>] in the yeast <italic>Saccharomyces cerevisiae</italic></article-title><source>Genetics</source><volume>137</volume><fpage>671</fpage><lpage>676</lpage></element-citation></ref><ref id="bib59"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Ter-Avanesyan</surname><given-names>MD</given-names></name><name><surname>Kushnirov</surname><given-names>VV</given-names></name><name><surname>Dagkesamanskaya</surname><given-names>AR</given-names></name><name><surname>Didichenko</surname><given-names>SA</given-names></name><name><surname>Chernoff</surname><given-names>YO</given-names></name><name><surname>Inge-Vechtomov</surname><given-names>SG</given-names></name><name><surname>Smirnov</surname><given-names>VN</given-names></name></person-group><year>1993</year><article-title>Deletion analysis of the SUP35 gene of the yeast <italic>Saccharomyces cerevisiae</italic> reveals two non-overlapping functional regions in the encoded protein</article-title><source>Molecular Microbiology</source><volume>7</volume><fpage>683</fpage><lpage>692</lpage><pub-id pub-id-type="doi">10.1111/j.1365-2958.1993.tb01159.x</pub-id></element-citation></ref><ref id="bib60"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Tipton</surname><given-names>KA</given-names></name><name><surname>Verges</surname><given-names>KJ</given-names></name><name><surname>Weissman</surname><given-names>JS</given-names></name></person-group><year>2008</year><article-title>In vivo monitoring of the prion replication cycle reveals a critical role for Sis1 in delivering substrates to Hsp104</article-title><source>Molecular Cell</source><volume>32</volume><fpage>584</fpage><lpage>591</lpage><pub-id pub-id-type="doi">10.1016/j.molcel.2008.11.003</pub-id></element-citation></ref><ref id="bib61"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>True</surname><given-names>HL</given-names></name><name><surname>Berlin</surname><given-names>I</given-names></name><name><surname>Lindquist</surname><given-names>SL</given-names></name></person-group><year>2004</year><article-title>Epigenetic regulation of translation reveals hidden genetic variation to produce complex traits</article-title><source>Nature</source><volume>431</volume><fpage>184</fpage><lpage>187</lpage><pub-id pub-id-type="doi">10.1038/nature02885</pub-id></element-citation></ref><ref id="bib62"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>True</surname><given-names>HL</given-names></name><name><surname>Lindquist</surname><given-names>SL</given-names></name></person-group><year>2000</year><article-title>A yeast prion provides a mechanism for genetic variation and phenotypic diversity</article-title><source>Nature</source><volume>407</volume><fpage>477</fpage><lpage>483</lpage><pub-id pub-id-type="doi">10.1038/35035005</pub-id></element-citation></ref><ref id="bib63"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Tuite</surname><given-names>MF</given-names></name><name><surname>Serio</surname><given-names>TR</given-names></name></person-group><year>2010</year><article-title>The prion hypothesis: from biological anomaly to basic regulatory mechanism</article-title><source>Nature Reviews Molecular Cell Biology</source><volume>11</volume><fpage>823</fpage><lpage>833</lpage><pub-id pub-id-type="doi">10.1038/nrm3007</pub-id></element-citation></ref><ref id="bib64"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Weibezahn</surname><given-names>J</given-names></name><name><surname>Schlieker</surname><given-names>C</given-names></name><name><surname>Bukau</surname><given-names>B</given-names></name><name><surname>Mogk</surname><given-names>A</given-names></name></person-group><year>2003</year><article-title>Characterization of a trap mutant of the AAA+ chaperone ClpB</article-title><source>The Journal of Biological Chemistry</source><volume>278</volume><fpage>32608</fpage><lpage>32617</lpage><pub-id pub-id-type="doi">10.1074/jbc.M303653200</pub-id></element-citation></ref><ref id="bib65"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Weibezahn</surname><given-names>J</given-names></name><name><surname>Tessarz</surname><given-names>P</given-names></name><name><surname>Schlieker</surname><given-names>C</given-names></name><name><surname>Zahn</surname><given-names>R</given-names></name><name><surname>Maglica</surname><given-names>Z</given-names></name><name><surname>Lee</surname><given-names>S</given-names></name><name><surname>Zentgraf</surname><given-names>H</given-names></name><name><surname>Weber-Ban</surname><given-names>EU</given-names></name><name><surname>Dougan</surname><given-names>DA</given-names></name><name><surname>Tsai</surname><given-names>FT</given-names></name><name><surname>Mogk</surname><given-names>A</given-names></name><name><surname>Bukau</surname><given-names>B</given-names></name></person-group><year>2004</year><article-title>Thermotolerance requires refolding of aggregated proteins by substrate translocation through the central pore of ClpB</article-title><source>Cell</source><volume>119</volume><fpage>653</fpage><lpage>655</lpage><pub-id pub-id-type="doi">10.1016/j.cell.2004.11.027</pub-id></element-citation></ref><ref