Normalising ChIP-seq data to RPM using a 1 or 2 count for paired-end data?
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9.9 years ago
James Ashmore ★ 3.5k

I want to normalise my paired-end ChIP-seq data (4 samples treated, 4 samples control) to reads per million (RPM). So far my calculation takes the number of reads mapped to a position, divides it by the total number of mapped reads in the sample, and then multiples this by one million. My question is, should the number of mapped paired-end reads be counted as 1 or 2 in the calculation? I believe Samtools reports the total number of mapped reads as half the actual number of paired-end reads which map?

My current pseudo script for normalising to RPM:

  • mappedReads = samtools view -c -F 4 input.bam
  • scalingFactor = 1000000 / mappedReads
  • bedtools genomecov -ibam input.bam -bg - scale scalingFactor -g chrom.sizes > output.bedGraph
  • bedGraphToBigWig input.bedGraph chrom.sizes output.bigWig
ChIP-Seq normalisation paired-end • 11k views
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For paired end data, rpm=fpm (fragments per million). So, it should be counted as one.

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Just to clarify, you are saying that each pair of reads should be counted as just one? So in a perfect world where 100% of my reads align, the number of total alignments would be half the total number of reads in the data?

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Yup. Count a pair of reads as one. For single end reads each read represents a fragment it is sequenced from whereas for paired-end, a pair of sequence represents the fragment it is sequenced from. As simple as that.

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9.9 years ago
Fidel ★ 2.0k

You can use deepTools to do the normalisation that you want. The output is a bigwig file. It is quite fast if you have multiple cores.

bamCoverage -b file.bam --normalizeUsingRPKM -o file.bw

The program first extends the read to match the paired-end length before computing the coverage. I opted to count paired end reads as 2 and not as 1 to avoid a bias when a read is not properly paired which could be a significant fraction.

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Thank you for the suggestion, I used Bowtie2 to map my reads but indicated to remove discordant and mixed alignments, in this case counting each pair of reads as 1 would be preferred

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One option is to filter your bam file to include only the first mate, then use it with bamCompare. If all your reads are properly paired this should work.

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I just pushed a commit to github enabling bamCoverage to select reads based on the SAM flag. Now you can do something like this to get what you want:

bamCoverage -b file.bam --normalizeUsingRPKM -o file.bw --samFlag 64

--samFlag 64 means to select only the first mate.

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9.9 years ago
Manvendra Singh ★ 2.2k

I think each read should be counted as 1

or

you can try MAnorm for normalization if it suits for your analysis or comparisons

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Initially I just want to create a coverage track for the normalised data.

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Okay, I agree with Fidel

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9.9 years ago
Ian 6.1k

In case you do not already know MACS2 will generate coverage plots for the non-redundant fragments used in the analysis (by default 1 unique fragment per strand) normalised to millions of reads using the --SPMR flag.

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I think MACS does not use the paired-end data to extend the reads. Does it extend the reads?

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MACS2 does not need to extend reads as it knows the start and end of the fragment by using the paired end reads information in the BAM file.

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For this you need to use the BAMPE mode of MACS2 which I am not sure it properly works. We tried it and didn't work, also I see numerous complains in the mailing list. Moreover, the bam file has to be sorted by name. I always use MACS2 for peak calling but not coverage tracks.

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