lectut btn-202-ppt-l35. genetic transformation
TRANSCRIPT
Genetic
Transformation
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Lecture- 35
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•The gene cloning method described by Stanley Cohen and coworkers
requires the introduction of the recombinant vector molecules into
suitable host cells. These researchers used transformation method to
introduce the recombinant plasmid molecules into E. coli cells.
•Transformation is the entry or introduction of naked DNA into the living
cells. In the year 1944 Oswald Avery, Colin MacLeod and Maclyn
McCarty proved that the genetic transformation discovered by
Frederick Griffith in 1928 in Diplococcus pneumoniae was due to the
introduction of naked DNA into the bacterial cells.
•The transfection method developed by Morton Mandel and Akiko Higa
(1970) for E. coli became the basis for the subsequent bacterial
transformation methods. The transformation of E. coli with the purified
plasmid DNA was achieved for the first time by Stanley Cohen and
coworkers in the year 1972.
INTRODUCTION
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Subsequently, the following organisms/cells of
organisms were transformed for the first time in the
years mentioned in brackets: yeast (1978), cultured
mammalian cells (1980), Drosophila melanogaster
(1982) and cultured plant cells (1983).
In 1987, B. M. Chassy and J. L. Flickinger
introduced the electroporation technique for
transformation of living cells. In the same year,
Theodore Klein, Edward Wolf, Ray Wu and John
Sanford developed high velocity microprojectiles to
deliver DNA into cells.
On the basis of this method a gene gun machine for
commercial use was developed by DuPont company.
Genetic transformation is the entry or
introduction of naked DNA into the living
cells.
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GENETIC TRANSFORMATION METHODS
Stimulation by chemicals
Encapsulation in liposomes
Electroporation
Microprojectile bombardment
Microinjection
Cell perforation using SiC whiskers
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STIMULATION BY CHEMICALS
1970: E. coli was transformed by calcium
chloride and heat shock treatments
1977: Lurquin and Kado demonstrated that
uptake of plasmid DNA by cowpea
protoplasts was stimulated by poly-L-
ornithine (PLO).
PLO, a polycation, possibly stimulates the
uptake of nucleic acids in plant protoplasts
by neutralising their surface charge.
PEG in the presence of calcium ions (CaCl2)
is used for transforming plant protoplasts.
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The technique involves incubating
protoplasts with naked DNA in the presence
of PEG and CaCl2
After gradual dilution of mixture, protoplasts
are collected, washed and finally plated on
selective medium.
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ENCAPSULATION IN LIPOSOMES
Liposomes are microscopic lipid molecules
which are produced when phospholipids are
dispersed in an aqueous phase.
Liposomes are large enough to allow
entrapment of DNA and can interact with a
variety of cells. Negatively charged
unilamellar liposomes are best suited for the
transfer of DNA and RNA into plant cells.
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ELECTROPORATION
The process by which macromolecules
present in the extra cellular medium are
internalized by living cells on exposure to
a brief electric pulse.
The technique allows introduction of DNA
into living cells/protoplasts by passing
short pulse of electricity which has a
voltage peak value of 250-350 volts with
RC constant in milliseconds range.
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MICROPROJECTILE BOMBARDMENT
Exogenous DNA molecules are adsorbed on
the surface of microscopic tungsten
microprojectiles which are then accelerated
to high velocities by a particle gun onto the
target cells.
The advantage in this approach is that a
naked DNA molecule can be directly
transferred into intact living cells or tissues.
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Particle gun for accelerating microprojectiles
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MICROINJECTION
Living cells/protoplasts are surface attached
on a slide by embedding in agro or polylysine
using a holding pipette.
The DNA is transferred by injecting it with
micro needles into the surface attached
cells/protoplasts.
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Microinjection by the holding pipette method13
CELL PERFORATION USING SiC WHISKERS
Recipient cells are perforated by vortexing in
the presence of SiC (silicon carbide)
whiskers along with DNA.
Cell perforation thereby allows direct entry of
exogenous DNA.
This method was initially used for genetic
transformation of maize suspension cells and
later extended to transform other plants.
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