STAR aligned reads minimum maping quality
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6.7 years ago
rob.costa1234 ▴ 310

I aligned RNAseq data with GRCH 37 and wonder what cut off of read quality is generally used when we perform downstream analysis. I know in HISAT2 generally read quality >20 is considered. I could not find any general rule of quality cutoff in STAR. Any suggestion?
RNA-Seq • 3.9k views
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when we perform downstream analysis.

I guess you are talking about differential expression analysis, but it doesn't hurt to be specific...

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6.7 years ago
GenoMax 147k

Take a look at this blog post by Dr. Simon Andrews and decide for yourself.

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6.7 years ago
caggtaagtat ★ 1.9k

Like mentioned in the blog post of genomax, I always go with the cutoff of 255, resulting in only uniquely mapped reads.
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