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Radioimmunoassay
&
Enzyme Linked Immunosorbent Assay
Presented By:- Sakshi Jaiswal
PHARM.D 1st year
y
• Principle: Uses an immune reaction [Antigen –
Antibody reaction] to estimate a ligand
Ag + Ag* + Ab 🡪 AgAb + Ag*Ab + Ag + Ab*
– Unbound Ag* and Ag washed out
– Radioactivity of bound residue measured
– Ligand conc is inversely related to radioactivity
[Ag : ligand to be measured ; Ag* radiolabelled ligand]
Principle of solid phase radioimmunoassay
Standard curve between the percent of bound
labelled antigen and concentration of unlabelled
antigen
Advantages & Disadvantages of RIA
• Advantages
– Highly specific: Immune reactions are specific
– High sensitivity : Immune reactions are sensitive
• Disadvantages
– Radiation hazards: Uses radiolabelled reagents
– Requires specially trained persons
– Labs require special license to handle radioactive
material
– Requires special arrangements for
• Requisition, storage of radioactive material
• radioactive waste disposal.
Requirements for RIA
1. Preparation & characterisation of the
Antigen [Ligand to be analysed]
2. Radiolabelling of the Antigen
3. Preparation of the Specific Antibody
4. Development of Assay System
Preparation & Radiolabelling of the
Antigen
• Antigens prepared by..
– Synthesis of the molecule
– Isolation from natural sources
• Radiolabelling [Tagging procedure]
– 3 H 14 C 125 I are used as radioactive tags
– Antigens are tagged to 3 H 14 C 125
– Tagging should NOT affect Antigenic specificity &
Antigenic activity !
Preparation of the Specific Antibody
• Antigen injected intradermally into rabbits or
guinea pigs 🡪 antibody production
• Antibodies recovered from the serum
• Some ligands are not Antigenic
– Hormones, Steroids, Drugs 🡪 HAPTENS
– Eg: Gastrin, Morphine,
– Haptens conjugated to albumin 🡪 antigenic
Development of the Assay System
• A crucial step is separation of unbound antigens
• This achieved by binding the antibodies to the
microtitre well surface [Solid phase RIA]
• Antigens bound to the fixed antibodies remain
stuck to the inner surface
• Decanting & washing the well removes unbound
antigens
• Other techniques of separation: Centrifugation
Assay Procedure
• Add known amounts of the test sample + labelled antigen
into the microtitre wells
• Incubate 🡪 allow the reaction to reach completion
• Decant & wash contents of the well 🡪 removes all unbound
antigens
• Radioactivity remaining in the Microtitre wells measured by
a Counter [GM counter , Scintillation counter etc]
• Intensity of radioactivity is inversely correlated with the
conc of antigens in the test sample
• Sensitive to very low conc of antigens
Enzyme Linked
Immunosorbent Assay
• Principle:
– Uses an immune reaction like RIA
– Differs from RIA in detection method
– Detection based on
• Enzyme catalysed reaction OR
• Fluorescent probe
• NOT radioactivity [great advantage!]
