Template:Team:KULeuven/27 August 2009/BlueLightReceptor

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(Difference between revisions)

Latest revision as of 09:24, 8 September 2009

The electroporations of 26/08 were checked.
- had some colonies. they were ented in liquid culture.
- LigC ( + ) did not grow. we figured that an insert of 35bp was too short to ligate so we decided to use as insert and + as vector . The following restriction digest was started:
  - was cut with SpeI and PstI
  - was cut with XbaI and PstI
The miniprep that was made to sequence the LigA construct on 26/08 was used again to perform a restriction digest (EcoRI and PstI). This was put on gel to check whether there actually was LigA-insert in the vector and whether the insert had the right length. The gel showed a signal at 1000 bp and at 2000 bp which coincides with the insert (BLp + GFP) and the vector.
A new setup to light the E.coli was engineered.
- Fresh cultures were made from the old ones (LB plate ligA 14/08 and the two liquid cultures from 26/08 were used as templates.)
- They were put in the 16°C room for about an hour
- A blue light (40W) was put on them for about an hour
- They were put in the 37°C incubator overnight

@@ Line 1: / Line 1: @@
-# the electroporations of 26/08 were checked.
+# The electroporations of 26/08 were checked.
 #*{{kulpart|pSB3K3}} had some colonies. they were ented in liquid culture.
-#*LigC ({{kulpart|BBa_J23101}} + {{kulpart|BBa_E0240}}) did not grow. we figured that an insert of 35bp was to short to ligate so we decided to use {{kulpart|BBa_E0240}} as insert and {{kulpart|BBa_J23101}} + {{kulpart|pSB1A2}} as vector . The following restriction digest was started:
+#*LigC ({{kulpart|BBa_J23101}} + {{kulpart|BBa_E0240}}) did not grow. we figured that an insert of 35bp was too short to ligate so we decided to use {{kulpart|BBa_E0240}} as insert and {{kulpart|BBa_J23101}} + {{kulpart|pSB1A2}} as vector . The following restriction digest was started:
 #** {{kulpart|BBa_J23101}} was cut with SpeI and PstI
 #** {{kulpart|BBa_E0240}} was cut with XbaI and PstI
-# the miniprep that was made to sequence the LigA construct on 26/08 was used again to perform a restriction digest (EcoRI and PstI). this was put on gel to check wether there actually was LigA-insert in the vector and wether the insert had the right length. the gel showed a signal at 1000 bp and at 2000 bp which coincides with the insert (BLp + GFP) and the vector.
+# The miniprep that was made to sequence the LigA construct on 26/08 was used again to perform a restriction digest (EcoRI and PstI). This was put on gel to check whether there actually was LigA-insert in the vector and whether the insert had the right length. The gel showed a signal at 1000 bp and at 2000 bp which coincides with the insert (BLp + GFP) and the vector.
-# a new set up to light the Ecoli was engineered.
+# A new setup to light the E.coli was engineered.
-#* fresh cultures were made from the old ones (LB plate ligA 14/08 and the two liquid cultures from 26/08 were used as templates.)
+#* Fresh cultures were made from the old ones (LB plate ligA 14/08 and the two liquid cultures from 26/08 were used as templates.)
-#* they were put in the 16°C room for about an hour
+#* They were put in the 16°C room for about an hour
-#* a blue light (40W) was put on them for about an hour
+#* A blue light (40W) was put on them for about an hour
-#* they were put in the 37°C incubator overnight
+#* They were put in the 37°C incubator overnight