04/09/13

(Difference between revisions)

Revision as of 09:07, 5 September 2013

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The double digest (pSB1C3) from yesterday was run on a 1% gel.
This was done in order to confirm that the digest worked and also to purify the pSB1C3 vector.

The two higher bands in tracks 2 and 3 are plasmids that were not digested.

The Zymoclean Gel DNA recovery Kit was used to perform the purification and its protocol was followed.
However the elution step was changed to 12ul of elution buffer, and this step was repeated.

Samples A (TodX), C (TodF) and E (ToBG) were digested with the enzymes XbaI and SpeI.

- The samples were incubated at 37C for 90 minutes
- Heat kill the enzymes by incubating the samples at 80C for 20 minutes

@@ Line 32: / Line 32: @@
 *However the elution step was changed to 12ul of elution buffer, and this step was repeated.
-==Double digest of TOD gene ligations==
+==Double digest of TOD genes PCR products==
+Samples A (TodX), C (TodF) and E (ToBG) were digested with the enzymes XbaI and SpeI.
+*Protocol
+{| border=1
+|Samples || A ||C ||E
+|-
+|Volume (ul)||20|| 23.5||21
+|-
+|SpeI (ul)||1|| 1|| 1
+|-
+|XbaI|| 0.5|| 0.5||0.5
+|-
+|Cutsmart Buffer|| 6|| 6||6
+|-
+|5mTris Hcl (ul)|| 32.5|| 29|| 31.5
+|}
+**The samples were incubated at 37C for 90 minutes
+**Heat kill the enzymes by incubating the samples at 80C for 20 minutes