Last night I designed and ordered the two complex primers I'll need to amplify and insert the SpcR gene. They won't get here until Monday, so today I did column and agarose-gel cleanups on the two other PCR fragments I'll be using
First I pooled what was left of the two PCR reactions (A and B). The volume of each was about equal to the amount I had run in my gel yesterday (left panel below). Then I did a column cleanup to get rid fo the bulk of the PPCR primers, using an old EconoSpin column that I'd revived by passing 0.2 N NaOH through it.
Then I ran all of the eluate from that column in one lane of a 1.2% agarose gel. I used only about 1/5 of the usual concentration of Ethidium Bromide, and I viewed the gel only with our hand-held long-wave UV lamp to avoid UV damage to the DNA. The bands were faint but clear and I cut them out together in one gel slice.
Then I used our new Zymoclean gel-recovery kit to dissolve the agarose and recover the DNA, and ran 3 µl of the resulting 24 µl in unused lanes of the same gel I used yesterday, to see how much DNA I had recovered.
The results look great. The bands are sharp and bright and the right sizes, and the intensities suggest that I've recovered most and perhaps all of the DNA I began with. So now this prep is in the fridge, waiting for the other piece of the construct.
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in The Biology Files
Not your typical science blog, but an 'open science' research blog. Watch me fumbling my way towards understanding how and why bacteria take up DNA, and getting distracted by other cool questions.
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