Team:Heidelberg/Delftibactin/DelRest

From 2013.igem.org

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This week the project DelRest was launched.
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In order to clone the Delftibactin cluster from <i>D. Acidovorans </i> into <i> E.coli </i>  we decided to use Gibson cloning. Therefore Gibson primers were designed to amplify our target backbone pSB4K5 with an overlap to DelA. Furthermore the Gibson primer connecting DelOP and DelAG introduces the ribosome binding site BBa_BNILS. Accordingly the Gibson primer for joining DelL with DelOP includes the ribosome binding site BBa_BNILS. The very last gibson primer used to amplify DelL consequently has an overlap to the beginning of the mRFP reporter gene connected to pSB4K5. Check out our vectormap if you are curious about the detailed primer design. The goal of this week was to amplify our previously assembled backbone with the intended overlaps as well as the desired genes from our host organism <i>D. Acidovorans </i>.
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In order to clone the Delftibactin cluster from <i>D. Acidovorans </i> we decided to use Gibson cloning. Therefore Gibson Primers were designed to amplify our target backbone pSB4K5 with an overlap to DelA. Furthermore the Gibson Primer designed to join DelOP with DelAF will introduce the ribosome binding site BBa_BNILS. Accordingly the Gibson Primer designed to join DelL with DelOP will introduce the ribosome binding site BBa_BAGAINNILSYOUNOOB.
 
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Revision as of 23:00, 1 October 2013

Del Rest. Creating a 31 kbp plasmid.

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Methods:

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