Team:DTU-Denmark/Notebook/3 July 2013

From 2013.igem.org

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(208 lab)
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=208 lab=
=208 lab=
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== Main purposes today ==
== Main purposes today ==
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Verify insert plated made Sunday. Run BioLector experiment.
Verify insert plated made Sunday. Run BioLector experiment.
==who were in the lab==
==who were in the lab==
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Kristian, Ariadni
Kristian, Ariadni
==Procedure==
==Procedure==
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Gel on colony PCR from yesterday.
Gel on colony PCR from yesterday.
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==Results==
==Results==
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[[File:03.07.13 Colony PCR.jpg|thumb|left|The gel from colony PCR. From left to right; Sec1, Sec2, Sec3, TAT2 1, TAT2 2, TAT2 3, TAT3 1, TAT3 2, TAT3 3, TAT3 1a, TAT3 2a. Where the different TATs are either with(TAT2) or without insertion of 2 additional amino acids to ease the primer design. 1kb plus ladder([http://www.invitrogen.com/site/us/en/home/Products-and-Services/Applications/DNA-RNA-Purification-Analysis/Nucleic-Acid-Gel-Electrophoresis/DNA-Ladders/Track-IT-Ladders.html invitrogen]) ]]
[[File:03.07.13 Colony PCR.jpg|thumb|left|The gel from colony PCR. From left to right; Sec1, Sec2, Sec3, TAT2 1, TAT2 2, TAT2 3, TAT3 1, TAT3 2, TAT3 3, TAT3 1a, TAT3 2a. Where the different TATs are either with(TAT2) or without insertion of 2 additional amino acids to ease the primer design. 1kb plus ladder([http://www.invitrogen.com/site/us/en/home/Products-and-Services/Applications/DNA-RNA-Purification-Analysis/Nucleic-Acid-Gel-Electrophoresis/DNA-Ladders/Track-IT-Ladders.html invitrogen]) ]]

Revision as of 13:21, 25 July 2013


Contents

208 lab


Main purposes today


Verify insert plated made Sunday. Run BioLector experiment.


who were in the lab


Kristian, Ariadni

Procedure


Gel on colony PCR from yesterday.

Setup of BioLector experiment.

MiniPrep selected colonies and make restriction digest analysis.

Results


The gel from colony PCR. From left to right; Sec1, Sec2, Sec3, TAT2 1, TAT2 2, TAT2 3, TAT3 1, TAT3 2, TAT3 3, TAT3 1a, TAT3 2a. Where the different TATs are either with(TAT2) or without insertion of 2 additional amino acids to ease the primer design. 1kb plus ladder([http://www.invitrogen.com/site/us/en/home/Products-and-Services/Applications/DNA-RNA-Purification-Analysis/Nucleic-Acid-Gel-Electrophoresis/DNA-Ladders/Track-IT-Ladders.html invitrogen])

No results from restriction analysis because we saw no bands on the gel. We assume that this is caused by the low DNA concentration.


Conclusion from today

TAT2 1 and TAT3 1a have the right bands on colony PCR and will be further analyzed.

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