# HG changeset patch
# User cshl-bsr
# Date 1459354306 14400
# Node ID 6610eedd9fae11b6d6fa3682d38e158e6c188bb7
# Parent 82bb8c455761ac5f483273b800d32aca2755b181
Uploaded
diff -r 82bb8c455761 -r 6610eedd9fae ._ezBAMQC
Binary file ._ezBAMQC has changed
diff -r 82bb8c455761 -r 6610eedd9fae BAMqc.sh
--- a/BAMqc.sh Wed Mar 30 12:03:10 2016 -0400
+++ /dev/null Thu Jan 01 00:00:00 1970 +0000
@@ -1,122 +0,0 @@
-#!/bin/sh
-
-### Galaxy Wrapper for BAMqc ###
-
-alignment_files=""
-refgene=""
-attrID=""
-rRNA=""
-outputHTML=""
-stranded=""
-mapq="30"
-lowBound="-250"
-upperBound="250"
-stepSize="5"
-labels=""
-cores="1"
-
-ARGS=$(getopt -o "r:f:R:o:s:p:q:" -- "$@")
-
-if [ $? -ne 0 ]; then
- echo "Invalid command-line parameters. Do not use this script outside of Galaxy" >&2
- exit 1
-fi
-
-eval set -- "$ARGS"
-
-while [ $# -gt 0 ]; do
- case "$1" in
- -r)
- refgene="$2"
- shift 2
- ;;
- -f)
- attrID="$2"
- shift 2
- ;;
- -R)
- rRNA="$2"
- shift 2
- ;;
- -o)
- outputHTML=$2
- shift 2
- ;;
- -s)
- stranded=$2
- shift 2
- ;;
- -q)
- mapq=$2
- shift 2
- ;;
-
- -p)
- cores=$2
- shift 2
- ;;
- --)
- shift
- break
- ;;
- esac
-done
-
-if [ "$cores" -gt 10 ];then
- cores="10"
-fi
-
-outputDir=`echo $outputHTML | sed 's/\.dat$/_files/'`
-if [ ! -d "$outputDir" ]; then
- mkdir $outputDir
-fi
-
-touch bamqc.log
-
-while [ "$#" -ne 0 ];
-do
- FILE="$1"
- LABEL=`echo $2 | sed 's/ /-/g; s/\[//; s/\]//;'`
- shift 2
- QNAME_SORTED=`samtools view -H ${FILE} | grep "SO:queryname"`
- if [ $? -ne 0 ]; then
- BASE=`basename ${FILE} \.dat`
- echo "Sorting BAM file (${LABEL}." >>samtools.log
- samtools sort -@ 5 -n ${FILE} ${BASE} 2>>samtools.log
- if [ $? -ne 0 ]; then
- echo "Error with samtools sorting for BAM file (${LABEL})." >&2
- cat samtools.log >&2
- exit 1
- fi
- echo "BAM file (${LABEL}) was re-sorted by query name." >>bamqc.log
- FILELIST="$FILELIST ${BASE}.bam"
- else
- FILELIST="$FILELIST $FILE"
- fi
- LABELLIST="$LABELLIST $LABEL"
-done
-
-CMD="ezBAMQC -i $FILELIST -l $LABELLIST -f $attrID -r $refgene -o Galaxy_BAMqc_output --stranded $stranded -q $mapq --rRNA $rRNA -t $cores"
-
-echo "BAMqc command: $CMD" >> bamqc.log
-echo >> bamqc.log
-
-$CMD 2>> bamqc.log
-
-if [ $? -ne 0 ]; then
- echo "BAMqc ran with errors" >&2
- cat bamqc.log >&2
- exit 1
-fi
-
