Pre-step: Install dependencies (if not present) deps.sh
1.Download static binary https://github.com/DecodeGenetics/popSTR/releases/download/2.0/popSTR and zip of source code https://github.com/DecodeGenetics/popSTR/archive/2.0.zip
2.Unzip source code: unzip popSTR-2.0
3.Move static binary to source code directory: mv popSTR popSTR-2.0
4.Run setup script: setUp.sh
1.Download zip of source code: https://github.com/DecodeGenetics/popSTR/archive/master.zip
2.Unzip source code: unzip master.zip
3.Move to source code directory: cd popSTR-master/
4.Run install script install.sh
5.Run setup script: setUp.sh
6.[Optional] To make sure installation succeeded, execute runSmall.sh with a bamList(described below) and path to reference: runSmall.sh bamList reference
This will genotype the samples in bamList over a set of markers from chr21 and write the results to ./vcfs/chr21_small_0.vcf. Two other files pnSlippage and markerSlippageChr21_0 are also generated. pnSlippage contains slippage rates for all samples in bamList and markerSlippageChr21_0 contains slippage and stutter rates for the genotyped markers.
To genotype samples listed in bamList for all markers on chrom in parallel where the number of markers run by each job is equal to markersPerJob :
runPerChrom bamList reference chrom markersPerJob
bamList- Two column file listing all samples to be genotyped, first column: A sample identifier. Second column: Path to the bam file. (An index (.bai file) for all bam files must exist in the same directory)reference- Path to a reference file the bam files inbamListwere aligned to.
PopSTR has three steps and one must iterate between steps 2 and 3 until convergence or use the kernel provided(Description here):
If you wish to manually run each step of the process, they are described below but we recommend using the provided runPerChrom.sh script
1. computeReadAttributes - Find useable reads, estimate their number of repeats and compute attributes for logistic regression.
Is run for a list of samples over a list of markers.
Call:
computeReadAttributes bamList outputDirectory <(cut -d ' ' -f 1-11,14- markerInfoFile) minFlankLength maxRepeatLength chrom reference expansions jumpToExpansions[Y/N]
Parameters:
-
bamList- Two column file listing all samples to be genotyped, first column: A sample identifier. Second column: Path to the bam file. (An index (.bai file) for all bam files must exist in the same directory) -
outputDirectory- A folder called attributes will be created in the directory if it doesn't exist. A folder called [chrom] (last parameter above) will be created in the attributes folder if it doesn't exist. One file will be created per marker, located at [outputDirectory]/attributes/[chrom]/[start]_[motif] where start is the start coordinate of the marker and motif is the marker's repeat motif. -
markerInfoFile- A file listing the markers to be genotyped, must only contain markers from one chromosome. Marker files for chr1-ch22 are provided. Format for markerInfoFile (cut command removes defaultSlippage and defaultStutter):chrom startCoordinate endCoordinate repeatMotif numOfRepeatsInRef 1000refBasesBeforeStart 1000refBasesAfterEnd repeatSeqFromRef minFlankLeft minFlankRight repeatPurity defaultSlippage defaultStutter fractionAinMotif fractionCinMotif fractionGinMotif fractionTinMotif -
minFlankLength- Minimum number of flanking bases required on each side of a repeat for a read to be considered useful. -
maxRepeatLength- All alleles with a basePair length above this number will be lumped together into a greater than allele. Should be set close to 0.5 * readLength in IN.bam. -
chrom- All markers in markerInfoFile must come from this chromosome. -
reference- Path to a fasta file containing the reference the reads were aligned/compressed to. Necessary for CRAM support. -
expansionsA list of known long repeat stretches in the reference, provided with the software -
jumpToExpansions[Y/N]Determines whether to examine reads aligned to other repeat locations in the genome with mates close to the marker being considered. Choosing Y will increase runtime but is more precise and intended when closely examinig possibly expanded regions.
First line contains an offset entry for each PN, to make seeking in the file possible.
The rest of the attribute-file has the following format for each sample specified in the bamList:
1:Sample id
2: Markerline
chrom startCoordinate endCoordinate repeatMotif numOfRepeatsInRef numOfReadsFound A1-initialization A2-initialization
3: Attribute lines (Number of lines is determined by numOfReadsFound from the Markerline):
numOfRepeatsInRead alignmentQualBefore alignmentQualAfter locationShift mateEditDist repeatPurity ratioOver20inRepeat repeatSeqFromRead
- numOfRepeatsInRead - The allele reported by the read, tells us how many repeats were found in the read.
