Team:Calgary/12 August 2010

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{{CalgaryNotebookTemplate|
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'''Thursday August 12, 2010'''
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Thursday August 12, 2010|
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[[Image:08.12.2010.CpxPDigest+ipbabdigest.jpg|thumb|400px|Chris's gel of CpxP digested as well as ibpAB digested. Lanes 2 through 8 are CpxP digested and Lanes 9-12 are ibpAB]]
[[Image:08.12.2010.CpxPDigest+ipbabdigest.jpg|thumb|400px|Chris's gel of CpxP digested as well as ibpAB digested. Lanes 2 through 8 are CpxP digested and Lanes 9-12 are ibpAB]]
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[[Image:08.12.2010ipbab-undigested.jpg|thumb|400px|Chris's gel of undigested ibpAB Promoter]]
[[Image:08.12.2010ipbab-undigested.jpg|thumb|400px|Chris's gel of undigested ibpAB Promoter]]
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[[Image:08 12 2010 ResDig malEandMalE31.jpg|thumb|400px|Restriction Digest with XbaI/SpeI of MalE and MalE31]]
<u>Chris</u>
<u>Chris</u>
Today, I started with a ton of plasmid preparations with I13504, iPBAB, I0500-I13504, and I13507 colonies. The concentrations are once again, available upon demand. Then, I began a digest of ibpAB to with the enzymes EcoRI and PstI to insert it into an AK Biobrick vector. I also digested the CpxP promoter that was inserted into AK plasmid with EcoRI and PstI. The results of the gel with the digested CpxP and ibpAB are shown on the first gel on the right. The second gel was the ibpAB promoter uncut in original state. Finally, I set up another digest for ibpAB to run with T4 DNA Ligase tomorrow as we are out of Quick Ligase.
Today, I started with a ton of plasmid preparations with I13504, iPBAB, I0500-I13504, and I13507 colonies. The concentrations are once again, available upon demand. Then, I began a digest of ibpAB to with the enzymes EcoRI and PstI to insert it into an AK Biobrick vector. I also digested the CpxP promoter that was inserted into AK plasmid with EcoRI and PstI. The results of the gel with the digested CpxP and ibpAB are shown on the first gel on the right. The second gel was the ibpAB promoter uncut in original state. Finally, I set up another digest for ibpAB to run with T4 DNA Ligase tomorrow as we are out of Quick Ligase.
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<u>Raida</u>
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Today I ran the gel electrophoresis of the restriction digest that Emily did on Thursday. The results are positive, the bands are at the right place : 1.2 and 3.9 kb. These will be sent down for sequencing tomorrow. I also ran a pcr of malEssdel and malE31ssdel to insert them in TOPO vector.
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I also worked on Ethics paper. I completed the Environment and synthetic biology portion of the paper.
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<u>Himika</u>
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Today I read more papers regarding inclusion body formation and modeling the same in SImbiology.
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<u>Alex</u>
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Today I performed a restriction digest of the plasmids attained from the K239000-I13504/I13507 constructions. Each tube contained 600ng of DNA, 0.5μl of EcoR1 and Spe1 enzymes.
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Latest revision as of 03:06, 27 October 2010

Thursday August 12, 2010

Chris's gel of CpxP digested as well as ibpAB digested. Lanes 2 through 8 are CpxP digested and Lanes 9-12 are ibpAB
Chris's gel of undigested ibpAB Promoter
Restriction Digest with XbaI/SpeI of MalE and MalE31

Chris

Today, I started with a ton of plasmid preparations with I13504, iPBAB, I0500-I13504, and I13507 colonies. The concentrations are once again, available upon demand. Then, I began a digest of ibpAB to with the enzymes EcoRI and PstI to insert it into an AK Biobrick vector. I also digested the CpxP promoter that was inserted into AK plasmid with EcoRI and PstI. The results of the gel with the digested CpxP and ibpAB are shown on the first gel on the right. The second gel was the ibpAB promoter uncut in original state. Finally, I set up another digest for ibpAB to run with T4 DNA Ligase tomorrow as we are out of Quick Ligase.


Raida Today I ran the gel electrophoresis of the restriction digest that Emily did on Thursday. The results are positive, the bands are at the right place : 1.2 and 3.9 kb. These will be sent down for sequencing tomorrow. I also ran a pcr of malEssdel and malE31ssdel to insert them in TOPO vector.

I also worked on Ethics paper. I completed the Environment and synthetic biology portion of the paper.


Himika

Today I read more papers regarding inclusion body formation and modeling the same in SImbiology.

Alex

Today I performed a restriction digest of the plasmids attained from the K239000-I13504/I13507 constructions. Each tube contained 600ng of DNA, 0.5μl of EcoR1 and Spe1 enzymes.