Team:Lethbridge/Notebook/Lab Work/Group2
From 2011.igem.org
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While these other aspects continue to elude success a plasmid preparation of SO4261, the ten residue arginine tag with a double transcriptional terminator, is transformed and a glycerol stock of it is made is made. <br> | While these other aspects continue to elude success a plasmid preparation of SO4261, the ten residue arginine tag with a double transcriptional terminator, is transformed and a glycerol stock of it is made is made. <br> | ||
'''Week 8 June 20 - 26''' <br> | '''Week 8 June 20 - 26''' <br> | ||
- | The xylE from puc19 is assembled with the arginine tag. The miscellaneous parts are also re-assembled into psb1c3. Both through PCR and restriction the gels do not show a positive result for the xylE-arg tag assembly. A blunt end ligation of mms6 into puc19 shows some white colonies. | + | The xylE from puc19 is assembled with the arginine tag. The miscellaneous parts are also re-assembled into psb1c3. Both through PCR and restriction the gels do not show a positive result for the xylE-arg tag assembly. A blunt end ligation of mms6 into puc19 shows some white colonies.<br> |
'''Week 9 June 27 - July 3''' <br> | '''Week 9 June 27 - July 3''' <br> | ||
- | The miscellaneous parts are restricted and run on a | + | 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> | ||
+ | <br> | ||
'''Week 11 July 11 - 17''' <br> | '''Week 11 July 11 - 17''' <br> | ||
'''Week 12 July 18 - 24''' <br> | '''Week 12 July 18 - 24''' <br> |
Revision as of 04:08, 15 September 2011
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