Team:Michigan/Oil Sands
From 2010.igem.org
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Since no nanodrop reading was made for the flu operon, no water was added and only the gel extraction was used | Since no nanodrop reading was made for the flu operon, no water was added and only the gel extraction was used | ||
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+ | '''Gel of constitutive promoter, KAN backbone and flu operon''' | ||
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+ | '''PCR purification of KAN backbone''' | ||
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+ | The PCR purification was performed with the 50 uL digest of the KAN backbone with EcoRI and SpeI according to the protocol in the protocol section of the wiki. | ||
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+ | 250 uL of buffer PB was used to mix with the digest before adding the mixture to the column |
Revision as of 18:11, 12 August 2010