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**cmbetts** · 08-07-2017, 09:33 AM

There's a couple reasons not to worry about it, but the primary ones are:
1) The denaturation temperature before RT isn't high enough to melt high MW gDNA
2) Even if gDNA was primed, the template switching mechanism requires the RT to hit a 5' end and neither the RT nor the PCR polymerase are anywhere processive enough to worry about capturing whole chromosomes.

**jteeee2** · 08-08-2017, 08:37 AM

If you're really interested DNase treating, we have had good success incorporating this product into the front end of several RNA Seq protocols (including SmartSeq). http://arcticzymes.com/technology/kits/heat-and-run/

We have seen that significant DNA contamination can affect the quality of the SmartSeq library, so I think it's definitely worth considering.

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DNase treatment for SMART Seq2

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