id="bib66"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Wickner</surname><given-names>RB</given-names></name></person-group><year>1994</year><article-title>[URE3] as an altered URE2 protein: evidence for a prion analog in <italic>Saccharomyces cerevisiae</italic></article-title><source>Science</source><volume>264</volume><fpage>566</fpage><lpage>569</lpage><pub-id pub-id-type="doi">10.1126/science.7909170</pub-id></element-citation></ref><ref id="bib67"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Winkler</surname><given-names>J</given-names></name><name><surname>Tyedmers</surname><given-names>J</given-names></name><name><surname>Bukau</surname><given-names>B</given-names></name><name><surname>Mogk</surname><given-names>A</given-names></name></person-group><year>2012</year><article-title>Chaperone networks in protein disaggregation and prion propagation</article-title><source>Journal of Structural Biology</source><volume>179</volume><fpage>152</fpage><lpage>160</lpage><pub-id pub-id-type="doi">10.1016/j.jsb.2012.05.002</pub-id></element-citation></ref><ref id="bib68"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Zhou</surname><given-names>P</given-names></name><name><surname>Derkatch</surname><given-names>IL</given-names></name><name><surname>Liebman</surname><given-names>SW</given-names></name></person-group><year>2001</year><article-title>The relationship between visible intracellular aggregates that appear after overexpression of Sup35 and the yeast prion-like elements [PSI<sup>+</sup>] and [PIN<sup>+</sup>]</article-title><source>Molecular Microbiology</source><volume>39</volume><fpage>37</fpage><lpage>46</lpage><pub-id pub-id-type="doi">10.1046/j.1365-2958.2001.02224.x</pub-id></element-citation></ref></ref-list></back><sub-article article-type="article-commentary" id="SA1"><front-stub><article-id pub-id-type="doi">10.7554/eLife.02949.018</article-id><title-group><article-title>Decision letter</article-title></title-group><contrib-group content-type="section"><contrib contrib-type="editor"><name><surname>Greenberg</surname><given-names>Peter</given-names></name><role>Reviewing editor</role><aff><institution>University of Washington</institution>, <country>United States</country></aff></contrib></contrib-group></front-stub><body><boxed-text><p>eLife posts the editorial decision letter and author response on a selection of the published articles (subject to the approval of the authors). An edited version of the letter sent to the authors after peer review is shown, indicating the substantive concerns or comments; minor concerns are not usually shown. Reviewers have the opportunity to discuss the decision before the letter is sent (see <ext-link ext-link-type="uri" xlink:href="http://elifesciences.org/review-process">review process</ext-link>). Similarly, the author response typically shows only responses to the major concerns raised by the reviewers.</p></boxed-text><p>[Editors’ note: this article was originally rejected after discussions between the reviewers, but the authors were invited to resubmit after an appeal against the decision.]</p><p>Thank you for choosing to send your work entitled “Prion propagation can occur in a prokaryote and requires the ClpB chaperone” for consideration at <italic>eLife</italic>. Your full submission has been evaluated by K (Vijay) VijayRaghavan (Senior editor) and 3 peer reviewers, one of whom, Peter Greenberg, is a member of our Board of Reviewing Editors, and the decision was reached after discussions between the reviewers.</p><p>The reviewers all thought this was an elegantly executed study but in the end that it did not constitute enough of an advance to merit publication in <italic>eLife</italic>. The specific reviews are self-explanatory. We are sorry we do not have better news at this time.</p><p><italic>Reviewer #1:</italic></p><p>The authors build on a previous study they published in which they showed that the yeast prion domain (Sup35NM) can take up an infectious prion form in a bacterial (<italic>E. coli</italic>) cell. In this important new paper they now go on to show that this prion form can be propagated over a large number of cell divisions in <italic>E. coli</italic> and that this propagation requires the Hsp104 bacterial ortholog of Hsp104, i.e. ClpB, to do so. They provide a very detailed description of their experimental strategy and, although the ability of <italic>E. coli</italic> to propagate the prion form of Sup35NM is certainly less efficient than one sees in yeast, nevertheless their data are convincing that propagation does indeed require ClpB. What they do not formally demonstrate is that it is the chaperone activity of ClpB that is important and this could be easily addressed by repeating their experiments with an appropriate ClpB mutant.