I made amplification of ITStotal. There was no problem with fresh leaves: I got app. 750 bp very bright bands, however with old herbarium specimens I met some other 800 bp and 1000bp bands beside 750 bp very bright band. Is this a problem for sequencing? if so what can I do to fix it?
Nor Aziyah MatRahim
Hi Burcu,
If your interest is to do sequencing, I guess that should not be a problem, since your fragment of interest is there. But you have to cut the 750 bp and do gel extraction procedure to extract the DNA from the agarose. For your case, you cannot use PCR purification because it will further extract the unwanted 800bp and 1000 bp.
Good luck!
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