Sbb14-Dingguo Chen: Difference between revisions
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==[[User:Dingguo Chen|Dingguo Chen]] 10:08, 18 March 2014 (PST)== | ==[[User:Dingguo Chen|Dingguo Chen]] 10:08, 18 March 2014 (PST)== | ||
Setting up digestion reactions for PCR products | Setting up digestion reactions for PCR products | ||
Results: | Results: | ||
not finished. Digested products were melt in ADB buffered and stored for | |||
next lab. | |||
Revision as of 12:31, 19 March 2014
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Team3: Organism: Thermotoga maritima Amino Acids: A,C,D,E,F,G,H,I,K,L
Protocols:
Design construction Files for All the Amino Acids.
Lab:
PCR(use expand polymerase) --> Run gel to check size of PCR parts --> Digestion Vector Digest Ligation(digest product + Vector + Ligase + ...)
--> Transformation --> Colonies selection and Screening.
Dingguo Chen 11:13, 4 March 2014 (PST)
PCR out the parts from the genome based on the designed construction files.
Dingguo Chen 12:20, 6 March 2014 (PST)
Run gel for soeing PCRs(Ala, Leu) and make sure they have the the correct size.
Run gel to check size of simple PCR products for other amino acides, then do zymo cleanup.
Results: All 4 soeing parts seem to have the correct sizes. for the normal PCRs, all but gul1 look good.
Dingguo Chen 11:45, 7 March 2014 (PST)
1. Redo PCRs for Glu1 2. Setting up Soeing PCRs.
Dingguo Chen 11:30, 11 March 2014 (PST)
Ran gel for PCR(Ala,and Leu). Results:
Soeing PCR on Ala doesn't work and need to redo.
Dingguo Chen 11:53, 13 March 2014 (PST)
Run gel for Ala Soeing PCR-increase the concentration of the templates to 5 ul each this time.
Results: We got PCR part that have the desired size.
Plan for next lab:
Do digestion and gel purification on all the PCR products.
Dingguo Chen 10:08, 18 March 2014 (PST)
Setting up digestion reactions for PCR products Results: not finished. Digested products were melt in ADB buffered and stored for next lab.
