Team:Calgary/9 July 2010
From 2010.igem.org
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{{CalgaryNotebookTemplate| | {{CalgaryNotebookTemplate| | ||
+ | Friday July 9, 2010| | ||
[[Image:07-09-2010-Himikagel.jpg|thumb|400px|Himika's gel electrophoresis of the restriction digest of parts listed below]] | [[Image:07-09-2010-Himikagel.jpg|thumb|400px|Himika's gel electrophoresis of the restriction digest of parts listed below]] | ||
[[Image:07.09.2010.R0040+I13507 set1.jpg|thumb|400px|Jeremy's construction of R0040+ 13507. Red and Normal colored cells present.]] | [[Image:07.09.2010.R0040+I13507 set1.jpg|thumb|400px|Jeremy's construction of R0040+ 13507. Red and Normal colored cells present.]] | ||
- | [[Image:07.09.2010.BbkpRFP.jpg|thumb|400px|Jeremy's Bbk RFP (attempt 1)]] | + | [[Image:07.09.2010.BbkpRFP.jpg|thumb|400px|Jeremy's Bbk RFP (attempt 1)]] |
<u>Himika</u> | <u>Himika</u> | ||
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I also designed primer along with Dave for sewing PCR of the ppRFP circuit. | I also designed primer along with Dave for sewing PCR of the ppRFP circuit. | ||
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<u>Chris</u> | <u>Chris</u> | ||
Today, I contacted the Qiagen representative about possible sponsorship and am awaiting a response. As well, this morning, I did plasmid preparations of several different overnight cultures of I0500. 7 overnight cultures were prepped using the Sigma Aldrich GenElute Plasmid Preparation kit (the protocol can be found in our Lab Protocols section). | Today, I contacted the Qiagen representative about possible sponsorship and am awaiting a response. As well, this morning, I did plasmid preparations of several different overnight cultures of I0500. 7 overnight cultures were prepped using the Sigma Aldrich GenElute Plasmid Preparation kit (the protocol can be found in our Lab Protocols section). | ||
+ | |||
<u>Jeremy</u> | <u>Jeremy</u> | ||
Today I worked on biobricking pRFP because the primers came in. Henry helped design suitable conditions for the PCR. There was problems with larger than normal bands, potentially due to annealing on the plasmid. The R0040 + I13507 parts had colonies that are red, further verification via sequencing for I13507 will be necessary to confirm it is consistent. | Today I worked on biobricking pRFP because the primers came in. Henry helped design suitable conditions for the PCR. There was problems with larger than normal bands, potentially due to annealing on the plasmid. The R0040 + I13507 parts had colonies that are red, further verification via sequencing for I13507 will be necessary to confirm it is consistent. | ||
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+ | <u>Dev</u> | ||
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+ | Results: Growth was obtained. Colonies showed fluorescence. | ||
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+ | |||
+ | <u>Alex</u> | ||
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+ | Today our new reverse primer for cpxp arrived. I diluted the primer down to ~5 micro molar, and then also diluted the forward primer, getting close with about 7 micro molar. Then we prepared a 5X master mix with our primers, and ran 5 PCR reactions. Today we also presented our project to our supervisors. | ||
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+ | |||
+ | <u>Patrick</u> | ||
+ | |||
+ | I helped the team make final preparations for our presentation to our supervisors. | ||
+ | |||
<u>Team</u> | <u>Team</u> | ||
- | We did a presentation of our overall project to our supervisors Dr. Cairine Logan and Dr. Anthony Schryvers as well as several graduate students and our lab technician Deirdre Lobb. This presentation was put together as a practice for the iGEM competition as well as to inform everyone on the status and goals of our project. | + | We did a presentation of our overall project to our supervisors Dr. Cairine Logan and Dr. Anthony Schryvers as well as several graduate students and our lab technician Deirdre Lobb. This presentation was put together as a practice for the iGEM competition as well as to inform everyone on the status and goals of our project. Changes to both the project as well as the presentation were suggested by our supervisors and modifications will be made. One of the main points which were made was the need for clarity in all slides. What we thought was easily understandable in figures turned out not to be so to others. Visual depictions of circuits and colour schemes will need to be modified in the future. |
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Latest revision as of 03:37, 23 August 2010
Friday July 9, 2010
Himika
Today I did a restriction digest of parts with EcoRI/SpeI in React II Buffer that I constructed and the plasmid switch I did on July 6th. The parts that I digested were:
- 3 colonies of E1010 in AC plasmid
- 2 colonies of E1010-B0015 construction done on July 6th
- I also ran 2 colonies of I13507
- 1 colony of E1010 in its original Kanamycin plasmid
Refer to the image for the results of the gel electrophoresis done of the restriction digests
I also designed primer along with Dave for sewing PCR of the ppRFP circuit.
Chris
Today, I contacted the Qiagen representative about possible sponsorship and am awaiting a response. As well, this morning, I did plasmid preparations of several different overnight cultures of I0500. 7 overnight cultures were prepped using the Sigma Aldrich GenElute Plasmid Preparation kit (the protocol can be found in our Lab Protocols section).
Jeremy
Today I worked on biobricking pRFP because the primers came in. Henry helped design suitable conditions for the PCR. There was problems with larger than normal bands, potentially due to annealing on the plasmid. The R0040 + I13507 parts had colonies that are red, further verification via sequencing for I13507 will be necessary to confirm it is consistent.
Dev
Results: Growth was obtained. Colonies showed fluorescence.
Alex
Today our new reverse primer for cpxp arrived. I diluted the primer down to ~5 micro molar, and then also diluted the forward primer, getting close with about 7 micro molar. Then we prepared a 5X master mix with our primers, and ran 5 PCR reactions. Today we also presented our project to our supervisors.
Patrick
I helped the team make final preparations for our presentation to our supervisors.
Team
We did a presentation of our overall project to our supervisors Dr. Cairine Logan and Dr. Anthony Schryvers as well as several graduate students and our lab technician Deirdre Lobb. This presentation was put together as a practice for the iGEM competition as well as to inform everyone on the status and goals of our project. Changes to both the project as well as the presentation were suggested by our supervisors and modifications will be made. One of the main points which were made was the need for clarity in all slides. What we thought was easily understandable in figures turned out not to be so to others. Visual depictions of circuits and colour schemes will need to be modified in the future.