Use of Translational Fusions to the Maltose-Binding Protein to Produce and Purify Proteins inPseudomonas syringaeand Assess Their Activity in Vivo

1 January 1996

journal article
Published by Scientific Societies in Molecular Plant-Microbe Interactions®

Vol. 9 (7) , 637-41
https://doi.org/10.1094/mpmi-9-0637

Abstract

A simple approach is described for the production and purification of proteins in Pseudomonas syringae. The strategy involves the use of the tac promoter, the maltose-binding protein, and the broad-host-range vector, pRK415. This approach was used to partially purify two proteins involved in coronatine biosynthesis from P. syringae. The activity of the fusions was demonstrated in vivo in complementation experiments using the appropriate mutants.

Keywords

PROTEINS
FUSIONS
MALTOSE BINDING
SYRINGAE
PURIFY
VIVO
PARTIALLY
BIOSYNTHESIS
PURIFICATION

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