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Introduction of Cloning Plasmids into Agrobacterium tumefaciens

 Last Update: 2021-01-15
 Source: Internet
 Author: User

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Most experiments utilizing Agrobacterium tumefaciens as a vector for the introduction of genes into plant cells commence in Escherichia coli . The sheer size and complexity of the Ti-plasmids precludes their direct manipulation. Thus, insertion is usually into a comparatively small binary vector, which is then propagated in E. coli , before being introduced into A. tumefaciens , where the larger, complementing vir plasmid mediates gene transfer to plants. Typically, the binary plasmid will be based on a broad host range replicon, of IncP, IncQ, or IncW derivation, capable of replication in both bacterial hosts. Its construction will have resulted in the binary plasmid possessing the following features:

1.	A selectable marker for bacterial cells;
2.	A selectable marker for plant cells;
3.	A multiple cloning site (MCS) and/or expression site; and
4.	The Ibft (LB) and right border (RB) from the Ti-plasmid T-DNA, positioned to define a pseudo T-DNA containing the plant selectable marker and the MCS.

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