Team:Alberta/Project/Chromosome Assembly
From 2009.igem.org
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Chromosomal AssemblyOnce sizable chunks of synthetic chromosome have been constructed, it becomes necessary to find a manner by which to assemble the pieces together and insert them into the cell, while simultaneously replacing corresponding regions of the original host chromosome. One approach would be to fabricate the entire construct in vitro in the form of a bacterial artificial chromosome (BAC) and then inactivate the host chromosome. However, we have adopted the approach of piecing together the chromosome in vivo by recombining synthetic sections into the original host chromosome. This provides a step-wise means of testing the functionality of smaller gene sets rather than attempting to find errors in an entire minimal chromosome. In Vivo ConstructionThis method requires a technique known as Lambda Red recombination. Synthetic sections produced via the BioBytes method can be transformed through electroporation as linear fragments. Once a fragment is in a cell, the Red recombination genes direct the section to a double crossover event at regions on the chromosome homologous to regions flanking the ends of the synthetic section. This results in the replacement of a large portion of the original chromosome with a synthetic construct. For a fully synthetic genome, this process can be repeated until only the original Ori remains. Advantages of Recombination of Building BAC's
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