Question

ChIP-seq reads trimming

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24 days ago

SEJAL • 0

ERROR: sequence and quality have different length:
@SRR16684719.6426858 6426858/1
CCCCTTCCTTTCTTTTTTGAGTTGGAGTTTCACTCTTGTTGCCCAGTCTGA
+
FFFFFFFFFF,FFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFF

I am trimming the fastq files with fastp, and it is showing this error, the file size after trimming is also very less as compared to the raw untrimmed fastq files. How can this be corrected? I have also tried aligning the files (using bowtie2) without trimming and it shows up the same error in the alignment output.

trimming chipseq fastp alignment bowtie2 • 403 views

ADD COMMENT • link updated 23 days ago by GenoMax 147k • written 24 days ago by SEJAL • 0

score 0 · Answer 1 · 2024-11-03

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23 days ago

GenoMax 147k

Looks like your data file is corrupt. Either download a new copy if you can or you will need to use something to remove these reads.

ADD COMMENT • link 23 days ago by GenoMax 147k

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I have tried downloading the file again and running the alignment, it shows the same error. Also, it is for many fastq files. Is there a tool to remove such reads from fastq files?

ADD REPLY • link 23 days ago by SEJAL • 0

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You can use one of the tools mentioned in this thread: is there a tool to recover corrupted fastq files

If you have a large number of fastq records getting removed then you really should be very careful. Removing a large number of sequences could make the data invalid.

ADD REPLY • link 23 days ago by GenoMax 147k