Advantages of ELISA
• Sensitive: nanogram levels or lower
• Reproducible
• Minimal reagents
• Qualitative & Quantitative
– Qualitative 🡪 Eg HIV testing
– quantitative assays 🡪 Eg Ther. Drug Monitoring
• Greater scope : Wells can be coated with Antigens OR
Antibodies
• Suitable for automation 🡪high speed
• NO radiation hazards
Types of ELISA
1. Noncompetitive binding assay or Sandwich
method
1. Antigen measuring system [Titrewells coated with
antibodies ; Enzyme labelled antibodies]
2. Antibody measuring system [Titrewells coated with
antigens ; Enzyme labelled antiantibodies]
2. Competitive binding assay [Titrewells coated with
antibodies ; Enzyme labelled antigens]
Noncompetitive or Sandwich Assay
• Antigen measuring system
– Titre wells coated with suitable antibody
– Add patient sample containing the antigen
– Incubate: till antigen antibody reaction is complete
– Wash🡪 remove unbound antigen
– Add Antibody labelled with Enzyme
– Incubate till antigen binds labelled antibody
– Wash 🡪 remove unbound labelled antibody
– Add substrate ; incubate
– Enzyme + Substrate 🡪 Product 🡪 measure colour
– Colour proportional to antigen in patient sample
Noncompetitive or Sandwich Assay
• Antibody measuring system
– Titre wells coated with suitable antigen
– Add patient sample containing the antibody
– Incubate: till antigen antibody reaction is complete
– Wash🡪 remove unbound antibody
– Add Antiantibody labelled with Enzyme
– Incubate till labelled antiantibodies binds antigen-
antibody complex
– Wash 🡪 remove unbound labelled antiantibody
– Add substrate ; incubate
– Enzyme + Substrate 🡪 Product 🡪 measure colour
– Colour proportional to antibody in patient sample
Diagram showing the principle of Non
competitive ELISA
Competitive binding assay
• Titrewells coated with antibodies
• Known quantities of patient sample containing antigen
+ antigen labelled with enzyme
• Incubate: till antigen antibody reaction is complete
• Wash🡪 remove unbound antigens
• Add substrate ; incubate
• Enzyme + Substrate 🡪 Product 🡪 measure colour
• Colour inversely related to antigen in patient sample
Diagram showing the principle of
Competitive ELISA
Enzyme labels
• Enzyme labels should have high specific reactivity
• Should be easily coupled to ligands & the labelled
complex must be stable
• The reactivity should be retained after linking of the
enzyme to the antigen/antibody
• The chosen enzymes should not be normally present in
the patient samples
• Examples of enzyme labels
– Horse radish peroxidase, Alkaline phosphatase, Glucose
oxidase
Applications of Immunoassays
[RIA & ELISA]
• Analysis of hormones, vitamins, metabolites, diagnostic
markers
– Eg. ACTH, FSH, T3, T4, Glucagon, Insulin, Testosterone,
vitamin B12, prostaglandins, glucocorticoids,
• Therapeutic drug monitoring:
– Barbiturates, morphine, digoxin,
• Diagnostic procedures for detecting infection
– HIV, Hepatitis A, B etc
THANK YOU

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ELISA and RIA

  • 1. Radioimmunoassay & Enzyme Linked Immunosorbent Assay Presented By:- Sakshi Jaiswal PHARM.D 1st year
  • 2. y • Principle: Uses an immune reaction [Antigen – Antibody reaction] to estimate a ligand Ag + Ag* + Ab 🡪 AgAb + Ag*Ab + Ag + Ab* – Unbound Ag* and Ag washed out – Radioactivity of bound residue measured – Ligand conc is inversely related to radioactivity [Ag : ligand to be measured ; Ag* radiolabelled ligand]
  • 3. Principle of solid phase radioimmunoassay
  • 4. Standard curve between the percent of bound labelled antigen and concentration of unlabelled antigen
  • 5. Advantages & Disadvantages of RIA • Advantages – Highly specific: Immune reactions are specific – High sensitivity : Immune reactions are sensitive • Disadvantages – Radiation hazards: Uses radiolabelled reagents – Requires specially trained persons – Labs require special license to handle radioactive material – Requires special arrangements for • Requisition, storage of radioactive material • radioactive waste disposal.
  • 6. Requirements for RIA 1. Preparation & characterisation of the Antigen [Ligand to be analysed] 2. Radiolabelling of the Antigen 3. Preparation of the Specific Antibody 4. Development of Assay System
  • 7. Preparation & Radiolabelling of the Antigen • Antigens prepared by.. – Synthesis of the molecule – Isolation from natural sources • Radiolabelling [Tagging procedure] – 3 H 14 C 125 I are used as radioactive tags – Antigens are tagged to 3 H 14 C 125 – Tagging should NOT affect Antigenic specificity & Antigenic activity !