-sed -i "s/\.\.\/Galaxy_BAMqc_output\///g;" Galaxy_BAMqc_output/bamqc_output.html
-
-cp -r Galaxy_BAMqc_output/data "$outputDir"
-cp -r Galaxy_BAMqc_output/figs "$outputDir"
-cp Galaxy_BAMqc_output/bamqc_output.html "$outputHTML"
-
-if [ $? -ne 0 ]; then
- echo "Copying BAMqc results failed" >&2
-fi
-
-echo "BAMqc results copied to $outputDir" >>bamqc.log
diff -r 82bb8c455761 -r 6610eedd9fae BAMqc.xml
--- a/BAMqc.xml Wed Mar 30 12:03:10 2016 -0400
+++ /dev/null Thu Jan 01 00:00:00 1970 +0000
@@ -1,109 +0,0 @@
-
-
-
- performs QC on BAM files for gene abundances and sample correlation
-
-
-
- BAMqc
- samtools
- R
-
-
-
-
- BAMqc.sh
-
- -r '${refdb}'
-
- -f '${attrID}'
-
- -R '${rRNAdb}'
-
- -s '$stranded'
-
- -o "$output"
-
- #set $core = len($files)
-
- -p $core
-
- #if str($cond_adv_options.adv_options) == 'yes':
- -q '$cond_adv_options.mapq'
- #end if
-
- #for $file in $files
- '$file.input'
- '$file.input.tag'
- #end for
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-
-**What it does**
-
-This tool takes the mapping results from RNA-Seq libraries (BAM), and performs rapid gene abundance quantification. If multiple files are provided, it will calculate and display correlation between each sample.
-
------
-
-The Galaxy wrapper for this tool is written by the `Cold Spring Harbor Laboratory`_ `Bioinformatics Shared Resources`_.
-
-ezBAMQC_ is written by the `Molly Hammell Laboratory`_ and the `Bioinformatics Shared Resources`_ at CSHL_.
-
-.. _CSHL: `Cold Spring Harbor Laboratory`_
-.. _ezBAMQC: http://hammelllab.labsites.cshl.edu/software#ezBAMQC
-.. _`Molly Hammell Laboratory`: http://hammelllab.labsites.cshl.edu/
-.. _`Cold Spring Harbor Laboratory`: http://www.cshl.edu/
-.. _`Bioinformatics Shared Resources`: http://bioinfo.cshl.edu/index.html
-
-
-
-
diff -r 82bb8c455761 -r 6610eedd9fae cshl_geneGTF.loc.sample
--- a/cshl_geneGTF.loc.sample Wed Mar 30 12:03:10 2016 -0400
+++ /dev/null Thu Jan 01 00:00:00 1970 +0000
@@ -1,20 +0,0 @@
-##
-## Location of gene annotations GTF
-##
-## Format is:
-## valueNamedbkeyID
-##
-## Name can contain spaces
-
-/localdata1/annotations/GTF/latest/hg19_refGene.gtf hg19 UCSC refSeq hg19 hg19_refgene
-/localdata1/annotations/GTF/latest/hg18_refGene.gtf hg18 UCSC refSeq hg18 hg18_refgene
