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SEMINAR PRESENTATION
ON
ANTHER CULTURE

PRESENTED TO:
by:
Dr.Harsh kumar sir
&
Biotech
Dr. Kundan sir

presented
DEEPTI
(msc.Ag.
1st sem)
ANTHER: A part of stamen
contaning pollen.
POLLEN: A fertilising powder
discharged from flowers anther.
ANTHER AND MICROSPORE(POLLEN)
CULTURE: It is the process of formation of
haploid plants from microspores (pollen)
cultured individually or anthers.
 Anther culture for production of
haploids reported in about 250 species.
Solanaceae, cruciferae, gramineae are most common.
 Anther/pollen culture is referred as
ANDROGENESIS : occurs when
pollen/microspore shift from a gametophytic to
sporophytic pathway of embryo formation.
 shift occur prior to premitotic & postmitotic :
either vegetative or generative divide to
undergo androgenesis.



In experiments using Datura innoxia,
induction frequencies of almost 100% and
a yield of more than one thousand
plantlets or calluses have occurred under
optimal conditions from one anther.
Success can be determined within 24
hours as cells begin to divide.
figure : Anther culture and
haploid plants regeneration.
(a) Anther at the onset of the culture. (b)
Anther after 6 days in culture. (c, d)
Embryos emerging from the anthers
after 30 days in culture, showing roots
(c) and shoots (d). (e–g) Plantlets with
cotyledons (e) and with leaves (f, g)
subcultured in growing medium. (h) 80day-old regenerated haploid plant from
anther culture (left-hand side).
–

1964, 1966 Datura innoxia (Guha and
Maheshwari), the Indian scientists.

–

1967 ( Bourgin and Nitsch ) : 1st haploid
plants from isolated anthers of Nicotiana.

–

during last decade : anther culture of rice,
wheat , maize, brassica, pepper and crop sp.
1.
2.
3.
4.
5.

Pathway I
Pathway II
Pathway III
Pathway IV
Pathway V
The microspores divide by an equal
division and two identical daughter cells
developed.
 Vegetative and generative cells are not
distinctly formed in the pathway.
 Example: Datura innoxia

The division of uninucleate microspores is
unusual , resulting in the formation of
vegetative and generative cell.
 The sporophyte arises through further
division in the vegetative cell and
generative cell does not divide.
 Examples: Nicotiana tabacum , Hordeum
vulgare , Triticum aestivum , Triticale.

The uninucleate microspore undergoes a
normal division but pollen embryos are formed
from generative cell alone.
 The vegetative cell does not divide.
 Examples: Hyoscyamus niger

Both generative and vegetative cell divide
further to the development of sporophyte.
 Examples: Datura metal, Atropa
belladona, Datura innoxia(occasionally).




PATHWAY V
In Brassica napus , 1st division is
symmetric and the pollen embryos
develop the vegetative cell.
Pathways to pollen
development

Normal pollen
development
1) Genotype of donor plant : determine the
frequency of pollen plant production.
_ eg. In Hordeum each genotype differs with
respect to androgenic response in anther
culture.
_ high responsive anthers should
be taken.
2) Anther wall factor : act as conditioning factors
and
promote culture growth.
_ report: glutamine alone or in combination
with
serine and myoinositol could replace the
anther
wall factor.
3) Stage of pollen : stage of pollen varies with
species.
_ before/after 1st pollen mitosis- Datura,
4) Physiological status of donor plant :
a) grown under best environmental
conditions with good anthers.
b) flowers obtained at the beginning
of flowering season are highly
responsive.
5) Pretreatment of anthers : appropriate
treatment required for good success of
haploid production(depend on donor plant
species).
# Temperature influence:
a) induction of androgenesis is
better if
stored at low temperature prior to
culture.e.g. maize , rye.
b) pretreatment of anthers at higher
temperature stimulates
androgenesis


response is not known but interference
with starch accumulation in pollen and
degradation of tapetum cellular
matrix,etc.may be involved.
Cold Treatment (3 to 5 C) Enhances
Symmetric Division of Microspores or
Division of Vegetative Nuclei
3 to 5 C
Vegetative
Microspore

Similar nuclei

Generative
3 to 5 C

Embryo
Cold Pretreatment of Anthers Enhances the
Embryogenic Response
Cold treatment imposed prior to the first pollen
mitosis increases the frequency of symmetric
divisions of the microspore leading to embryo
formation.
% Anthers
Producing Embryos