</p><p>The chaperone activity of ClpB depends on its oligomerisation and its ATPase activity and numerous chaperone-defective mutants have been described. Such an experiment should be straightforward and well within the grasps of the authors. Given the important implications of their findings, i.e. that <italic>E. coli</italic> has the chaperone machinery to propagate a (heterologous) prion; I think it necessary that they demonstrate that it is indeed the chaperone activity that is essential. Of course it remains to be established if <italic>E. coli</italic> (or any other bacterial spp) has endogenous prion-forming proteins but the findings reported here give one confidence that they are there, we just have to find a way of detecting them. By showing the dependency on ClpB, the authors open up one strategy to do so.</p><p><italic>Reviewer #2:</italic></p><p>The manuscript submitted by Hochschild and colleagues addresses the ability of <italic>E. coli</italic> to support propagation of the [PSI+] prion of yeast through the self-assembly and inheritance of aggregates of the prion-determining domain (NM) of the Sup35 protein. The significance of this work to the field and its ability to advance the current state of knowledge are somewhat limited:</p><p>1) Previous work from Hochschild and colleagues (Garrity et al. PNAS 2010) demonstrated that NM can form SDS-resistant aggregates that, when introduced into yeast cytosol, induce the appearance of [PSI+]. In the current work, the authors reveal that this state is maintained in <italic>E. coli</italic> through multiple generations and that its propagation, unlike its initiation, is independent of another yeast prion protein New1. These principles have been previously established in yeast, and it’s unclear how their extension into <italic>E. coli</italic> advances our understanding of the process or its evolutionary conservation.</p><p>2) The authors demonstrate that ClpB, the bacterial homologue of Hsp104, is required for propagation of NM aggregates in <italic>E. coli</italic>. Previous work from the Masison lab has demonstrated that, when expressed in yeast, ClpB and its Hsp70 co-chaperone DnaK are sufficient to support [PSI+], so the fact that ClpB can do so within its native environment is not surprising. Moreover, this result simply reports a genetic interaction without mechanistic insight. Is ClpB performing the same function in <italic>E. coli</italic> as Hsp104 does in yeast?</p><p>Together, these studies only represent an incremental advance over previous work in the field.</p><p><italic>Reviewer #3:</italic></p><p>Yuan et al present evidence for the establishment of yeast prion propagation in the prokaryote <italic>E. coli</italic>. This is dependent on the presence of both the yeast PIN factor New1 and the bacterial Hsp104 homologue ClpB. A PIN factor is required for conversion of Sup35 from psi- to PSI+ (the prion form) and Hsp104 has long been known to be required for the propagation of nearly all yeast prions known. Thus the key finding of this carefully done paper is that ClpB the E coli homologue of yeast Hsp104 is also analogous (having the same function). Since most homologues are analogues and many yeast proteins can function in <italic>E. coli</italic>, at one level this result is not too surprising. It does however suggest that fundamentally there are no huge differences between the cytosol of yeast and <italic>E. coli</italic> in regards to prion propagation apart from the presumable absence of PIN factors in <italic>E. coli</italic>. This work sets the stage for further genetic analysis of yeast prion propagation in <italic>E. coli</italic>.</p><p>Since both of these systems are genetically well characterized some overall conclusions about the fundamentals of in vivo prion propagation may well be able to be reached in future work, though such work is prone to false negative results as there can be many trivial reasons for lack of functional complementation when working in such evolutionarily distant systems. The authors make a distinction between prion establishment and prion propagation, but these are really more tightly linked as one cannot establish a prion without propagating it. They do come out on the side of ClpB and New1 both being required for prion propagation but indeed since both were simultaneously depleted in the experiments shown in <xref ref-type="fig" rid="fig6">Figure 6</xref>, it seems more likely that they are both required for both the establishment and propagation phases. Even given the fuzziness of the distinction is not clear if ClpB is required for the propagation alone or if it is just required for prion establishment. Does expression of NM make <italic>E. coli</italic> sick? If it does then that raises the possibility that strains that propagate prions are able to sequester it as a less toxic form. This in combination with the observation that the vast majority of ClpB+ colonies fail to propagate NM raises the possibility that <italic>E. coli</italic> host mutations are also necessary for prion propagation and that <italic>E. coli</italic> is coming up with various other ways to get around this sickness. The various forms of aggregates observed raises the issue of which are prion-like and which are non-propagating. The real definition of prion I guess is ability to propagate, more than its SDS insolubility. This distinction should be made clearer throughout the manuscript.