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SYNOPSIS --
 Introduction of se
Definition of se
 Types of se
 Steps of se
 Methods of se
 In monocot and Dicot
 Factor affecting
 Applications
 Conclusion
 Reference
• Process by which somatic cells or tissue develops into
differentiated embryo.
• Somatic embryos are formed from plant cells that are not normally
involved in the development of embryo, i.e. ordinary plant tissue.
• Somatic embryogenesis is the process in which a single cell or a
small group of cells follow a development pathway that leads to
reproducible regeneration of non-zygotic embryos which are
capable of producing a complete plant.
• However, the two ways of inducing somatic embryogenesis
include:
• Direct somatic embryogenesis: In this process, the embryo is
developed without any intermediate callus stage. The embryo can
be developed by directly inducing the explant for the genesis.
• Indirect somatic embryogenesis: In this process, the development of
an embryo occurs with an intermediate callus stage. So, it is a
multistep process.
• 1. Induction: It is the initiative phase where cells of callus are induced to
divide and differentiate into groups of meristematic cells called embryogenic
clumps (ECS).
• These Ecs develop into initial stages of somatic embryo i.e. globular stage.
• 2. Maturation: In this phase somatic embryo develop into mature embryos
by differentiating from globular to heart shaped and the mature embryo here
undergoes biochemical changes to acquire hardness.
• 3. Conversion: Embryos germinate to produce seedlings.
• Leaf petiole or root segments from seven day old seedlings or cambium
tissue from storage root can be used as explant.
• Following aseptic technique, explants are placed individually on a semi-
solid MS medium.
• Culture are incubated in the dark.
• In this medium the explant will produce sufficient callus tissue.
• After 4 week of callus growth, cell suspension culture is to be initiated by
transferring callus tissue to a 250 ml flask containing 20-25ml of liquid
medium of same composition as used for callus growth (without agar).
• Flask are placed on a horizontal gyratory shaker at 25*C.
• The presence or absence of light is not critical at this stage.
• Cell suspension are sub- cultured every 4 week by transferring 5 ml to 65
ml of fresh liquid medium.
• After 3-4 week, the culture would contain numerous embryos in different
stage of development.
• Somatic embryos can be placed on agar medium devoid of 2, 4-D for
plantlet development.
• Plantlets are finally transferred to pots for subsequent development.
• The addition of reduced nitrogen in the medium helps in both embryo in
association and maturation.
• In the absence of iron, embryo development fails to pass from the globular to
the heart shaped stage.
• Growth regulators in the medium specially oxygen or oxygen in combination
with cytokinins appear essential for the onset of growth and the induction of
embryogenesis.
• Cytokinins are important in somatic maturation and specially cotyledons
development.
• The addition of activated charcoal to the medium has proved to the useful for
somatic embryo development.
• Environment conditions of light, temperature, density of embryogenic cell in
medium a important.
• Regarding culture vessel the position of embryos and the physical state of
medium have little effect.
• Large scale propagation compared to zygotic embryo.
• More useful than organogenesis.
• Useful for mutagenic studies and mutant production.
• Useful for genetic manipulation technique.
• Useful for pathogen- free plant production.
• A good source of protoplast culture.

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SE Embryogenesis Process & Factors

  • 1.
  • 2. SYNOPSIS --  Introduction of se Definition of se  Types of se  Steps of se  Methods of se  In monocot and Dicot  Factor affecting  Applications  Conclusion  Reference
  • 3. • Process by which somatic cells or tissue develops into differentiated embryo. • Somatic embryos are formed from plant cells that are not normally involved in the development of embryo, i.e. ordinary plant tissue. • Somatic embryogenesis is the process in which a single cell or a small group of cells follow a development pathway that leads to reproducible regeneration of non-zygotic embryos which are capable of producing a complete plant.
  • 4.
  • 5. • However, the two ways of inducing somatic embryogenesis include: • Direct somatic embryogenesis: In this process, the embryo is developed without any intermediate callus stage. The embryo can be developed by directly inducing the explant for the genesis. • Indirect somatic embryogenesis: In this process, the development of an embryo occurs with an intermediate callus stage. So, it is a multistep process.
  • 6. • 1. Induction: It is the initiative phase where cells of callus are induced to divide and differentiate into groups of meristematic cells called embryogenic clumps (ECS). • These Ecs develop into initial stages of somatic embryo i.e. globular stage. • 2. Maturation: In this phase somatic embryo develop into mature embryos by differentiating from globular to heart shaped and the mature embryo here undergoes biochemical changes to acquire hardness. • 3. Conversion: Embryos germinate to produce seedlings.
  • 7.
  • 8.
  • 9. • Leaf petiole or root segments from seven day old seedlings or cambium tissue from storage root can be used as explant. • Following aseptic technique, explants are placed individually on a semi- solid MS medium. • Culture are incubated in the dark. • In this medium the explant will produce sufficient callus tissue. • After 4 week of callus growth, cell suspension culture is to be initiated by transferring callus tissue to a 250 ml flask containing 20-25ml of liquid medium of same composition as used for callus growth (without agar).
  • 10. • Flask are placed on a horizontal gyratory shaker at 25*C. • The presence or absence of light is not critical at this stage. • Cell suspension are sub- cultured every 4 week by transferring 5 ml to 65 ml of fresh liquid medium. • After 3-4 week, the culture would contain numerous embryos in different stage of development. • Somatic embryos can be placed on agar medium devoid of 2, 4-D for plantlet development. • Plantlets are finally transferred to pots for subsequent development.
  • 11. • The addition of reduced nitrogen in the medium helps in both embryo in association and maturation. • In the absence of iron, embryo development fails to pass from the globular to the heart shaped stage. • Growth regulators in the medium specially oxygen or oxygen in combination with cytokinins appear essential for the onset of growth and the induction of embryogenesis. • Cytokinins are important in somatic maturation and specially cotyledons development.
  • 12. • The addition of activated charcoal to the medium has proved to the useful for somatic embryo development. • Environment conditions of light, temperature, density of embryogenic cell in medium a important. • Regarding culture vessel the position of embryos and the physical state of medium have little effect.
  • 13. • Large scale propagation compared to zygotic embryo. • More useful than organogenesis. • Useful for mutagenic studies and mutant production. • Useful for genetic manipulation technique. • Useful for pathogen- free plant production. • A good source of protoplast culture.