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**Jon_Keats** · 07-17-2013, 08:37 PM

what read length, not bad if 100mers

**JJP** · 07-18-2013, 01:19 AM

Sorry I knew I had forgotten to mention something, the reads have a length of 101.

**jp.** · 07-30-2013, 06:07 PM

Dear Jon
I have posted the same problem here;

tophat: option --read-gap-length not recognized? - SEQanswers

http://seqanswers.com/forums/showthread.php?p=112098#post112098

Discussion of next-gen sequencing related bioinformatics: resources, algorithms, open source efforts, etc

any solution ?

Originally posted by Jon_Keats View Post

what read length, not bad if 100mers

**rnastar** · 08-08-2013, 01:55 PM

I just finished running tophat on about 20 cancer samples and my concordant pair alignment rate ranged between 50-60% for 50 bp reads. Should I be worried? Will this have an impact on the downstream cufflinks/cuffdiff analysis?

**westerman** · 08-09-2013, 06:07 AM

I presume you are talking about *human* samples. The 50-60% rate is low. I suspect that since the samples are more-or-less uniform in their mapping rate then you won't have too many problems with cufflinks/cuffdiff aside from not having as much data to work with.

Did you run non-cancer controls? Or are those part of the "20" you mention above. How about replicates -- technical and biological?

**rnastar** · 08-12-2013, 06:08 AM

Yes, human samples. We did run non-cancer controls but they did not have this problem. What do you think this means? Is this more a reflection of biology or an indication of a technical issue? We do not have any technical replicates, only biological.

**westerman** · 08-12-2013, 09:16 AM

The lack of technical replicates is not a big concern -- although they can help troubleshooting usually the technical process is flawless. Although when problems do occur you really wish that you had technical reps. :-)

As for the question "is a 50-60% concordant rate normal for cancer samples when the non-cancer samples have a higher concordant rate?" ... I am going to have to skip on answering this. I simply do not have enough experience with human cancer samples to say one way or another. Cancer genome rearrangements can be widespread so may 50-60% if expected. Can anyone with more human experience chime in?

BTW: You may wish to make a new thread on this topic with the keywords "human"
and "cancer" in it. That might attract more knowledgeable people.

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