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PLANT TISSUE
CULTURE
PRESENTED BY: MOHD NADEEM
M.Sc. BIOCHEMISTRY 3rd SEMESTER
Definition
the culture of plant seeds, organs,
tissues, cells, or protoplasts on
nutrient media under sterile
conditions.
HISTORY
STERILIZATION METHODS
Callus
 Equimolar amounts of auxin and cytokinin
stimulate cell division. Leads to a mass
proliferation of an unorganised mass of cells
called a callus.
 Requirement for support ensures that scale-
up is limited (Ginseng saponins successfully
produced in this way).
Cell suspension culture
 When callus pieces are agitated in a liquid
medium, they tend to break up.
 Suspensions are much easier to bulk up than
callus since there is no manual transfer or
solid support.
Types of In Vitro Culture
 Culture of intact plants (seed and seedling
culture)
 Embryo culture (immature embryo culture)
 Organ culture
1. shoot tip culture
2. root culture
3. leaf culture
4. anther culture
 Callus culture
 Cell suspension culture
 Protoplast culture
Micropropagation
 Embryogenesis
 Direct embryogenesis
 Indirect embryogenesis
 Organogenesis
 Organogenesis via callus formation
 Direct adventitious organ formation
 Microcutting
 Meristem and shoot tip culture
 Bud culture
Steps of Micropropagation
 Stage 0 – Selection & preparation of the mother plant
 sterilization of the plant tissue takes place
 Stage I - Initiation of culture
 explant placed into growth media
 Stage II - Multiplication
 explant transferred to shoot media; shoots can be constantly
divided
 Stage III - Rooting
 explant transferred to root media
 Stage IV - Transfer to soil
 explant returned to soil; hardened off
Features of Micropropagation
 Clonal reproduction
 Way of maintaining heterozygozity
 Multiplication Stage can be recycled many times
to produce an unlimited number of clones
 Routinely used commercially for many ornamental
species, some vegetatively propagated crops
 Easy to manipulate production cycles
 Not limited by field seasons/environmental influences
 Disease-free plants can be produced
 Has been used to eliminate viruses from donor plants
Embryo Culture
 Embryo culture developed from the need to rescue embryos
(embryo rescue) from wide crosses where fertilization occurred,
but embryo development did not occur
 These techniques have been further developed for the production
of plants from embryos developed by non-sexual methods (haploid
production discussed later)
Anther/Microspore Culture Factors
 Genotype
 As with all tissue culture techniques
 Growth of mother plant
 Usually requires optimum growing conditions
 Correct stage of pollen development
 Need to be able to switch pollen development from gametogenesis to
embryogenesis
 Pretreatment of anthers
 Cold or heat have both been effective
 Culture media
 Additives, Agar vs. ‘Floating’
PROTOPLAST ISOLATION
DIRECT GENE TRANSFER
PLANT TISSUE CULTURE TECHNIQUES
PLANT TISSUE CULTURE TECHNIQUES

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PLANT TISSUE CULTURE TECHNIQUES

  • 1. PLANT TISSUE CULTURE PRESENTED BY: MOHD NADEEM M.Sc. BIOCHEMISTRY 3rd SEMESTER
  • 2. Definition the culture of plant seeds, organs, tissues, cells, or protoplasts on nutrient media under sterile conditions.
  • 5.
  • 6.
  • 7.
  • 8.
  • 9. Callus  Equimolar amounts of auxin and cytokinin stimulate cell division. Leads to a mass proliferation of an unorganised mass of cells called a callus.  Requirement for support ensures that scale- up is limited (Ginseng saponins successfully produced in this way).
  • 10. Cell suspension culture  When callus pieces are agitated in a liquid medium, they tend to break up.  Suspensions are much easier to bulk up than callus since there is no manual transfer or solid support.
  • 11.
  • 12.
  • 13. Types of In Vitro Culture  Culture of intact plants (seed and seedling culture)  Embryo culture (immature embryo culture)  Organ culture 1. shoot tip culture 2. root culture 3. leaf culture 4. anther culture  Callus culture  Cell suspension culture  Protoplast culture
  • 14.
  • 15.
  • 16. Micropropagation  Embryogenesis  Direct embryogenesis  Indirect embryogenesis  Organogenesis  Organogenesis via callus formation  Direct adventitious organ formation  Microcutting  Meristem and shoot tip culture  Bud culture
  • 17. Steps of Micropropagation  Stage 0 – Selection & preparation of the mother plant  sterilization of the plant tissue takes place  Stage I - Initiation of culture  explant placed into growth media  Stage II - Multiplication  explant transferred to shoot media; shoots can be constantly divided  Stage III - Rooting  explant transferred to root media  Stage IV - Transfer to soil  explant returned to soil; hardened off
  • 18. Features of Micropropagation  Clonal reproduction  Way of maintaining heterozygozity  Multiplication Stage can be recycled many times to produce an unlimited number of clones  Routinely used commercially for many ornamental species, some vegetatively propagated crops  Easy to manipulate production cycles  Not limited by field seasons/environmental influences  Disease-free plants can be produced  Has been used to eliminate viruses from donor plants
  • 19. Embryo Culture  Embryo culture developed from the need to rescue embryos (embryo rescue) from wide crosses where fertilization occurred, but embryo development did not occur  These techniques have been further developed for the production of plants from embryos developed by non-sexual methods (haploid production discussed later)
  • 20.
  • 21. Anther/Microspore Culture Factors  Genotype  As with all tissue culture techniques  Growth of mother plant  Usually requires optimum growing conditions  Correct stage of pollen development  Need to be able to switch pollen development from gametogenesis to embryogenesis  Pretreatment of anthers  Cold or heat have both been effective  Culture media  Additives, Agar vs. ‘Floating’
  • 23.
  • 24.
  • 25.
  • 26.
  • 27.
  • 28.