Team:Cambridge/Gibson/Introduction

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(Gibson Assembly)
(Gibson Assembly)
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Gibson Assembly is a cutting-edge DNA ligation technique developed by Dan Gibson at JCVI in 2009 [http://www.nature.com/nmeth/journal/v6/n5/abs/nmeth.1318.html].  
Gibson Assembly is a cutting-edge DNA ligation technique developed by Dan Gibson at JCVI in 2009 [http://www.nature.com/nmeth/journal/v6/n5/abs/nmeth.1318.html].  
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It is an enzymatic assembly technique for ligating sequences of DNA with short overlapping end sections (~40 bp). These overlapping regions can be easily added to the ends of a length of DNA by using PCR with primers which have added "flaps".
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It is an enzymatic assembly technique for ligating two or more sequences of DNA when they have overlapping end sequence at their joining point (~40bp). These overlapping regions can be easily added to the ends of any length of DNA by using PCR with primers which have added "flaps". Thus PCR followed by Gibson allows you to join any two blunt ended pieces of DNA.
== Advantages ==
== Advantages ==

Revision as of 20:00, 23 October 2010