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Topic :- Plant Tissue Culture
Prepared By :-
Bhadani Smit Ramjibhai
Roll No.:- 17BPH095
Program :- B.Pharm(IV)
Subject:-
Pharmacognosy
PLANT TISSUE CULTURE
PLANT TISSUE CULTURE
• Plant tissue culture is a collection of
techniques used to maintain or grow plant
cells, tissues or organs under sterile conditions
on a nutrient culture medium of known
composition. Plant tissue culture is widely
used to produce clones of a plant in a method
known as micropropagation .
Advantages of Plant Tissue Culture
• The production of exact copies of plants that
produce particularly good flowers, fruits.
• To quickly produce mature plants.
• The production of multiples of plants in the
absence of seeds.
• The regeneration of whole plants from plant
cells that have been genetically modified.
• The production of plants in sterile containers
that allows them to be moved with greatly
reduced chances of transmitting diseases,
pests, and pathogens.
• The production of plants from seeds that
otherwise have very low chances of
germinating and growing, i.e.: orchids and
Nepenthes.
• To clear particular plants of viral and other
infections and to quickly multiply these plants
as 'cleaned stock' for horticulture and
agriculture.
ADVANTAGES OF PLANT TISSUE
CULTURE
1) Availability of raw material
2) Variation in supplies and quality
3) Patent rights
4) Easy purification of the compounds
5) Modification of chemical structure
6) Disease free and desired product
7) Crop improvement
EXPLANT
• Any part of a plant taken out and grown in
test tube under sterile conditions in special
nutrient media is called explant.
METHODS OF PLANT TISSUE CULTURE
• Plant tissue culture includes two major methods:
(A) Type of in vitro growth-callus and suspension
cultures.
(B) Type of explant— single cell culture, shoot and
root cultures, somatic embryo culture, meristem
culture, anther culture and haploid production,
protoplast culture and somatic hybridisation,
embryo culture, ovule culture, ovary culture, etc.
Environmental Conditions
• There are three important aspects in vitro
culture
1) Nutrient medium
2) Aseptic condition
3) Aeration of the tissue
Nutrient Medium
• Medium depends upon the type of plant tissue or
cell used for culture
o Generally nutrient consist of
o inorganic salts (both micro & macro elements)
o a carbon source (usually sucrose)
o Vitamins (eg. nicotinic acid, thiamine, pyridoxine
o Amino acids (eg. arginine)
o Growth regulators (eg. auxins)
o An optimum pH (5.7) is also vary important
Aseptic Condition
• Nutrient medium contains sugar which
increases growth of microbes
• These microbes compete with growing tissue
and finally kill it.
• It is important to maintain aseptic condition.
• Sterilization is very important to stop the
growth of microbes.
Aeration of the Tissue
• Proper aeration of the cultured tissue is also
an important aspect of culture technique.
• It is achieved by occasionally stirring the
medium by stirring or by automatic shaker.
Types of Plant Tissue
Culture
Callus Culture
• In Callus culture, cell division in explant forms a callus.
• Callus is irregular unorganized and undifferentiated
mass of actively dividing cells.
• Darkness & solid medium gelled by agar stimulates
callus formation.
• The medium contains the auxins and BAP (Benzyl
amino purines). Both are growth regulators (
Hormones).
• This stimulates cell division in explant.
• Callus is obtained within 2-3 weeks.
Callus culture and Sub culture
Maintenance
• After sufficient time of callus growth on the same
medium following changes will occur :-
o Depletion of nutrient in the medium
o Gradual loss of water
o Accumulation of metabolic toxins
• Hence for maintenance of growth in callus it is
necessary to subculture the callus.
• Subculture should be repeated after 4-5 weeks
Single Cell Culture
• As stated earlier, cells derived from a single
cell through mitosis constitute a clone and the
process of obtaining clones is called cloning
(asexual progeny of a single individual make
up a clone). There are two popular techniques
for single cell culture.
Root tip culture
• Tips of the lateral roots are sterilized, excised and
transferred to fresh medium.
• The lateral roots continue to grow and provide
several roots.
• After 7 days that are used to initiate stock or
experiment.
• Thus the root material derived from a single
radical.
