Question

RNA-seq different reads numbers of two samples is trouble?

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2.9 years ago

szp770 ▴ 10

Hi, for RNA-seq analysis, I did experiments for two samples, each with two repeats, sample1(both repeat1 and repeat2) have 70M raw reads, but sample2(both repeat1 and repeat2) only have 30M raw reads, so for the differential analysis, is it a trouble? Thanks!

RNA-Seq R seq python linux • 652 views

ADD COMMENT • link updated 2.9 years ago by MatthewP ★ 1.4k • written 2.9 years ago by szp770 ▴ 10

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I think there are multiple factors you need to consider.

The treatment/Biological conditions (What if the treatment is impacting on global gene expression program)
RNA quantity/quality
prior to sequencing Number of cells (Maybe)
Sequencing depth
Alignment rate
Alignment to the specific genomic regions (What if the majority of reads are aligning to the other genomic regions and not on the exons)

etc. etc.

I would just give it try and check the results.

ADD REPLY • link 2.9 years ago by Nitin Narwade ★ 1.6k

score 0 · Answer 1 · 2021-06-01

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2.9 years ago

MatthewP ★ 1.4k

Different read depth(coverage) is not a problem for differential analysis, for example you can use DESeq2. But I would recommend to have at least 3 repeats each sample, not 2 repeats. Here I mean biology repeats.

ADD COMMENT • link 2.9 years ago by MatthewP ★ 1.4k