Team:Harvard/Template:NotebookDataAugust

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====Redoing the isothermal assembly/transformation for Pos con 77 and the 3 controls====
====Redoing the isothermal assembly/transformation for Pos con 77 and the 3 controls====
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Today we redid the isothermal assembly for Pos con 77, Zif268, OZ052, and OZ123 using our [[Lab_Notebook:_July#Isothermal_Assembly_of_Pos_Con_77.2C_Zif_268.2C_and_OZs|previous protocol]].  We also performed a chemical transformation using Top 10 ChemComp cells, and plated them with 100 ul each plate.  We will have to wait and see whether colonies grow tomorrow.
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Today we redid the isothermal assembly for Pos con 77, Zif268, OZ052, and OZ123 using our previous protocol.  We also performed a chemical transformation using Top 10 ChemComp cells, and plated them with 100 ul each plate.  We will have to wait and see whether colonies grow tomorrow.
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We also performed a cross junction PCR on the isothermal assembly product to make sure that it worked, using our [[Lab_Notebook:_July#PCR_of_expression_plasmid_cross-junction|usual protocol]]. The gel (pictured below) shows appropriately sized bands for the cross junction.
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We also performed a cross junction PCR on the isothermal assembly product to make sure that it worked, using our usual protocol. The gel (pictured below) shows appropriately sized bands for the cross junction.
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In order to further troubleshoot our less-than-ideal gels for our digestion product, we ran a third digestion reaction, using the second recipe. This time we simultaneously digested our oligo, and our cross junction (which had been shown to work before). We also ran the unpurified PCR product from recipe 2 on this gel.  
In order to further troubleshoot our less-than-ideal gels for our digestion product, we ran a third digestion reaction, using the second recipe. This time we simultaneously digested our oligo, and our cross junction (which had been shown to work before). We also ran the unpurified PCR product from recipe 2 on this gel.  
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See [[#Yesterday's last digestion and PCR results|tomorrow's entry]] for the gel image.
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See tomorrow's entry for the gel image.
Our digestion of the cross junction appeared to have worked, while once again, we got unusually large bands for our oligo.
Our digestion of the cross junction appeared to have worked, while once again, we got unusually large bands for our oligo.
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We performed a PCR to clone out Zif268 so that we can later assemble Zif and GFP into our reporter plasmid. We used the Zif clone Forward and Zif clone Reverse primers (Primer index: 148 and 149). We had an annealing temperature of 62* and an extension time of 90 seconds. Our expected product was ~3 kb.
We performed a PCR to clone out Zif268 so that we can later assemble Zif and GFP into our reporter plasmid. We used the Zif clone Forward and Zif clone Reverse primers (Primer index: 148 and 149). We had an annealing temperature of 62* and an extension time of 90 seconds. Our expected product was ~3 kb.
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See [[#Yesterday's last digestion and PCR results|tomorrow's entry]] for the gel. Our PCR appeared to have worked, and we have a strong band at our expected product size.
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See tomorrow's entry for the gel. Our PCR appeared to have worked, and we have a strong band at our expected product size.
===Team Wolfe===
===Team Wolfe===
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Once again, we got unusually low yields. We decided to test the quality of our spec, to see if that was the problem. We grew PZE22G(which does not have spec resistance) in spec to see if it grew. By the end of the day, nothing had grown.  
Once again, we got unusually low yields. We decided to test the quality of our spec, to see if that was the problem. We grew PZE22G(which does not have spec resistance) in spec to see if it grew. By the end of the day, nothing had grown.  
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Still, we decided to PCR the miniprep product, since any DNA that is in the product should be amplified. We performed our [[Lab_Notebook:_July#PCR_of_expression_plasmid_cross-junction|usual protocol]] for a cross junction PCR, but we repeated the reaction for 30 cycles.  
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Still, we decided to PCR the miniprep product, since any DNA that is in the product should be amplified. We performed our usual protocol for a cross junction PCR, but we repeated the reaction for 30 cycles.  
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'''PCRs of Zif 268 and GFP'''
'''PCRs of Zif 268 and GFP'''
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We decided to perform more PCRs to clone out Zif 268, since it will have to be gel purified. This reaction had the same conditions as [[#PCR of Zif268 to create GFP Reporter Strain|yesterday's]].
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We decided to perform more PCRs to clone out Zif 268, since it will have to be gel purified. This reaction had the same conditions as yesterday's.
We also received the GFP plate today, so we decided to perform a colony PCR in order to get out the sequence that encodes GFP. We used our GFP Forward and GFP Reverse (Primer Index: 146 and 147) for the reaction, had an annealing temperature of 58*, and an extension time of 30 seconds. The expected product size was ~700 bp.  
We also received the GFP plate today, so we decided to perform a colony PCR in order to get out the sequence that encodes GFP. We used our GFP Forward and GFP Reverse (Primer Index: 146 and 147) for the reaction, had an annealing temperature of 58*, and an extension time of 30 seconds. The expected product size was ~700 bp.  

Revision as of 22:12, 19 September 2011