Team:Washington/Magnetosomes/Background

From 2011.igem.org

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[[File:Igem2011 GibsonToolkit.png|left|300px|link=https://2011.igem.org/Team:Washington/Magnetosomes/GibsonVectors]]  
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;'''What's in the Gibson Assembly Toolkit?'''<br/>
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;'''What's in the Gibson Assembly Toolkit?'''
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* Five plasmid backbones <br/>
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* Five plasmid backbones
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* 2 High copy vectors for gene extraction and cloning <br/>
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* 2 High copy vectors for gene extraction and cloning: '''pGA1A3, pGA1C3'''
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** pGA1A3, pGA1C3 <br/>
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* 1 medium copy expression vector: '''pGA3K3'''
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* 1 medium copy expression vector <br/>
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* 2 low copy expression vectors: '''pGA4A5, pGA4C5'''
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** pGA3K3 <br/>
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* 2 low copy expression vectors <br/>
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** pGA4A5, pGA4C5 <br/>
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Revision as of 03:46, 23 September 2011


iGEM Toolkits: Background


As with the expansion of the iGEM competition, many iGEM teams have started to investigate the possibility of working with large-scale genomes. Large-scale gene manipulation often requires the use of tools which allow multiple gene inserts as to bring the cloning project from single gene level to a multiple gene level. However, the current BioBrick standard vectors available through iGEM are not designed for multiple-insert cloning. Therefore, the UW iGEM team decided to research methods to improve cloning efficiency and as a result, two "toolkits" were submitted to the registry.



Gibson Assembly Toolkit

To expand on work started by the 2010 UW IGEM team, this year we developed and submitted a set of plasmid backbones for BioBricks that are optimized for Gibson assembly. Based on the bglBrick standard [http://dspace.mit.edu/bitstream/handle/1721.1/46747/BBFRFC21.pdf?sequence=1 RFC 21], these "pGA" vectors comprise the Gibson Assembly Toolkit. These vectors have much higher cloning efficiencies than the equivalent pSB vector and are fully compliant with BioBrick [http://www.synbio.org.uk/gibson/downloads/files/RFC57.pdf RFC 57] developed by the 2010 Cambridge iGEM team.

Igem2011 GibsonToolkit.png
What's in the Gibson Assembly Toolkit?
  • Five plasmid backbones
  • 2 High copy vectors for gene extraction and cloning: pGA1A3, pGA1C3
  • 1 medium copy expression vector: pGA3K3
  • 2 low copy expression vectors: pGA4A5, pGA4C5








Magnetosome Toolkit

In addition, we were also ambitious about assembling a large gene-construct of over 16 kb. Therefore, utilizing our pGA vectors and Gibson cloning methods, the Magnetosome Toolkit was developed with the goal to build magnetic E.Coli; a novel characteristic expressed solely by magnetotactic bacteria, such as Magnetospirillum magneticum strain AMB-1.


Igem2011 MagnetToolkit.png

What’s in the Magnetosome Toolkit?

  • A set of the 18 essential genes for the various steps of magnetosome formation.
  • Our favorite genes in pGA vectors
  • A table compiling individual gene functions from our literature search