100

3C

80
5C
60

C

40
C

20
0
Tobacco

Datura
PLANT SPECIES

ANDROGENIC
RESPONSE

Brassica napus

Heat treatment(320 c for 8
hrs ), gamma- rays,
colchicine

Hordeum vulgare

Stress by mannitol, calcium
and ABA

Nicotiana tabacum(tobacco)

Glutamine and sugar
starvation
(transfer to high glucose
medium)
Cold treatment( 4 - 100 c for 3-

Triticum aestivum
6) Effect of light : pretreatment of anthers at
elevated temperatures( 3 0 c) stimulate
androgenesis in some Brassica and
Capsicum.
7) Culture medium :
- it vary with the genotype and age of the anther.
- culture maintained on an auxin medium for
longer period develop a friable callus.
- a compound related to auxin namely 2,3,5triiodobenzoic acid(TIBA) gives +ve result at low
concentration.
- incorporation of activated charcoal/2chloroethyl-phosphate stimulates androgenesis
DIFFERENT TYPES RELATED CULTURE
OF PLANT
MEDIUM
SPECIES
Nicotiana tabaccum
and
Datura innoxia

Simple agar plates containing
only sucrose

Solanaceae species

Complete nutrient medium

Non- solanaceae plants

Medium fortified with growth
adjuvents (yeast extract, casein
hydrosylate, coconut milk)

Maize anthers

N6 and Yu-Pei

Wheat anthers

Potato – 2 medium(potato-1 +
six low salt concentration)
1) Selection of explants(eg. Flower bud)
2) preparation of explant
3) disinfection of bud
4) selected buds are pretreated
5) surface sterlization
6) inoculation
7) transfer to culture room
8) transplanted to small pots in
greenhouse





simple.
less time consuming.
responsive.






Requires skill to remove anthers without
causing damage.
Not much successful in case of cereal
crop.
Risk of chimera and callus formation from
anther wall.
1. Often fail to grow in-vitro.
2. Tissue or callus comprises a chimera of
diploid, tetraploid and haploid cells.
3. Formation of albinos especially with cereals
and effect the loss of plants due to albinism.
4. It is not economically viable for haploid
production.
5. Callus in a medium supplemented with growth
regulators is usually detrimental for haploid
production.
THANKS
thank you

