Team:Lethbridge/Notebook/Lab Work/Group2
From 2011.igem.org
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The miscellaneous parts are restricted and run on a gel along with mini-preps of the mms6 colonies that were grown in liquid LB media and while all the remaining miscellaneous parts are consistent with expected results, the mms6 is blank on the gel. A PCR of the mms6 in puc19 also gives the same result on an agarose gel. The xylE and re-assembled, plated, possible colonies are picked and grown in liquid LB media and cultures are mini-prepped.<br> | The miscellaneous parts are restricted and run on a gel along with mini-preps of the mms6 colonies that were grown in liquid LB media and while all the remaining miscellaneous parts are consistent with expected results, the mms6 is blank on the gel. A PCR of the mms6 in puc19 also gives the same result on an agarose gel. The xylE and re-assembled, plated, possible colonies are picked and grown in liquid LB media and cultures are mini-prepped.<br> | ||
'''Week 10 July 4 - 10''' <br> | '''Week 10 July 4 - 10''' <br> | ||
- | After restricting and running on a gel all the xylE-arg tag assemblies came back negative. | + | After restricting and running on a gel all the xylE-arg tag assemblies came back negative. The lack of progress on xylE and mms6 being suspicious, new approachs are used. PCR products of both xylE and mms6 with the fusion standard are gel extracted using a Qiagen gel extraction kit. These gel extractions have DNA presence confirmed on a gel and are then used in a blunt end ligation with puc19 and a restriction free cloning attempt with psb1c3. Neither first attempt succeeds. <br> |
'''Week 11 July 11 - 17''' <br> | '''Week 11 July 11 - 17''' <br> | ||
- | <br> | + | Sequencing data from samples sent to genewiz come back showing k331025 and k331008, a signal sequence for localization to the outer membrane of ''E. coli'' is the correct sequence and confirmed suspicions regarding what was thought to be xylE in puc19. Six more attempts at restriction free cloning fail to produce results, including attempts to use non gel extracted PCR products that have had the original plasmid digested. <br> |
'''Week 12 July 18 - 24''' <br> | '''Week 12 July 18 - 24''' <br> | ||
'''Week 13 July 25 - 31''' <br> | '''Week 13 July 25 - 31''' <br> |
Revision as of 04:52, 15 September 2011
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