- alignmentQualBefore - Quality of realignment on left side of repeat. Ranges from 0 to 1 and higher values indicate more reliable reads.
- alignmentQualAfter - Quality of realignment on right side of repeat. Ranges from 0 to 1 and higher values indicate more reliable reads.
- locationShift - Measures changes from original alignment during the realignment of flanking sequences, common values lie between 0 and 4.
- mateEditDist - Edit distance of aligned base pairs of the mate sequence to the reference, higher values of this attribute are suspicious.
- repeatPurity - Measures how well the repeat sequence from the read matches the repeat sequence from the reference. Ranges from 0 to 1 and higher values indicate more reliable reads.
- ratioOver20inRepeat - Measures the ratio of bases in the repeat sequence with high quality scores. Ranges from 0 to 1 and higher values indicate more reliable reads.
- repeatSeqFromRead - Repeat sequence from the read.
Is run for a list of samples over a list of markers.
Call:
computePnSlippage -ML markerList -PL pnList -AD attributesDirectory -OF outputFile -IN iterationNumber -FP firstPnIdx -NPN minPnsPerMarker -MS markerSlippageFile -MD modelAndLabelDir
Parameters:
-
markerList- List of markers to estimate the slippage over, must all come from the same chromosome. Format for markerList:chrom start end motif -
pnList- List of samples to estimate slippage for, should only have a single column with same sample identifiers as in column one of bamList used in computeReadAttributes call. -
attributesDirectory- Should be the same as the "outputDirectory" parameter in the computeReadAttributes call + /attributes/chrom where chrom is the chromosome of the markers in markerList. -
outputFile- Slippage rate will be written to a file with _iterationNumber appended to this name, i.e. in iteration 0 outputFile_0 will be created. OBS:if the file already exists, the slippage rates estimated will be appended to it. If iterationNumber > 0 the program will also look for outputFile_[iterationNumber - 1] to get slippage estimates from previous iteration. -
iterationNumber- Zero based number of iteration. -
firstPnIdx- Index of the first sample in pnList within the bamList passed to the computeReadAttributes command, to enable faster seeking within the attributes files. -
minPnsPerMarker- Minimum number of individuals used to estimate slippage at a given marker so the slippage can be considered reliable. Slippage rates estimated using a small number of samples might not be accurate. -
markerSlippageFile- ONLY applicable if iterationNumber > 0! Should be a path to the markerSlippage file created by msGenotyper in the last iteration. iterationNumber will be appended to the path. -
modelAndLabelDir- ONLY applicable if iterationNumber > 0! Should be modelAndLabelDir supplied in the msGenotyper call for this chrom. The program will find within the folder for chrom the label files created in iteration number [iterationNumber] of msGenotyper. It will also locate a file for each marker containing the current logistic regression model for that marker.
3. msGenotyper - Determine genotypes, estimate marker slippage rates and train logistic regression models.
Is run for a list of samples(preferably all samples in bamList from computeReadAttributes command) over a list of markers from the same chromosome.
Call:
msGenotyper -AD attDir -PNS pnList -ML markerList -I intervalIndex -MS markerSlippageFile -MD modelAndLabelDir -IN iterationNumber -FP firstPnIdx -VD vcfOutputDirectory -VN vcfFileName
Parameters:
attDir- A concatenation of the outputDirectory and chrom paratmeters: [outputDirectory]/[chrom] from the computeReadAttributes call of the chromosome being genotyped.pnList- Should be the outputFile parameter supplied in the computePnSlippage call.markerList- List of markers to genotype, has only 2 columns: start and motifintervalIndex- If splitting the chromosome this parameter indicates the index of the interval specified. When this functionality is not desired the user can specify any number, it will be appended to names of all output files as "_intervalIndex" and must be manually removed before performing subsequent iterations.markerSlippageFile- The marker slippage rates estimated will be written to [markerSlippageFile][iterationNumber]_[intervalIndex] and if iterationNumber>1 the marker slippage rates estimated in the previous iteration will be read from [markerSlippageFile][iterationNumber-1]_[intervalIndex]modelAndLabelDir- In this folder a files called [start]_[motif][iterationNumber] and model_[start]_[motif] will be created for each marker. If iteration number>1 the labels and models from the previous iteration will be read.iterationNumber- One based number of iteration.firstPnIdx- Index of the first sample in pnList within the bamList passed to the computeReadAttributes command, to enable faster seeking within the attributes files.vcfOutputDirectory- ONLY applicable if iteration number == 5! Directory to place vcf-files containing genotypes for all individuals at all markers contained within the interval being considered.vcfFileName- ONLY applicable if iteration number == 5! Genotypes will be written to a vcf-file [vcfOutputDirectory]/[vcfFileName]_[intervalIndex].vcf.