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Anther culture

  • 1. SEMINAR PRESENTATION ON ANTHER CULTURE PRESENTED TO: by: Dr.Harsh kumar sir & Biotech Dr. Kundan sir presented DEEPTI (msc.Ag. 1st sem)
  • 2. ANTHER: A part of stamen contaning pollen. POLLEN: A fertilising powder discharged from flowers anther.
  • 3. ANTHER AND MICROSPORE(POLLEN) CULTURE: It is the process of formation of haploid plants from microspores (pollen) cultured individually or anthers.  Anther culture for production of haploids reported in about 250 species. Solanaceae, cruciferae, gramineae are most common.  Anther/pollen culture is referred as ANDROGENESIS : occurs when pollen/microspore shift from a gametophytic to sporophytic pathway of embryo formation.  shift occur prior to premitotic & postmitotic : either vegetative or generative divide to undergo androgenesis. 
  • 4.
  • 5.  In experiments using Datura innoxia, induction frequencies of almost 100% and a yield of more than one thousand plantlets or calluses have occurred under optimal conditions from one anther. Success can be determined within 24 hours as cells begin to divide.
  • 6. figure : Anther culture and haploid plants regeneration. (a) Anther at the onset of the culture. (b) Anther after 6 days in culture. (c, d) Embryos emerging from the anthers after 30 days in culture, showing roots (c) and shoots (d). (e–g) Plantlets with cotyledons (e) and with leaves (f, g) subcultured in growing medium. (h) 80day-old regenerated haploid plant from anther culture (left-hand side).
  • 7. – 1964, 1966 Datura innoxia (Guha and Maheshwari), the Indian scientists. – 1967 ( Bourgin and Nitsch ) : 1st haploid plants from isolated anthers of Nicotiana. – during last decade : anther culture of rice, wheat , maize, brassica, pepper and crop sp.
  • 9. The microspores divide by an equal division and two identical daughter cells developed.  Vegetative and generative cells are not distinctly formed in the pathway.  Example: Datura innoxia 
  • 10. The division of uninucleate microspores is unusual , resulting in the formation of vegetative and generative cell.  The sporophyte arises through further division in the vegetative cell and generative cell does not divide.  Examples: Nicotiana tabacum , Hordeum vulgare , Triticum aestivum , Triticale. 
  • 11. The uninucleate microspore undergoes a normal division but pollen embryos are formed from generative cell alone.  The vegetative cell does not divide.  Examples: Hyoscyamus niger 
  • 12. Both generative and vegetative cell divide further to the development of sporophyte.  Examples: Datura metal, Atropa belladona, Datura innoxia(occasionally).   PATHWAY V In Brassica napus , 1st division is symmetric and the pollen embryos develop the vegetative cell.
  • 14.
  • 15. 1) Genotype of donor plant : determine the frequency of pollen plant production. _ eg. In Hordeum each genotype differs with respect to androgenic response in anther culture. _ high responsive anthers should be taken.
  • 16. 2) Anther wall factor : act as conditioning factors and promote culture growth. _ report: glutamine alone or in combination with serine and myoinositol could replace the anther wall factor. 3) Stage of pollen : stage of pollen varies with species. _ before/after 1st pollen mitosis- Datura,
  • 17. 4) Physiological status of donor plant : a) grown under best environmental conditions with good anthers. b) flowers obtained at the beginning of flowering season are highly responsive.
  • 18. 5) Pretreatment of anthers : appropriate treatment required for good success of haploid production(depend on donor plant species). # Temperature influence: a) induction of androgenesis is better if stored at low temperature prior to culture.e.g. maize , rye. b) pretreatment of anthers at higher temperature stimulates androgenesis
  • 19.  response is not known but interference with starch accumulation in pollen and degradation of tapetum cellular matrix,etc.may be involved.
  • 20. Cold Treatment (3 to 5 C) Enhances Symmetric Division of Microspores or Division of Vegetative Nuclei 3 to 5 C Vegetative Microspore Similar nuclei Generative 3 to 5 C Embryo
  • 21. Cold Pretreatment of Anthers Enhances the Embryogenic Response Cold treatment imposed prior to the first pollen mitosis increases the frequency of symmetric divisions of the microspore leading to embryo formation. % Anthers Producing Embryos 100 3C 80 5C 60 C 40 C 20 0 Tobacco Datura
  • 22. PLANT SPECIES ANDROGENIC RESPONSE Brassica napus Heat treatment(320 c for 8 hrs ), gamma- rays, colchicine Hordeum vulgare Stress by mannitol, calcium and ABA Nicotiana tabacum(tobacco) Glutamine and sugar starvation (transfer to high glucose medium) Cold treatment( 4 - 100 c for 3- Triticum aestivum
  • 23. 6) Effect of light : pretreatment of anthers at elevated temperatures( 3 0 c) stimulate androgenesis in some Brassica and Capsicum. 7) Culture medium : - it vary with the genotype and age of the anther. - culture maintained on an auxin medium for longer period develop a friable callus. - a compound related to auxin namely 2,3,5triiodobenzoic acid(TIBA) gives +ve result at low concentration. - incorporation of activated charcoal/2chloroethyl-phosphate stimulates androgenesis
  • 24. DIFFERENT TYPES RELATED CULTURE OF PLANT MEDIUM SPECIES Nicotiana tabaccum and Datura innoxia Simple agar plates containing only sucrose Solanaceae species Complete nutrient medium Non- solanaceae plants Medium fortified with growth adjuvents (yeast extract, casein hydrosylate, coconut milk) Maize anthers N6 and Yu-Pei Wheat anthers Potato – 2 medium(potato-1 + six low salt concentration)
  • 25. 1) Selection of explants(eg. Flower bud) 2) preparation of explant 3) disinfection of bud 4) selected buds are pretreated 5) surface sterlization 6) inoculation 7) transfer to culture room 8) transplanted to small pots in greenhouse
  • 26.
  • 28.    Requires skill to remove anthers without causing damage. Not much successful in case of cereal crop. Risk of chimera and callus formation from anther wall.
  • 29. 1. Often fail to grow in-vitro. 2. Tissue or callus comprises a chimera of diploid, tetraploid and haploid cells. 3. Formation of albinos especially with cereals and effect the loss of plants due to albinism. 4. It is not economically viable for haploid production. 5. Callus in a medium supplemented with growth regulators is usually detrimental for haploid production.