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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="article-commentary" 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">02904</article-id><article-id pub-id-type="doi">10.7554/eLife.02904</article-id><article-categories><subj-group subj-group-type="display-channel"><subject>Insight</subject></subj-group><subj-group subj-group-type="heading"><subject>Genes and chromosomes</subject></subj-group><subj-group subj-group-type="sub-display-channel"><subject>Gene Therapy</subject></subj-group></article-categories><title-group><article-title>Delivering the second revolution in site-specific nucleases</article-title></title-group><contrib-group><contrib contrib-type="author" corresp="yes" id="author-9822"><name><surname>Hackett</surname><given-names>Perry B</given-names></name><xref ref-type="aff" rid="aff1"/><xref ref-type="fn" rid="conf1"/><x> is in the </x></contrib><contrib contrib-type="author" id="author-13565"><name><surname>Somia</surname><given-names>Nikunj V</given-names></name><xref ref-type="aff" rid="aff2"/><xref ref-type="fn" rid="conf1"/><x> is in the </x></contrib><aff id="aff1"><institution content-type="dept">Department of Genetics, Cell Biology and Development</institution>, <institution>University of Minnesota</institution>, <addr-line><named-content content-type="city">Minneapolis</named-content></addr-line>, <country>United States</country> <email>hacke004@umn.edu</email></aff><aff id="aff2"><institution content-type="dept">Department of Genetics, Cell Biology and Development</institution>, <institution>University of Minnesota</institution>, <addr-line><named-content content-type="city">Minneapolis</named-content></addr-line>, <country>United States</country></aff></contrib-group><pub-date date-type="pub" publication-format="electronic"><day>08</day><month>05</month><year>2014</year></pub-date><pub-date pub-type="collection"><year>2014</year></pub-date><volume>3</volume><elocation-id>e02904</elocation-id><permissions><copyright-statement>© 2014, Hackett and Somia</copyright-statement><copyright-year>2014</copyright-year><copyright-holder>Hackett and Somia</copyright-holder><license xlink:href="http://creativecommons.org/licenses/by/3.0/"><license-p>This article is distributed under the terms of the <ext-link ext-link-type="uri" xlink:href="http://creativecommons.org/licenses/by/3.0/">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="elife02904.pdf"/><related-article ext-link-type="doi" id="ra1" related-article-type="commentary-article" xlink:href="10.7554/eLife.01911"/><abstract><p>Viruses have been used to deliver two types of site-specific nucleases into cells for targeted gene editing.</p></abstract><kwd-group kwd-group-type="author-keywords"><title>Author keywords</title><kwd>protein transduction</kwd><kwd>zinc-finger nucleases</kwd><kwd>transcription activator-like effector nucleases</kwd><kwd>lentiviral vector</kwd><kwd>gag</kwd><kwd>gene therapy</kwd></kwd-group><kwd-group kwd-group-type="research-organism"><title>Research organism</title><kwd>human</kwd><kwd>viruses</kwd></kwd-group></article-meta></front><body><boxed-text><p><bold>Related research article</bold> Cai Y, Bak RO, Mikkelsen JG. 2014. Targeted genome editing by lentiviral protein transduction of zinc-finger and TAL-effector nucleases. <italic>eLife</italic> <bold>3</bold>:e01911. doi: <ext-link ext-link-type="uri" xlink:href="http://dx.doi.org/10.7554/eLife.01911">10.7554/eLife.01911</ext-link></p><p><bold>Image</bold> A schematic of a virus containing site-specific nucleases (blue and green dots) and templates (red squiggles) for gene editing</p><p><inline-graphic xlink:href="elife02904inf001"/></p></boxed-text><p>Microorganisms rely on enzymes called restriction endonucleases to protect them against viruses. These restriction enzymes work by breaking the DNA in the virus into short fragments that are no longer active (<xref ref-type="bibr" rid="bib14">Linn and Arber, 1968</xref>). When isolated and purified, these restriction enzymes can also be used to cut DNA from different sources into fragments that can then be recombined into new sequences with specific properties. When site-specific endonucleases were first used to fashion recombinant DNA molecules in the early 1970s, they revolutionised research in molecular and cellular biology (<xref ref-type="bibr" rid="bib7">Cohen et al., 1973</xref>; <xref ref-type="bibr" rid="bib6">Cohen, 2013</xref>). The power of this approach was immediately recognised, but worries about potential biohazards (<xref ref-type="bibr" rid="bib1">Berg et al., 1974</xref>) suppressed the technology for a couple of years, before common sense and appropriate experimentation demonstrated its safety (<xref ref-type="bibr" rid="bib2">Berg and Singer, 1995</xref>).