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PREPARED BY: VIPIN KUMAR SHUKLA
ASSISTANT PROFESSOR
DEPARTMENT OF BIOTECHNOLOGY
PRESENTATION 0N HYBRIDOMA
TECHNOLOGY
Introduction:
 Hybridoma technology is a method of
forming hybrid cell lines (called
Hybridoma) by fusing a specific
 Antibody-producing B-cell with a
myeloma cell (cancerous cell).
 The antibodies produced by the
Hybridoma are of a single
specificity and are therefore
monoclonal antibodies.
HISTORY:
 In 1975, these technology developed by Georges
J.F.Kohler and Cesar Milstein. And in 1984, they
shared a Nobel prize for this discovery.
 They make a hybrid cell that will make a numbers of
monoclonal antibodies against antigen .
PRINCIPLE:
 The hybrid cell has the capacity of antibody
production derived from B-cells (spleen cell ).
 At the same time it can divide continuously by the
quality derived from myeloma cell.
 By combining the desired qualities of both the cells,
the technology ensures large, antibody production of
single specificity.
 Specific Hybridoma(spleen cell and myeloma cell)
obtain monoclonal antibodies in artificial media, this
technology called as HYBRIDOMA
TECHNOLOGY.
Continued……
 The selection of Hybridoma cells is based on inhibiting
the nucleotide (consequently the DNA) synthesizing
machinery.
 De novo synthesis and salvage pathway are the two
pathways through which mammalian cells can synthesize
nucleotides.
 HAT (hypoxanthine Aminopterin and Thymidine)
medium – Only Hybridoma cells can proliferate in HAT
medium.
General Flow Diagram of Hybridoma
Technology
MONOCLONAL ANTIBODY:
 Monoclonal antibodies (mab) are antibodies that are
identical because they are produced by one type of
immune cell, all clones of a single parent cell.
 Basically produced by white blood cell which is called
as plasma cell.
 Is used for treatment of cancerous cells and as anti-
venom( anti snake venom).
PROCEDURE:
 Immunization of specific animal which generate
Hybridoma cell with spleen cell.
 Isolation of myeloma cells.
 Fusion between spleen cell and myeloma cell.
 Selection of HAT medium.
 Isolation of Hybridoma cell.
 Screening of Hybridoma cell
Immunization of specific animal:
 An antigen immunized to an animal (like mice) via
intravenously(directly to blood) by injection.
 Where in spleen it activate B-cell which produce
plasma cell (spleen cell).
 Plasma cell to produce monoclonal antibodies.
 Isolation of plasma cell from spleen of animal.
Isolation of myeloma cells:
 Myeloma cells are cancerous cells which is
isolated from bone-marrow.
 Myeloma cells are generally immortal in nature
(that which never dies) and has multiplication
property.
Fusion of spleen cell and myeloma cell:
 It requires PEG (poly ethylene glycol) medium for
fusion.
 It can also done by electro fusion.
 Fusion between spleen cell and myeloma cell
produced five different types of cells.
 Fused plasma
 Fused myeloma
 Hybridoma
 Unfused plasma
 Unfused myeloma
Selection of HAT medium.
( Hypoxanthine, Aminopterin, Thymidine)
 Before multiplication of Anti-body, it has to synthesize new
copy of DNA and for that it require synthesis of nucleotide.
 For synthesis of nucleotide mainly two pathways are there:
 1. Salvage pathway
 2. De-novo Synthesis
 In 1 , Salvage pathway it requires degraded part of old
nucleotide to produce new nucleotide.
 In 2, De-novo synthesis it synthesized completely new
nucleotide by small molecules (sugar, amino-acid).
Continued…….
 So in HAT medium, Cells not synthesized by De-novo
synthesis due to presence of Aminopterin in HAT medium
which blocks Di-hydro follate enzyme which is
necessary for these synthesis.
 For synthesis in salvage pathway it must requires
HGPRT enzyme (Hypoxanthine Guanine Phospho-
Ribosyl Transferase).
 Where hypoxanthine and Thymidine are used as
precursors.
Isolation of Hybridoma cell:
Spleen cell have HGPRT enzyme
Myeloma cell doesn’t have HGPRT enzyme
Fused plasma present
2. Fused myeloma absent
3. Hybridoma present
4. Unfused plasma present
5. Unfused myeloma absent
Continued……
 Fused myeloma and unfused myeloma didn’t have
HGPRT enzyme so, can’t survive in HAT medium.
 Fused plasma and unfused plasma have HGPRT
enzyme but didn’t have long-life.
 Hybrid cell has HGPRT enzyme from spleen
cell as well as they have the ability to multiply
repeatedly as myeloma cell.
 So, isolation of hybrid cell because is only cell
which survive in HAT medium.
Screening of Hybridoma cell:
 ELISA screening method which done by incubating
Hybridoma culture in which secondary enzyme gets
conjugate and formation of colored product shows
positive Hybridoma.
