Team:UPO-Sevilla/Notebook/08 10
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<h1>August, 10th</h1> | <h1>August, 10th</h1> | ||
- | <h2> | + | <h2>Production Team</h2> |
- | + | <p>We repeated SDM reactions for <i>fecA*</i> (UPO28) and <i>gltD**</i> (UPO17) from the beginning. This time we used <i>Taq expand enzyme</i> instead of <i>Pfu</i>. In the results, we did not obtain any product of amplification in the first PCR reaction of SDM. Next we made the second PCR reaction of SDM by using the former PCR reaction products of SDM. Again the results were not satisfactory.</p> | |
+ | |||
+ | <h2>Assembly Team</h2> | ||
<p>Transformation of <i>E. coli</i> DH5α with ligations made the day before.</p> | <p>Transformation of <i>E. coli</i> DH5α with ligations made the day before.</p> | ||
- | <p> | + | <p>BamI-PstI digestions were analyzed by 1% agarose electrophoresis gel: colony 4 and 5 were positive.</p> |
+ | |||
+ | <p>The 2+28 and 28+3 day before transformation plates had not white colonies. Colonies from UPO7+2+28 plate were strange. We will repeat these devices using low copy vectors. We set up inocula of positive candidate colonies.</p> | ||
+ | |||
+ | <p>We made preparative digestion of UPO 4, 5 and 11 (in Mr. Gene vector) and ran them in 1% agarose gel. The spots were purified using GFX. Ligations with pSB1C3 and transformations were made.</p> | ||
+ | |||
+ | |||
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Latest revision as of 00:26, 27 October 2010
August, 10th
Production Team
We repeated SDM reactions for fecA* (UPO28) and gltD** (UPO17) from the beginning. This time we used Taq expand enzyme instead of Pfu. In the results, we did not obtain any product of amplification in the first PCR reaction of SDM. Next we made the second PCR reaction of SDM by using the former PCR reaction products of SDM. Again the results were not satisfactory.
Assembly Team
Transformation of E. coli DH5α with ligations made the day before.
BamI-PstI digestions were analyzed by 1% agarose electrophoresis gel: colony 4 and 5 were positive.
The 2+28 and 28+3 day before transformation plates had not white colonies. Colonies from UPO7+2+28 plate were strange. We will repeat these devices using low copy vectors. We set up inocula of positive candidate colonies.
We made preparative digestion of UPO 4, 5 and 11 (in Mr. Gene vector) and ran them in 1% agarose gel. The spots were purified using GFX. Ligations with pSB1C3 and transformations were made.
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