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PROTOPLAST AND IMMOBILIZATION
            BY
       Dr.U.Srinivasa,
          M.Pharm, Ph.D.
   Definition :
   Protoplast is a cell without a cell wall are called
    protoplast.
   They contain all the normal cell organelles plus
    the nucleus.
   The cell wall of a plant cell can be decomposed
    and removed by the treatment of the lytic
    enzymes like cellulose and pectinase
Isolation of protoplast
   Protoplasts can be isolated from all types of
    actively growing young and healthy tissues.
    METHODS OF ISOLATION :

    1.Mechanical method

    2. Enzymatic method

    3. Combination of above methods
   During the process of isolation, the
    cells    are   first   separated   by
    mechanical method and subsequently
    protoplasts are isolated by enzymatic
    method
Mechanical method
   The cells are first placed in a suitable
    plasmolyticum .This treatment makes the
    protoplasms of these plasmolysed cells
    shrink away from their cell walls( this
    makes the removal of cell wall easy)
   Further ,they are cut with a knife.
   Then the protoplasts are released from the cells
    through the cell wall , and then the tissue is
    again deplasmolysed.
   Advantages :
   It is suitable method for the isolation of protoplasts from
    vacuolated cells. Eg onion bulbs, scales, radish roots
   Dis advantages :
   Poor yield
   Unsuitable     for   the   isolation   of   protoplasts   from
    meristematic cells
   Unsuitable for the isolation of protoplasts from          less
    vacuolated cells
Enzymatic method
   Protoplasts can be isolated from aIt is widely
    used   method.The      isolation   of   protoplasts
    requires digestion of cell wall and middle
    lamellae. This is affected by the use of
    enzymes
   variety of tissues including leaves, roots, in vitro
    shoot culture and cell suspension culture
Steps
   1.Sterilization of leaves
   2. Peeling of the epidermis
   3. Enzymatic treatment
   4. Isolation and cleaning of the protoplasts
   Sterilization of leaves –
   Fully expanded leaves are sterilized by the
    following procedure
   A. dipping in 70% ethyl alcohol for about a
    minute and then with 2% solution of sodium
    hypochlorite for 20-30 minutes
   B. rinsing with sterile distilled water three
    times.
   Peeling of the epidermal layer :
   The lower epidermis is carefully peeled off
    and the stripped leaves are cut into small
    pieces.
   This operation must be carried out under
    aseptic conditions
   Mesophyll protoplasts can be isolated from
    the peeled leaf segments while epidermis
    yields epidermal protoplasts
   Enzymatic treatment :
   There are two methods
   1.Direct method ( 1 step)
   2.Sequential method (2 steps)
   Direct method :
   Here simultaneous treatment with macerase
    ( pectinase ) and cellulose enzymes is carried
    out.
   0.5% macerase and 2% cellulose enzyme in
    13% sorbitol or mannitol at pH 5.4
•   Sequential method :
•   1 step – Sample is treated with macerase
    ( pectinase ) enzyme for isolation of cells
     2 step – Isolated cells are treated with cellulose
    enzyme for protoplast isolation
    In both cases , peeled leaf segments are placed
    with the lower surface downwards in a petridish
    containing enzyme mixture
Purification
   The    isolated    protoplasts    are   usually
    associated with a range of cell debris and
    broken cell organelles .
   Methods used for purification :
   1. Sedimentation
   2. Flotation
Applications
   Suitable for the isolation of cell organelles
    and chromosomes
   Suitable for the isolation of mutants
   To affect genetic transformations through
    DNA or organelle uptake
   Study of cell wall formation, membrane
    transport , ultra structures
Immobilization of Enzyme
Definition
“Enzymes physically confined or localized in
 a certain defined region of space with retention of their
 catalytic activities , and which can be used repeatedly
 and continuously".
 Immobilization is a process of aggregate formation and
 adhesion on a matrix under controlled conditions.
Advantages
   1) No purification of enzyme after production
   2) High enzyme activity (high reactor activity)
   3) Enhanced operational stability
   4) Low enzyme cost
   5) Application of multienzyme        reaction is
    possible
How to stabilize enzyme?

•   Addition of substrate analogues

•   Addition of sugar alcohols (e.g. sorbitol)

•   Addition of cofactors (e.g. calcium ion)

•    Immobilization: reuse & long-term
    stability !
Methods of immobilization
1.Direct intercellular binding due to natural affinity .
  Eg: Adhesion, adsorption,agglutination
2.Covalent bonding on inert matrices
3.Embedding
4.Cross linking with biopolyfunctional reagents
5. Purely physical retensions in diverse pore size
  eg: entrapment, microencapsulation
Agents used

   Agarose gel
   Alginate gel
   Chitosan
   Polyacrylamide
   Polyurethane foam
   Polyethylene oxide
Enzyme Immobilization
Immobilization by Binding

•   Adsorption:
•   Electrostatic interactions (van der Waals forces, ionic
    and hydrogen bonds betweeen the cell surface and
    the support materials
•   cell wall composition: determined by distribution of
    carboxyl and amino groups of the peptide amino acids
    of cell wall surface (ex) yeast cells are negative
    charge, thus choose a positively charged support
•   Advantages: ability to regenerate the support
•   Disadvantsges: low stability (desorption of cells due
    to changes of pH and/or ionic strength)
•   Covalent-binding methods
•   Advantages:
•   Free of diffusional limitations
•   High operational stability
•   Uniform binding
•   Disadvantages:
•   Toxicity of the coupling agents(loss of activity and
    cell   viability,   not   acceptable   in   food   and
    pharmaceutical fields)
•   Hard to regenerate the supports

