Revision as of 14:57, 4 August 2013

3 August 2013

lab 208

Main purpose

Who was in the lab

Henrike, Kristian

Procedure

Gel electrophoresis

Run 1% agarose gel on overnight PCR products.

Miniprep

Isolate plasmids from samples Sec2, cycAX, TAT 3-1a, TAT 3-2, TAT 2-1 using ethanol precipitation. Actually should have used the Midiprep kit from QIAgen. After ethanol precipitation continued with Midiprep kit step from step 9.

Purification gel

Purification of Nir 2 fragment by gel purification.

Results

Gels

1% agarose gel

1kb ladder
Nir1 high
Nir1 high
Nir1 low
Nir1 low
broad band ladder
43
43
Nir2 GC
Nir2 GC
neg for Nir
AMO
AMO
neg for AMO
1 kb ladder

Conclusion

The gel verified that Nir1 high is the right fragment but also confirmed that the recurrent fragment on approx. 16 kb from whole Nir isolation is not Nir but unspecific product.

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@@ Line 8: / Line 8: @@
 ==Who was in the lab==
 <hr/>
+Henrike, Kristian
 ==Procedure==
@@ Line 20: / Line 21: @@
 Isolate plasmids from samples Sec2, cycAX, TAT 3-1a, TAT 3-2, TAT 2-1 using [[Team:DTU-Denmark/Methods/Plasmid_isolation|ethanol precipitation]]. Actually should have used the Midiprep kit from QIAgen.
 After ethanol precipitation continued with Midiprep kit step from step 9.
+===Purification gel===
+Purification of Nir 2 fragment by gel purification.
 ==Results==
@@ Line 48: / Line 53: @@
 ==Conclusion==
 <hr/>
+The gel verified that Nir1 high is the right fragment but also confirmed that the recurrent fragment on approx. 16 kb from whole Nir isolation is not Nir but unspecific product.
 Navigate to the [[Team:DTU-Denmark/Notebook/2_August_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/4_August_2013|Next]] Entry
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Team:DTU-Denmark/Notebook/3 August 2013

From 2013.igem.org