</p></body></sub-article><sub-article article-type="reply" id="SA2"><front-stub><article-id pub-id-type="doi">10.7554/eLife.02949.019</article-id><title-group><article-title>Author response</article-title></title-group></front-stub><body><p>Reviewer #1:</p><p><italic>[…] They provide a very detailed description of their experimental strategy and, although the ability of E. coli to propagate the prion form of Sup35NM is certainly less efficient than one sees in yeast, nevertheless their data are convincing that propagation does indeed require ClpB. What they do not formally demonstrate is that it is the chaperone activity of ClpB that is important and this could be easily addressed by repeating their experiments with an appropriate ClpB mutant</italic>.</p><p><italic>The chaperone activity of ClpB depends on its oligomerisation and its ATPase activity and numerous chaperone-defective mutants have been described. Such an experiment should be straightforward and well within the grasps of the authors. Given the important implications of their findings, i.e. that E. coli has the chaperone machinery to propagate a (heterologous) prion; I think it necessary that they demonstrate that it is indeed the chaperone activity that is essential. Of course it remains to be established if E. coli (or any other bacterial spp) has endogenous prion-forming proteins but the findings reported here give one confidence that they are there, we just have to find a way of detecting them. By showing the dependency on ClpB, the authors open up one strategy to do so</italic>.</p><p>We fully agree with the reviewer that our study would be enhanced by demonstrating that it is in fact the disaggregase activity of ClpB that is required for the propagation of the Sup35-NM prion in <italic>E. coli</italic>. The reviewer suggests that it would be relatively straightforward to address this point by using appropriate ClpB mutants. Indeed, we have already initiated such experiments and aim to test two well characterized ClpB mutants that are (i) specifically deficient in ATPase activity and (ii) specifically defective in substrate translocation through the ClpB pore. We hypothesize that neither of these mutants will support propagation of the Sup35-NM prion.</p><p>Reviewer #2:</p><p><italic>The manuscript submitted by Hochschild and colleagues addresses the ability of E. coli to support propagation of the [PSI+] prion of yeast through the self-assembly and inheritance of aggregates of the prion-determining domain (NM) of the Sup35 protein. The significance of this work to the field and its ability to advance the current state of knowledge are somewhat limited. […] Together, these studies only represent an incremental advance over previous work in the field</italic>.</p><p>In response to reviewer #2, we wish to clarify why we believe our findings are broadly significant. Specifically, our findings establish that prion biology can operate in the bacterial domain of life and thus they provide the first demonstration of protein-based inheritance in a non-eukaryote. Additionally, as pointed out by reviewer #1, our study lays the foundation for a search for endogenous prion-like mechanisms in bacteria (reviewer #1 says, “the findings reported here give one confidence that they [endogenous bacterial prion proteins] are there, we just have to find a way of detecting them. By showing the dependency on ClpB, the authors open up one strategy to do so”). The second reviewer’s assessment that our study represents only “an incremental advance of previous work in the field” appears to be in reference to the field of fungal prion biology. We agree with the reviewer that our findings do not significantly deepen the mechanistic understanding of prion propagation in the endogenous fungal system. Rather we believe that the significance of our work is that we have uncovered a foundation for prion biology in another domain of life.</p><p>The reviewer also suggests that our findings with regard to ClpB are “not surprising”. However, given a prominently published study from the Shorter lab, which concludes, based on experiments performed <italic>in vitro</italic>, that ClpB is incapable of remodeling prion-like amyloid aggregates, we believe our findings will be surprising to at least some investigators in the field. (In demonstrating that ClpB is capable of remodeling prion-like aggregates, our findings complement those from the Masison lab, which we discuss; we note, however, that Masison and colleagues found that the ability of ClpB to support [PSI+] in yeast was dependent on the fungal Hsp40-family Sis1 protein, whereas our work shows that no fungal accessory factors are required in the endogenous bacterial setting.) Specifically, our results and those of the Masison lab challenge a prevalent view in the yeast prion field – namely that the ability to remodel prion-like aggregates is an Hsp104 innovation specific to fungal systems. Instead, our results raise the possibility that this ability predates the split between bacteria and yeast and has been conserved in their respective chaperone systems.</p><p>Finally, the reviewer asks if ClpB is performing the same function in <italic>E. coli</italic> as Hsp104 does in yeast. As discussed above (response to reviewer #1), we agree that this is an important question and are currently performing experiments to address this point.