Team:BCCS-Bristol/Calendar-Notebook/11 July 2008

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Revision as of 13:57, 24 July 2008

Home	The Team	The Project	Submitted Parts	Modelling	Wet Lab	Calendar	Miscellaneous

Used the 0.3% swimming agar from yesterday and the overnight culture that gave us some lively bacteria. Made 2 wells in the plates using a pippette tip in the left hole put some 7% aspartate solution, in the right we put some water (control). then innnoculated in centre of plate. put aspartate in well in the morning and innoculated afternoon (arond 5 hours later) to allow chemotactic gradient to set up.

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+<html><link rel="stylesheet" href="http://www.chofski.co.uk/iGEM/bccs-igem.css" type="text/css"></html>
+__NOTOC__
+<div class="bccsNavBar">
+{|  align="center"
+!align="center"|[[Team:BCCS-Bristol|Home]]
+!align="center"|[[Team:BCCS-Bristol/Team|The Team]]
+!align="center"|[[Team:BCCS-Bristol/Project|The Project]]
+!align="center"|[[Team:BCCS-Bristol/Parts|Submitted Parts]]
+!align="center"|[[Team:BCCS-Bristol/Modeling|Modelling]]
+!align="center"|[[Team:BCCS-Bristol/Notebook|Wet Lab]]
+!align="center"|[[Team:BCCS-Bristol/Calendar|Calendar]]
+!align="center"|[[Team:BCCS-Bristol/Misc|Miscellaneous]]
+|}
+<br>
+</div>
 Used the 0.3% swimming agar from yesterday and the overnight culture that gave us some lively bacteria. Made 2 wells in the plates using a pippette tip in the left hole put some 7% aspartate solution, in the right we put some water (control). then innnoculated in centre of plate. put aspartate in well in the morning and innoculated afternoon (arond 5 hours later) to allow chemotactic gradient to set up.