Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Friday, 19 August 2011)
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About the PCR of the lysis cassette for the new Gibson assembly, Nadine found out that she designed the reverse primer on a terminator (BBa_B0010) that was also present 400bp before, allowing the primer to anneal perfectly after 1400bp instead of 1800bp.
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About the PCR of the lysis cassette for the new Gibson assembly, Nadine found out that she designed the reverse primer on a terminator (BBa_B0010) that was also present 400bp before, allowing the primer to anneal perfectly after 1400bp instead of 1800bp. This mistake was also present in the primer designed for the 3-part Gibson assembly, but we didn't notice at this time. She designed a new primer, skipping the final terminator because there will be another terminator in the Gibson-assembled plasmid.

Revision as of 08:02, 22 August 2011