</p><p>Reviewer #3:</p><p><italic>Yuan et al present evidence for the establishment of yeast prion propagation in the prokaryote E. coli. This is dependent on the presence of both the yeast PIN factor New1 and the bacterial Hsp104 homologue ClpB. A PIN factor is required for conversion of Sup35 from psi- to PSI+ (the prion form) and Hsp104 has long been known to be required for the propagation of nearly all yeast prions known. Thus the key finding of this carefully done paper is that ClpB the E coli homologue of yeast Hsp104 is also analogous (having the same function). Since most homologues are analogues and many yeast proteins can function in E. coli, at one level this result is not too surprising. It does however suggest that fundamentally there are no huge differences between the cytosol of yeast and E. coli in regards to prion propagation apart from the presumable absence of PIN factors in E. coli. This work sets the stage for further genetic analysis of yeast prion propagation in E. coli</italic>.</p><p><italic>Since both of these systems are genetically well characterized some overall conclusions about the fundamentals of in vivo prion propagation may well be able to be reached in future work, though such work is prone to false negative results as there can be many trivial reasons for lack of functional complementation when working in such evolutionarily distant systems. The authors make a distinction between prion establishment and prion propagation, but these are really more tightly linked as one cannot establish a prion without propagating it. They do come out on the side of ClpB and New1 both being required for prion propagation but indeed since both were simultaneously depleted in the experiments shown in</italic> <xref ref-type="fig" rid="fig6"><italic>Figure 6</italic></xref><italic>, it seems more likely that they are both required for both the establishment and propagation phases. Even given the fuzziness of the distinction is not clear if ClpB is required for the propagation alone or if it is just required for prion establishment. Does expression of NM make E. coli sick? If it does then that raises the possibility that strains that propagate prions are able to sequester it as a less toxic form. This in combination with the observation that the vast majority of ClpB+ colonies fail to propagate NM raises the possibility that E. coli host mutations are also necessary for prion propagation and that E. coli is coming up with various other ways to get around this sickness. The various forms of aggregates observed raises the issue of which are prion-like and which are non-propagating. The real definition of prion I guess is ability to propagate, more than its SDS insolubility. This distinction should be made clearer throughout the manuscript</italic>.</p><p>The reviewer suggests that the distinction between prion establishment and prion propagation is a fuzzy one. We suspect that we did not make the distinction clear enough in our manuscript. We believe (i) that there is a clear conceptual distinction between the <italic>de novo</italic> formation phase and the propagation phase and (ii) that our <italic>E. coli</italic>-based system provides us with a rigorous experimental strategy to distinguish between these two phases. Conceptually, the <italic>de novo</italic> formation of prion-like aggregates from soluble protein within a given cell (which can be facilitated by protein overproduction) represents “establishment”, whereas the maintenance of these aggregates in progeny cells under conditions that do not permit <italic>de novo</italic> formation represents “propagation”. Accordingly, the strict [PIN+] dependence of Sup35-NM aggregate formation in our bacterial system allows for a clean separation between a <italic>de novo</italic> formation phase (which occurs in our “starter” cultures) and a propagation phase (which occurs after plating). Specifically, the detection of prion-like aggregates in cells that have arisen multiple generations after the loss of the vector encoding New1 (the source of [PIN+] in our system) is evidence for propagation (i.e. protein-based inheritance).</p><p>Based on these considerations (which we believe we can articulate more clearly in a revised text), we disagree with the reviewer’s comment that it is “not clear if ClpB is required for propagation alone or if it is just required for prion establishment”. If ClpB were required just for prion establishment, then depleting the cells of ClpB <italic>after</italic> the establishment phase would not have resulted in Round-1 progeny clones that uniformly lack prion-like aggregates (see <xref ref-type="fig" rid="fig6">Figure 6</xref>).</p><p>We agree with the reviewer’s last substantive point: “The real definition of prion I guess is ability to propagate, more than its SDS insolubility. This distinction should be made clearer throughout the manuscript”. We will carefully revise the text to avoid confusion on this critical point.</p></body></sub-article></article> |