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**pbluescript** · 04-21-2011, 04:41 AM

It is due to overcycling your PCRs, so it could also be due to too much input. I have attached an example of two libraries where I tried different numbers of PCR cycles. The gel shows 6-18 cycles in 2-cycle steps from left to right. In this case, I took the 8 cycle libraries.
Here's another thread talking about this issue:

How to eliminate PE dimers from final product? - SEQanswers

http://seqanswers.com/forums/showthread.php?t=8894

Application of sequencing to RNA analysis (RNA-Seq, whole transcriptome, SAGE, expression analysis, novel organism mining, splice variants)

Attached Files

PCRovercycling.jpg (7.5 KB, 335 views)

**jlove** · 04-22-2011, 12:34 PM

Update: it was indeed over-cycling that created the problem. I believe that I was getting the amplicons partially hybridizing at the adapter regions and forming Ys which ran larger on the bioA. 10 cycles (vs 18) completely solved the problem. Thanks pbluescript for the ideas!

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TruSeq libraries - double sizing?

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