How to deal with Bubble Library for sequencing?

09 May 2022 1 7K Report

Hi all,

1. How do you identify if you have bubble library or just insufficient size selection?

2. How to deal with bubble library? Would reconditioning PCR work? Is it recommended to use single primer or both forward and reverse primers?

3. How to quantify bubble library for library pooling? qPCR? How?

Thanks.

Lux

C. Kiran

Heat the libraries for 3-5 mins in 90'c and recheck the QC. Concentration will decrease if it is bubble libraries.

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