-/localdata1/annotations/GTF/latest/mm10_refGene.gtf mm10 UCSC refSeq mm10 mm10_refgene
-/localdata1/annotations/GTF/latest/mm9_refGene.gtf mm9 UCSC refSeq mm9 mm9_refgene
-/localdata1/annotations/GTF/latest/dm3_refGene.gtf dm3 UCSC refSeq dm3 dm3_refgene
-/localdata1/annotations/GTF/refseq_2015_01_20/rn5_refGene.gtf rn5 UCSC refSeq rn5 rn5_refgene
-#/localdata1/annotations/GTF/latest/rn4_refGene.gtf rn4 UCSC refSeq rn4 rn4_refgene
-#/localdata1/annotations/GTF/latest/ce6_refGene.gtf ce6 UCSC refSeq ce6 ce6_refgene
-#/localdata1/annotations/GTF/latest/ce10_refGene.gtf ce10 UCSC refSeq ce10 ce10_refgene
-#/localdata1/annotations/GTF/igenomes_2014_08_28/ZmAGPv2_iGenome_genes.gtf Maize (AGPv2) iGenomes gene info ZmAGPv2 ZmAGPv2_genes
-#/localdata1/annotations/GTF/igenomes_2014_08_28/ZmAGPv3_iGenome_genes.gtf Maize (AGPv3) iGenomes gene info ZmAGPv3 ZmAGPv3_genes
-#/localdata1/annotations/GTF/igenomes_2014_08_28/tair10_iGenome_genes.gtf Arabidopsis (TAIR10) iGenomes gene info
diff -r 82bb8c455761 -r 6610eedd9fae cshl_rRNA_BED.loc.sample
--- a/cshl_rRNA_BED.loc.sample Wed Mar 30 12:03:10 2016 -0400
+++ /dev/null Thu Jan 01 00:00:00 1970 +0000
@@ -1,19 +0,0 @@
-##
-## Location of rRNA BED files
-##
-## Format is:
-## valueNamedbkeyID
-##
-## Name can contain spaces
-
-#/localdata1/annotations/BED_files/rRNA/hg19_rmsk_rRNA.bed hg38 repeatMasker rRNA hg38 hg38_rRNA
-/localdata1/annotations/BED_files/rRNA/hg19_rmsk_rRNA.bed hg19 repeatMasker rRNA hg19 hg19_rRNA
-/localdata1/annotations/BED_files/rRNA/hg18_rmsk_rRNA.bed hg18 repeatMasker rRNA hg18 hg18_rRNA
-/localdata1/annotations/BED_files/rRNA/mm10_rmsk_rRNA.bed mm10 repeatMasker rRNA mm10 mm10_rRNA
-/localdata1/annotations/BED_files/rRNA/mm9_rmsk_rRNA.bed mm9 repeatMasker rRNA mm9 mm9_rRNA
-#/localdata1/annotations/BED_files/rRNA/dm6_rmsk_rRNA.bed dm6 repeatMasker rRNA dm6 dm6_rRNA
-/localdata1/annotations/BED_files/rRNA/dm3_rmsk_rRNA.bed dm3 repeatMasker rRNA dm3 dm3_rRNA
-/localdata1/annotations/BED_files/rRNA/rn5_rmsk_rRNA.bed rn5 repeatMasker rRNA rn5 rn5_rRNA
-#/localdata1/annotations/BED_files/rRNA/rn4_rmsk_rRNA.bed rn4 repeatMasker rRNA rn4 rn4_rRNA
-#/localdata1/annotations/BED_files/rRNA/ce6_rmsk_rRNA.bed ce6 repeatMasker rRNA ce6 ce6_rRNA
-#/localdata1/annotations/BED_files/rRNA/ce10_rmsk_rRNA.bed ce10 repeatMasker rRNA ce10 ce10_rRNA
