I am capturing B cells from Lung tissue using LCM, and then isolating the DNA for various downstream assays. When I finish DNA isolation using the Qiamp mini kit, I am getting good quantity and quality of DNA. One thing I am doing is running a PCR on one of our known primer sets with my DNA samples. the primer set is around 500 bp and has not exhibited any bands after several attempts. I also ran a PCR on a primer set which is about 100 bp and this resulted in appropriate bands. Could this be because the DNA was fragmented during some part of the LCM process? Please let me know if anyone can help. Thanks!

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