Team:University of Ottawa/23 July 2008

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Latest revision as of 18:34, 7 August 2008

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Today in the lab

Dan

PCR amplification of T123

I wanted to do PCR amplification of 0A and 0B, however PCR blocks were full, I will do this tomorrow

6 tubes of PCR reaction were prepared for T123, hopefuly this will give me the amount of DNA that I need for a successful ligation.

Transformation of p2S and p2D

p2S and p2D were transformed in E. coli

Chris

Minipreparation of AtCRE

Used minprep kit and protocol to isolate AtCRE from inoculated cells.

Measured absorbance of resulting DNA samples to determine concentrations

Confirmation of AtCRE

Performed a digestion of AtCRE with EcoRI against a water control and a positive control (DQ2325601 digested with EcoRI)

Ran product on a 1% gel for 40 minutes at 80V

Two of six samples showed desired bands.

Matt

Ligation of PTP2 with pSSA42

Attempted another ligation of PTP2/pSSA42 this time with 1:1, 3:1, Vector with ligase, H2O, Vector without ligase.

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 __TOC__
 ==Today in the lab==
@@ Line 7: / Line 80: @@
 :'''Transformation of p2S and p2D'''
 ::<li>p2S and p2D were transformed in E. coli
+'''Chris'''
+:'''Minipreparation of AtCRE'''
+::<li> Used minprep kit and protocol to isolate AtCRE from inoculated cells.
+::<li> Measured absorbance of resulting DNA samples to determine concentrations
+:'''Confirmation of AtCRE'''
+::<li> Performed a digestion of AtCRE with EcoRI against a water control and a positive control (DQ2325601 digested with EcoRI)
+::<li> Ran product on a 1% gel for 40 minutes at 80V
+::<li> Two of six samples showed desired bands.
+'''Matt'''
+:'''Ligation of PTP2 with pSSA42'''
+::<li>Attempted another ligation of PTP2/pSSA42 this time with 1:1, 3:1, Vector with ligase, H2O, Vector without ligase.

Team:University of Ottawa/23 July 2008

From 2008.igem.org

Latest revision as of 18:34, 7 August 2008

Contents

Today in the lab