\ No newline at end of file
diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC.zip
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._MANIFEST.in
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._Makefile
Binary file ezBAMQC/._Makefile has changed
diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._README.rst
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._doc
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._ezBAMQC
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._setup.py
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._src
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/._test-data
Binary file ezBAMQC/._test-data has changed
diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/Makefile
--- a/ezBAMQC/Makefile Wed Mar 30 12:03:10 2016 -0400
+++ b/ezBAMQC/Makefile Wed Mar 30 12:11:46 2016 -0400
@@ -1,6 +1,6 @@
# Makefile for ezBAMQC, utilities for the Sequence Alignment/Map format.
#
-# Version 0.6.5
+# Version 0.6.7
#
# Copyright (C) 2015 Bioinformatics Shared Resource, CSHL.
# Portions copyright (C) 2015 Cold Spring Harbor Laboratory.
diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/README.rst
--- a/ezBAMQC/README.rst Wed Mar 30 12:03:10 2016 -0400
+++ b/ezBAMQC/README.rst Wed Mar 30 12:11:46 2016 -0400
@@ -1,184 +1,186 @@
-.. image:: https://raw.githubusercontent.com/mhammell-laboratory/bamqc/master/doc/bamqc-icon.png
- :width: 200 px
- :alt: generated at codeology.braintreepayments.com/mhammell-laboratory/bamqc
- :align: right
- :target: http://codeology.braintreepayments.com/mhammell-laboratory/bamqc
-
-=====
-ezBAMQC
-=====
-*"ezBAMQC, a tool to check the quality of mapped next generation sequencing files."*
-
-:Description:
-
- ezBAMQC is a tool to check the quality of either one or many mapped next-generation-sequencing datasets. It conducts comprehensive evaluations of aligned sequencing data from multiple aspects including: clipping profile, mapping quality distribution, mapped read length distribution, genomic/transcriptomic mapping distribution, inner distance distribution (for paired-end reads), ribosomal RNA contamination, transcript 5’ and 3’ end bias, transcription dropout rate, sample correlations, sample reproducibility, sample variations. It outputs a set of tables and plots and one HTML page that contains a summary of the results. Many metrics are designed for RNA-seq data specifically, but ezBAMQC can be applied to any mapped sequencing dataset such as RNA-seq, CLIP-seq, GRO-seq, ChIP-seq, DNA-seq and so on. ::
-
-:Links:
-
- `Github Page `_
-
- `Pypi Page `_
-
- `MHammell Lab `_
-
-:Authors:
- Ying Jin, David Molik, and Molly Hammell
-
-:Version: 0.6.5
-
-:Contact:
- Ying Jin (yjin@cshl.edu)
-
-Installation guide for ezBAMQC for from source installs
-=====================================================
-
-When installing ezBAMQC there are several options, but the main point is: since ezBAMQC uses C++ STD 11 you'll need a version of GCC that can support that, this useally means 4.8 or 4.9. beyond that, you'll need Python, R and Corrplot for interfacing with the C code.
-
-:Intallation:
- `Source Code `_
-
- `Pypi `_
-
-:Prerequisites:
- * `python2.7 `_
- * `R `_
- * `corrplot `_
- * `GCC 4.8.1 or greater `_ GCC 4.9.1 or greater is recomended for PyPi install
-
-:Notes:
- * While there are multiple methods of installing the prerequistes it may help to look at (if using a yum based linux distro):*
- * `Devtoolset-3 `_ for GCC compilers
- * `IUS `_ for Python2.7
- * `Software Collections `_ for collections of software (like devtoolset 3 or python)
- * `rpmfinder `_ for searching rpms across mutliple systems
-
-Setup
-=====
-
-1) Make sure that the GCC comiler is in your PATH:
-
-::
-
- export PATH=/path/to/gcc:$PATH
-
-2) Make sure that python2.7 is in your PYTHONPATH:
-
-::
-
- export PYTHONPATH=/path/to/python2.7/site-packages:$PYTHONPATH
-
-3) There are three methods of installation of ezBAMQC, from source, from setup.py, and from pypi, once prequistes are setup.
-
-From Source
-~~~~~~~~~~~
-
-1) Download source
-
-2) Unpack tarball and go to the directory of the package:
-
-::
-
- tar xvfz bamqc-0.6.6.tar.gz
-
- cd bamqc-0.6.6
-
-3) Run make:
-
-::
-
- make
-
-From Setup.py
-~~~~~~~~~~~~~
-
-::
-
- python2.7 setup.py install
-
-From Pypi
-~~~~~~~~~
-
-::
-
- pip2.7 install BAMqc
-
-Usage
-=====
-
-::
-
- ezBAMQC [-h] -i alignment_files [alignment_files ...] -r [refgene]
- [-f [attrID]] [--rRNA [rRNA]] -o [dir] [--stranded [stranded]]
- [-q [mapq]] [-l labels [labels ...]] [-t NUMTHREADS]
-
-optional arguments:
-
-::
-
- -h, --help show this help message and exit.
- -i, --inputFile alignment files. Could be multiple SAM/BAM files separated by space. Required.
- -r, --refgene gene annotation file in GTF format. Required
- -f the read summation at which feature level in the GTF file. DEFAULT: gene_id.
- --rRNA rRNA coordinates in BED format.
- -o, --outputDir output directory. Required.
- --stranded strandness of the library?
- yes : sense stranded
- reverse : reverse stranded
- no : not stranded
- DEFAULT: yes.
- -q, --mapq Minimum mapping quality (phred scaled) for an alignment to be called uniquely mapped. DEFAULT:30
- -l, --label Labels of input files. DEFAULT:smp1 smp2 ...
