Team:Penn State/Notebook

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<h1 style="color: green"> Cas9 Project</h1>
<h1 style="color: green"> Cas9 Project</h1>
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<p style="color: green; "><b>June 23-29</b></p>
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<p>PCR amplification of NOS 1 and NOS 2 terminators from pmdc107. PCR amplification of GFP, NOS 3, CMV35s, CMV35s(2), and mCherry. All PCR products were gel extracted and then PCR amplified again.</p>
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<p style="color: green; "><b>June 30-July 6</b></p>
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<p>PCR amplification of mCherry again from pNigel7 for higher yields, then it was gel extracted. Picked colonies and grew cultures of bacteria containing pMDC107. </p>
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<p style="color: green; "><b>July 7-13</b></p>
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<p>Miniprep of bacteria containing pmdc107 and pNigel7, made save cultures of both. Ran gradient PCR of mCherry due to it’s failure the first tries. </p>
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<p style="color: green; "><b>July 14-20</b></p>
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<p>Gradient PCR for NOS 2 terminator then a “band stab” PCR from the band in the gel. PCR amplification of Actin 8. PCR amplification of GFP, Nos1, and Nos2 from newer pmdc107.</p>
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<p style="color: green; "><b>July 21-27</b></p>
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<p>Having trouble isolating mCherry still, PCR with taq polymerase and phusion polymerase to eliminate factors. Also, PCR of Nos2 with taq polymerase for same reasons as mCherry. PCR amplification of dCas9 with phusion polymerase.</p>
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<p style="color: green; "><b>July 28- Aug 3</b></p>
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<p>PCR amplification of dCas9 from the band last week, in addition to starting from plasmid DNA. Tried again with lower annealing temperatures. They were successful and the bands were then gel extracted. At this point all of the components have been isolated and PCR amplified to our specifications. </p>
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<p style="color: green; "><b>Aug 4-10</b></p>
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<p>Calculations were started for a Gibson Assembly for all of the components. In addition, dCas9 was PCR amplified again using different annealing temperatures and again using different DNA. Two CBAR’s were ran to assemble CMV35s, GFP, Nos1, Nos2, CMV35s(2), mCherry, and Nos3. It was unsuccessful and more calculations were done to troubleshoot the problem.</p>
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<p style="color: green; "><b>Aug 11-17</b></p>
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<p>Tried smaller Gibson Assemblies putting together CMV35s with GFP, Nos1 with Nos2, and CMV35s(2) with mcherry and Nos3. All three CBAR’s were successful and were rescue PCR amplified. Then, CBAR of g-blocks for viral promoters, all were successful and also rescue PCR amplified. PCR amplification of Actin, Myosin, Profilin from the Arabidopsis thaliana genome.</p>
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<p style="color: green; "><b>Aug 18-24</b></p>
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<p>PCR products were all ran on a gel and only 2 viral promoters and the Actin, Myosin, and Profilin were successful.</p>
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<p>**From here the Project switched focus from Cas9 to the promoter project for consolidation purposes and time constraints**</p>
<h1 style="color: green"> Promoter Project</h1>
<h1 style="color: green"> Promoter Project</h1>

Revision as of 18:27, 27 September 2013

Cas9 Project

June 23-29

PCR amplification of NOS 1 and NOS 2 terminators from pmdc107. PCR amplification of GFP, NOS 3, CMV35s, CMV35s(2), and mCherry. All PCR products were gel extracted and then PCR amplified again.

June 30-July 6

PCR amplification of mCherry again from pNigel7 for higher yields, then it was gel extracted. Picked colonies and grew cultures of bacteria containing pMDC107.

July 7-13

Miniprep of bacteria containing pmdc107 and pNigel7, made save cultures of both. Ran gradient PCR of mCherry due to it’s failure the first tries.

July 14-20

Gradient PCR for NOS 2 terminator then a “band stab” PCR from the band in the gel. PCR amplification of Actin 8. PCR amplification of GFP, Nos1, and Nos2 from newer pmdc107.

July 21-27

Having trouble isolating mCherry still, PCR with taq polymerase and phusion polymerase to eliminate factors. Also, PCR of Nos2 with taq polymerase for same reasons as mCherry. PCR amplification of dCas9 with phusion polymerase.

July 28- Aug 3

PCR amplification of dCas9 from the band last week, in addition to starting from plasmid DNA. Tried again with lower annealing temperatures. They were successful and the bands were then gel extracted. At this point all of the components have been isolated and PCR amplified to our specifications.

Aug 4-10

Calculations were started for a Gibson Assembly for all of the components. In addition, dCas9 was PCR amplified again using different annealing temperatures and again using different DNA. Two CBAR’s were ran to assemble CMV35s, GFP, Nos1, Nos2, CMV35s(2), mCherry, and Nos3. It was unsuccessful and more calculations were done to troubleshoot the problem.

Aug 11-17

Tried smaller Gibson Assemblies putting together CMV35s with GFP, Nos1 with Nos2, and CMV35s(2) with mcherry and Nos3. All three CBAR’s were successful and were rescue PCR amplified. Then, CBAR of g-blocks for viral promoters, all were successful and also rescue PCR amplified. PCR amplification of Actin, Myosin, Profilin from the Arabidopsis thaliana genome.

Aug 18-24

PCR products were all ran on a gel and only 2 viral promoters and the Actin, Myosin, and Profilin were successful.

**From here the Project switched focus from Cas9 to the promoter project for consolidation purposes and time constraints**

Promoter Project

**The components of this project are the same as those in Cas9 and because of this, the notebook starts in August**

Aug 11-17

Re-isolated cytoskeletal promoter, Actin, from Arabidopsis thaliana genome. Actin was unsuccessful so it was PCR amplified again. A genomic isolation was performed from Arabidopsis leaves. Gel extractions of Myosin, Actin, MMV, and ClCuV.

Aug 18-24

PCR of myosin and profilin were both successful. CBAR 1 and CBAR 2 were performed again as described in cas9 notebook. In addition, FiMV promoter was put together again with CBAR. All were successful except the CBAR’s that were rescue PCR amplified. It was determined that the annealing temperatures were not compatible for CBAR 1 and 2 amplification so new primers were ordered. FiMV was successfully PCR amplified and was gel extracted. An intermediate CBAR of CMV35s(2) with mCherry (CBAR 3.5) was conducted and successfully amplified. Each component of the construct was CBARed again successfully and a CBAR of those parts was conducted to assemble the entire construct. It was unsuccessful.

Aug 25-31

More intermediate CBAR’s were conducted to piece together CBAR 1 with CBAR 2 from above, named CA. Also, CBAR 3.5 and Nos3 were joined together and named CB. Both attempts were unsuccessful and were tried again.

Sept 1-7

Began biobrick assembly by PCR amplifying Actin, Profilin, ClCuV, MMV, CesA 7, CesA 8, and Myosin with new primers that had the correct restriction enzymes on them. Continuation of trying for successful CBAR reactions with a series of new calculations, new primers, and new annealing temperatures during rescue PCR.

Sept 8-14

Restriction enzyme digest of all of the biobrick components and pSB1C3. The was some success with CBAR 1 and CBAR 3.5, but nothing could be amplified to standards.

Sept 15-21

Biobrick parts were individually ligated into vectors and transformed. Colonies were picked, cultures were grown and mini prepped to be sent to sequencing. Continued to troubleshoot CBAR reactions and look into a different method for assembly.

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