 Used for multiplying the Hybridoma cells
 In-vivo
 In-vitro
Continued…..
 In-vivo procedure involves introduction of Hybridoma
cells into the peritoneal cavity of the animal , then
from ascetic fluid antibodies are isolated.
 In-vitro method involves culturing of Hybridoma
cells in suitable culture media and then antibodies are
isolated and purified.
 Once a Hybridoma colony is established, it will
continually grow in culture medium like RPMI-1640
and produce antibodies.
 Storage: liquid nitrogen.
APPLICATION OF HYBRIDOMA
TECHNOLOGY
 Serological:
 Identification of ABO blood group
 Diagnosis:
 Detection of pregnancy by assaying of hormones with monoclonal.
 Separation of one substance from a mixture of very similar
molecules.
 Immunopurification:
 Purification of individual interferon using monoclonal.
 Inactivation of T-lymphocytes responsible for rejection of organ
transplants.
 Therapy:
 Removal of tumor cell from bone marrow.
 Treatment of acute renal failure.
 Treatment malignant leukemic cells, B cell lymphomas, and a
variety of allograft rejections after transplantation.
ADVANTAGES AND DISADVANTAGES
OF MONOCLONAL ANTIBODIES
 Advantages-
 Represent a homogeneous state of a single molecular
species.
 Each Mab is specific to a given antigenic determinant.
 Disadvantages-
 Hybridoma technology is laborious and time
consuming.
 There is no guarantee that Mab produced is totally
virus-free, despite the purification.
 For this reason, US Food and Drug Administration
insists that Mab for human use should be totally free
from all pathogenic organisms, including viruses.
REFERENCES
 Satyanarayana, U. 2016. Biotechnology. Books and Allied
(P) Ltd, Kolkata. pp. 213-226.
 Gupta, P.K. 2016. Biotechnology and Genomics. Rastogi
Publications, Meerut. pp. 299-311.
 Owen, J.A., Punt J., Stanford, S.A. and Patricia, P.J. 2013.
Kuby Immunology. 7th Ed. W.H. Freeman and Company,
New York. pp.645- 655.
 Singh, B.D. 2017. Biotechnology Expanding Horizons.
Kalyani Publishers, New Delhi. pp. 172-174.
 Dubey, R.C. and Maheshwari, D.K. 2018. A Textbook of
Microbiology. S Chand and Company Limited, New
Delhi. pp. 662-663.
Presentation 0 n hybridoma technology

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Presentation 0 n hybridoma technology

  • 1. PREPARED BY: VIPIN KUMAR SHUKLA ASSISTANT PROFESSOR DEPARTMENT OF BIOTECHNOLOGY PRESENTATION 0N HYBRIDOMA TECHNOLOGY
  • 2. Introduction:  Hybridoma technology is a method of forming hybrid cell lines (called Hybridoma) by fusing a specific  Antibody-producing B-cell with a myeloma cell (cancerous cell).  The antibodies produced by the Hybridoma are of a single specificity and are therefore monoclonal antibodies.
  • 3. HISTORY:  In 1975, these technology developed by Georges J.F.Kohler and Cesar Milstein. And in 1984, they shared a Nobel prize for this discovery.  They make a hybrid cell that will make a numbers of monoclonal antibodies against antigen .
  • 4. PRINCIPLE:  The hybrid cell has the capacity of antibody production derived from B-cells (spleen cell ).  At the same time it can divide continuously by the quality derived from myeloma cell.  By combining the desired qualities of both the cells, the technology ensures large, antibody production of single specificity.  Specific Hybridoma(spleen cell and myeloma cell) obtain monoclonal antibodies in artificial media, this technology called as HYBRIDOMA TECHNOLOGY.
  • 5. Continued……  The selection of Hybridoma cells is based on inhibiting the nucleotide (consequently the DNA) synthesizing machinery.  De novo synthesis and salvage pathway are the two pathways through which mammalian cells can synthesize nucleotides.  HAT (hypoxanthine Aminopterin and Thymidine) medium – Only Hybridoma cells can proliferate in HAT medium.
  • 6. General Flow Diagram of Hybridoma Technology
  • 7. MONOCLONAL ANTIBODY:  Monoclonal antibodies (mab) are antibodies that are identical because they are produced by one type of immune cell, all clones of a single parent cell.  Basically produced by white blood cell which is called as plasma cell.  Is used for treatment of cancerous cells and as anti- venom( anti snake venom).
  • 8. PROCEDURE:  Immunization of specific animal which generate Hybridoma cell with spleen cell.  Isolation of myeloma cells.  Fusion between spleen cell and myeloma cell.  Selection of HAT medium.  Isolation of Hybridoma cell.  Screening of Hybridoma cell
  • 9. Immunization of specific animal:  An antigen immunized to an animal (like mice) via intravenously(directly to blood) by injection.  Where in spleen it activate B-cell which produce plasma cell (spleen cell).  Plasma cell to produce monoclonal antibodies.  Isolation of plasma cell from spleen of animal.
