Team:Freiburg/Description

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(Difference between revisions)
(The Concept)
(Bacterial artificial chromosom)
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Molecular Microbiology 70 (2008) 341–351<br/><br/>
Molecular Microbiology 70 (2008) 341–351<br/><br/>
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==Bacterial artificial chromosom==
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==Bacterial artificial chromosome==
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Bacterial artificial chromosome, a vector, based on the single copy plasmid F-factor from Escherichia coli, which can host inserts from bacteria or other sources between 150 and 350 kilo base pairs (kbp) but up to 700 kbp, and hold them for more then 100 generations. The BAC vector has some common gene components that are: the oriS and repE which are responsible for the not bidirectional replication. The parA and parB genes which control the copy number of the BAC. In addition to it there is a selection marker commonly an antibiotic resistance and finally the cloning segment with the restrictions sites. This cloning segment will be flanked by a T7 and SP6 promoter. Usually BACs are used to build up libraries or genetically screening, through its stability. <br/>
Bacterial artificial chromosome, a vector, based on the single copy plasmid F-factor from Escherichia coli, which can host inserts from bacteria or other sources between 150 and 350 kilo base pairs (kbp) but up to 700 kbp, and hold them for more then 100 generations. The BAC vector has some common gene components that are: the oriS and repE which are responsible for the not bidirectional replication. The parA and parB genes which control the copy number of the BAC. In addition to it there is a selection marker commonly an antibiotic resistance and finally the cloning segment with the restrictions sites. This cloning segment will be flanked by a T7 and SP6 promoter. Usually BACs are used to build up libraries or genetically screening, through its stability. <br/>
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To have a BAC which contains our precipitator, the lysis cassette and the most parts of our light inducible systems should not to be underestimated. It would be an easy, timesaving and stable construct.
To have a BAC which contains our precipitator, the lysis cassette and the most parts of our light inducible systems should not to be underestimated. It would be an easy, timesaving and stable construct.
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O'Connor M, Peifer M, Bender W (1989). "Construction of large DNA segments in Escherichia coli". Science 244 (4910): 1307–1312.
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Shizuya H, Birren B, Kim U-J, Mancino V, Slepak T, Tachiiri Y, Simon M (1992). "Cloning and stable maintenance of 300-kilobase-pair fragments of human DNA in Escherichia coli using an F-factor-based vector". Proc Natl Acad Sci USA 89 (18): 8794–8797.
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Revision as of 21:08, 20 September 2011


This is the wiki page
of the Freiburger student
team competing for iGEM 2011.
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