Team:Yeshiva NYC/Notebook

From 2009.igem.org

(Difference between revisions)

Revision as of 04:06, 22 September 2009

Faige's Work:

May 26-June 2: Made LB-media agar plates with different antibiotics (Cam, Kan, and Amp); learned techniques

June 3: Received primers for leader sequences

June 4: Purified genomic XL1-Blue DNA

June 5-10: Unsuccessful PCR with 3 primers; digestion, ligation, and transformation (DLT) of 3 ccdB plasmid DNA

June 11: Miniprepped ccdB

June 12-19: Continued toggling with annealing temperatures for all 8 primers, 2 were successful!

June 22-24: DLT of ccdB with two successful leader sequence PCR reactions; DLT of RBS; DLT of promoter

June 25: Three-way DLT of RBS and promoter into ccdB plasmid

June 29: Received 6 long primers (for the 6 unsuccessful ones) and ran PCR with them, 4 were successful!

June 30-July 9: Resumed tweaking conditions for two remaining unsuccessful primers; DLT of 4 recently successful leader sequence PCR reactions, and three-way DLT of each of first 2 successful leader sequences with RBS/promoter into ccdB; DLT of RFP DNA; received RFP primers

July 10-14: Three-way DLT of the 4 later successes with RBS and promoter; three-way DLT of cytoslac with 2 earlier leader sequence/RBS/promoter

July 15: Ran PCR with RFP primers; tweaked conditions for unsuccessful ligation reactions

July 16-21: Three-way DLT of RFP and 1 earlier leader sequence/RBS/promoter; DLT of RFP DNA [as a simple Biobrick(BB)]; continued tweaking of previously unsuccessful DLTs; gel extraction of cytoslac digests (to remove resistance)

July 22-23: Transformation of RFP BBs into BL21 DE3 cells; Three-way DLT of RFP with other 5 successful leader sequence/RBS/promoter combinations; DLT of pure cytoslac with 4 recently successful leader sequence/RBS/promoter combinations; transformed 2 successful cytoslac/leader sequence/RBS/promoter combos into BL21 DE3 cells

July 24: Made 2XYT-media liquid cultures of BL21 DE3 cells and stimulated with IPTG; Also added IPTG to a plates of BL21 DE3 cells. No expression.

@@ Line 1: / Line 1: @@
 Faige's Work:
-May 26-June 2: Made agar plates with different antibiotics; learned techniques
+May 26-June 2: Made LB-media agar plates with different antibiotics (Cam, Kan, and Amp); learned techniques
 June 3: Received primers for leader sequences
@@ Line 7: / Line 7: @@
 June 4: Purified genomic XL1-Blue DNA
-June 5-10: Unsuccessful PCR of 3 primers; digestion, ligation, and transformation (DLT) of 3 ccdB plasmid DNA
+June 5-10: Unsuccessful PCR with 3 primers; digestion, ligation, and transformation (DLT) of 3 ccdB plasmid DNA
 June 11: Miniprepped ccdB
@@ Line 17: / Line 17: @@
 June 25: Three-way DLT of RBS and promoter into ccdB plasmid
-June 29: Received 6 long primers (for the 6 unsuccessful ones) and ran PCR on them, 4 were successful!
+June 29: Received 6 long primers (for the 6 unsuccessful ones) and ran PCR with them, 4 were successful!
 June 30-July 9: Resumed tweaking conditions for two remaining unsuccessful primers; DLT of 4 recently successful leader sequence PCR reactions, and three-way DLT of each of  first 2 successful leader sequences with RBS/promoter into ccdB; DLT of RFP DNA; received RFP primers
@@ Line 23: / Line 23: @@
 July 10-14: Three-way DLT of the 4 later successes with RBS and promoter; three-way DLT of cytoslac with 2 earlier leader sequence/RBS/promoter
-July 15: Ran PCR on RFP primers; tweaked conditions for unsuccessful ligation reactions
+July 15: Ran PCR with RFP primers; tweaked conditions for unsuccessful ligation reactions
 July 16-21: Three-way DLT of RFP and 1 earlier leader sequence/RBS/promoter; DLT of RFP DNA [as a simple Biobrick(BB)]; continued tweaking of previously unsuccessful DLTs; gel extraction of cytoslac digests (to remove resistance)