User:Mary Mendoza/Notebook/CHEM 571 Experimental Biological Chemistry I/2012/10/17

(Difference between revisions)

Revision as of 12:26, 27 October 2012

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Transferred 5 μL of the mutated plasmid into a new sterilized tube; leaving out one tube containing 45 μL.
Simultaneously, added 1 μL of the gel loading dye 6x blue into the 5 μL plasmid and added 1 μL of DpnI into the 45 μL plasmid.
The sample containing the DpnI was placed in a VWR analog heatblock at 37°C.
The agarose gel was prepared by dissolving 1.23 g of agarose in 35 mL of TAE buffer. The agarose was heated in a microwave for 35s.
When the solution is clear, the agarose was poured into the gel electrophoresis tray with the comb in place.
A wait period of 30 min. was allotted for the gel to solidify. Upon observing the gel is already in its solidified state, the comb was gently removed to avoid breakage.
The chamber containing the gel tray was filled with TAE buffer to the point where the gel is completely submerged of the buffer.

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 * When the solution is clear, the agarose was poured into the gel electrophoresis tray with the comb in place.
 * A wait period of 30 min. was allotted for the gel to solidify. Upon observing the gel is already in its solidified state, the comb was gently removed to avoid breakage.
-*
+* The chamber containing the gel tray was filled with TAE buffer to the point where the gel is completely submerged of the buffer.