Team:University of Ottawa/18 June 2008

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(New page: __TOC__ ==Today in the lab== '''Dan and Matt''' :'''Performed digestion of Tet plasmids''' :<li> T123, D12, and S1 were all digested with NcoI and EcoRV, results appeared to be as expected...)
 
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__TOC__
__TOC__
==Today in the lab==
==Today in the lab==
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:'''Innoculated BY4741'''
:'''Innoculated BY4741'''
:<li>BY4741 was innoculated in 5 mL of 2xYPD + 1/10 20% glucose. However the BY4741 strain was 2 months old.
:<li>BY4741 was innoculated in 5 mL of 2xYPD + 1/10 20% glucose. However the BY4741 strain was 2 months old.
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'''Chris'''
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:<li>Too few colonies grew on incubated plates; linear AtCRE may not have ligated properly
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:'''Comparison of Ligated and Unligated Samples
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:<li>To determine of recircularisation worked, the ligated and unligated samples of AtCRE were run on a 0.8% gel for about 50 minutes. A difference was expected between the two samples when visualised.
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:<li>Neither sample turned up on the gel; concentrations of both were too low. This prompted a re-examination of AtCRE concentrations by absorbance.
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:<li>The concentrations of both samples were incredibly low; ligation did not work.
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:'''Starting Over'''
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:<li>Digested AtCRE: 37 uL DNA, 1 uL EagI, 5 uL Buffer 3, 7 uL water.

Latest revision as of 22:54, 28 October 2008

Untitled Document

 

 


Contents

Today in the lab

Dan and Matt

Performed digestion of Tet plasmids
  • T123, D12, and S1 were all digested with NcoI and EcoRV, results appeared to be as expected however EcoRI should have been used instead of EcoRV in order to obtain a better resolution
  • Innoculated BY4741
  • BY4741 was innoculated in 5 mL of 2xYPD + 1/10 20% glucose. However the BY4741 strain was 2 months old.
  • Chris

  • Too few colonies grew on incubated plates; linear AtCRE may not have ligated properly
  • Comparison of Ligated and Unligated Samples
  • To determine of recircularisation worked, the ligated and unligated samples of AtCRE were run on a 0.8% gel for about 50 minutes. A difference was expected between the two samples when visualised.
  • Neither sample turned up on the gel; concentrations of both were too low. This prompted a re-examination of AtCRE concentrations by absorbance.
  • The concentrations of both samples were incredibly low; ligation did not work.
  • Starting Over
  • Digested AtCRE: 37 uL DNA, 1 uL EagI, 5 uL Buffer 3, 7 uL water.