Team:UQ-Australia/Notebook/Experiment2

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Latest revision as of 12:27, 21 October 2009

Experiment 2

Transformation of pSUTp. pG.pmt and pSUTp

The bacteria used for this transformation reaction was DH5α Max efficiency cells strain (chemical competent) pSUTp. pG. pmt and pSUTp solution collected from 02/10/09 (click HERE fore further details) (Can you please put the link to 02/10.09 nanodrop result here?) were diluted to 10ng/uL solution to use for the transformation reaction.

Transformation control: pUC19

Click HERE for detailed protocol of transformation reaction.
While bacteria containing pSUTp.pG.pmt and pUC 19 were cultured on two separate Amp plates, bacteria with pSUTp was grown on Kan plate.
Incubate went overnight at 370C.
Results: Bacteria colonies were shown on plate in following morning
08/10/09: Pick isolate colonies from pSUTp and pSUTp.pG.pmt cultures.

Click HERE for detailed protocol of picking colonies.

4 colonies from pSUTp culture were picked and transfered into new tubes named pSUTp Kan 1-4
4 colonies from pSUTp.pG.pmt were picked and transferred into new tubes named pSUTp.pG.pmt Amp 1-4

NOTE: MerT and MerP primers arrived.

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-==Miniprep Procedure==
+==Experiment 2==
-'''Production of Cleared Lysate'''
+'''Transformation of pSUTp. pG.pmt and pSUTp'''
-. Pellet 1-10ml overnight cultures for 5 minutes
+The bacteria used for this transformation reaction was DH5α Max efficiency cells strain (chemical competent)
+pSUTp. pG. pmt  and pSUTp solution collected from 02/10/09 (click HERE fore further details)                            (Can you please put the link to 02/10.09 nanodrop result here?) were diluted to 10ng/uL solution to use for the transformation reaction.
-. Thoroughly re-suspend pellet with 250ul Cell Resuspension Solution
+'''Transformation control: pUC19'''
+*Click HERE for detailed protocol of transformation reaction.
+*While bacteria containing pSUTp.pG.pmt and pUC 19 were cultured on two separate Amp plates, bacteria with pSUTp was grown on Kan plate.
+*Incubate went overnight at 370C.
+*Results: Bacteria colonies were shown on plate in following morning
+*08/10/09: Pick isolate colonies from pSUTp and pSUTp.pG.pmt cultures.
-. Add 250ul Cell Lysis Solution to each sample; invert 4 times to mix
+Click HERE for detailed protocol of picking colonies.
+*4 colonies from pSUTp culture were picked and transfered into new tubes named pSUTp  Kan 1-4
-. Add 10ul Alkaline Protease Solution; invert 4 times to mix. Incubate 5 minutes at room temperature
+*4 colonies from pSUTp.pG.pmt were picked and transferred into new tubes named  pSUTp.pG.pmt Amp 1-4
+NOTE: MerT and MerP primers arrived.
-. Add 350 ul Neutralizer Solution; invert 4 times to mix
-. Centrifuge at top speed for 10 minutes at room temperature.
-'''Binding of Plasmid DNA'''
-. Insert Spin Column into Collection Tube
-. Decant cleared lysate into Spin Column
-. Centrifuge at top speed for 1 minute at room temperature. Discard flowthrough and reinsert Column into Collection Tube.
-'''Washing'''
-. Add 750ul Wash Solution (ethanol added). Centrifugeat top speed for 1 minute. Discard flowthrough and reinsert column into Collection Tube
-. Repeat step 10 with 250ul Wash Solution
-. Centrifuge at top speed for 2 minutes at room temperature
-'''Elution'''
-. Transfer Spin Column to a sterile 1.5ml microcentrifuge tube, being careful not to transfer any of the Column Wash Solution with the Spin Column.
-. Add 100ul of Nuclease-free Water to the Spin Column. Centrifuge at top speed for 1 minute at room temperature.
-. Discard column and store DNA at -20'C or below.