• Such genetically uniform root cultures are
referred to as a clone of isolated roots.
Leaves culture
• Leaves (800µm) may be detached from
shoots, surface sterilized and place in healthy
condition for long period.
• Growth rate in the culture depends on their
stages of maturity at excision.
• Young leaves have more growth potential
then the nearly mature ones.
Shoot tip culture
• The excised shoot tips (100-1000µm long) of
many plant species can be cultured on
relatively simple nutrient media.
• This media must contains growth hormones
and will often form roots and develop into
whole plants.
Complete flower culture
• Flowers (2days after pollination) are excised,
sterilized by immersion in 5% calcium
hypochloride, washed with sterilized water.
• Transfer this to culture tubes containing an
agar medium.
• Fruits, which develop are smaller than their
natural counterpart, size can be increases by
supplementing the medium with appropriate
combination of growth hormones.
Anther Culture
• Young flower buds are removed from the
plant & surface sterilized.
• The anthers are then excised and transferred
to an appropriate nutrient medium.
• The plantlet are formed after 4-5 weeks of
inoculation.
• Many plantlets are produced from the single
anther.
Pollens culture
• Pollen grains are removed from the anther.
• Anthers are placed in a 5ml liquid medium in
petri dish.
• Petri dishes containing the pollen grains in
the culture media are sealed with parafilm &
incubated at 28ºC in dark for 14 days.
• 3-4 weeks may be required to obtain haploid
plantlets.
Application of tissue culture
• Tissue culture is used to conserve the rare
species in the forest.
• A plant breeder may use tissue culture to
screen cells rather than plants.
• Large-scale growth of plant cells in liquid
culture as a source of secondary products, like
recombinant proteins used as
biopharmaceuticals.
• To cross distantly related species by
protoplast fusion.
• Help in crop improvement.
• Creation of additional genetic variation.
• Selection of plants resistant to toxins, viruses
etc.
• Suitable for breeding of tree species.
• Production of many plants that are clone to
each other.
• Production of disease free plants.
• Tissue culture have a advantage of time sever,
With the help of root culture plants are ready
to grow which save time.

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Plant tissue culture

  • 1. Topic :- Plant Tissue Culture Prepared By :- Bhadani Smit Ramjibhai Roll No.:- 17BPH095 Program :- B.Pharm(IV) Subject:- Pharmacognosy
  • 3. PLANT TISSUE CULTURE • Plant tissue culture is a collection of techniques used to maintain or grow plant cells, tissues or organs under sterile conditions on a nutrient culture medium of known composition. Plant tissue culture is widely used to produce clones of a plant in a method known as micropropagation .
  • 4. Advantages of Plant Tissue Culture • The production of exact copies of plants that produce particularly good flowers, fruits. • To quickly produce mature plants. • The production of multiples of plants in the absence of seeds. • The regeneration of whole plants from plant cells that have been genetically modified.
  • 5. • The production of plants in sterile containers that allows them to be moved with greatly reduced chances of transmitting diseases, pests, and pathogens. • The production of plants from seeds that otherwise have very low chances of germinating and growing, i.e.: orchids and Nepenthes. • To clear particular plants of viral and other infections and to quickly multiply these plants as 'cleaned stock' for horticulture and agriculture.
  • 6. ADVANTAGES OF PLANT TISSUE CULTURE 1) Availability of raw material 2) Variation in supplies and quality 3) Patent rights 4) Easy purification of the compounds 5) Modification of chemical structure 6) Disease free and desired product 7) Crop improvement
  • 7. EXPLANT • Any part of a plant taken out and grown in test tube under sterile conditions in special nutrient media is called explant.
  • 8. METHODS OF PLANT TISSUE CULTURE • Plant tissue culture includes two major methods: (A) Type of in vitro growth-callus and suspension cultures. (B) Type of explant— single cell culture, shoot and root cultures, somatic embryo culture, meristem culture, anther culture and haploid production, protoplast culture and somatic hybridisation, embryo culture, ovule culture, ovary culture, etc.
