Elisa seminar final2

deepak deshkar
deepak deshkarTeacher in medical college en D.Y.Patil medical college,kolhapur
Enzyme-Linked ImmunoSorbant Assay … By Dr. Deshkar DW
1798 - First demonstration of vaccination smallpox vaccination  (Edward Jenner) 1890 - Demonstration of antibody activity against diphtheria and tetanus  toxins. 1890 - Beginning of humoral theory of immunity.  (Emil von Behring & Shibasaburo Kitasato) 1900 - Antibody formation theory (Paul Ehrlich) 1938 - Antigen-Antibody binding hypothesis (John Marrack) 1948 - antibody production in plasma B cells 1959 -1962 - Discovery of antibody structure E nzyme  L inked  I mmuno S orbent  A ssay {ELISA}   History
[object Object],[object Object],[object Object],[object Object],[object Object],E nzyme  L inked  I mmuno S orbent  A ssay {ELISA}   History
[object Object],[object Object],[object Object],[object Object],E nzyme  L inked  I mmuno S orbent  A ssay {ELISA}
Components ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object],[object Object],Components
[object Object],[object Object],[object Object],Components
Components ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
Four major advantages of ELISA Data analysed statistically  ELISA  Enzyme Linked Immunosorbent Assay   Why ELISA? Versatile  Simple  Sensitive  Quantifiable  Many systems using different combinations of reagents are possible  Uses micro-titre plates and allied equipment  Enzyme catalyst amplification  Colour  Passive attachment to solid phase  High Capacity  Ideal range of sensitivity for diagnosis  Read by eye  Easy separation of bound and unbound reactants by washing step  Rapid Cheap  Kits feasible  Multi-channel spectrophotometers  Data can be stored
ELISA : Pros and Cons ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
General Procedure Of ELISA ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
A Microtiter plate (96-well) used for ELISA
General Procedure Of ELISA
Reading plates • Select proper wave-length on machine. •  Carefully wipe bottom of plate to remove excess moisture. Plates that are wet may diffuse your light source, giving inaccurate readings. • Mix the plate. This will distribute color evenly. Some machines have a ‘mix’ setting. General Procedure Of ELISA
HOMOGENOUS ELISA There is no need for phase separation. It is less sensitive than heterogenous  ELISA. Uses: It is suitable for determination of low molecular weight substances. e.g drug monitoring. PRINCIPAL: Enzyme labeled Ag & unknown Ag compete together for Ab-binding sites . The enzyme labeled Ag that remain free is enzymatically active & can be determined in the presence of the bound form.
HETEROGENOUS ELISA ,[object Object],[object Object],[object Object],[object Object],[object Object]
TYPES OF ELISA ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
DIRECT ELISA ,[object Object],[object Object],[object Object],[object Object],[object Object]
DIRECT ELISA
DIRECT ELISA
DIRECT ELISA
[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],DIRECT ELISA
[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],INDIRECT ELISA
INDIRECT ELISA
INDIRECT ELISA
[object Object],[object Object],[object Object],[object Object],[object Object],INDIRECT ELISA
[object Object],[object Object],[object Object],INDIRECT ELISA
SANDWICH ELISA ,[object Object],[object Object],[object Object],[object Object],[object Object]
SANDWICH ELISA
SANDWICH ELISA TYPES ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
SANDWICH DIRECT
SANDWICH DIRECT
SANDWICH INDIRECT
SANDWICH INDIRECT
COMPETITIVE ELISA ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
COMPETITIVE ELISA
ELISA Reverse method & device  (ELISA-R m&d) ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
ADVANTAGES ,[object Object],[object Object],[object Object],[object Object]
PRECAUTIONS Negative control with strong signal  The excessive background signal can be caused by  inadequate rinsing of plates, reagents not sufficiently  diluted, inadequate blocking of plates or non-specific  binding of enzyme conjugate. The appearance of color in  negative control wells may also indicate cross-reactivity of  secondary antibody with components in the antigen  sample.
PRECAUTIONS  contd….. ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],PRECAUTIONS  contd…..
APPLICATIONS ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
APPLICATIONS  contd…. ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
Thank You
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Elisa seminar final2

  • 1. Enzyme-Linked ImmunoSorbant Assay … By Dr. Deshkar DW
  • 2. 1798 - First demonstration of vaccination smallpox vaccination (Edward Jenner) 1890 - Demonstration of antibody activity against diphtheria and tetanus toxins. 1890 - Beginning of humoral theory of immunity. (Emil von Behring & Shibasaburo Kitasato) 1900 - Antibody formation theory (Paul Ehrlich) 1938 - Antigen-Antibody binding hypothesis (John Marrack) 1948 - antibody production in plasma B cells 1959 -1962 - Discovery of antibody structure E nzyme L inked I mmuno S orbent A ssay {ELISA} History
  • 3.
  • 4.
  • 5.
  • 6.
  • 7.
  • 8.
  • 9. Four major advantages of ELISA Data analysed statistically ELISA Enzyme Linked Immunosorbent Assay Why ELISA? Versatile Simple Sensitive Quantifiable Many systems using different combinations of reagents are possible Uses micro-titre plates and allied equipment Enzyme catalyst amplification Colour Passive attachment to solid phase High Capacity Ideal range of sensitivity for diagnosis Read by eye Easy separation of bound and unbound reactants by washing step Rapid Cheap Kits feasible Multi-channel spectrophotometers Data can be stored
  • 10.
  • 11.
  • 12. A Microtiter plate (96-well) used for ELISA
  • 14. Reading plates • Select proper wave-length on machine. • Carefully wipe bottom of plate to remove excess moisture. Plates that are wet may diffuse your light source, giving inaccurate readings. • Mix the plate. This will distribute color evenly. Some machines have a ‘mix’ setting. General Procedure Of ELISA
  • 15. HOMOGENOUS ELISA There is no need for phase separation. It is less sensitive than heterogenous ELISA. Uses: It is suitable for determination of low molecular weight substances. e.g drug monitoring. PRINCIPAL: Enzyme labeled Ag & unknown Ag compete together for Ab-binding sites . The enzyme labeled Ag that remain free is enzymatically active & can be determined in the presence of the bound form.
  • 16.
  • 17.
  • 18.
  • 22.
  • 23.
  • 26.
  • 27.
  • 28.
  • 30.
  • 35.
  • 37.
  • 38.
  • 39. PRECAUTIONS Negative control with strong signal The excessive background signal can be caused by inadequate rinsing of plates, reagents not sufficiently diluted, inadequate blocking of plates or non-specific binding of enzyme conjugate. The appearance of color in negative control wells may also indicate cross-reactivity of secondary antibody with components in the antigen sample.
  • 40.
  • 41.
  • 42.
  • 43.