Team:Johns Hopkins/Notebook/GROUP 5: MATa Specific Promoters II
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- | Restriction Enzyme Digested and the insert | + | Restriction Enzyme Digested and the insert appears promising. Ready for sequence submission for Ste 2 promotor. |
Status Report by: Alexandra McMillan | Status Report by: Alexandra McMillan | ||
Revision as of 03:51, 30 October 2008
GROUP 5: MATa Specific Promoters II
Summary for MATa Specific Promoters II Group
Part Description: Ste2 Promoter Reverse Summary here: We were able to grow colonies with sequence verified Ste2 promoters. The promoter is currently located in a glycerol stock in pGEM vector. One attempt to transfer to the iGEM vector has been made, unsuccessfully. This was due to a mistake in protocol however, so final transfer to the iGEM vector should still be straightforward. Progress on this bio-brick has been paused in order to focus on MFA1, which is more applicable to our project design because this Ste2 designed for the wrong direction. Part no.: BBa_K110015 Part Description: MFA1 Promoter Forward Summary here: We have been unable to get successful, sequence verified clones with our MFA1 promoter thus far. We currently have a few samples of DNA ready to be tested by restriction enzyme digest, and then, hopefully, sequencing.
For more information about the parts go to: http://partsregistry.org/cgi/partsdb/pgroup.cgi?pgroup=iGEM2008& group=Johns_Hopkins
Up to today... Since then -- we have been troubleshooting and working on getting higher concentrations and using the correct stock plates. Several delays have occurred,and we should be close to ligating into the iGEM vector
8/24 Restriction Enzyme Digested and the insert appears promising. Ready for sequence submission for Ste 2 promotor. Status Report by: Alexandra McMillan
8/21 Due to low concentrations, we needed to concentrate our DNA before preceeding. Ethanol precipitation using EtOH/NaAc and 100 ul of miniprep mix was complete of the BBa_K110015 and BBa_K11009 minipreps.
8/18 Miniprep products were < 100 ng/ul. Restriction digest. There appear to be correct size inserts. Gel image coming. Results look promising.
8/15 DNA miniprep of BBa_K110015 and BBa_K11009 cultures
8/13 Incubated inoculations of old colony plates
By 7/19/08 We successfuly transformed both BB 15 and 9 and ran a gel that came out with faint bands. We digested BB 9 and 15.
Date: 7/11/08 status report by Rick Carrick Part no.: BBa_K110015, Part Description: MFA1 Part Location (in build a genome lab): PCR successful?; Y (on moodle somewhere) Cloning of PCR product successful: Y Sequencing of cloned PCR product successful:N Joining of validated part to adjacent part(s) status: Not done Problems to be solved: None so far Current status of this part: This parts must be restriction enzyme digested and sequenced next.
Date: 7/11/08 status report by Rick Carrick Part no.: BBa_K110009 Part Description: Ste2 Part Location (in build a genome lab): PCR successful?; Y (on moodle somewhere) Cloning of PCR product successful: Y Sequencing of cloned PCR product successful:N Joining of validated part to adjacent part(s) status: Not done Problems to be solved: None so far Current status of this part: This part must be restriction enzyme digested and sequenced next