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In Vitro Developmental Pathways. Explant - Piece of tissue put into culture -Tissue selection depends on purpose, species, many factors.

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Presentation on theme: "In Vitro Developmental Pathways. Explant - Piece of tissue put into culture -Tissue selection depends on purpose, species, many factors."— Presentation transcript:

1 In Vitro Developmental Pathways

2 Explant - Piece of tissue put into culture -Tissue selection depends on purpose, species, many factors

3 Explants Pieces of organs –Leaves –Stems –Roots –Cotyledons –Embryos –Other

4 Explants Specific cell types –Leaf tissue –Embryo –Pollen –Endosperm –Nucellus

5 Callus Unorganized, growing mass of cells Dedifferentiation of explant –Loosely arranged thinned walled, outgrowths from explant –No predictable site of organization or differentiation Auxin + cytokinin Often can be maintained indefinitely by subculture, but may lose ability to redifferentiate Compact vs friable Habituation

6 Three stages of callus culture Induction: Cells in explant dedifferentiate and begin to divide Proliferative Stage: Rapid cell division Differentiation stage (sometimes): organogenesis or embryogenesis

7 Induction © 1998-2003, Branch of Shemyakin&Ovchinnikov IBCh RAS

8 Division E. Sutton, UC Davis

9 Callus © 1998-2003, Branch of Shemyakin&Ovchinnikov IBCh RAS

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12 Differentiation Organogenesis Somatic embryogenesis

13 Cell and Suspension Culture Cell Cultures? Suspension Cultures

14 Suspension cultures Can be initiated from any part of the plant. Usually initiated from friable callus already growing in culture. Transferred into liquid medium.

15 Agitation Breakdown of cell aggregates into smaller clumps of cells Maintains a uniform distribution of cells and cell clumps in the medium Provides gas exchange

16 Medium Same as for callus culture? Gamborg B5 Conditioning

17 Growth Curve E. Sutton, UC Davis

18 Batch Cultures A certain number of cells is used to inoculate the culture, in a given volume Erlenmeyer flask: volume should be about 20% of flask capacity for aeration. Roller cultures

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21 Continuous Culture Bioreactors Closed continuous cultures: Remove some of the media and replace with fresh. Continuous removal or periodic. Terminate growth at harvest. Start over. Open continuous culture: Not only remove some of media, but cells too. Maintain cell density at optimal level. Can be grown for years.

22 Why is it possible to regenerate in vitro? Totipotency –Initial state –Competence –Determination –Differentiation

23 Only occurs in a few cells in culture. Why? Pre-determination prior to culture Newly formed meristems may act as sinks  Meristematic centers might actually produce compounds that inhibit neighboring cells.

24 Organogenesis The formation of organs (such as leaves, shoots, roots) on a plant organ, usually of a different kind.

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26 Organogenesis Rule of thumb: Auxin/cytokinin 10:1- 100:1 induces roots. 1:10-1:100 induces shoots Intermediate ratios around 1:1 favor callus growth.

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30 Indirect organogenesis Explant → Callus → Meristemoid → Primordium

31 Indirect Organogenesis Dedifferentiation –Less committed, more plastic developmental state Induction –Cells become organogenically competent and fully determined for primordia production –Change in culture conditions? Differentiation

32 © 1998-2003, Branch of Shemyakin&Ovchinnikov IBCh RAS

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37 Direct Organogenesis

38 Somatic Embryogenesis lParthenocarpy lApomixis lIn vitro somatic embryogenesis

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46 Soybean – Wayne Parrot, UGA

47 Somatic Embryos Bipolar Not connected to explant or callus cells by vascular tissue In most woody plants, tissue must be juvenile or reproductive

48 Indirect Somatic Embryogenesis

49 Induction Auxins required for induction –Proembryogenic masses form –2,4-D most used –NAA, dicamba also used

50 Development Auxin must be removed for embryo development Continued use of auxin inhibits embryogenesis Stages are similar to those of zygotic embryogenesis –Globular –Heart –Torpedo –Cotyledonary –Germination (conversion)

51 Maturation Require complete maturation with apical meristem, radical, and cotyledons Often obtain repetitive embryony Storage protein production necessary Often require ABA for complete maturation ABA often required for normal embryo morphology –Fasciation –Precocious germination

52 Germination May only obtain 3-5% germination Sucrose (10%), mannitol (4%) may be required Drying (desiccation) –ABA levels decrease –Woody plants –Final moisture content 10-40% Chilling –Decreases ABA levels –Woody plants

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56 Rubber tree from somatic embryo CIRAD

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63 Factors that Influence SE Genotype Growth regulators Carbon source Nitrogen

64 Maturation and Germination (Conversion)

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