</p><p>The use of naturally occurring restriction endonucleases limited what could be achieved by gene therapy. These enzymes generally cleave DNA molecules after every few hundred to few thousand base pairs, which is good enough for constructing recombinant DNAs for use in research. Gene therapy, on the other hand, requires the ability to cleave a DNA molecule at a specific site in a genome comprising billions of basepairs.</p><p>Forty years after restriction enzymes were first used to cleave DNA strands, a new revolution employing artificial site-specific nucleases has overtaken biological sciences. This began with the creation of hybrid enzymes, composed of protein sequences called zinc fingers and an endonuclease domain taken from a naturally occurring restriction enzyme (<xref ref-type="bibr" rid="bib12">Kim et al., 1996</xref>). Like a natural restriction enzyme, a zinc finger nuclease (ZFN) operates as a dimer, with one zinc finger binding to each strand of a double-stranded DNA molecule. With ZFNs cleaving both strands of DNA at the same place, researchers can either disable a gene, or introduce specific changes in the sequence by adding a ‘template DNA’ molecule (<xref ref-type="bibr" rid="bib3">Bibikova et al., 2002</xref>) as part of a process called homology-directed repair (<xref ref-type="bibr" rid="bib16">Urnov et al., 2010</xref>). These processes are called gene editing.</p><p>Since the introduction of ZFNs, two more highly adaptable methods have been developed. The first method employs TALENs (transcription activator-like endonucleases), which are like ZFNs but use alternative pairs of polypeptides in place of the zinc fingers (<xref ref-type="bibr" rid="bib4">Bogdanove and Voytas, 2011</xref>). The second method, called CRISPR-Cas, cleaves specific DNA sequences that have been targeted by designer RNA sequences (<xref ref-type="bibr" rid="bib10">Haurwitz et al., 2010</xref>). TALENs and the CRISPR-Cas system are considered easier to engineer and more reliable than ZFNs (<xref ref-type="bibr" rid="bib9">Gaj et al., 2013</xref>). Now, in <italic>eLife</italic>, Yujia Cai, Rasmus Bak and Jacob Mikkelsen of Aarhus University in Denmark present a new method that could bring these gene-editing techniques a step closer to mainstream medical use (<xref ref-type="bibr" rid="bib5">Cai et al., 2014</xref>).</p><p>Despite the immense potential of gene editing, deploying it has been problematic. For many types of gene therapy, proteins and the nucleic acid molecules that encode ZFN, TALEN and CRISPR activities must be introduced into the cells of an individual. However, the immune response protects all the cells in the body from invasion, so until the immune system can be effectively controlled to prevent this response, most gene editing is limited to single cells. This has certain advantages: several molecular transfer technologies can be used to introduce DNA molecules, RNA molecules or the proteins that direct DNA cleavage into cells. Moreover, working with single cells also offers the opportunity to screen gene-edited genomes for unwanted mutations that can arise when the nucleases cut the DNA at a different, related sequence to the one that should be targeted. If just the right amounts of nuclease and template are introduced into a cell, this ‘off-targeting’ can be reduced—which is important for ensuring gene therapy is safe.</p><p>Viruses called integration- and replication-deficient lentiviruses (IDLVs) can penetrate the cellular barriers to introduce precise levels of site-specific nucleases and templates into cells (<xref ref-type="bibr" rid="bib8">Cornu and Cathomen, 2007</xref>; <xref ref-type="bibr" rid="bib15">Lombardo et al., 2007</xref>). These viruses are highly engineered versions of human immunodeficiency virus type 1 (HIV-1). Appropriately modified IDLVs are able to infect a range of cell types and deliver both their genetic cargos and their viral proteins. Thus, genes encoding ZFNs and templates for homology directed repair could be delivered to cells in whole animals (<xref ref-type="bibr" rid="bib11">Joglekar et al., 2013</xref>).</p><p>Cai, Bak and Mikkelsen hypothesised that they could deliver functional nucleases in the lentiviral particles while blocking the integration of viral DNA into the genome (<xref ref-type="bibr" rid="bib5">Cai et al., 2014</xref>). The technique exploits the fact that viruses are made from long proteins that are split into shorter, functional proteins by a viral enzyme. In this case, Cai et al. fused either ZFN- or TALEN-nuclease encoding sequences to the <italic>gag</italic> (group-specific antigens) set of genes in the IDLVs (<xref ref-type="fig" rid="fig1">Figure 1</xref>). This combined genetic sequence created a single ‘fusion protein’, which could cut out specific target genes in several mammalian cell lines. In addition, using fusion proteins makes it possible to control the level of nuclease polypeptides entering cells simply by introducing different numbers of viral particles. This contrasts with previously used methods that instead deliver the genes encoding ZFNs or TALENs. As these genes are expressed at variable levels inside the cell, depending on the stability and integration of the delivered DNA, precise control of the number of nucleases is not possible.