Team:Grenoble-EMSE-LSU/Documentation/Notebook/August

From 2013.igem.org

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                                           <h3>Thursday</h3>
                                           <h3>Thursday</h3>
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    <p>- PCR of mRFP and KR for pJT106b with EcoRI restriction sites on both primers</br>
+
    <p></p>
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- Try to digest mRFP and KR with EcoRI but forget pJT106b so there is no control, don’t know if the digestion was efficient or not.</br></p>
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                                           <h3>Friday</h3>
                                           <h3>Friday</h3>
    <p></p>
    <p></p>
                                         <h2>Week 2</h2>
                                         <h2>Week 2</h2>
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                                          <p>- Have some trouble with the digestion of pJT106b. The restriction enzyme used - EcoRI - seems to have a star-activity and cut the plasmid everywhere.</br>
 +
After these 3 experiences it can be said that the problem comes from the plasmid since the buffers and the RE work on and another plasmid.</br>
 +
After talking about it with the advisors, they said that during the Miniprep, it still may be some ethanol after the elution. And ethanol can led to the inhibition or the star-activity of the RE.</br>
 +
To avoid this, before the elution, the column is warm up to 70°C for 5min in order for the ethanol to evaporate.</br>
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</p>
                                           <h3>Monday</h3>
                                           <h3>Monday</h3>
    <p></p>
    <p></p>
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    <p></p>
    <p></p>
                                             <h2>Week 3</h2>
                                             <h2>Week 3</h2>
 +
- Redo the PCR for pJT106b with mRFP and KR, and do another miniprep with the new protocol to extract pJT106b.</br>
 +
- Try again the digestion with lower amount of DNA to be sure that it works to avoid losing to much DNA. it works for different different gel but another problem was encountered. After the gel extraction, done to purified the vector the amount of DNA was too low (<2ng/µL) to do the next experiences. So different wells were use for one column but it was  still not enough (<5ng/µL for 50µL). Try to precipitate the DNA in a fewer volume but it didn’t reach the expected goal.</br>
 +
10 wells were used for 1 column, and the concentration that we got was of 16.6ng/µL for 30µL. It is not a lot but it is enough for doing the dephosphorylation - to prevent the plasmid to recircularise.</br>
                                               <h3>Monday</h3>
                                               <h3>Monday</h3>
                                               <h3>Tuesday</h3>
                                               <h3>Tuesday</h3>

Revision as of 19:17, 24 September 2013

Grenoble-EMSE-LSU, iGEM


Grenoble-EMSE-LSU, iGEM

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