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HYBRIDOMA CELL
S I T I H A M I D A H S E A D | E V Y M A S T U R A S H U K R I
1
WHAT IS
HYBRIDOMA
CELL?
W H AT I S C O N T R I B U T I O N O F T H E C E L L?
2
INTRODUCTION
• Hydridoma cell is fusion of 2 cells in order to obtain or express a specific monoclonal
antibodies.
B-cells Tumor
cell HYBRIDOMA
B-
lymphocytes
myeloma
3
WHAT IS MONOCLONAL ANTIBODIES?
• Monoclonal antibodies artificially produced against a specific antigen in order to bind
to their target antigens.
• Uses of monoclonal antibodies are:
CANCER RHEUMATOID ARTHRITIS
CARDIOVASCULAR
DISEASES
ULCERATIVE COLITIS
4
Jens
Martensson
Method of culturing
hybridoma cells
1. Immunisation of mouse
2. Isolation of B cells from spleen
3. Cultivation of myeloma cells
4. Fusion of myeloma and B cells
5. Separation of cell lines
6. Screening suitable cell lines
7. In vitro / in vivo
8. Harvesting
Jens
Martensson
1. Immunisation of mouse
 2-4 weeks old mice are immunized with antigen against
which to raised monoclonal antibodies by subcutaneous
injection.
 Series of injections of the antigen over the course of
several weeks.
2.Isolation of B cells from
spleen
 B cells are isolated from the spleen of immunized mice.
Jens
Martensson
3. Cultivation of myeloma cells
 Myeloma cells are isolated from bone marrow.
 The myeloma cells used are HGPRT ( Hypoxanthine-
guanine phosphoribosyl transferase) mutant cells which
raised by mutation using 8-azaguanine.
4. Fusion of myeloma and B
cells Using electrofusion: cells are allowed to fused with the
application of electric field.
 By using PEG medium (Polyethylene Glycol)
Jens
Martensson
5. Separation of cell lines
 HAT (Hyphoxanthine Aminopterine Thymidine)
medium is used for the selection of hybrid cells.
 .B cells are HGPRT+ and can survive in the HAT
medium but the undergo normal cell death after some
division.
 Myeloma cells are HGPRT deficient so the cells could
not survive in HAT medium since Aminopterin blocks
the pathway that allows for nucleotide synthesis.
 Hybrid cells has HGPRT enzyme from B cells as well
as they have the ability to multiply repeatedly as
myeloma cells. So, only hybrid cells can survive in
Jens
Martensson
6. Screening suitable cell lines
 Screening technique used is called ELISA.
 The hybridoma culture supernatant, secondary enzyme labeled conjugate, and chromogenic
substrate.
 Then it is incubated and the formation of a colored product indicates a positive hybridoma.
 Alternatively, immunocytochemical screening can also be used.
Jens
Martensson
7.Methods multiplying hybridoma cell
 Introduce of hybridoma cells into peritoneal
cavity of mice.
 Ascetic fluid is isolated from the mice.
 Isolate antibodies from ascetic fluid.
 Culturing of hybridoma cells in suitable culture
media (
 Antibodies is isolated and purified.
Jens
Martensson
8. Harvesting
 Once a hybridoma colony is established, it will continually
grow in culture medium like RPMI-1640 (with antibiotics
and fetal bovine serum) and produce antibodies.
 Multiwell plates are used initially to grow the hybridomas.
 After selection, they are changed to tissue culture flasks to
provides enough cells for cryopreservation and supernatant
for subsequent investigations.
ADVANTAGES OF HYBRIDOMA
In vitro
• reduce the use of mice at the antibody-production stage
• ease of culture for production, compared with use of animals, and because of economic
considerations.
• decrease the need for laboratory personnel experienced in animal handling.
In Vivo
• produces very high mAb.
• high concentration of the desired mAb in mouse ascites fluid avoids the effects of contaminants
in in vitro batch-culture fluid when comparable quantities of mAb are used.
• reduce the need to teach the antibody producer tissue-culture methods.
12
DISADVANTAGE OF HYBRIDOMA
• Some cell may do not grow well in culture or are lost in culture.
• Require the use of FBS, which limits some antibody uses.
• In batch tissue-culture methods, mAb concentration tends to be low in the
supernatant
In vitro
• involves the continued use of mice requiring daily observation.
• can be expensive if immunodeficient mice in a barrier facility must be used.
• can contain various mouse proteins and other contaminants that might require
purification.
In vivo
13
CONCLUSION
• Hybridoma is fusion of two cell between tumor cell and Beta cell which specifically
beta lymphocytes cell from mice.
• The hydridoma is used to produce monoclonal antibodies to treat cancer disease such
as cardiovascular disease and ulcerative diseases
• Hybridoma can be cultured either in vitro or in vivo .
14
REFERENCES
• National Research Council (US) Committee on Methods of Producing Monoclonal
Antibodies. Monoclonal Antibody Production. Washington (DC): National Academies
Press (US); 1999. 4, Summary of Advantages and Disadvantages of In Vitro and In Vivo
Methods.Available from: https://www.ncbi.nlm.nih.gov/books/NBK100200/
• Prospecs Protein Cloning, https://www.prospecbio.com/monoclonal_antibodies
• Arya George. 2018. Hybridoma Technology. Slide. Mar Ivanios College
Trivandrum.Linkedln
15