When finishing an iteration of msGenotyper, these steps must be taken before starting the next iteration of computePnSlippage.
-
MarkerSlippage-files for all intervals must be concatenated into a single file for that chromosome. For example if one has just finished iteration 1 and the chromosome has been split into 20 intervals, the following command must be run in the directory containing the interval-split markerSlippage-files:
for i in {1..22}; do cat markerSlippageFile1_${i} >> markerSlippageFile1; done
A specific vcf file will be created for each interval and when all intervals have finished running these must be manually concatenated into a single file.
`grep ^# [vcfOutputDirectory]/vcfFileName_1.vcf > [vcfOutputDirectory]/vcfFileName.vcf`
`for i in {1..[numIntervals]}; do grep -v ^# [vcfOutputDirectory]/vcfFileName_${i}.vcf >> [vcfOutputDirectory]/vcfFileName.vcf; done`
To circumvent the iterative part using your entire dataset it is possible to train only slippage rates for a selected set of markers (a kernel) and run the "Default" versions of computePnSlippage and msGenotyper to obtain genotypes directly.
A kernel containing 8779 markers on chr21(HG38 coordinates) is supplied along with the software (kernelSlippageRates, kernelModels(1 file for each marker in the kernel) and kernelMarkersInfo).
To use the kernel one must follow the same three steps as before with slight changes:
1. Run computeReadAttributes as described in the iterative version for all chromosomes on all PNs to be genotyped.
Call:
`computePnSlippageDefault -PL pnList -AD attributesDirectory -OF outputFile -FP firstPnIdx -MS kernelSlippageRates -MD pathToKernelModelsFiles`
Parameters:
pnList- List of samples to estimate slippage for, should only have a single column with same sample identifiers as in column one of bamList used in computeReadAttributes call.attributesDirectory- outputDirectory/attributes/chr21 Parameter 2 from running computeReadAttributes with kernelMarkersInfo from the kernel as parameter number 3 appended with attributes and chr21 as shown.outputFile- Slippage rate will be written(appended if file exists) to this file.firstPnIdx- Index of the first sample in pnList within the bamList passed to the computeReadAttributes command, to enable faster seeking within the attributes files.kernelSlippageRates- supplied in the kernel tarball, contains slippage rates and other info for kernel markers.pathToKernelModelsFiles- Folder supplied in the kernel tarball. Logistic regression models for all markers in the kernel.
Call:
`msGenotyperDefault -ADCN attributesDirectory/chromNum/ -PNS pnSlippageFile -MS markerSlippageFile -VD vcfOutputDirectory -VN vcfFileName -ML markerList -I intervalIndex -FP firstPnIdx`
Parameters:
-
attributesDirectory/chromNum/- Should be a path to output files from running computeReadAttributes in the standard way followed by the name of the chromosome to be genotyped. This directory will be searched for attribute files for all markers in the markerList file. -
pnSlippageFile- This file should contain the output of computePnSlippageDefault for all individuals to be genotyped and have 2 columns, sample identifier and slippage rate. -
markerSlippageFile- Slippage rates for all markers to be genotyped will be written to a file called [markerSlippageFile]_[intervalIndex]. -
vcfOutputDirectory- Directory to place vcf-files containing genotypes for all individuals at all markers in the markerList file. -
vcfFileName- Genotypes will be written to a vcf-file vcfOutputDirectory/vcfFileName_[intervalIndex].vcf -
markerList- List of markers to estimate the slippage over, must all come from the same chromosome. Format for markerList:chrom start end motif -
intervalIndex- If splitting the chromosome this parameter indicates the index of the interval specified. When this functionality is not desired the user can specify any number, it will be appended to names of all output files as "_intervalIndex" and must be manually removed before performing subsequent iterations. -
firstPnIdx- Index of the first sample in pnSlippageFile within the bamList passed to the computeReadAttributes command, to enable faster seeking within the attributes files.