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**jteeee2** · 06-10-2016, 04:31 AM

Could you please attach Bioanalyzer traces of your pre and post capture libraries? That information may help troubleshoot the issue.

**bsvega** · 06-10-2016, 06:13 AM

We use QIAxcell instead of bioanalyzer. I am attaching the files.

Attached Files

**jteeee2** · 06-10-2016, 06:57 AM

Thanks for attaching these. The only pertinent comment I have about the traces is that the average library size is a bit larger than we commonly see for captures. Was genomic DNA used as the starting material?

The NextSeq can typically handle fragments of that size with no problem, however. You simply see a significant bias towards smaller fragments being able to cluster effectively. One thing we have seen with Agilent capture libraries is the presence of a poly-G tract at the beginning of the read that can really screw up the NextSeq's base calling software. How does the base diversity look on the run? Are you seeing high "G" calls anywhere?

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low clustering for Sureselect exome v6 on NextSeq

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