Team:Caltech/week11

From 2014.igem.org

(Difference between revisions)

Latest revision as of 00:53, 15 September 2014

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Week Eleven
Monday, 8/25/14	lamBCDA & fsrABC Reception Systems agrBCDA Reception System and Combinatorial Promoters

Tuesday, 8/26/14	lamBCDA & fsrABC Reception Systems agrBCDA Reception System and Combinatorial Promoters

Wednesday, 8/27/14	lamBCDA & fsrABC Reception Systems agrBCDA Reception System and Combinatorial Promoters

Thursday, 8/28/14	lamBCDA & fsrABC Reception Systems agrBCDA Reception System and Combinatorial Promoters Re-ran a Gibson assembly of pAA009 Transformed Gibson products into JM109 cells

Friday, 8/29/14	lamBCDA & fsrABC Reception Systems agrBCDA Reception System and Combinatorial Promoters Picked 10 Gibson colonies from yesterday Ran colony PCR on re-suspended colonies, inoculated liquid cultures of picked colonies Ran gel of colony PCR products, but no good bands were obtained

Saturday, 8/30/14	Export Systems Redo of cloning of agr system: Ran PCR reactions to construct appropriate backbone for pTG002 & modified gblock insert for pTG002. DpnI digested PCR product for pTG002 backbone. PCR purified DpnI digested pTG002 backbone and pTG002 modified gblock insert PCR products. Ran purified products on a gel. Ran Gibson assembly reaction between pTG002-backbone & pTG002-insert. Transformed Gibson reaction mix into JM109. Cells were then plated & incubated overnight. De-FLAGging pTG005 for LC/MS analysis: Ran PCR reaction to exclude 3xFLAG from pTG005. Ran DpnI digest and then PCR purification on PCR product. Ran PCR product on a gel to verify creation of the appropriate DNA fragment. Ran a round-the-horn ligation reaction on the purified PCR product. Transformed the reaction mix into JM109. Cells were then plated & incubated overnight.

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-Redo of cloning of agr system:
+<br>Redo of cloning of agr system:
-<ul><li>
+<ul><li>Ran PCR reactions to construct appropriate backbone for pTG002 & modified gblock insert for pTG002.</li>
+    <li>DpnI digested PCR product for pTG002 backbone.</li>
+    <li>PCR purified DpnI digested pTG002 backbone and pTG002 modified gblock insert PCR products.</li>
+    <li>Ran purified products on a gel.</li>
+    <li>Ran Gibson assembly reaction between pTG002-backbone & pTG002-insert.</li>
+    <li>Transformed Gibson reaction mix into JM109. Cells were then plated & incubated overnight.</li>
+</ul>
+De-FLAGging pTG005 for LC/MS analysis:
+<ul><li>Ran PCR reaction to exclude 3xFLAG from pTG005.</li>
+    <li>Ran DpnI digest and then PCR purification on PCR product.</li>
+    <li>Ran PCR product on a gel to verify creation of the appropriate DNA fragment.</li>
+    <li>Ran a round-the-horn ligation reaction on the purified PCR product.</li>
+    <li>Transformed the reaction mix into JM109. Cells were then plated & incubated overnight.</li>
 </ul>
 </td>

Team:Caltech/week11

From 2014.igem.org

Latest revision as of 00:53, 15 September 2014

Week Eleven

Monday, 8/25/14

Tuesday, 8/26/14

Wednesday, 8/27/14

Thursday, 8/28/14

Friday, 8/29/14

Saturday, 8/30/14