- -t, --threads Number of threads to use. DEFAULT:1
-
-Example:
-
-::
-
- ezBAMQC -i test-data/exp_data/treat1.bam test-data/exp_data/treat2.bam test-data/exp_data/treat3.bam -r test-data/exp_data/hg9_refGene.gtf -q 30 --rRNA test-data/exp_data/hg19_rRNA.bed -o exp_output2
-
- Please find the example output from folder test-data.
-
-FAQ
-====
-Q: Why use ezBAMQC?
-
-A: ezBAMQC is efficient and easy to use. With one command line, it reports a comprehensive evaluation of the data with a set of plots and tables.The ability to assess multiple samples together with high efficiency make it especially useful in cases where there are a large number of samples from the same condition, genotype, or treatment. ezBAMQC was written in C++ and supports multithreading. A mouse RNA-seq sample with 120M alignments can be done in 8 minutes with 5 threads.
-
-Q: Why the total number of reads reported by ezBAMQC does not match with samtools flagstat?
-
-A: The difference is because of non-uniquely mapped reads or multiply aligned reads (multi-reads). Samtools flagstat counts each multiple aligment as a different reads, but ezBAMQC counts reads accoriding to the read ID, i.e., each individual read will be counted once no matter that it is a uniquely mapped read or multi-read.
-
-Q: What is "Low Quality Reads" ?
-
-A: Reads marked as qc fail accoriding to SAM format or reads with mapping quality lower than the value set by the option -q will be considered as "Low Quality Reads".
-
-Q: How the setting of option -q alter the results?
-
-A: Reads with low quality, i.e., did not pass -q cutoff, are only counted in Total Reads, Mapped Reads, and Mappability by mapping quality plot. The rest of the report does not include low quality reads.
-
-Q: Do multi-reads (non-uniquely mapped reads) have been considered in Read distribution and gene quantification?
-
-A: No. Only uniquely mapped reads were counted.
-
-
-Acknowledgements
-================
-
-#) Samtools contributors
-#) Users' valuable feedback
-
-Copying & Distribution
-======================
-
-ezBAMQC is free software: you can redistribute it and/or modify
-it under the terms of the GNU General Public License as published by
-the Free Software Foundation, either version 3 of the License, or
-(at your option) any later version.
-
-This program is distributed in the hope that it will be useful,
-but *WITHOUT ANY WARRANTY*; without even the implied warranty of
-*MERCHANTABILITY or FITNESS FOR A PARTICULAR PURPOSE*. See the
-GNU General Public License for more details.
-
-You should have received a copy of the GNU General Public License
-along with ezBAMQC. If not, see `this website `_
+=======
+ezBAMQC
+=======
+
+*"ezBAMQC, a tool to check the quality of mapped next generation sequencing files."*
+
+:Codeology Icon:
+
+ .. image:: https://raw.githubusercontent.com/mhammell-laboratory/bamqc/master/doc/bamqc-icon.gif
+ :alt: generated at codeology.braintreepayments.com/mhammell-laboratory/bamqc
+ :align: right
+ :target: http://codeology.braintreepayments.com/mhammell-laboratory/bamqc
+
+:Description:
+
+ ezBAMQC is a tool to check the quality of either one or many mapped next-generation-sequencing datasets. It conducts comprehensive evaluations of aligned sequencing data from multiple aspects including: clipping profile, mapping quality distribution, mapped read length distribution, genomic/transcriptomic mapping distribution, inner distance distribution (for paired-end reads), ribosomal RNA contamination, transcript 5’ and 3’ end bias, transcription dropout rate, sample correlations, sample reproducibility, sample variations. It outputs a set of tables and plots and one HTML page that contains a summary of the results. Many metrics are designed for RNA-seq data specifically, but ezBAMQC can be applied to any mapped sequencing dataset such as RNA-seq, CLIP-seq, GRO-seq, ChIP-seq, DNA-seq and so on.
