I am performing plasmid DNA extraction using the akaline lysis method as described by a lab below (attached file). I wonder if I need to do any additional steps if I dissolve the extracted DNA sample in TE-RNAase pH8.0 buffer? Is there anything to note when preparing the solution?
Michael J. Benedik
No additional steps, the DNA should dissolve readily. Sometimes you end up with a bit of insoluble crud that is cell debris. Just mix the solution well with the pellet and the DNA will dissolve and any undissolved junk after a bit of time can be centrrigured down and ignored.
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