Number Of Reads In A Sam File Which Are Assigned To Each Chromosome?
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13.0 years ago
KCC ★ 4.1k

Given a sam file which was produced by using bwa to align a fastq of reads to a reference genome, how can I enumerate the number of reads which were assigned to each chromosome of the reference genome?

alignment sam • 31k views
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13
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13.0 years ago

Your question refers to SAM format, but in the event that you may also have a sorted/indexed BAM, you can simply do the following to get this very quickly.

samtools idxstats aln.bam | cut -f 1,3
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9.9 years ago

The solution based on samtools idxstats aln.bam should be used with caution. This is because AFAIK the numbers reported by samtools idxstats (& flagstat) represent the number of alignments of reads that are mapped to chromosomes, not the (non-redundant) number of reads, as stated in the documentation. I stumbled across this by observing that the total numbers reported by samtools idxstats (& flagstat) exceeded the total number of reads in my input fastq files. See further discussion on this issue in the comments on this post: http://left.subtree.org/2012/04/13/counting-the-number-of-reads-in-a-bam-file/

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Incidentally, I wrote a program that calculates read coverage from a sam file (number of reads mapped to each sequence, average depth, median depth, standard deviation, fraction of bases covered, etc).

pileup.sh in=mapped.sam out=coverage.txt

It has a toggle for including or ignoring secondary alignments; secondary=false or secondary=true (default).

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When generating your SAM file make sure it has the header section before using pileup.sh.

samtools view -h file.bam > file.sam

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Example pipe with filtering:

cat file.bam | samtools view -h -F 0x4 -F 0x100 | samtools idxstats -  |  cut -f 1,3
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Brian, I'd be interested to read the source code of your program, but your link is broken. Could I ask you to provide a new link?

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Sometimes Sourceforge goes down for a few hours for maintenance, or something. I put the latest version (35.14) on my Google drive; please let me know if you still have trouble accessing it.

https://drive.google.com/file/d/0B3llHR93L14wTzZSMjZvdjdmYzg/view?usp=sharing

The source code for pileup.sh is mainly in /bbmap/current/jgi/CoveragePileup.java

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13.0 years ago

based on the first column only:

awk ' $1 !~ /@/ {print $1}' toy.sam | uniq -c

if you want to count only aligned reads you can also use awk to count only aligned reads.

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Won't $1 denote the query name? $3 is the chrom

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Oops that's right

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Oops, you're correct.

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9.3 years ago
Kamil ★ 2.3k

Here's how I count the number per sequence of primary alignments with proper read pairs:

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3.6 years ago

Now there is a more convenient way with seqkit bam:

seqkit bam -C mybam.bam
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7.1 years ago

This is the Samtools Solution + bash

Enjoy

PROCESSORS=10
BAM=blah.bam | blah.sam

samtools view --threads $PROCESSORS $BAM | cut -f 3 | sort | uniq -c | sort -nr | sed -e 's/^ *//;s/ /\t/' | awk 'OFS="\t" {print $2,$1}' | sort -n -k1,1 > Chr_freqs.txt
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