Revision as of 20:05, 30 July 2008

Untitled Document

Today in the lab

Chris

PCR Amplification of PTP2

Began running experimentation alongside Matt to increase chances of success

Ran 5 samples, including two water controls as per Cory's request.

Master mix: 50 uL Buffer, 5 uL dNTP, 12.5 uL F60 and F61, 2.5 uL DNA (at 25 ng/uL), 142.5 uL water.

Digestion of PSSA42

Ran five samples and one water control

Per tube: 3 uL water, 3 uL Buffer 3, 3 uL BSA, 1.5 uL XhoI and BamHI, 16 uL DNA template.

Incubated at 37 C for one hour

PCR Cleanup

Used PCR cleanup kit to purify PTP2

Measured absorbance of resulting DNA samples. The concentrations were found to be very low; PCR did not work. It was later determined that DNA template was not added, by accident.

PCR Amplification of PTP2

Ran PCR with same constraints as previously. Let run overnight.

Tammy and Dan

0.8% Agarose Gel Electrophoresis of T123 PCR Products

Each PCR reaction tube (50 μL) was divided into 2 and ran on 2 separate wells

Agarose Gel Extraction

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+='''Today in the lab'''=
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+=='''Chris'''==
 :'''PCR Amplification of PTP2'''
 ::<li> Began running experimentation alongside Matt to increase chances of success
@@ Line 86: / Line 158: @@
 :'''PCR Amplification of PTP2'''
 ::<li> Ran PCR with same constraints as previously. Let run overnight.
+=='''Tammy and Dan'''==
+:'''0.8% Agarose Gel Electrophoresis of T123 PCR Products'''
+::<li> Each PCR reaction tube (50 &mu;L) was divided into 2 and ran on 2 separate wells
+:'''Agarose Gel Extraction'''

Team:University of Ottawa/29 July 2008

From 2008.igem.org

Revision as of 20:05, 30 July 2008

Today in the lab

Contents

Chris

Tammy and Dan