Question

Quality control ChiP-Seq

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9.8 years ago

marina-orlova ▴ 90

Hello

I'm trying to improve quality of reads (ChiP-Seq, drosophila melanogaster).

Initially the quality was very bad

I tried using Trimmomatic with parameters TRAILING:20 and MINLEN:50

After that, per base quality became good.

Next, I searched for overrepresented sequences with BLAST and found out that most of them are from drosophila genome, others (such as GAAGAGAAGA, TTTTTTTTT etc.) - are not from it. Besides, these overrepresented sequences have much in common.

Please advise what I should do with overrepresented sequences - cut them or don't do anything.

ChIP-Seq QC trimming • 3.3k views

ADD COMMENT • link updated 2.3 years ago by Ram 43k • written 9.8 years ago by marina-orlova ▴ 90

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If those are not adapters, keep the overpresented sequences, but trim off the bad quality bases by Trimmomatic

ADD REPLY • link updated 2.3 years ago by Ram 43k • written 9.7 years ago by Ming Tommy Tang ★ 3.9k

Ram · Accepted Answer · 2014-07-12

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9.8 years ago

Devon Ryan 104k

Don't do anything unless they're adapters, which they probably aren't since you already trimmed things.

BTW, depending on what exactly was being IP'd, one might expect some highly overrepresented sequences (in fact, that might be the whole point of the experiment).

ADD COMMENT • link 9.8 years ago by Devon Ryan 104k

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So, do you think I should just start mapping in spite of the low quality showed by fastqc?

ADD REPLY • link updated 2.4 years ago by Ram 43k • written 9.8 years ago by marina-orlova ▴ 90

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You should always quality and adapter trim. Aside from that, just map the remaining reads.