Template:Team:KULeuven/24 August 2009/BlueLightReceptor

(Difference between revisions)

Revision as of 11:53, 1 September 2009

plates with ligA were put under blue light. the LEDs were put on their max capacity.
restriction digest with
- tubes (1,3,5,7,9) of ligA (BLP + ) cut with EcoRI en PstI
- promotor cut with EcoRI en SpeI (4x)
gel electroforese with the RD of ligA and followed by a gel extraction:
- note: tube 5 of ligA was loaded poorly on the gel and could not be used.
- note: the samples of promotor were barly visible. only 2 of the 4 samples were recoverd by extraction.

4. enting of liquid cultures with kanamycin and

@@ Line 1: / Line 1: @@
 # plates with ligA were put under blue light. the LEDs were put on their max capacity.
 # restriction digest with
-#*tubes (1,3,5,7,9) of ligA (BLP + E0240) cut with EcoRI en PstI
+#*tubes (1,3,5,7,9) of ligA (BLP + {{kulpart|BBa_E0240}}) cut with EcoRI en PstI
-#*promotor J23101 cut with EcoRI en SpeI (4x)
+#*promotor {{kulpart|BBa_J23101}} cut with EcoRI en SpeI (4x)
-#gel electroforese with the RD of ligA and J23101 followed by a gel extraction:
+#gel electroforese with the RD of ligA and {{kulpart|BBa_J23101}} followed by a gel extraction:
 #* note: tube 5 of ligA was loaded poorly on the gel and could not be used.
-#* note: the samples of promotor J23101 were barly visible. only 2 of the 4 samples were recoverd by extraction.
+#* note: the samples of promotor {{kulpart|BBa_J23101}} were barly visible. only 2 of the 4 samples were recoverd by extraction.
 {| border ="1" align="center"
 !| Part || concentration (ng/&mu;l) || 260/280 &lambda; ||
@@ Line 21: / Line 21: @@
 | {{kulpart|BBa_J23101}} (B) ||12,8|| 2,57 ||
 |}
-. enting of liquid cultures with kanamycin and pSB3K3
+. enting of liquid cultures with kanamycin and {{kulpart|pSB3K3}}