<fig id="fig1" position="float"><label>Figure 1.</label><caption><title>Modified viruses can deliver the enzymes and templates needed for gene editing.</title><p>The lentiviral particles created by Cai et al. had glycoproteins (VSV; pale orange) on their surface, which enabled them to infect of a wide range of cell types. The lentiviral particles also contained site-specific nucleases (thick black lines) that targeted specific sequences in the DNA of the host cell, and a DNA template (thick red line) that was added to the genome of the host cell. Cai et al. demonstrated that their approach worked with two types of site-specific nuclease (SSN): zinc finger nucleases (ZFNs) and transcription activator-like endonucleases (TALENs). The modified lentiviral ‘genome’ is illustrated at the top: when this is expressed as a polypeptide inside the host cell, it is cleaved by protease (PROT; red stars). The gene for the SSN was inserted into the <italic>gag</italic> sequence of genes in the virus. Cai et al. also made a number of other important modifications: the normal lentiviral promoter that marks the start of a gene was replaced by a different promoter (called CMV), and the gene in the <italic>pol</italic> sequence that encodes an enzyme called integrase (INT) was modified (red slash) to inactivate the integration activity. The virus used was actually an RNA virus, so reverse transcriptase (RT; brown stars) was used to convert the RNA into DNA. The bottom of the figure shows the DNA of the host cell. The SSNs bind to the DNA (double blue lines) at the sites indicated by the red stars, and the cleavage site is shown by the lightning bolt. VSV: vesicular stomatitis virus; CMV: cytomegalovirus.</p></caption><graphic xlink:href="elife02904f001"/></fig></p><p>Mikkelsen and colleagues demonstrated that genes in up to about 20% of cultured cells could be disrupted by IDLV-mediated protein transfer, and that the incoming viral genomes could provide DNA templates to support specific gene editing, albeit at a lower rate than cleavage of the DNA target site. However, the rates of TALEN-mediated gene editing were substantially reduced compared with that by ZFNs (due to the polypeptides in the TALEN being inactivated).</p><p>Although the rates of gene editing reported by Cai et al. are low and variable, they approach the levels required for effective gene therapy in whole animals—including humans. As this is the first demonstration of the use of gag-modified IDLVs for gene editing in animal cells, there is room for improving the design of the IDLVs and the way they are delivered. One challenge is to eliminate the possibility of a recombination event occurring between a circular form of the template, which would lead to unwanted sequences being inserted into the chromosome. The platform could also be adapted to work with the CRISPR system. Moreover, Mikkelsen and colleagues speculate on the basis of preliminary data that this method of delivery of site-specific nucleases may reduce off-targeting rates through its ability to carefully control the levels of nuclease in the cells.</p><p>The aim of researchers during the original site-specific endonuclease revolution, to repair parts of the human genome using gene editing techniques, was derided some years ago as ‘not only naïve but also wrong-headed’ (<xref ref-type="bibr" rid="bib13">Lewin, 1970</xref>). This second revolution brings us closer to proving that notion wrong.</p></body><back><fn-group content-type="competing-interest"><fn fn-type="conflict" id="conf1"><label>Competing interests:</label><p>The authors declare that no competing interests exist.