Team:University of Lethbridge/Notebook/GeneralLabOctober

From 2008.igem.org

(Difference between revisions)
m (Ocotber 10, 2008)
m (October 11, 2008)
Line 59: Line 59:
-Ran a gel of the reporter system plasmids that Munima Isolated yesterday to determine to outcome.
-Ran a gel of the reporter system plasmids that Munima Isolated yesterday to determine to outcome.
 +
 +
[[Image:Reporter(Oct11).jpg| 250 px]]
-Set up a Restriction Digest of the Reporter System Parts. pLacI is cut with SpeI and PstI, RFP sub and TetR sub are cut with XbaI and PstI.
-Set up a Restriction Digest of the Reporter System Parts. pLacI is cut with SpeI and PstI, RFP sub and TetR sub are cut with XbaI and PstI.

Revision as of 19:25, 11 October 2008

Back to The University of Lethbridge Main Notebook

Contents

October 1, 2008

Roxanne

-Inactivated the Enzymes in the morning

-Ran a gel of the tested pLacI, along with the previously cut RFP and TetR in the afternoon on 1% Agarose Gel in TAE.

-the iGEM pLacI had a faint band, RFP looks good (half of it cut), TetR looks like it either didn't cut at all, or only cut once. Only used 2 uL for each sample, will try running with more.

October 4, 2008

Roxanne

-Reran the pLacI tests, RFP and TetR on a 1% Agarose Gel in TAE.

-Repicked pLacI x2, RFP and TetR colonies into LB+amp media since I've been having trouble with ligations. Brent suggested using lots of DNA in the ligation (<100 ng) to make ure that the ligation does in fact work this time.

Argh.jpg


October 5, 2008

Roxanne

-plasmid prepped the pLacI x2, RFP and TetR subcultures. Lost one of the pLacI cultures (cells wouldn't lyse). Had some left over pLacI - 2 culture, attempted to plasmid prep those cells.

-Ran a gel of the plasmid preps.

-Restriction Digest the pLacI - 1, RFP and TetR plasmids obtained today, as well as recutting the TetR plasmid from last time, since it appears as though it didn't cut at all, or only cut once. I will be using the iGEM enzymes. Left to cut overnight at 37.0C

-picked some pLacI colonies from a different plate. Maybe I'll have better luck there. Incubate in LB+amp media at 37.0C for 15 hours.

Oct5gel.jpg

Ocotber 6, 2008

Roxanne

-Running a gel of the parts which were Restriction Digested yesterday.

-Plasmid Prepping the new pLacI subcultures which were incubated overnight.

-Run a gel of the plasmid prep.

Oct6.jpg 2xOct6.jpg

-Yay!!!! The Enzymes Work!!!

Christa, Munima

Made 68 LB + Amp (100 ug/mL) plates and stored them in the iGEM 4 C fridge.

Made 72 5 mL culture tubes of LB liquid media. Stored in the iGEM glass cabinet.


October 10, 2008

Munima

Objective: Isolate more plasmids for continued work on the reporter system.

Plasmid prepped 3 mL of culture for various plasmids for the reporter system: pLacI, TetR sub, pLacI-3, RFP sub, and GFP sub. They are labelled with their name and today's date in 1.5 mL microfuge tubes (50 uL of elution solution). They are stored in the "iGEM Plasmids" box in the -20 C freezer.

October 11, 2008

Roxanne

-Ran a gel of the reporter system plasmids that Munima Isolated yesterday to determine to outcome.

Reporter(Oct11).jpg

-Set up a Restriction Digest of the Reporter System Parts. pLacI is cut with SpeI and PstI, RFP sub and TetR sub are cut with XbaI and PstI.