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Anther and-pollen-culture

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HISTORY  W.TULECKE(1953) First observed that mature pollen grains of Ginkgo biloba (gymnosperm) can be induced to prolifrate in culture to form haploid callus. S.GUHA AND S.C MAHESWARI(1964)  First reported the direct deveiopment of embroys from microspores of Datura innoxia by the culture of excised anther. J.P. BOURGIN AND J.P.NITSCH(1967)  Obtained complete haploid plantlents from anther culture of Nicotiana tabacum.
Anther culture  Culturing of anther obtained from unopened flower bud in the nutrient medium under aseptic condition.  callus tissue or embryoids that give rise to haploid plantlets either though organogenesis or embryogenesis.
Pollen culture  Pollen or microspore culture is an in vitro technique by which the pollen grains preferably at the uninucleated stage, are squeezed out aseptically from the intact anther and then cultured on nutrient medium.  the microspores develop into haploid embryoids or callus tissue that give rise to haploid plantlets by embryogenesis or organogenesis.
Androgenesis  Androgenesis is the in vitro development of haploid plants originating from totipotent pollen grains through a series of cell division and differentiation.  It is of two types.  Direct androgenesis  Indirect androgenesis
Androgenesis 1)Direct androgeneis:- The microspores behaves like a zygote and undergoes chance to form enbryoid which ultimately give rise to a plantlet. 2) Indirect Androgenesis:- The microspores divide repeatedly to form a callus tissue which differentiates into haploid plantlets.
Principle of anther and pollen culture  The production of haploid plants is to exploit the totipotency of microspore .  In this process the normal development and function of the pollen cell to become a male gamete is stopped and is diverted forcely to a new metabolic pathway for vegetative cell division .
Factors influencing anther culture 1) Genotype of donor plants:- The genotype of the donor plant plays a significant role in determining the frequency of pollen production.  Example :- Horedum of each genotype differs with respect to androgenic response in anther culture. 2) Anther wall factor:- The anther wall provide the nourishment in the development of isolated pollen of a number of species.  There are reports that glutamine alone or in combination with serine and myo inositol could replace the anther wall
Factors influencing anther culture 3) CULTURE MEDIUM:- For anther culture, medium requirements vary with genotype and the age of the anther as well as condition under which donor plants are grown.  Incorporation of activated charcoal into the medium has stimulated the induction of androgenesis.  The iron in the medium plays a very important role for the induction of haploids .  Potato extracts, coconut milk and growth regulators like auxin and cytokinin are used for anther and pollen culture.
Factors influencing anther culture
Factors influencing anther culture Effect of temperature:- Temperature enhance the induction frequency of microspore androgensis.  The low temperature treatment to anther or flower bud enhance the haploid formation.  The low temperature effects the number of factors such as dissolution of microtubules lowering of absicisic acid maintenance of higher ratio of viable pollen capable of embryognesis.
Factor influencing anther culture Physiological status of donor plant  Physiological status of donor plant such as water stress nitrogen requirement and age of donor plant highly affect the pollen embryogenesis.  Plants starved of nitrogen may give more responsive anthers compared to those that are well fed with nitrogenous fertilizers.
Method of anther and pollen culture
Procedure for Anther culture  1.collection of unopened flower buds  2.surface sterilized with tween 80 and mercuric chloride  3.Anthers excised from flower buds and kept seperately  4.Anthers in first meiotic division is selected by acetocarmine test  5.Inoculated in the medium containing glutamine, L-serine and inositol
 6. Incubated the culture at 25 C for 15 days. Here, anthers grow in to embryoids.  7. embryoids transfer to rooting medium under 3000 lux illumination after 4-5 weeks the embryoids became plantlets.  8.After aclimatization, transferto green house
Procedure for pollen culture  1.Anther collected from flower buds and pollen grains are isolated and inoculated in the nutrients medium with the concentration of pollen 0.5ml.  2.Nitsh (1974) medium is used for pollen culture  3. Anthers are place on the medium  some times nurse culture may used.  4. A paper disc is placed over anther or callus. 
continued  O.5ml pollen suspension is poured on the disc  Petridh covered with lid and incubated at 50 C for 4 weeks. Pollengrains grown in to individual clones with 60% efficacy.  Clones are transferred to callus induction medium to produce calli.  Calli transfered to shooting medium and then to rooting medium to produce ploantlets
Advantage of pollen culture over anther culture  During anther culture there is always the possibility that somatic cells of the anther that are diploid will also respond to the culture condition and so produce unwanted diploid calli or plantlets.  Sometimes the development of microspores inside the anther may be interrupted due to growth inhibiting substances leaking out of the anther wall in contact with nutrient medium.
Importance of pollen and anther culture  Utility of anther and pollen culture for basic research cytogenetic studies.  Study of genetic recombination in higher plants.  Study of mode of differentiation from single cell to whole organism.  Study of factor controlling pollen embryogenesis of higher plants.  Formation of double haploid that are homozygous and fertile.
2) for mutation study. 3) for plant breeding and crop improvement. 4) to obtain the secondary metabolites. Eg. Hyoscyamus niger obtain by anther culture having higher alkaloid content. 5) Haploids are used in molecular biology and genetic engineering. Example:- Haploid tissue of Arabidopsis and Lycopersicon have been used for the transfer and expression of three genes from Escherchia coli....

