Matt Gethers/CRI, Thailand/Labwork/Isolating HmgR/Week of 6.16.08

=6.16.08=

The primers BT2736 and BT2737 arrived today. I added 277 and 315 &mu;l of TE to them respectively to create 100 &mu;M Stocks. I then diluted each 1 &mu;l in 99 &mu;l H20 to have my own 1 &mu;M stocks. I placed the TE stocks in the -20 in the latest box and I put my aliquots in my -20.

Now that I have the primers, I can plan to do the PCR. Here's the protocol. I should check if I'm still using Pfu (I think so).

=6.17.08=

To Do:


 * Run the PCR to amplify the HmgR ORF. If the other PCR worked, I can run both the Upstream fragment and HmgR amplification together because they both use the same annealing temp (55o).
 * Assuming the HmgR ORF PCR works, digest with NdeI and BamHI. I might as well run out on a gel to get rid of unwanted fragments.
 * Get pET-11a and digest with NdeI and BamHI to prepare for insertion of HmgR ORF.
 * Do a gel clean up of the excised bands.

=6.18.08=

To Do:
 * Try a gradient PCR for the annealing temperature for the amplification of the HmgR ORF.
 * What should be the temperature bounds? Try 50oC to 65oC (5 degrees below the annealing temp of the lower primer to well above the annealing temp of the higher primer).
 * Run the gradient PCR products on a gel to see if any products show up.
 * If bands show up, note the temperature and rerun the PCR with a larger volume at the best temperature (I can further optimize if I so choose).
 * If no bands show up, I should probably repeat the gradient PCR as my run was a little abnormal :-).

Summary:

The gradient PCR worked - actually, each annealing temperature worked and it doesn't seem that there's a particularly efficient temperature between 50 and 65 degrees. I excised the bands (8 of them with 5 &mu;l of product in each lane) and did a gel clean up, capturing everything on one column. Tomorrow I'll try digesting.

=6.19.08=

To Do:


 * Digest gel-extracted PCR product with NdeI and BamHI
 * Run out digested product on a gel, excise, gel purify.
 * Ligate digested product into pET-11a (already digested).
 * Transform into some cloning strain?
 * If the pET-11a doesn't allow for the Blue-White selection, how will I go about selecting colonies with the insert? Screening?

Summary:

I forgot I had the cultural orientation today, so everything is postponed until Friday.

=6.20.08=

To Do:


 * Digest gel-extracted PCR product with NdeI and BamHI
 * Run out digested product on a gel, excise, gel purify.
 * Ligate digested product into pET-11a (already digested).
 * Transform into DH5 &alpha;.
 * If the pET-11a doesn't allow for the Blue-White selection, how will I go about selecting colonies with the insert? Screening?

Summary:

Digestion, gel, and ligation complete. Also finished transformation. Placed plates in 37o incubator at 16:45.