</p></fn></fn-group><ref-list><title>References</title><ref id="bib1"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Berg</surname><given-names>P</given-names></name><name><surname>Baltimore</surname><given-names>D</given-names></name><name><surname>Boyer</surname><given-names>HW</given-names></name><name><surname>Cohen</surname><given-names>SN</given-names></name><name><surname>Davis</surname><given-names>RW</given-names></name><name><surname>Hogness</surname><given-names>DS</given-names></name><name><surname>Nathans</surname><given-names>D</given-names></name><name><surname>Roblin</surname><given-names>R</given-names></name><name><surname>Watson</surname><given-names>JD</given-names></name><name><surname>Weissman</surname><given-names>S</given-names></name><name><surname>Zinder</surname><given-names>ND</given-names></name></person-group><year>1974</year><article-title>Potential biohazards of recombinant DNA molecules</article-title><source>Science</source><volume>185</volume><fpage>303</fpage><pub-id pub-id-type="doi">10.1126/science.185.4148.303</pub-id></element-citation></ref><ref id="bib2"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Berg</surname><given-names>P</given-names></name><name><surname>Singer</surname><given-names>MF</given-names></name></person-group><year>1995</year><article-title>The recombinant DNA controversy: Twenty years later</article-title><source>Proceedings of the National Academy of Sciences of the USA</source><volume>92</volume><fpage>9011</fpage><lpage>9013</lpage><pub-id pub-id-type="doi">10.1073/pnas.92.20.9011</pub-id></element-citation></ref><ref id="bib3"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Bibikova</surname><given-names>M</given-names></name><name><surname>Golic</surname><given-names>M</given-names></name><name><surname>Golic</surname><given-names>KG</given-names></name><name><surname>Carroll</surname><given-names>D</given-names></name></person-group><year>2002</year><article-title>Targeted chromosomal cleavage and mutagenesis in Drosophila using zinc-finger nucleases</article-title><source>Genetics</source><volume>161</volume><fpage>1169</fpage><lpage>1175</lpage></element-citation></ref><ref id="bib4"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Bogdanove</surname><given-names>AJ</given-names></name><name><surname>Voytas</surname><given-names>DF</given-names></name></person-group><year>2011</year><article-title>TAL efffectors: customizable proteins for DNA targeting</article-title><source>Science</source><volume>333</volume><fpage>1843</fpage><lpage>1844</lpage><pub-id pub-id-type="doi">10.1126/science.1204094</pub-id></element-citation></ref><ref id="bib5"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Cai</surname><given-names>Y</given-names></name><name><surname>Bak</surname><given-names>RO</given-names></name><name><surname>Mikkelsen</surname><given-names>JG</given-names></name></person-group><year>2014</year><article-title>Targeted genome editing by lentiviral protein transduction of zinc-finger and TAL-effector nucleases</article-title><source>eLife</source><volume>3</volume><fpage>e01911</fpage><pub-id pub-id-type="doi">10.7554/eLife.01911</pub-id></element-citation></ref><ref id="bib6"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Cohen</surname><given-names>SN</given-names></name></person-group><year>2013</year><article-title>DNA cloning: a personal view after 40 years</article-title><source>Proceedings of the National Academy of Sciences of the USA</source><volume>110</volume><fpage>15521</fpage><lpage>15529</lpage><pub-id pub-id-type="doi">10.1073/pnas.1313397110</pub-id></element-citation></ref><ref id="bib7"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Cohen</surname><given-names>SN</given-names></name><name><surname>Chang</surname><given-names>AC</given-names></name><name><surname>Boyer</surname><given-names>HW</given-names></name><name><surname>Helling</surname><given-names>RB</given-names></name></person-group><year>1973</year><article-title>Construction of biologically functional bacterial plasmids in vitro</article-title><source>Proceedings of the National Academy of Sciences of the USA</source><volume>70</volume><fpage>3240</fpage><lpage>3244</lpage><pub-id pub-id-type="doi">10.1073/pnas.70.11.3240</pub-id></element-citation></ref><ref id="bib8"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Cornu</surname><given-names>TI</given-names></name><name><surname>Cathomen</surname><given-names>T</given-names></name></person-group><year>2007</year><article-title>Targeted genome modifications using integrase-deficient lentiviral vectors</article-title><source>Molecular Therapy</source><volume>15</volume><fpage>2107</fpage><lpage>2113</lpage><pub-id pub-id-type="doi">10.1038/sj.mt.6300345</pub-id></element-citation></ref><ref id="bib9"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Gaj</surname><given-names>T</given-names></name><name><surname>Gersbach</surname><given-names>CA</given-names></name><name><surname>Barbas</surname><given-names>CF</given-names><suffix>III</suffix></name></person-group><year>2013</year><article-title>ZFN, TALEN, and CRISPR/Cas-based methods for genome engineering</article-title><source>Trends in Biotechnology</source><volume>31</volume><fpage>397</fpage><lpage>404</lpage><pub-id pub-id-type="doi">10.1016/j.tibtech.2013.04.004</pub-id></element-citation></ref><ref