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Protoplast isolation and immobiliz by Dr.U.Srinivasa

  • 1. PROTOPLAST AND IMMOBILIZATION BY Dr.U.Srinivasa, M.Pharm, Ph.D.
  • 2. Definition :  Protoplast is a cell without a cell wall are called protoplast.  They contain all the normal cell organelles plus the nucleus.  The cell wall of a plant cell can be decomposed and removed by the treatment of the lytic enzymes like cellulose and pectinase
  • 3. Isolation of protoplast  Protoplasts can be isolated from all types of actively growing young and healthy tissues. METHODS OF ISOLATION : 1.Mechanical method 2. Enzymatic method 3. Combination of above methods
  • 4. During the process of isolation, the cells are first separated by mechanical method and subsequently protoplasts are isolated by enzymatic method
  • 5. Mechanical method  The cells are first placed in a suitable plasmolyticum .This treatment makes the protoplasms of these plasmolysed cells shrink away from their cell walls( this makes the removal of cell wall easy)  Further ,they are cut with a knife.
  • 6. Then the protoplasts are released from the cells through the cell wall , and then the tissue is again deplasmolysed.
  • 7. Advantages :  It is suitable method for the isolation of protoplasts from vacuolated cells. Eg onion bulbs, scales, radish roots  Dis advantages :  Poor yield  Unsuitable for the isolation of protoplasts from meristematic cells  Unsuitable for the isolation of protoplasts from less vacuolated cells
  • 8. Enzymatic method  Protoplasts can be isolated from aIt is widely used method.The isolation of protoplasts requires digestion of cell wall and middle lamellae. This is affected by the use of enzymes  variety of tissues including leaves, roots, in vitro shoot culture and cell suspension culture
  • 9. Steps  1.Sterilization of leaves  2. Peeling of the epidermis  3. Enzymatic treatment  4. Isolation and cleaning of the protoplasts
  • 10. Sterilization of leaves –  Fully expanded leaves are sterilized by the following procedure  A. dipping in 70% ethyl alcohol for about a minute and then with 2% solution of sodium hypochlorite for 20-30 minutes  B. rinsing with sterile distilled water three times.
  • 11. Peeling of the epidermal layer :  The lower epidermis is carefully peeled off and the stripped leaves are cut into small pieces.  This operation must be carried out under aseptic conditions  Mesophyll protoplasts can be isolated from the peeled leaf segments while epidermis yields epidermal protoplasts
  • 12. Enzymatic treatment :  There are two methods  1.Direct method ( 1 step)  2.Sequential method (2 steps)
  • 13. Direct method :  Here simultaneous treatment with macerase ( pectinase ) and cellulose enzymes is carried out.  0.5% macerase and 2% cellulose enzyme in 13% sorbitol or mannitol at pH 5.4
  • 14. Sequential method : • 1 step – Sample is treated with macerase ( pectinase ) enzyme for isolation of cells 2 step – Isolated cells are treated with cellulose enzyme for protoplast isolation In both cases , peeled leaf segments are placed with the lower surface downwards in a petridish containing enzyme mixture
  • 15. Purification  The isolated protoplasts are usually associated with a range of cell debris and broken cell organelles .  Methods used for purification :  1. Sedimentation  2. Flotation
  • 16. Applications  Suitable for the isolation of cell organelles and chromosomes  Suitable for the isolation of mutants  To affect genetic transformations through DNA or organelle uptake  Study of cell wall formation, membrane transport , ultra structures
  • 17. Immobilization of Enzyme Definition “Enzymes physically confined or localized in a certain defined region of space with retention of their catalytic activities , and which can be used repeatedly and continuously". Immobilization is a process of aggregate formation and adhesion on a matrix under controlled conditions.
  • 18. Advantages  1) No purification of enzyme after production  2) High enzyme activity (high reactor activity)  3) Enhanced operational stability  4) Low enzyme cost  5) Application of multienzyme reaction is possible
  • 19. How to stabilize enzyme? • Addition of substrate analogues • Addition of sugar alcohols (e.g. sorbitol) • Addition of cofactors (e.g. calcium ion) • Immobilization: reuse & long-term stability !
  • 20. Methods of immobilization 1.Direct intercellular binding due to natural affinity . Eg: Adhesion, adsorption,agglutination 2.Covalent bonding on inert matrices 3.Embedding 4.Cross linking with biopolyfunctional reagents 5. Purely physical retensions in diverse pore size eg: entrapment, microencapsulation
  • 21. Agents used  Agarose gel  Alginate gel  Chitosan  Polyacrylamide  Polyurethane foam  Polyethylene oxide
  • 23. Immobilization by Binding • Adsorption: • Electrostatic interactions (van der Waals forces, ionic and hydrogen bonds betweeen the cell surface and the support materials • cell wall composition: determined by distribution of carboxyl and amino groups of the peptide amino acids of cell wall surface (ex) yeast cells are negative charge, thus choose a positively charged support • Advantages: ability to regenerate the support • Disadvantsges: low stability (desorption of cells due to changes of pH and/or ionic strength)
  • 24. Covalent-binding methods • Advantages: • Free of diffusional limitations • High operational stability • Uniform binding • Disadvantages: • Toxicity of the coupling agents(loss of activity and cell viability, not acceptable in food and pharmaceutical fields) • Hard to regenerate the supports