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Team:UFAM Brazil/7-10-2014
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| - | The colonies from the transformation in Escherichia coli DH5α and RR1 with the Biobrick Transformation Efficiency Kit as a control and the DNA diluted from the 2013 | + | The colonies from the transformation in <i>Escherichia coli</i> DH5α and RR1 with the Biobrick Transformation Efficiency Kit as a control and the DNA diluted from the 2013 DNA Part Kit (BBa_E0840) greeeew!!!! Although we were not sure if we could trust in the results. We made an inoculum using liquid LB medium from the transformed cells (BBa_E0840 and Transformation Efficiency Kit) to make a miniprep and check the electrophoretical profile from the transformation. To get more satisfactory results we are going to repeat the transformation process with only the lining RR1, shown in the following : |
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Revision as of 21:09, 15 October 2014
07/10/2014 | ||
The colonies from the transformation in Escherichia coli DH5α and RR1 with the Biobrick Transformation Efficiency Kit as a control and the DNA diluted from the 2013 DNA Part Kit (BBa_E0840) greeeew!!!! Although we were not sure if we could trust in the results. We made an inoculum using liquid LB medium from the transformed cells (BBa_E0840 and Transformation Efficiency Kit) to make a miniprep and check the electrophoretical profile from the transformation. To get more satisfactory results we are going to repeat the transformation process with only the lining RR1, shown in the following : - Negative control - no DNA; - Positive control from the Transformation Efficiency Kit; - BBa_E0840 (Biodetection Biobrick); - BBa_K346004 (Bioaccumulation Biobrick). We have followed iGEM’s Transformation Protocol. LB plates – agar with 20ug/ml of chloranphenicol. Waiting for our synthesis to arrive!! | ||
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