Team:Harvard/Template:NotebookDataJuly3

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(Construction of OZ052 and OZ123: Joining the Finger with Homology regions)
(Transformation for OZ plasmids)
 
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Our concentrations were better than they have been in the past; notably, after the addition of buffer P2, our solution actually turned a bright blue (indicating lysis of the cells), which we had not seen before.
Our concentrations were better than they have been in the past; notably, after the addition of buffer P2, our solution actually turned a bright blue (indicating lysis of the cells), which we had not seen before.
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We then ran a PCR on our miniprep product, to check for our desired insert. We used our [[#PCR of expression plasmid cross-junction|usual protocol]] for a PCR of the expression plasmid cross-junction.   
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We then ran a PCR on our miniprep product, to check for our desired insert. We used our usual protocol for a PCR of the expression plasmid cross-junction.   
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====Sending out our expression colonies for sequencing====
====Sending out our expression colonies for sequencing====
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We sent out the samples from [[#Expression Plasmid Sequencing Results|yesterday]] that had no more than 1 SNP for reverse sequencing. In addition, we also sent out 78 and 79 for forward and reverse sequencing.  
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We sent out the samples from yesterday that had no more than 1 SNP for reverse sequencing. In addition, we also sent out 78 and 79 for forward and reverse sequencing.  
*Reverse sequencing: 77.1, 77.3, 77.4, 78.1, 80.1, 80.2, 80.4, 81.1, 81.4, 82.1, 83.4, 84.1, 84.4, Zif268
*Reverse sequencing: 77.1, 77.3, 77.4, 78.1, 80.1, 80.2, 80.4, 81.1, 81.4, 82.1, 83.4, 84.1, 84.4, Zif268
*Forward and reverse sequencing: 781, 78.2, 78.3, 78.4, 79.1, 79.2, 79.3, 79.4
*Forward and reverse sequencing: 781, 78.2, 78.3, 78.4, 79.1, 79.2, 79.3, 79.4
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====Gel Extraction and Isothermal Assembly of OZ fingers+homology====
====Gel Extraction and Isothermal Assembly of OZ fingers+homology====
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We ran a gel extraction of our PCR product from [[#Construction of OZ052 and OZ123: Joining the Finger with Homology regions|yesterday]], so that we could use it for isothermal assembly later.  Strangely, we got bands that were larger than our largest theoretical product.
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We ran a gel extraction of our PCR product from yesterday, so that we could use it for isothermal assembly later.  Strangely, we got bands that were larger than our largest theoretical product.
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*Also replated the 7/20 lambda red culture to see if we can get any good cells (1.5mL).</div>
*Also replated the 7/20 lambda red culture to see if we can get any good cells (1.5mL).</div>
<div id="722" style="display:none">
<div id="722" style="display:none">
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==July 22nd==
==July 22nd==
===Team ZF===
===Team ZF===
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To this end, we redid the PCRs for everything in preparation for the resequencing, using the junction primers and [[#PCR of expression plasmid cross-junction|the previous protocol]].  The resulting gels can be observed below:
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To this end, we redid the PCRs for everything in preparation for the resequencing, using the junction primers and the previous protocol.  The resulting gels can be observed below:
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====Transformation for OZ plasmids====
====Transformation for OZ plasmids====
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Today, we took the results of the isothermal assembly from yesterday and did chemical transformation to introduce the plasmids into the Top 10 ChemComp bacteria, using [[Protocols#Cultures|our protocol for chemical transformations]]. They were left to recover for approximately 1.5 hours. We plated 2 dilutions, 10 ul and 50 ul, and left them overnight at 37* in the incubator.
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Today, we took the results of the isothermal assembly from yesterday and did chemical transformation to introduce the plasmids into the Top 10 ChemComp bacteria, using [https://2011.igem.org/Team:Harvard/Protocols#Cultures our protocol for chemical transformations]. They were left to recover for approximately 1.5 hours. We plated 2 dilutions, 10 ul and 50 ul, and left them overnight at 37* in the incubator.
===Team Wolfe===
===Team Wolfe===

Latest revision as of 20:53, 4 August 2011