Team:WashU/Week6
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- | + | First, we reinnoculated the ligation cultures.<br> | |
- | + | Then, we maxipreped PsbA2 and used the nanodrop to see how much DNA resulted from the prep. | |
- | + | Next, we digested the ligations, miniprepped and digested them, made a gel, and ran the gel. [PICTURE] | |
- | + | In addition, we started a 20 degree culture of <i>E. coli</i> with the Z construct and our construct CS42S. | |
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- | + | We miniprepped the <i>E. coli</i>which had taken up double plasmids (Z and C plasmids). We digested these and then ran them on a gel. [PICTURE] | |
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+ | Finally, we replated ligation 2, our most successful ligation of plasmid PSL2131 and construct CS42S. | ||
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Revision as of 19:36, 19 July 2012