id="bib10"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Haurwitz</surname><given-names>RE</given-names></name><name><surname>Jinek</surname><given-names>M</given-names></name><name><surname>Wiedenheft</surname><given-names>B</given-names></name><name><surname>Doudna</surname><given-names>JA</given-names></name></person-group><year>2010</year><article-title>Sequence- and structure-specific RNA processing by a CRISPR endonuclease</article-title><source>Science</source><volume>329</volume><fpage>1355</fpage><lpage>1358</lpage><pub-id pub-id-type="doi">10.1126/science.1192272</pub-id></element-citation></ref><ref id="bib11"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Joglekar</surname><given-names>AV</given-names></name><name><surname>Hollis</surname><given-names>RP</given-names></name><name><surname>Kuftinec</surname><given-names>G</given-names></name><name><surname>Senadheera</surname><given-names>SR</given-names></name><name><surname>Chan</surname><given-names>R</given-names></name><name><surname>Kohn</surname><given-names>DB</given-names></name></person-group><year>2013</year><article-title>Integrase-defective lentiviral vectors as a delivery platform for targeted modification of adenosine deaminase locus</article-title><source>Molecular Therapy</source><volume>21</volume><fpage>1705</fpage><lpage>1717</lpage><pub-id pub-id-type="doi">10.1038/mt.2013.106</pub-id></element-citation></ref><ref id="bib12"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Kim</surname><given-names>YG</given-names></name><name><surname>Cha</surname><given-names>J</given-names></name><name><surname>Chandrasegaran</surname><given-names>S</given-names></name></person-group><year>1996</year><article-title>Hybrid restriction enzymes: zinc finger fusions to Fok I cleavage domain</article-title><source>Proceedings of the National Academy of Sciences of the USA</source><volume>93</volume><fpage>1156</fpage><lpage>1160</lpage><pub-id pub-id-type="doi">10.1073/pnas.93.3.1156</pub-id></element-citation></ref><ref id="bib13"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Lewin</surname><given-names>B</given-names></name></person-group><year>1970</year><article-title>Second ages of molecular biology</article-title><source>Nature</source><volume>227</volume><fpage>1009</fpage><lpage>1013</lpage><pub-id pub-id-type="doi">10.1038/2271009a0</pub-id></element-citation></ref><ref id="bib14"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Linn</surname><given-names>S</given-names></name><name><surname>Arber</surname><given-names>W</given-names></name></person-group><year>1968</year><article-title>Host specificity of DNA produced by Escherichia coli, X. In vitro restriction of phage fd replicative form</article-title><source>Proceedings of the National Academy of Sciences of the USA</source><volume>59</volume><fpage>1300</fpage><lpage>1306</lpage><pub-id pub-id-type="doi">10.1073/pnas.59.4.1300</pub-id></element-citation></ref><ref id="bib15"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Lombardo</surname><given-names>A</given-names></name><name><surname>Genovese</surname><given-names>P</given-names></name><name><surname>Beausejour</surname><given-names>CM</given-names></name><name><surname>Colleoni</surname><given-names>S</given-names></name><name><surname>Lee</surname><given-names>YL</given-names></name><name><surname>Kim</surname><given-names>KA</given-names></name><name><surname>Ando</surname><given-names>D</given-names></name><name><surname>Urnov</surname><given-names>FD</given-names></name><name><surname>Galli</surname><given-names>C</given-names></name><name><surname>Gregory</surname><given-names>PD</given-names></name><name><surname>Holmes</surname><given-names>MC</given-names></name><name><surname>Naldini</surname><given-names>L</given-names></name></person-group><year>2007</year><article-title>Gene editing in human stem cells using zinc finger nucleases and integrase-defective lentiviral vector delivery</article-title><source>Nature Biotechnology</source><volume>25</volume><fpage>1298</fpage><lpage>1306</lpage><pub-id pub-id-type="doi">10.1038/nbt1353</pub-id></element-citation></ref><ref id="bib16"><element-citation publication-type="journal"><person-group person-group-type="author"><name><surname>Urnov</surname><given-names>FD</given-names></name><name><surname>Rebar</surname><given-names>EJ</given-names></name><name><surname>Holmes</surname><given-names>MC</given-names></name><name><surname>Zhang</surname><given-names>HS</given-names></name><name><surname>Gregory</surname><given-names>PD</given-names></name></person-group><year>2010</year><article-title>Genome editing with engineered zinc finger nucleases</article-title><source>Nature Reviews Genetics</source><volume>11</volume><fpage>636</fpage><lpage>646</lpage><pub-id pub-id-type="doi">10.1038/nrg2842</pub-id></element-citation></ref></ref-list></back></article>