Difference between revisions of "Team:Potsdam/Protocols"

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<b>1. Aim </b><br>
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<b>1. Aim </b><br><br>
 
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1. Is the insert DNA in the plasmid present or absent? </div>
 
1. Is the insert DNA in the plasmid present or absent? </div>
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2. Much easier than to isolate and purify the vector. </div>
 
2. Much easier than to isolate and purify the vector. </div>
 
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<b> 2. Good to know before the start </b> <br>
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<b> 2. Good to know before the start </b> <br><br>
 
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1. Take typical measures to prevent PCR cross over contamination, keep your bench clean, wear gloves, use sterile tubes and filter pipet tips.
 
1. Take typical measures to prevent PCR cross over contamination, keep your bench clean, wear gloves, use sterile tubes and filter pipet tips.
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<b>3. Are you working with <i> A. E.coli </i> or B. yeast?</b>
 
<b>3. Are you working with <i> A. E.coli </i> or B. yeast?</b>
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<b>A.step by step for <i>E.coli</i>: </b> <br>  
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<b>A.step by step for <i>E.coli</i>: </b> <br> <br>
 
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1. Resuspend colonies. </div>
 
1. Resuspend colonies. </div>

Revision as of 16:21, 31 October 2017

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Our research work

We are describing our research work. Below you can find the protocols we used.

Protocols