Team:Alberta/Notebook

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<font size=5> &nbsp;&nbsp;&nbsp;iGem Notebook</font>
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<font size=5> iGen Diary </font>
 
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<div class="underline"><font size=5>May</font></div>
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Rick and Tom recruited and learning basic laboratory protocols, such as making competent cells, restriction digests, cell transformation, gel electrophoresis.
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Rick and Tom began coming in to the lab regularly and started learning basic laboratory protocols, such as making competent cells, restriction digests, cell transformation, gel electrophoresis, ect.
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Rick, Tom, Spencer, and Easwar learned how to use PCR today, with varying degrees of success.
Rick, Tom, Spencer, and Easwar learned how to use PCR today, with varying degrees of success.
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|Today Tom finally managed to get a PCR to work, though it took him about twelve attempts.
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Today Tom finally managed to get a PCR to work, though it took him about twelve attempts.
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|June 4
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|Made working stock of puc19 and then transformed Top10 with puc19. Overnight cultures were also set up in preparation for the making of competent cells
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|[[https://2012.igem.org/Team:Alberta/Notebook Top page]]
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|June 5
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|Competent cells were made today using a standard procedure which took the entire day.
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<div class="underline"><font size=5>June</font></div>
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|June 6
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|The competent cells were tested with basic puc19 transformation, and the transformation worked.
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June 4
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|June 7-8
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|Today multiple PCRs were run on puc19 with two of the color genes and a C1 gene.
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Made working stock of puc19 and then transformed Top10 with puc19. Overnight cultures were also set up in preparation for the making of competent cells
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|June 11
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</font>
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|Made pUC19 plasmid with the new color genes and C1 and transformed it into cells.
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|June 18-21
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June 5
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|We cloned a variety of different (9) promoters into our color gene plasmids, in order to get a sense of relative promoter strengths. we also seqencing those construct to check they are correct
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|June 22- july 3
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Competent cells were made today using a standard procedure which took the entire day. The competent cell procedure is described elsewhere in this wiki.
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|We PCR new RBS  colour genes and regulatory promoters. we then made those constructs into kanamycin resistant plasmid backbone and transform them into Top 10 cells.
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|July 4-5
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June 6
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|Torrin and Sarah Join. we perform the same work again on TG1.  
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|July 6
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The competent cells were tested with basic puc19 transformation, and the transformation worked with acceptable efficiency.
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|Tom checked overnights of origin cut site strains and chose colonies to be sequenced.
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|July 9-10
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|Today Tom Used the successful origin cut site plasmid with Amp Resistance and replaced that resistance with Chlr.
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June 7-8
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Torrin and Sarah are creating and testing chemical gradient plates, and learning additional laboratory procedure.
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Rick and Spencer is making competent cells of TG1 so that we can test our current parts in an E.Coli strain that grows faster than our current Top10.
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|Rick and Easwar are drop in LacI and Tet R repressor into chloranphenicol construct.
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Today multiple PCRs were run on puc19 with two of the color genes and a repressor gene.
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|July 11
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|We continued our experiments with making chemical gradients on agar plates.
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June 11
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Made pUC19 plasmid with various color genes and C1 and transformed it into cells.
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June 18-21
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We cloned a variety of different promoters (nine total) into our color gene plasmids in order to get a sense of relative promoter strengths. We also sent off to sequencing those construct to check that they are correct.
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June 22- July 3
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We used PCR to add new RBS  colour genes and regulatory promoters to our constructs. We then pieced those constructs into kanamycin resistant plasmid backbone and transform them into Top 10 cells.
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{|align="right"
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|[[https://2012.igem.org/Team:Alberta/Notebook Top page]]
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<div class="underline"><font size=5>July</font></div>
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July 4-5
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</font>
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<font size=2>
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Torrin and Sarah join the team. We performed the same work on the TG1 strain of E.Coli as a learning exercise.  
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July 6
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Creation of a plasmid with a cut site near the origin of replication began today. This plasmid will be used in order to modify the promoter on the plasmid's origin of replication.
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July 9-10
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Today Tom Used the successful origin cut site plasmid with Amp Resistance and replaced that resistance with Chlr.

Latest revision as of 21:56, 18 September 2012




   iGem Notebook


May


May.9-11.2012

Rick and Tom began coming in to the lab regularly and started learning basic laboratory protocols, such as making competent cells, restriction digests, cell transformation, gel electrophoresis, ect.


May. 24

Rick, Tom, Spencer, and Easwar learned how to use PCR today, with varying degrees of success.


May 31

Today Tom finally managed to get a PCR to work, though it took him about twelve attempts.

[Top page]


June


June 4

Made working stock of puc19 and then transformed Top10 with puc19. Overnight cultures were also set up in preparation for the making of competent cells


June 5

Competent cells were made today using a standard procedure which took the entire day. The competent cell procedure is described elsewhere in this wiki.


June 6

The competent cells were tested with basic puc19 transformation, and the transformation worked with acceptable efficiency.


June 7-8

Today multiple PCRs were run on puc19 with two of the color genes and a repressor gene.


June 11

Made pUC19 plasmid with various color genes and C1 and transformed it into cells.


June 18-21

We cloned a variety of different promoters (nine total) into our color gene plasmids in order to get a sense of relative promoter strengths. We also sent off to sequencing those construct to check that they are correct.


June 22- July 3

We used PCR to add new RBS colour genes and regulatory promoters to our constructs. We then pieced those constructs into kanamycin resistant plasmid backbone and transform them into Top 10 cells.

[Top page]


July


July 4-5

Torrin and Sarah join the team. We performed the same work on the TG1 strain of E.Coli as a learning exercise.


July 6

Creation of a plasmid with a cut site near the origin of replication began today. This plasmid will be used in order to modify the promoter on the plasmid's origin of replication.


July 9-10

Today Tom Used the successful origin cut site plasmid with Amp Resistance and replaced that resistance with Chlr.