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Anther and-pollen-culture

  • 1.
  • 2. HISTORY  W.TULECKE(1953) First observed that mature pollen grains of Ginkgo biloba (gymnosperm) can be induced to prolifrate in culture to form haploid callus. S.GUHA AND S.C MAHESWARI(1964)  First reported the direct deveiopment of embroys from microspores of Datura innoxia by the culture of excised anther. J.P. BOURGIN AND J.P.NITSCH(1967)  Obtained complete haploid plantlents from anther culture of Nicotiana tabacum.
  • 3. Anther culture  Culturing of anther obtained from unopened flower bud in the nutrient medium under aseptic condition.  callus tissue or embryoids that give rise to haploid plantlets either though organogenesis or embryogenesis.
  • 4. Pollen culture  Pollen or microspore culture is an in vitro technique by which the pollen grains preferably at the uninucleated stage, are squeezed out aseptically from the intact anther and then cultured on nutrient medium.  the microspores develop into haploid embryoids or callus tissue that give rise to haploid plantlets by embryogenesis or organogenesis.
  • 5. Androgenesis  Androgenesis is the in vitro development of haploid plants originating from totipotent pollen grains through a series of cell division and differentiation.  It is of two types.  Direct androgenesis  Indirect androgenesis
  • 6. Androgenesis 1)Direct androgeneis:- The microspores behaves like a zygote and undergoes chance to form enbryoid which ultimately give rise to a plantlet. 2) Indirect Androgenesis:- The microspores divide repeatedly to form a callus tissue which differentiates into haploid plantlets.
  • 7. Principle of anther and pollen culture  The production of haploid plants is to exploit the totipotency of microspore .  In this process the normal development and function of the pollen cell to become a male gamete is stopped and is diverted forcely to a new metabolic pathway for vegetative cell division .
  • 8. Factors influencing anther culture 1) Genotype of donor plants:- The genotype of the donor plant plays a significant role in determining the frequency of pollen production.  Example :- Horedum of each genotype differs with respect to androgenic response in anther culture. 2) Anther wall factor:- The anther wall provide the nourishment in the development of isolated pollen of a number of species.  There are reports that glutamine alone or in combination with serine and myo inositol could replace the anther wall
  • 9. Factors influencing anther culture 3) CULTURE MEDIUM:- For anther culture, medium requirements vary with genotype and the age of the anther as well as condition under which donor plants are grown.  Incorporation of activated charcoal into the medium has stimulated the induction of androgenesis.  The iron in the medium plays a very important role for the induction of haploids .  Potato extracts, coconut milk and growth regulators like auxin and cytokinin are used for anther and pollen culture.
  • 11. Factors influencing anther culture Effect of temperature:- Temperature enhance the induction frequency of microspore androgensis.  The low temperature treatment to anther or flower bud enhance the haploid formation.  The low temperature effects the number of factors such as dissolution of microtubules lowering of absicisic acid maintenance of higher ratio of viable pollen capable of embryognesis.
  • 12. Factor influencing anther culture Physiological status of donor plant  Physiological status of donor plant such as water stress nitrogen requirement and age of donor plant highly affect the pollen embryogenesis.  Plants starved of nitrogen may give more responsive anthers compared to those that are well fed with nitrogenous fertilizers.
  • 13. Method of anther and pollen culture
  • 14. Procedure for Anther culture  1.collection of unopened flower buds  2.surface sterilized with tween 80 and mercuric chloride  3.Anthers excised from flower buds and kept seperately  4.Anthers in first meiotic division is selected by acetocarmine test  5.Inoculated in the medium containing glutamine, L-serine and inositol
  • 15.  6. Incubated the culture at 25 C for 15 days. Here, anthers grow in to embryoids.  7. embryoids transfer to rooting medium under 3000 lux illumination after 4-5 weeks the embryoids became plantlets.  8.After aclimatization, transferto green house
  • 16. Procedure for pollen culture  1.Anther collected from flower buds and pollen grains are isolated and inoculated in the nutrients medium with the concentration of pollen 0.5ml.  2.Nitsh (1974) medium is used for pollen culture  3. Anthers are place on the medium  some times nurse culture may used.  4. A paper disc is placed over anther or callus. 
  • 17. continued  O.5ml pollen suspension is poured on the disc  Petridh covered with lid and incubated at 50 C for 4 weeks. Pollengrains grown in to individual clones with 60% efficacy.  Clones are transferred to callus induction medium to produce calli.  Calli transfered to shooting medium and then to rooting medium to produce ploantlets
  • 18. Advantage of pollen culture over anther culture  During anther culture there is always the possibility that somatic cells of the anther that are diploid will also respond to the culture condition and so produce unwanted diploid calli or plantlets.  Sometimes the development of microspores inside the anther may be interrupted due to growth inhibiting substances leaking out of the anther wall in contact with nutrient medium.
  • 19. Importance of pollen and anther culture  Utility of anther and pollen culture for basic research cytogenetic studies.  Study of genetic recombination in higher plants.  Study of mode of differentiation from single cell to whole organism.  Study of factor controlling pollen embryogenesis of higher plants.  Formation of double haploid that are homozygous and fertile.
  • 20. 2) for mutation study. 3) for plant breeding and crop improvement. 4) to obtain the secondary metabolites. Eg. Hyoscyamus niger obtain by anther culture having higher alkaloid content. 5) Haploids are used in molecular biology and genetic engineering. Example:- Haploid tissue of Arabidopsis and Lycopersicon have been used for the transfer and expression of three genes from Escherchia coli....