  • 10. Isolation of myeloma cells:  Myeloma cells are cancerous cells which is isolated from bone-marrow.  Myeloma cells are generally immortal in nature (that which never dies) and has multiplication property.
  • 11. Fusion of spleen cell and myeloma cell:  It requires PEG (poly ethylene glycol) medium for fusion.  It can also done by electro fusion.  Fusion between spleen cell and myeloma cell produced five different types of cells.  Fused plasma  Fused myeloma  Hybridoma  Unfused plasma  Unfused myeloma
  • 12. Selection of HAT medium. ( Hypoxanthine, Aminopterin, Thymidine)  Before multiplication of Anti-body, it has to synthesize new copy of DNA and for that it require synthesis of nucleotide.  For synthesis of nucleotide mainly two pathways are there:  1. Salvage pathway  2. De-novo Synthesis  In 1 , Salvage pathway it requires degraded part of old nucleotide to produce new nucleotide.  In 2, De-novo synthesis it synthesized completely new nucleotide by small molecules (sugar, amino-acid).
  • 13. Continued…….  So in HAT medium, Cells not synthesized by De-novo synthesis due to presence of Aminopterin in HAT medium which blocks Di-hydro follate enzyme which is necessary for these synthesis.  For synthesis in salvage pathway it must requires HGPRT enzyme (Hypoxanthine Guanine Phospho- Ribosyl Transferase).  Where hypoxanthine and Thymidine are used as precursors.
  • 14. Isolation of Hybridoma cell: Spleen cell have HGPRT enzyme Myeloma cell doesn’t have HGPRT enzyme Fused plasma present 2. Fused myeloma absent 3. Hybridoma present 4. Unfused plasma present 5. Unfused myeloma absent
  • 15.
  • 16. Continued……  Fused myeloma and unfused myeloma didn’t have HGPRT enzyme so, can’t survive in HAT medium.  Fused plasma and unfused plasma have HGPRT enzyme but didn’t have long-life.  Hybrid cell has HGPRT enzyme from spleen cell as well as they have the ability to multiply repeatedly as myeloma cell.  So, isolation of hybrid cell because is only cell which survive in HAT medium.
  • 17. Screening of Hybridoma cell:  ELISA screening method which done by incubating Hybridoma culture in which secondary enzyme gets conjugate and formation of colored product shows positive Hybridoma.  Used for multiplying the Hybridoma cells  In-vivo  In-vitro
  • 18.
  • 19. Continued…..  In-vivo procedure involves introduction of Hybridoma cells into the peritoneal cavity of the animal , then from ascetic fluid antibodies are isolated.  In-vitro method involves culturing of Hybridoma cells in suitable culture media and then antibodies are isolated and purified.  Once a Hybridoma colony is established, it will continually grow in culture medium like RPMI-1640 and produce antibodies.  Storage: liquid nitrogen.
  • 20.
  • 21. APPLICATION OF HYBRIDOMA TECHNOLOGY  Serological:  Identification of ABO blood group  Diagnosis:  Detection of pregnancy by assaying of hormones with monoclonal.  Separation of one substance from a mixture of very similar molecules.  Immunopurification:  Purification of individual interferon using monoclonal.  Inactivation of T-lymphocytes responsible for rejection of organ transplants.  Therapy:  Removal of tumor cell from bone marrow.  Treatment of acute renal failure.  Treatment malignant leukemic cells, B cell lymphomas, and a variety of allograft rejections after transplantation.
  • 22. ADVANTAGES AND DISADVANTAGES OF MONOCLONAL ANTIBODIES  Advantages-  Represent a homogeneous state of a single molecular species.  Each Mab is specific to a given antigenic determinant.  Disadvantages-  Hybridoma technology is laborious and time consuming.  There is no guarantee that Mab produced is totally virus-free, despite the purification.  For this reason, US Food and Drug Administration insists that Mab for human use should be totally free from all pathogenic organisms, including viruses.
  • 23.
  • 24. REFERENCES  Satyanarayana, U. 2016. Biotechnology. Books and Allied (P) Ltd, Kolkata. pp. 213-226.  Gupta, P.K. 2016. Biotechnology and Genomics. Rastogi Publications, Meerut. pp. 299-311.  Owen, J.A., Punt J., Stanford, S.A. and Patricia, P.J. 2013. Kuby Immunology. 7th Ed. W.H. Freeman and Company, New York. pp.645- 655.  Singh, B.D. 2017. Biotechnology Expanding Horizons. Kalyani Publishers, New Delhi. pp. 172-174.  Dubey, R.C. and Maheshwari, D.K. 2018. A Textbook of Microbiology. S Chand and Company Limited, New Delhi. pp. 662-663.