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From 2012.igem.org

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Contents 1 June 1.1 June 10th-16th 1.1.1 June 13th, Wednesday 1.1.2 June 14th, Thursday 1.1.3 June 15th, Friday 1.2 June 17th-23rd 1.3 June 24th-30th 1.3.1 June 28th, Wednesday 2 July

June

June 10th-16th

June 13th, Wednesday

• Set up PCR for four fragments of the nah operon as well as the pBMT-1 backbone, using primers designed to mutate cut-sites concurrently with Gibson Assembly. Also set up a PCR for the entire nah operon. Due to length of the fragments, a longer extension time was chosen.
• If Gibson Assembly fails, but we are able to PCR the entire 10kb nah operon, an alternate method of mutation using three sequential site-directed mutageneses will be pursued.
  • Work done by: Caleb, Claire, Dylan, Spencer, Steven, and Swati

June 14th, Thursday

• PCR only amplified nah1, nah3, and nah4 - longer fragments (nah2, the full nah operon, and pBMT-1) were not identified on the PCR product gel. Set up another PCR with shorter extension time.

June 15th, Friday

• PCR of four out of five products visible on gel. Set up PCR of pBMT-1, final fragment required for Gibson Assembly of the nah operon.

June 17th-23rd

June 24th-30th

June 28th, Wednesday

• Gel purified arsR construct

July

=August=