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Hybridoma Cell Production of Monoclonal Antibodies

  • 1. HYBRIDOMA CELL S I T I H A M I D A H S E A D | E V Y M A S T U R A S H U K R I 1
  • 2. WHAT IS HYBRIDOMA CELL? W H AT I S C O N T R I B U T I O N O F T H E C E L L? 2
  • 3. INTRODUCTION • Hydridoma cell is fusion of 2 cells in order to obtain or express a specific monoclonal antibodies. B-cells Tumor cell HYBRIDOMA B- lymphocytes myeloma 3
  • 4. WHAT IS MONOCLONAL ANTIBODIES? • Monoclonal antibodies artificially produced against a specific antigen in order to bind to their target antigens. • Uses of monoclonal antibodies are: CANCER RHEUMATOID ARTHRITIS CARDIOVASCULAR DISEASES ULCERATIVE COLITIS 4
  • 5. Jens Martensson Method of culturing hybridoma cells 1. Immunisation of mouse 2. Isolation of B cells from spleen 3. Cultivation of myeloma cells 4. Fusion of myeloma and B cells 5. Separation of cell lines 6. Screening suitable cell lines 7. In vitro / in vivo 8. Harvesting
  • 6. Jens Martensson 1. Immunisation of mouse  2-4 weeks old mice are immunized with antigen against which to raised monoclonal antibodies by subcutaneous injection.  Series of injections of the antigen over the course of several weeks. 2.Isolation of B cells from spleen  B cells are isolated from the spleen of immunized mice.
  • 7. Jens Martensson 3. Cultivation of myeloma cells  Myeloma cells are isolated from bone marrow.  The myeloma cells used are HGPRT ( Hypoxanthine- guanine phosphoribosyl transferase) mutant cells which raised by mutation using 8-azaguanine. 4. Fusion of myeloma and B cells Using electrofusion: cells are allowed to fused with the application of electric field.  By using PEG medium (Polyethylene Glycol)
  • 8. Jens Martensson 5. Separation of cell lines  HAT (Hyphoxanthine Aminopterine Thymidine) medium is used for the selection of hybrid cells.  .B cells are HGPRT+ and can survive in the HAT medium but the undergo normal cell death after some division.  Myeloma cells are HGPRT deficient so the cells could not survive in HAT medium since Aminopterin blocks the pathway that allows for nucleotide synthesis.  Hybrid cells has HGPRT enzyme from B cells as well as they have the ability to multiply repeatedly as myeloma cells. So, only hybrid cells can survive in
  • 9. Jens Martensson 6. Screening suitable cell lines  Screening technique used is called ELISA.  The hybridoma culture supernatant, secondary enzyme labeled conjugate, and chromogenic substrate.  Then it is incubated and the formation of a colored product indicates a positive hybridoma.  Alternatively, immunocytochemical screening can also be used.
  • 10. Jens Martensson 7.Methods multiplying hybridoma cell  Introduce of hybridoma cells into peritoneal cavity of mice.  Ascetic fluid is isolated from the mice.  Isolate antibodies from ascetic fluid.  Culturing of hybridoma cells in suitable culture media (  Antibodies is isolated and purified.
  • 11. Jens Martensson 8. Harvesting  Once a hybridoma colony is established, it will continually grow in culture medium like RPMI-1640 (with antibiotics and fetal bovine serum) and produce antibodies.  Multiwell plates are used initially to grow the hybridomas.  After selection, they are changed to tissue culture flasks to provides enough cells for cryopreservation and supernatant for subsequent investigations.
  • 12. ADVANTAGES OF HYBRIDOMA In vitro • reduce the use of mice at the antibody-production stage • ease of culture for production, compared with use of animals, and because of economic considerations. • decrease the need for laboratory personnel experienced in animal handling. In Vivo • produces very high mAb. • high concentration of the desired mAb in mouse ascites fluid avoids the effects of contaminants in in vitro batch-culture fluid when comparable quantities of mAb are used. • reduce the need to teach the antibody producer tissue-culture methods. 12
  • 13. DISADVANTAGE OF HYBRIDOMA • Some cell may do not grow well in culture or are lost in culture. • Require the use of FBS, which limits some antibody uses. • In batch tissue-culture methods, mAb concentration tends to be low in the supernatant In vitro • involves the continued use of mice requiring daily observation. • can be expensive if immunodeficient mice in a barrier facility must be used. • can contain various mouse proteins and other contaminants that might require purification. In vivo 13
  • 14. CONCLUSION • Hybridoma is fusion of two cell between tumor cell and Beta cell which specifically beta lymphocytes cell from mice. • The hydridoma is used to produce monoclonal antibodies to treat cancer disease such as cardiovascular disease and ulcerative diseases • Hybridoma can be cultured either in vitro or in vivo . 14
  • 15. REFERENCES • National Research Council (US) Committee on Methods of Producing Monoclonal Antibodies. Monoclonal Antibody Production. Washington (DC): National Academies Press (US); 1999. 4, Summary of Advantages and Disadvantages of In Vitro and In Vivo Methods.Available from: https://www.ncbi.nlm.nih.gov/books/NBK100200/ • Prospecs Protein Cloning, https://www.prospecbio.com/monoclonal_antibodies • Arya George. 2018. Hybridoma Technology. Slide. Mar Ivanios College Trivandrum.Linkedln 15

Notas del editor

  1. This is the question that your experiment answers
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