Team:Yale/Parts

From 2011.igem.org

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<h1>BioBricks:</h1>
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<h1>BioBricks</h1>
The following constructs were generated in the pSB1AK8 vector:
The following constructs were generated in the pSB1AK8 vector:
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<h1>Figures</h1>
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<img src="https://static.igem.org/mediawiki/2011/a/a9/Yale-Cloning-strategy.jpg" />
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Figure 1: Representation of cloning strategy
<groupparts>iGEM011 Yale</groupparts>
<groupparts>iGEM011 Yale</groupparts>
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Revision as of 15:17, 28 September 2011

iGEM Yale

BioBricks

The following constructs were generated in the pSB1AK8 vector:

  • T7 promoter-RBS-eGFP-TEV-RiAFP-His-Terminator
  • T7 promoter-RBS-RiAFP-His-Terminator
  • T7 promoter-RBS-eGFP-ZeAFP-His-Terminator
  • T7 promoter-RBS-His-eGFP-TEV-TmAFP-Terminator
  • T7 promoter-RBS-His-eGFP-TmAFP-Terminator
  • T7 promoter-RBS-His-MBP-TEV-TmAFP-Terminator

In the pSB1A3 vector:

  • RBS-ZeAFP
  • In the pSB1C3 vector (submitted to the registry, parts BBa_K652000 to BBa_K652004):
  • T7-RBS-eGFP-TEV-RiAFP-His-Terminator
  • T7-RBS-RiAFP-His-Terminator
  • T7-RBS-His-eGFP-TEV-TmAFP-Terminator
  • T7-RBS-eGFP-TmAFP-His-Terminator
  • RBS-ZeAFP-Terminator

A plasmid containing the TmAFP antifreeze protein was kindly provided by the Fass lab. A plasmid containing the type III ZeAFP antifreeze protein was kindly provided by the Davies lab. The DNA sequence encoding the 12kDa RiAFP was codon-optimized for E. coli, synthesized, and generously sponsored by Integrated DNA Technologies.

All genes were PCR-amplified with primers of the following form:
  • Forward primer: Biobrick prefix-RBS-20bp homology to start of gene
  • Reverse primer: Reverse complement of 20bp homology to end of gene-TAA-terminator-suffix

All primer designs can be found in the protocols section.

PCR products were PCR purified and gel purified, then cut with XbaI and PstI and ligated to the pSB1AK8 plasmid (containing a T7 promoter) cut with SpeI and PstI. Successful ligation was verified by colony PCR, a double digest, and sequencing. Several antifreeze constructs were transferred from the pSB1AK8 vector to the pSB1C3 vector for submission to the registry. The pSB1C3 linearized vector and the biobricks in the pSB1AK8 vector were digested with EcoRI and PstI. The pSB1AK8 vector was CIP treated prior to ligation. Colonies were selected on chloramphenicol plates, and colony PCR and sequencing were used to verify the constructs.

Figures

<img src="Yale-Cloning-strategy.jpg" /> Figure 1: Representation of cloning strategy <groupparts>iGEM011 Yale</groupparts>