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**steven** · 03-18-2010, 11:06 AM

?! strange indeed!
statistical significance may be an important point here.. is the bias constant across chromosomes?
s.

**bioinfosm** · 03-18-2010, 12:33 PM

What aligner are you using? Probably you could use a different one and see what happens to the bias

**maubp** · 03-19-2010, 03:20 AM

I'd also suggest taking your references and reverse complementing them. Then repeat the alignment on the RC reference and see what happens. If this is just a software artefact, then you should see more reads on the new forward strand (i.e. what was the reverse strand in the original reference).

**steven** · 03-22-2010, 01:56 AM

My bet would be a single genomic position (on the forward strand) that gets a gazillion of copies of a single read (generated by a contaminant, an amplification artifact, an incorrect filter, or something else).

**steven** · 04-05-2010, 05:42 AM

Originally posted by dawe View Post

Hi all,
this may be something known... anyway, tags coming from Illumina sequencing method (GA II here) seem to map preferentially on forward strand... I haven't check if there is a statistically significant variation, but apparently tags aligned on forward strand are 2-5% more (in various ChIP-seq and also in genome resequencing).
I wonder which could be the source of this variation... The library prep? The cluster generation? The aligner? None of these steps makes sense to me...

d

Hi,
any news regarding this issue?
thanks,
s.

**dawe** · 04-05-2010, 07:00 AM

Originally posted by steven View Post

Hi,
any news regarding this issue?
thanks,
s.

Not yet... I've been busy on other issue but I will investigate this further...

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Forward strand bias?

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