Team:Calgary/12 June 2009

From 2009.igem.org

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Friday Team Meeting
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Revision as of 05:12, 21 August 2009

University of Calgary

UNIVERSITY OF CALGARY



THIS MONTH

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NOTEBOOK PAGE INDEX
Carol
Chinmoyee
Emily
Fahd
Iman
Jamie
Jeremy
Katie
Kevin
Mandy
Patrick
Prima
Stefan
Vicki



CALENDAR

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JUNE 12, 2009


CAROL

Descriptive Title of What You’re Doing

WIKI CODING HERE

CHINMOYEE

Three Gene Repressilator Presentation

Presented Ander's Modeling examples of the Three Gene Repressilator .

Looked at the Optimization Toolbox:


EMILY

Friday Team Meeting

  • Had a team meeting where each subproject presented their recent work. Lab group talked about verification of genes of interest in TOPO vectors, BBK ampliciation PCR and cloning into Biobrick vectors (psB1AC3 and psB1AK3).


FAHD

Descriptive Title of What You're Doing

WIKI CODING HERE


IMAN

Descriptive Title of What You're Doing

WIKI CODING HERE


JAMIE

Descriptive Title of What You're Doing

WIKI CODING HERE


JEREMY

Descriptive Title of What You're Doing

WIKI CODING HERE


KATIE

Descriptive Title of What You're Doing

WIKI CODING HERE


KEVIN

Team meeting

No lab experiments were performed


MANDY

Descriptive Title of What You're Doing

WIKI CODING HERE


PATRICK

Descriptive Title of What You're Doing

WIKI CODING HERE


PRIMA

Descriptive Title of What You're Doing

WIKI CODING HERE


STEFAN

Descriptive Title of What You're Doing

WIKI CODING HERE


VICKI

Purification of gradient PCR product

Purpose: to purify the LuxOD47A BBk that was produced yesterday in the gradient PCR

Protocol: Please refer to the protocol page. Concentrations were measured after the product was purified.


Restriction digest of LuxOD47A BBk (insert) and psB1AC3 (vector)

Purpose: The LuxOD47A BBk DNA from yesterday’s gradient PCR is in linear form. This will prepare the ends so that it can be inserted into a BioBrick vector.

Protocol:

This is the restriction digest component of the construction protocol, which we describe on our protocol page. We attempted the construction with 2 different sets of enzymes: 6 tubes with cuts at XbaI and PstI , and 6 tubes with cuts at EcoRI and PstI. Both were prepared in REact 2 buffer. Once prepared, the tubes were left in the water bath at 37 degrees C for 6.5 hours; heatshocked at 65 degrees C on a heating block to deactivate the restriction enzymes in the tube; and placed in the -20 degrees C freezer.


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