Team:BYU Provo/Notebook/Cholera - Enzyme/September/Period2/Dailylog
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+ | <font size="4">'''9/18/13'''</font> | ||
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+ | We transformed the DspB in the pet15b plasmid into the BL21 strain of competent E. Coli cells. We then set up overnights of Colony 1 of DspB/pIG91 and Colony 1 of AmyA/pIG91. | ||
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+ | We also set up overnights of V. cholerae in preparation for setting up and running our Enzyme Assay on Friday in order to test the enzymatic action of AmyA in breaking down V. cholerae biofilms. We will use various amounts of or purified AmyA protein with urea as a positive control and untreated biofilm as a negative control. | ||
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+ | <font size="4">'''9/19/13'''</font> | ||
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+ | We ran plasmid preps for our DspB/pIG91 and AmyA/pIG91 overnights from yesterday using the plasmid prep protocol on the protocol page. The purified plasmids were labeled and placed in the freezer. | ||
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+ | <font size="4">'''9/20/13'''</font> | ||
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+ | We revised our Enzyme Assay protocol today (see Enzyme Assay Revised on protocols page). Rather than growing our biofilms in the 96-well plate, we are going to grow them and run all the treatments in test tubes. In the 96-well plate we were seeing too much variation in growth conditions from the interior of the plate to the exterior as the wells have different air flows and evaporation rates. We will set up our assay to test AmyA enzymatic degradation of V. cholerae biofilms tomorrow. | ||
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+ | <font size="4">'''9/21/13'''</font> | ||
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+ | We set up our large-scale AmyA Enzyme Assay using the following setup. We will test AmyA at different concentrations and over different time periods to find the best enzymatic response. | ||
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Revision as of 03:08, 23 September 2013
Cholera - Enzymes Notebook: September 15 - September 27 Daily Log
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9/16/13 The
9/18/13 We transformed the DspB in the pet15b plasmid into the BL21 strain of competent E. Coli cells. We then set up overnights of Colony 1 of DspB/pIG91 and Colony 1 of AmyA/pIG91. We also set up overnights of V. cholerae in preparation for setting up and running our Enzyme Assay on Friday in order to test the enzymatic action of AmyA in breaking down V. cholerae biofilms. We will use various amounts of or purified AmyA protein with urea as a positive control and untreated biofilm as a negative control.
9/19/13 We ran plasmid preps for our DspB/pIG91 and AmyA/pIG91 overnights from yesterday using the plasmid prep protocol on the protocol page. The purified plasmids were labeled and placed in the freezer.
9/20/13 We revised our Enzyme Assay protocol today (see Enzyme Assay Revised on protocols page). Rather than growing our biofilms in the 96-well plate, we are going to grow them and run all the treatments in test tubes. In the 96-well plate we were seeing too much variation in growth conditions from the interior of the plate to the exterior as the wells have different air flows and evaporation rates. We will set up our assay to test AmyA enzymatic degradation of V. cholerae biofilms tomorrow.
9/21/13 We set up our large-scale AmyA Enzyme Assay using the following setup. We will test AmyA at different concentrations and over different time periods to find the best enzymatic response.
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