+
+:Links:
+
+ `Github Page `_
+
+ `Pypi Page `_
+
+ `MHammell Lab `_
+
+:Authors:
+ Ying Jin, David Molik, and Molly Hammell
+
+:Version: 0.6.7
+
+:Contact:
+ Ying Jin (yjin@cshl.edu)
+
+Installation guide for ezBAMQC for from source installs
+=======================================================
+
+When installing ezBAMQC there are several options, but the main point is: since ezBAMQC uses C++ STD 11 you'll need a version of GCC that can support that, this useally means 4.8 or 4.9. beyond that, you'll need Python, R and Corrplot for interfacing with the C code.
+
+:Intallation:
+ `Source Code `_
+
+ `Pypi `_
+
+:Prerequisites:
+ * `python2.7 `_
+ * `R `_
+ * `corrplot `_
+ * `GCC 4.8.1 or greater `_ GCC 4.9.1 or greater is recomended for PyPi install
+
+:Notes:
+ * While there are multiple methods of installing the prerequistes it may help to look at (if using a yum based linux distro):*
+ * `Devtoolset-3 `_ for GCC compilers
+ * `IUS `_ for Python2.7
+ * `Software Collections `_ for collections of software (like devtoolset 3 or python)
+ * `rpmfinder `_ for searching rpms across mutliple systems
+
+Setup
+=====
+
+1) Make sure that the GCC comiler is in your PATH:
+
+::
+
+ export PATH=/path/to/gcc:$PATH
+
+2) Make sure that python2.7 is in your PYTHONPATH:
+
+::
+
+ export PYTHONPATH=/path/to/python2.7/site-packages:$PYTHONPATH
+
+3) There are three methods of installation of ezBAMQC, from source, from setup.py, and from pypi, once prequistes are setup.
+
+From Source
+~~~~~~~~~~~
+
+1) Download source
+
+2) Unpack tarball and go to the directory of the package:
+
+::
+
+ tar xvfz bamqc-0.6.7.tar.gz
+
+ cd bamqc-0.6.7
+
+3) Run make:
+
+::
+
+ make
+
+From Setup.py
+~~~~~~~~~~~~~
+
+::
+
+ python2.7 setup.py install
+
+From Pypi
+~~~~~~~~~
+
+::
+
+ pip2.7 install BAMqc
+
+Usage
+=====
+
+::
+
+ ezBAMQC [-h] -i alignment_files [alignment_files ...] -r [refgene]
+ [-f [attrID]] [--rRNA [rRNA]] -o [dir] [--stranded [stranded]]
+ [-q [mapq]] [-l labels [labels ...]] [-t NUMTHREADS]
+
+optional arguments:
+
+::
+
+ -h, --help show this help message and exit.
+ -i, --inputFile alignment files. Could be multiple SAM/BAM files separated by space. Required.
+ -r, --refgene gene annotation file in GTF format. Required
+ -f the read summation at which feature level in the GTF file. DEFAULT: gene_id.
+ --rRNA rRNA coordinates in BED format.
+ -o, --outputDir output directory. Required.
+ --stranded strandness of the library?
+ yes : sense stranded
+ reverse : reverse stranded
+ no : not stranded
+ DEFAULT: yes.
+ -q, --mapq Minimum mapping quality (phred scaled) for an alignment to be called uniquely mapped. DEFAULT:30
+ -l, --label Labels of input files. DEFAULT:smp1 smp2 ...
+ -t, --threads Number of threads to use. DEFAULT:1
+
+Example:
+
+::
+
+ ezBAMQC -i test-data/exp_data/treat1.bam test-data/exp_data/treat2.bam test-data/exp_data/treat3.bam -r test-data/exp_data/hg9_refGene.gtf -q 30 --rRNA test-data/exp_data/hg19_rRNA.bed -o exp_output2
+
+ Please find the example output from folder test-data.
+
+FAQ
+===
+Q: Why use ezBAMQC?
+
+A: ezBAMQC is efficient and easy to use. With one command line, it reports a comprehensive evaluation of the data with a set of plots and tables.The ability to assess multiple samples together with high efficiency make it especially useful in cases where there are a large number of samples from the same condition, genotype, or treatment. ezBAMQC was written in C++ and supports multithreading. A mouse RNA-seq sample with 120M alignments can be done in 8 minutes with 5 threads.
