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Method for Specific Integration of
T7 RNA Polymerase Gene into the Chromosome of Corynebacteria
- T7 Promoter based Shuttle Vector and Shuttle Vector System
Introduction
E.coli has been the host of choice for
the production of recombinant proteins since the last many
years. However being a gram negative bacteria, the secretion
of proteins is limited in E.coli. It forms inclusion bodies
from which the recombinant protein has to be isolated by using
harsh chemical treatment. Besides, not only is the reducing
environment in the cytoplasm not conducive for several proteins,
the periplasmic space of this bacteria has got several proteases,
which degrade the expressed proteins reducing their yield
considerably. For these reasons, a method for effectuating
a specific integration of T7 RNA polymerase gene into the
chromosomal DNA of Corynebacteria to obtain high success rates
of getting the desired strain .has been developed. This enable
to construct E.coli Cornebacteria shuttle vector as well as
Cornebacteria - T7 shuttle vector system.
The method involve integration of T7 RNA
polymerase gene into the chromosome of corynebacteria (Cacetoacidophilum).
The said method for specific integration uses an E.coli plasmid
pGP1-2 carrying the gene for kanamycin resistance, the genes
for T7 RNA Polymerase and the cl repressor. This plasmid is
digested with restriction enzyme Bam H1 and ligated to the
Sau3A1dugested genomic DNA of C, acetoacidophilum.. Thereafter
a ligation mixture is used to transform C, acetoacidophilum..
protoplasts. Transformants are then screened for Kanamycin
resistance and seniitivity to aminoglycoside such as streptomycin,
to ensure targeting of plasmid vector pGP1-2 into the chromosome
of C, acetoacidophilum. The process will lead to the modification
of the chromosomal DNA of C, acetoacidophilum, which now enables
the said bacterium designated B-30T7R to express T7 RNA polymerase.
These cells are then processed for isolation of pGP1-2 to
detect plasmid DNA. The absence of plasmid DNA establishes
that the plasmid has integrated into the chromosome of the
cell. It was also noticed that this chromosomal integration
did not affect the growth of this strain. Figure 1 outlines
the strategy adopted for the integration of T7 RNA polymerase
gene of plasmid pGP1-2 into the genomic DNA of C, acetoacidophilum.
Special Features:
Screening of the clones is simple and
cost effective No expensive chemical is required for regulation
No adverse effect is noticed on cell growth There is no protease
induction when the temperature is raised to 400 C Expensive
chemicals is not required Provide a novel shuttle vector pBKET29aS
and a novel vector system, Provides a method for obtaining
optimum expressed proteins in a transformed gram positive
bacteria.
Prospective Users:
Pharmaceutical industries
Type of Technology:
Process
Status of IPR Protection:
Indian Patent Application No 96/DEL/2002
dated 5.2.2002 with title "Method for Specific integration
of T7 RNA Polymerase gene into the Chromosome of Corynebacteria
and resultant novel Corynebacteria -T7 promoter based shuttle
vector and shuttle vector system "
Contact for
more information
The Director
Foundation for Innovation and Technology Transfer
Indian Institute of Technology Delhi
Hauz Khas, New Delhi-110016
Tel : 91-011-26597167, 26857762, 26581013
Fax : 91-011-26851169
E-mail : mdfitt@gmail.com
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