  • 8. Preparation of the Specific Antibody • Antigen injected intradermally into rabbits or guinea pigs 🡪 antibody production • Antibodies recovered from the serum • Some ligands are not Antigenic – Hormones, Steroids, Drugs 🡪 HAPTENS – Eg: Gastrin, Morphine, – Haptens conjugated to albumin 🡪 antigenic
  • 9. Development of the Assay System • A crucial step is separation of unbound antigens • This achieved by binding the antibodies to the microtitre well surface [Solid phase RIA] • Antigens bound to the fixed antibodies remain stuck to the inner surface • Decanting & washing the well removes unbound antigens • Other techniques of separation: Centrifugation
  • 10. Assay Procedure • Add known amounts of the test sample + labelled antigen into the microtitre wells • Incubate 🡪 allow the reaction to reach completion • Decant & wash contents of the well 🡪 removes all unbound antigens • Radioactivity remaining in the Microtitre wells measured by a Counter [GM counter , Scintillation counter etc] • Intensity of radioactivity is inversely correlated with the conc of antigens in the test sample • Sensitive to very low conc of antigens
  • 11. Enzyme Linked Immunosorbent Assay • Principle: – Uses an immune reaction like RIA – Differs from RIA in detection method – Detection based on • Enzyme catalysed reaction OR • Fluorescent probe • NOT radioactivity [great advantage!]
  • 12. Advantages of ELISA • Sensitive: nanogram levels or lower • Reproducible • Minimal reagents • Qualitative & Quantitative – Qualitative 🡪 Eg HIV testing – quantitative assays 🡪 Eg Ther. Drug Monitoring • Greater scope : Wells can be coated with Antigens OR Antibodies • Suitable for automation 🡪high speed • NO radiation hazards
  • 13. Types of ELISA 1. Noncompetitive binding assay or Sandwich method 1. Antigen measuring system [Titrewells coated with antibodies ; Enzyme labelled antibodies] 2. Antibody measuring system [Titrewells coated with antigens ; Enzyme labelled antiantibodies] 2. Competitive binding assay [Titrewells coated with antibodies ; Enzyme labelled antigens]
  • 14. Noncompetitive or Sandwich Assay • Antigen measuring system – Titre wells coated with suitable antibody – Add patient sample containing the antigen – Incubate: till antigen antibody reaction is complete – Wash🡪 remove unbound antigen – Add Antibody labelled with Enzyme – Incubate till antigen binds labelled antibody – Wash 🡪 remove unbound labelled antibody – Add substrate ; incubate – Enzyme + Substrate 🡪 Product 🡪 measure colour – Colour proportional to antigen in patient sample
  • 15. Noncompetitive or Sandwich Assay • Antibody measuring system – Titre wells coated with suitable antigen – Add patient sample containing the antibody – Incubate: till antigen antibody reaction is complete – Wash🡪 remove unbound antibody – Add Antiantibody labelled with Enzyme – Incubate till labelled antiantibodies binds antigen- antibody complex – Wash 🡪 remove unbound labelled antiantibody – Add substrate ; incubate – Enzyme + Substrate 🡪 Product 🡪 measure colour – Colour proportional to antibody in patient sample
  • 16. Diagram showing the principle of Non competitive ELISA
  • 17. Competitive binding assay • Titrewells coated with antibodies • Known quantities of patient sample containing antigen + antigen labelled with enzyme • Incubate: till antigen antibody reaction is complete • Wash🡪 remove unbound antigens • Add substrate ; incubate • Enzyme + Substrate 🡪 Product 🡪 measure colour • Colour inversely related to antigen in patient sample
  • 18. Diagram showing the principle of Competitive ELISA
  • 19. Enzyme labels • Enzyme labels should have high specific reactivity • Should be easily coupled to ligands & the labelled complex must be stable • The reactivity should be retained after linking of the enzyme to the antigen/antibody • The chosen enzymes should not be normally present in the patient samples • Examples of enzyme labels – Horse radish peroxidase, Alkaline phosphatase, Glucose oxidase
  • 20. Applications of Immunoassays [RIA & ELISA] • Analysis of hormones, vitamins, metabolites, diagnostic markers – Eg. ACTH, FSH, T3, T4, Glucagon, Insulin, Testosterone, vitamin B12, prostaglandins, glucocorticoids, • Therapeutic drug monitoring: – Barbiturates, morphine, digoxin, • Diagnostic procedures for detecting infection – HIV, Hepatitis A, B etc