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**nilshomer** · 06-11-2011, 10:09 AM

Originally posted by guo View Post

Hi. everyone.

Should we transform the fastq file from solid2fastq (Bfast) before mapping with bwa?
I mean from "0123123" to "ACTGACT", something likewise plus some other format issues?

Before, I proced without any transformation, then got malformed .sai file and some "segmentation fault" which I haven't specified yet.

Any suggestions? Thank you

Make sure you use the solid2fastq within BWA if you are going to use BWA. On the other hand, if you are using bfast+bwa, make sure you see the command line parameters in BFAST's solid2fastq.

**nilshomer** · 09-03-2011, 05:20 AM

Originally posted by NanYu View Post

I'm wondering in the postprocess step, if BFAST will do something like: choose the best for F and second best for R within a pair because that is within the expected distance, yet the best for R is in another chromsome.
I know it is a rare scenario and maybe I should not worry about it.

It could happen when using the insert size distance in the probability calculation, though it is rare.

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