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**nucacidhunter** · 09-23-2016, 11:44 PM

I think the problem is other modifications not the RT enzyme. Your reactions has produced the large transcript drived cDNA. You can get rid of smaller fragments by bead clean up.

Edit: RT enzyme contamination and alternatives has been discussed:

RNA-seq from single cells? - SEQanswers

http://seqanswers.com/forums/showthread.php?p=196705&highlight=single+cell+rnaseq#post196705

Techniques and protocol discussions on sample preparation, library generation, methods and ideas

**plyguy69** · 09-26-2016, 07:18 AM

Thanks Nucacidhunter

Those cDNA products shown were analyzed after one SPRI bead clean up. You're right I can remove the majority of the lower bp nonspecific products by a second bead clean up (have tried and it worked). We are just concerned about these products showing up in the new lots of Primescript and don't want to rush into HiSeq runs until we know for sure what's going on....

**nucacidhunter** · 09-26-2016, 02:05 PM

Looking at your negative control trace might give some idea about their origin.

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