Difference between revisions of "Part:BBa K4268001:Experience"
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| − | [[File: T-suny-oneonta-t7-capsid assembly protein colony PCR figure.png|500px|thumb|center|Figure 1: Colony PCR of five colonies (clones) suspected of | + | [[File: T-suny-oneonta-t7-capsid assembly protein colony PCR figure.png|500px|thumb|center|Figure 1: Colony PCR of five colonies (clones) suspected of containing the Capsid Assembly Protein insert. The insert length is 768bp and the predicted size of the PCR product when using VF/VR primers is 1073 bp.]] |
| − | The gel indicates that | + | The gel indicates that colonies 1 and 2 are likely to contain the correct insert and thus, the Capsid Assembly Protein was successfully cloned into a Level 0 Golden Gate Assembly basic part. |
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<I>Username</I> | <I>Username</I> | ||
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| − | Enter the review | + | Enter the review information here. |
|}; | |}; | ||
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Latest revision as of 18:21, 8 October 2022
The part was received, resuspended, and cloned into the level 0 Golden Gate vector, PSB1C00. The ligation was then transformed into DH5α cells. After overnight growth, white colonies (indicative of a replacement of the RFP reporter cassette) were subjected to screening for the correct insert using colony PCR with the VF/VR primer pair.
The gel indicates that colonies 1 and 2 are likely to contain the correct insert and thus, the Capsid Assembly Protein was successfully cloned into a Level 0 Golden Gate Assembly basic part.
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UNIQ4638f3866825d19c-partinfo-00000000-QINU UNIQ4638f3866825d19c-partinfo-00000001-QINU