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**dpryan** · 06-07-2012, 09:28 AM

For SNP calling you need to mark PCR duplicates. That works better with paired-end reads, so of the options I'd do 50bp paired-end. Paired-end reads will also be beneficial for mapping in general. You'll also be better able to differentiate isoforms with paired-end reads, if that's important to you.

**dhanapala** · 06-08-2012, 09:01 AM

Thanks dpryan

Since we have reference genome for Soybean

So do you mean the 50bp PE is good option and still all above four analysis can be done ?

How about the exon expression ? Is it possible too ?

**alexdobin** · 06-08-2012, 11:43 AM

I would recommend doing 2x100bp

Paired-end reads are preferred for de-convolution of isoform expression such as done by Cufflinks.
On the other hand, longer reads allow for much more accurate detection of the splice junctions.

**adaptivegenome** · 06-08-2012, 05:09 PM

PE first priority, longer reads second. Any reason you can't do 100?

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