  • 9. Environmental Conditions • There are three important aspects in vitro culture 1) Nutrient medium 2) Aseptic condition 3) Aeration of the tissue
  • 10. Nutrient Medium • Medium depends upon the type of plant tissue or cell used for culture o Generally nutrient consist of o inorganic salts (both micro & macro elements) o a carbon source (usually sucrose) o Vitamins (eg. nicotinic acid, thiamine, pyridoxine o Amino acids (eg. arginine) o Growth regulators (eg. auxins) o An optimum pH (5.7) is also vary important
  • 11. Aseptic Condition • Nutrient medium contains sugar which increases growth of microbes • These microbes compete with growing tissue and finally kill it. • It is important to maintain aseptic condition. • Sterilization is very important to stop the growth of microbes.
  • 12. Aeration of the Tissue • Proper aeration of the cultured tissue is also an important aspect of culture technique. • It is achieved by occasionally stirring the medium by stirring or by automatic shaker.
  • 13. Types of Plant Tissue Culture
  • 14. Callus Culture • In Callus culture, cell division in explant forms a callus. • Callus is irregular unorganized and undifferentiated mass of actively dividing cells. • Darkness & solid medium gelled by agar stimulates callus formation. • The medium contains the auxins and BAP (Benzyl amino purines). Both are growth regulators ( Hormones). • This stimulates cell division in explant. • Callus is obtained within 2-3 weeks.
  • 15. Callus culture and Sub culture
  • 16. Maintenance • After sufficient time of callus growth on the same medium following changes will occur :- o Depletion of nutrient in the medium o Gradual loss of water o Accumulation of metabolic toxins • Hence for maintenance of growth in callus it is necessary to subculture the callus. • Subculture should be repeated after 4-5 weeks
  • 17. Single Cell Culture • As stated earlier, cells derived from a single cell through mitosis constitute a clone and the process of obtaining clones is called cloning (asexual progeny of a single individual make up a clone). There are two popular techniques for single cell culture.
  • 18.
  • 19. Root tip culture • Tips of the lateral roots are sterilized, excised and transferred to fresh medium. • The lateral roots continue to grow and provide several roots. • After 7 days that are used to initiate stock or experiment. • Thus the root material derived from a single radical. • Such genetically uniform root cultures are referred to as a clone of isolated roots.
  • 20.
  • 21. Leaves culture • Leaves (800µm) may be detached from shoots, surface sterilized and place in healthy condition for long period. • Growth rate in the culture depends on their stages of maturity at excision. • Young leaves have more growth potential then the nearly mature ones.
  • 22. Shoot tip culture • The excised shoot tips (100-1000µm long) of many plant species can be cultured on relatively simple nutrient media. • This media must contains growth hormones and will often form roots and develop into whole plants.
  • 23.
  • 24. Complete flower culture • Flowers (2days after pollination) are excised, sterilized by immersion in 5% calcium hypochloride, washed with sterilized water. • Transfer this to culture tubes containing an agar medium. • Fruits, which develop are smaller than their natural counterpart, size can be increases by supplementing the medium with appropriate combination of growth hormones.
  • 25. Anther Culture • Young flower buds are removed from the plant & surface sterilized. • The anthers are then excised and transferred to an appropriate nutrient medium. • The plantlet are formed after 4-5 weeks of inoculation. • Many plantlets are produced from the single anther.
  • 26.
  • 27. Pollens culture • Pollen grains are removed from the anther. • Anthers are placed in a 5ml liquid medium in petri dish. • Petri dishes containing the pollen grains in the culture media are sealed with parafilm & incubated at 28ºC in dark for 14 days. • 3-4 weeks may be required to obtain haploid plantlets.
  • 28.
  • 29. Application of tissue culture • Tissue culture is used to conserve the rare species in the forest. • A plant breeder may use tissue culture to screen cells rather than plants. • Large-scale growth of plant cells in liquid culture as a source of secondary products, like recombinant proteins used as biopharmaceuticals.
  • 30. • To cross distantly related species by protoplast fusion. • Help in crop improvement. • Creation of additional genetic variation. • Selection of plants resistant to toxins, viruses etc. • Suitable for breeding of tree species. • Production of many plants that are clone to each other. • Production of disease free plants.
  • 31. • Tissue culture have a advantage of time sever, With the help of root culture plants are ready to grow which save time.