Bam to RPM Bedgraph Conversion
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6.7 years ago

I want to convert my ChIP-seq bam files to an RPM bedgraph file. I want to use the following command:

bedtools genomecov -bg -split -scale 1000000 -trackline -trackopts “name=bam_file_name description=bam_file” -ibam bamfilename > bedgraphfilename

I want to clarify that, for an rpm file, I should use the value one million following the "-scale"? Or should the scale factor be 6 because it assumes a 10 base?

Thanks in advance!

ChIP-Seq • 4.2k views
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I tried the scaling factor command and receive the following output: (standard_in) 1: illegal character: \342 (standard_in) 1: illegal character: \200 (standard_in) 1: illegal character: \234 -bash: 1000000/10743694": No such file or directory

I checked the spacing between all the parts of the command and they are correct. Does anyone know what I am doing wrong?

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6.7 years ago
ATpoint 85k

The value of -scale is the one that each value in column 4 of the bg is multiplied with, means you have to calculate the scaling factor externally. Here is a two-liner that can do it:

 ## Scaling factor for single-end data, counting every mapped read (bitwise flag = 0)
 TmpScale=$(bc <<< "scale=6;1000000/$(samtools view -f 0 -c in.bam)")

 ## Now get the actual bedGraph:
 echo '==> RPM scaling factor:' $TmpScale
 bedtools genomecov -bga -ibam in.bam -scale $TmpScale | sort -k1,1 -k2,2n > out.bedGraph

For matters of completeness, there are tools that can output a RPM-normalized bedGraph or bigwig in one go, like deeptools bamCoverage. Still, both genomecov and deeptools are pretty slow. There is a newer tool, mosdepth, which outputs a compressed bedGraph and is lightning fast. The RPM-normalization can be done using something like awk once the bedGraph has been generated.

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Thank you for your reply.

1) Do I need to download specific packages to carry out these commands? 2) Can I just lift over these commands, or are all the arrow characters you've used unimportant?

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Would it be possible for you to explain what exactly your first command is doing?

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It counts total number of mapped reads in the bam file, and uses it to calculate a per-million scaling factor. Still, I recommend deeptools bamCoverage for creating browser tracks. Is offers many options that are quiet convinient.

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Thanks, makes sense. Last question: how would it work for paired-end data?

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Thinking about it again, for single end, I would probably do -f 0 -F 256 (read mapped, and not supplementary alignment), and for paired, -f 1 -F 256 (read paired, but not supplementary). Bitwise flags explained here.

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Sorry to bother you again, but do you happen to know if bamCoverage requires for your input Bam file to be sorted? It doesn't look like but I can't seem to find a definitive answer anywhere.. It definitely seems to want a .bai to be present in the same directory as your bam file.

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It requires indexed BAM, and indexing requires sorted BAM, so yes bamCoverage requires sorted BAM. Use samtools sort to sort your bam and then samtools index to index the sorted bam.

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