+
+Q: Why the total number of reads reported by ezBAMQC does not match with samtools flagstat?
+
+A: The difference is because of non-uniquely mapped reads or multiply aligned reads (multi-reads). Samtools flagstat counts each multiple aligment as a different reads, but ezBAMQC counts reads accoriding to the read ID, i.e., each individual read will be counted once no matter that it is a uniquely mapped read or multi-read.
+
+Q: What is "Low Quality Reads" ?
+
+A: Reads marked as qc fail accoriding to SAM format or reads with mapping quality lower than the value set by the option -q will be considered as "Low Quality Reads".
+
+Q: How the setting of option -q alter the results?
+
+A: Reads with low quality, i.e., did not pass -q cutoff, are only counted in Total Reads, Mapped Reads, and Mappability by mapping quality plot. The rest of the report does not include low quality reads.
+
+Q: Do multi-reads (non-uniquely mapped reads) have been considered in Read distribution and gene quantification?
+
+A: No. Only uniquely mapped reads were counted.
+
+
+Acknowledgements
+================
+
+#) Samtools contributors
+#) Users' valuable feedback
+
+Copying & Distribution
+======================
+
+ezBAMQC is free software: you can redistribute it and/or modify
+it under the terms of the GNU General Public License as published by
+the Free Software Foundation, either version 3 of the License, or
+(at your option) any later version.
+
+This program is distributed in the hope that it will be useful,
+but *WITHOUT ANY WARRANTY*; without even the implied warranty of
+*MERCHANTABILITY or FITNESS FOR A PARTICULAR PURPOSE*. See the
+GNU General Public License for more details.
+
+You should have received a copy of the GNU General Public License
+along with ezBAMQC. If not, see `this website `_
diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/doc/._CONTACTS
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/doc/._bamqc-icon.gif
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/doc/._bamqc-icon.png
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diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/ezBAMQC
--- a/ezBAMQC/ezBAMQC Wed Mar 30 12:03:10 2016 -0400
+++ b/ezBAMQC/ezBAMQC Wed Mar 30 12:11:46 2016 -0400
@@ -12,7 +12,7 @@
@status:
-@version: 0.6.6
+@version: 0.6.7
'''
@@ -872,7 +872,7 @@
f.write("nz_gene_mm[i] = length(which(M1[,i]>0))/nz_genes * 100 } \n")
- f.write("bplt <- barplot(nz_gene_mm,beside=T,border='NA',space=1.5,ylim=c(0,100),ylab='Genes reproducibly detected (%)',col='blue',names.arg=colnames(MM))\n")
+ f.write("bplt <- barplot(nz_gene_mm,beside=T,border='NA',space=1.5,ylim=c(0,100),ylab='Genes reproducibly detected (%)',col='blue',names.arg=colnames(MM),las=2)\n")
f.write("text(y= nz_gene_mm+2, x= bplt, labels=paste(as.character(round(nz_gene_mm,digits=1)),'%',sep=''), xpd=TRUE)\n")
@@ -956,7 +956,7 @@
- f.write('barplot(Fn_mm,main="Gene abundance (RPM)",xlab="Sample",ylab="Frequency",col=c("green","blue","red","yellow"),legend=xname)\n')
