hi, I am performing DNA extraction from cervical swab using QIAGEN QIAAMP DNA MINI KIT and I am incubating my samples at 56c for 1 hour but the thing I am noticing is that I am not getting enough cell density after my PCR reaction. is it due to genomic DNA shearing or fault of my primer or I am not doing correct cell lysis?
kindly solve my query.
Mauricio de la Rosa-Garza
There are many things to consider before giving proper feedback.
It would help a lot if you first give us the following information:
1. What do you mean by cell density after PCR reaction?
2. If you are analyzing your PCR results through gel electrophoresis, a picture of the results with detailed information would be very helpful.
3. Are you evaluating DNA quantity/quality somehow? (e.g. nanodrop)
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