Team:University of Ottawa/25 June 2008

From 2008.igem.org

Revision as of 17:54, 30 June 2008

Today in the Lab

Matt

PCR Amplification

F60, F61 primers used for PTP2 cassette. I also labelled all the primers we received that we will be using for the next few months.

I decided to use the Kaern Lab protocol for PCR Amplification.

The PTP2 PCR product was then run on a gel - gel results were as expected with 2275 size band.

Glycerol Stock

Glycerol stock of plasmids D12, S1, T123, pSS042 with LB + glycerol was performed.

Dan

Ran gel of pSSA42, S1, D12, T123 plasmids

This time the marker was added and expected results were obtained. SB, DA, TB, and 42B colonies were chosen for glycerol stock.

Cleaned out DNA box

Cleaned out all DNA that will not be used from our box

Our names are getting complicated so I am renaming our DNA using the following legend (all other DNA was discarded)

Plasmid	Strain	New Name
587	7B	7
598	8B	8
600	0A	0
601	1C	1
S1	SB	S
D12	DA	D
T123	TB	T
pSSA42	42B	42

PCR amplification of S, D, T, 7 and 8

S, D, and T plasmids were PCR amplified using primers F69 and F70

The 0 and 1 plasmids were amplified according to the following chart: (Primer F66 is :Int TetR Repl F (*PstI) (B). primer F67 is Int GFP Repl F(*SphI) (A), and primer F68 is:Int SSRE R(*ClaI )

Sample	F66	F67	F68
0A		Y	Y
1A		Y	Y
0B	Y		Y
1B	Y		Y

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