+ f.write('barplot(Fn_mm,main="Gene abundance (RPM)",xlab="Sample",ylab="Frequency",col=c("green","blue","red","yellow"),legend=xname,las=2)\n')
f.write("dev.state = dev.off()\n")
@@ -1022,7 +1022,7 @@
- f.write('barplot(Fn_mm,xlab="Sample",main="Mapping Quality",ylim=c(0,1),ylab="Frequency",col=c("blue","green","yellow","orange","red"),legend=xname)\n')
+ f.write('barplot(Fn_mm,xlab="Sample",main="Mapping Quality",ylim=c(0,1),ylab="Frequency",col=c("blue","green","yellow","orange","red"),legend=xname,las=2)\n')
f.write("dev.state = dev.off()\n")
diff -r 82bb8c455761 -r 6610eedd9fae ezBAMQC/setup.py
--- a/ezBAMQC/setup.py Wed Mar 30 12:03:10 2016 -0400
+++ b/ezBAMQC/setup.py Wed Mar 30 12:11:46 2016 -0400
@@ -89,28 +89,28 @@
sys.exit()
BAMQC_HEADER = [
- 'src/bamqc/Constants.h',
- 'src/bamqc/Coverage_prof.h',
- 'src/bamqc/GeneFeatures.h',
- 'src/bamqc/InnerDist_prof.h',
- 'src/bamqc/IntervalTree.h',
- 'src/bamqc/Mappability.h',
- 'src/bamqc/parseBAM.h',
- 'src/bamqc/ReadDup_prof.h',
- 'src/bamqc/Results.h',
- 'src/bamqc/rRNA.h'
+ 'src/ezBAMQC/Constants.h',
+ 'src/ezBAMQC/Coverage_prof.h',
+ 'src/ezBAMQC/GeneFeatures.h',
+ 'src/ezBAMQC/InnerDist_prof.h',
+ 'src/ezBAMQC/IntervalTree.h',
+ 'src/ezBAMQC/Mappability.h',
+ 'src/ezBAMQC/parseBAM.h',
+ 'src/ezBAMQC/ReadDup_prof.h',
+ 'src/ezBAMQC/Results.h',
+ 'src/ezBAMQC/rRNA.h'
]
BAMQC_SOURCE = [
- 'src/bamqc/Coverage_prof.cpp',
- 'src/bamqc/GeneFeatures.cpp',
- 'src/bamqc/InnerDist_prof.cpp',
- 'src/bamqc/IntervalTree.cpp',
- 'src/bamqc/Mappability.cpp',
- 'src/bamqc/parseBAM.cpp',
- 'src/bamqc/ReadDup_prof.cpp',
- 'src/bamqc/Results.cpp',
- 'src/bamqc/rRNA.cpp'
+ 'src/ezBAMQC/Coverage_prof.cpp',
+ 'src/ezBAMQC/GeneFeatures.cpp',
+ 'src/ezBAMQC/InnerDist_prof.cpp',
+ 'src/ezBAMQC/IntervalTree.cpp',
+ 'src/ezBAMQC/Mappability.cpp',
+ 'src/ezBAMQC/parseBAM.cpp',
+ 'src/ezBAMQC/ReadDup_prof.cpp',
+ 'src/ezBAMQC/Results.cpp',
+ 'src/ezBAMQC/rRNA.cpp'
]
###TODO HAVE TO SPLIT INTO TWO AND MAKE THE A FILE
@@ -174,7 +174,7 @@
BAMqc_CFLAGS = ['-fpermissive','-O3','-std=c++11','-Wno-error=declaration-after-statement']
BAMqc_DFLAGS = [('_FILE_OFFSET_BITS','64'),('_LARGEFILE64_SOURCE',''),('_CURSES_LIB','1')]
BAMqc_INCLUDES = ['./src/htslib']
-BAMqc_HEADERS = ['./src/bamqc']
+BAMqc_HEADERS = ['./src/ezBAMQC']
BAMqc_EXTRA = ['build/lib.linux-x86_64-2.7/htslib.so']
htslib_CFLAGS = ['-Wno-error=declaration-after-statement']
@@ -182,7 +182,7 @@
htslib_DFLAGS = [('_FILE_OFFSET_BITS','64'),('_USE_KNETFILE','')]
setup(name = "ezBAMQC",
- version = "0.6.5",
+ version = "0.6.7",
description = 'Quality control tools for NGS alignment file',
keywords = 'Quality control BAM file',
# make sure to add all the nessacary requires
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--- a/tool_data_table_conf.xml.sample Wed Mar 30 12:03:10 2016 -0400
+++ /dev/null Thu Jan 01 00:00:00 1970 +0000
@@ -1,12 +0,0 @@
-cat
-
-
- value, name, dbkey, id
-
-
-
-
- value, name, dbkey, id
-
-
-
\ No newline at end of file