Team:Harvard/Template:NotebookDataJuly4

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===Team ZF===
===Team ZF===
====Result of OZ052 and OZ123 Transformation====
====Result of OZ052 and OZ123 Transformation====
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[[#Transformation for OZ plasmids|Last Friday]] we plated out the transformed bacteria for the two OZ controls in 10 ul and 50 ul volumes.  They both yielded colonies, but the 10 ul plates only had a handful while the 50 ul plates had around 15-20 colonies each.  We picked four colonies from each plate and grew them in LB/spec so that tomorrow we can perform a miniprep and send them off for sequencing.  We should know the final verdict by Wednesday regarding which ones are good or bad.
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Last Friday we plated out the transformed bacteria for the two OZ controls in 10 ul and 50 ul volumes.  They both yielded colonies, but the 10 ul plates only had a handful while the 50 ul plates had around 15-20 colonies each.  We picked four colonies from each plate and grew them in LB/spec so that tomorrow we can perform a miniprep and send them off for sequencing.  We should know the final verdict by Wednesday regarding which ones are good or bad.
====Glycerol stockmaking====
====Glycerol stockmaking====
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We got the sequencing results back from last Friday, and took the following colonies to make into glycerol stock solutions: 77.1, 79.2, 80.1, 81.1 (x2 for both FH bottom and Myc 198), 82.1, 83.4, 84.1, Zif268.  These colonies are a subset of the "good" colonies from our [[Lab_Notebook:_July#Sequencing_Results|sequencing results]] from Sunday.  We mixed 120 ul of bacteria in mid-log with 300 ul of 80% glycerol to make the final solution, which was stored at -80 degrees C.
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We got the sequencing results back from last Friday, and took the following colonies to make into glycerol stock solutions: 77.1, 79.2, 80.1, 81.1 (x2 for both FH bottom and Myc 198), 82.1, 83.4, 84.1, Zif268.  These colonies are a subset of the "good" colonies from our sequencing results from Sunday.  We mixed 120 ul of bacteria in mid-log with 300 ul of 80% glycerol to make the final solution, which was stored at -80 degrees C.
====Restriction enzyme test====
====Restriction enzyme test====
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*OZ123 - 76, 126</div>
*OZ123 - 76, 126</div>
<div id="726" style="display:none">
<div id="726" style="display:none">
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==July 26==
==July 26==
===Team ZF===
===Team ZF===
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The miniprep lysis step looked good, and the samples turned blue after lysis.
The miniprep lysis step looked good, and the samples turned blue after lysis.
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We then performed a junction PCR using the [[Lab_Notebook:_July#PCR_of_expression_plasmid_cross-junction|previous protocol]], and checked the products on a gel:
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We then performed a junction PCR using the previous protocol, and checked the products on a gel:
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===Team ZF===
===Team ZF===
====Transformation plating results====
====Transformation plating results====
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We got no growth on any of the plated transformed bacteria for either the ElectroComp or ChemComp bacteria.  To check whether the isothermal assembly itself was the problem, we ran a junction PCR using our [[Lab_Notebook:_July#PCR_of_expression_plasmid_cross-junction|previous protocol]] on the isothermal assembly mix, along with a positive control (Myc981):
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We got no growth on any of the plated transformed bacteria for either the ElectroComp or ChemComp bacteria.  To check whether the isothermal assembly itself was the problem, we ran a junction PCR using our previous protocol on the isothermal assembly mix, along with a positive control (Myc981):
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Latest revision as of 19:22, 3 August 2011