Team:KULeuven/29 July 2008

From 2008.igem.org

(Difference between revisions)
(Wet Lab)
Line 4: Line 4:
=== Wet Lab ===
=== Wet Lab ===
-
Only one ligation succeeded (R0084+B0032). We think that the others failed because the vectors weren't properly cut. Therefore, we will try another digest. This time we will cut the vector with ''Xba'' I, and only when this works, we will cut it with ''Eco''R I. We do this because ''Xba'' I has problems with cleaving close to the end of DNA fragments.
+
* Only one ligation succeeded (R0084+B0032). We think that the others failed because the vectors weren't properly cut. Therefore, we tried another digest. This time we cut the vector with ''Xba'' I, and only when this worked, we cut it with ''Eco''R I. We did this because ''Xba'' I has problems with cleaving close to the ends of DNA fragments. The problem is that ''Xba'' I doesn't seem to cut. Perhaps there's something wrong with the enzyme. We are trying to overcome this problem by allowing the restriction with ''Xba'' I to continue overnight.
 +
* Some more plasmids were isolated from the cells using the Qiagen MiniPrep Kit. It concerns parts used in the filter and in the inverter (J23022, J23109, J23032, I712074, B0015, R0084, B0032 and  B0034, C0012, R0011, F1610). We also digested some of these isolated plasmids. The ones that were cut with ''Eco''R I and ''Spe'' I succeeded (R0084, J23109 and I712074) and were cut out of the agarose gel and purified. The ones that were cut with ''Xba'' I failed (J23022, J23032 and B0015) - we didn't get the expected result with gel electrophoresis.
=== Dry Lab ===
=== Dry Lab ===

Revision as of 18:09, 29 July 2008

<< return to notebook return to homepage >>
< previous friday ← yesterday tomorrow → next monday >

Contents

Lab Work

Wet Lab

  • Only one ligation succeeded (R0084+B0032). We think that the others failed because the vectors weren't properly cut. Therefore, we tried another digest. This time we cut the vector with Xba I, and only when this worked, we cut it with EcoR I. We did this because Xba I has problems with cleaving close to the ends of DNA fragments. The problem is that Xba I doesn't seem to cut. Perhaps there's something wrong with the enzyme. We are trying to overcome this problem by allowing the restriction with Xba I to continue overnight.
  • Some more plasmids were isolated from the cells using the Qiagen MiniPrep Kit. It concerns parts used in the filter and in the inverter (J23022, J23109, J23032, I712074, B0015, R0084, B0032 and B0034, C0012, R0011, F1610). We also digested some of these isolated plasmids. The ones that were cut with EcoR I and Spe I succeeded (R0084, J23109 and I712074) and were cut out of the agarose gel and purified. The ones that were cut with Xba I failed (J23022, J23032 and B0015) - we didn't get the expected result with gel electrophoresis.

Dry Lab

Modeling

Mainly chillin' out, memory was finished and complete model is functional.

Wiki

Modeling section got taken care of some more, work on new dropdown menu proceeds...

Remarks

Quote Of The Day

Sigrid: Het is te hopen dat de getransduceerde cellen een groeischeut krijgen. Stefanie: Daar wacht ik nu al 22 jaar op!