User:University of Washington/9 September 2008

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==LuxR from AraC and TetR(Faifan)==
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-Ran gel of the PCR products x14 colonies, got no DNA in all lanes-probably because cells weren't lysed or there weren't any cells at all from the beginning(resuspension wasn't good enough to disperse the cells in dH2O)
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-Resuspended 28 colonies into 20 ul dH2O (14 from yesterday's resuspension, 14 from plate), boiled at 100 degree Celsius for 16 mins.
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-Did Colony PCR again
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*mix 12.6ul dH2O + 2 Buffer + 0.4ul 10mM-dNTP + 0.8ul 50mM-MgCl2 + 1ul 10mM-VF2 + 1ul 10mM-VR + 0.2ul Taq + 2ul Template
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*Thermocycling
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**1 : 95 : 1 min
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**30: 95 : 30 s
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**__: 53 : 30 s
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**__: 72 : 1 min
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**1 : 72 : 7 mins
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**1 : 4 : forever
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-Grew overnight of MG1655Z1 from stock in Tsy
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Back to [[Team:University_of_Washington/Notebook#Notebook]]
Back to [[Team:University_of_Washington/Notebook#Notebook]]

Latest revision as of 22:57, 9 September 2008

LuxR from AraC and TetR(Faifan)

-Ran gel of the PCR products x14 colonies, got no DNA in all lanes-probably because cells weren't lysed or there weren't any cells at all from the beginning(resuspension wasn't good enough to disperse the cells in dH2O)

-Resuspended 28 colonies into 20 ul dH2O (14 from yesterday's resuspension, 14 from plate), boiled at 100 degree Celsius for 16 mins.

-Did Colony PCR again

  • mix 12.6ul dH2O + 2 Buffer + 0.4ul 10mM-dNTP + 0.8ul 50mM-MgCl2 + 1ul 10mM-VF2 + 1ul 10mM-VR + 0.2ul Taq + 2ul Template
  • Thermocycling
    • 1 : 95 : 1 min
    • 30: 95 : 30 s
    • __: 53 : 30 s
    • __: 72 : 1 min
    • 1 : 72 : 7 mins
    • 1 : 4 : forever

-Grew overnight of MG1655Z1 from stock in Tsy


Back to Team:University_of_Washington/Notebook#Notebook