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Biochemistry clinical practice CLS 432Dr. Samah Kotb Nasr El-deen
ENZYME LINKED IMMUNO SORBENT ASSAY (ELISA) & RADIO IMMUNO ASSAY(RIA)
Lecturer of Biochemistry2015
ENZYME LINKED IMMUNOSORBENT ASSAY
CONTENTS
Introduction to ELISAPrinciple & procedureMaterials neededTypes of ELISAAdvantages & disadvantages of ELISAApplications
ELISA
RIAIntroduction to RIAPrinciple & procedureMaterials neededAdvantages & disadvantages of RIAInstrumentationApplications
INTRODUCTION TO ELISA
• ELISA, or enzyme-linked immunosorbent assay, are quantitative immunological procedures in which the Ag-Ab reaction is monitored by enzyme measurements.
• The term ELISA was first used by Engvall & Perlma in 1971.
• The ELISA test, or the enzyme immunoassay (EIA), was the first screening test commonly employed for HIV. It has a high sensitivity.
Why known as ......? Enzyme Linked Immunosorbent Assay
1. Antigen of interest is absorbed on to plastic surface (‘sorbent’).
2. Antigen is recognised by specific antibody (‘immuno’).3. This antibody is recognised by second antibody
(‘immuno’) which has enzyme attached (‘enzyme-linked’).
4. Substrate reacts with enzyme to produce product, usually coloured.
BASIC PRINCIPLE OF ELISA
Use an enzyme to detect the binding of antigen (Ag) antibody (Ab).
The enzyme converts a colorless substrate (chromogen) to a colored product, indicating the presence of Ag : Ab binding.
An ELISA can be used to detect either the presence of Antigens or antibodies in a sample depending how the test is designed.
ELISA was dveloped in 1970 and became rapidly accepted.
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Materials Needed
• Testing sample.• Antibody (1st, 2nd) / Antigen.• Polystyrene microtiter plate.• Blocking buffer.• Washing buffer.• Substrate.• Enzyme.
ANTIGEN (Ag)
Any molecule that induces production of antibodies when introduced in the body of an animal is called antigen. OR
any “thing”, foreign to the immune system. e.g. bacteria, viruses, (or their parts), pollen, etc.
Protein molecule.Carbohydrate molecule.Microorganisms.Allergens.Viruses Etc.
SYMBOL FOR ANTIGEN
ANTIBODY ( Ab)
• Antibody: proteins produced by the immune system which help defend against antigens.
SYMBOL FOR ANTIBODY
Y
Antibodies (Immunoglobulins)
Specimen Sample For ELISA
SERUM
CSF
SPUTUM
URINE
SEMEN
SUPERNATANT OF CULUTRE
STOOL
Enzymes Used in Elisa
Horseradish peroxidase (most commonly used).Alkaline Phosphatase.β-galactosidase.Lactoperoxidase.Tetra Methyl benzidine is a chromogenic substrate
used in staining procedures in immunohistochemistry .
In case of peroxidase, the substrate hydrogen peroxide is converted into water and o2 in the presence of electron donors(like diaminobenzidine or 4-chloronaphthol which themselves oxidized in the reaction).
Oxidation of diaminobenzidine produces dark brown color while that of 4-chlorornaphthol yields purple color which is the basis of ELISA.
ENZYME SUBSTRATE• Initially the substrate should be colorless• After degradation by the enzyme it should be strongly
colored or fluorescent.
ENZYME SUBSTRATE CHROMOGEN STOPPING
Alkaline Phosphatase
p-NPP p-NPP+ diethandamine+MgCl2
1 M NaOH
Horse radish Peroxidase
H2O2 Tetramethylbenzidine + Phosphate – Citrate buffer
1 M H2SO4
Horse radish Peroxidase
H2O2 O – Phenylenediamine + HCl
1 M HCl
Substrate
Primary antibody
Enzyme
Secondary antibody
Different antigens in sample
Coloured product
Basic Steps Of Enzyme-Linked
ImmunosorbantAssay
TYPES OF ELISA
– Indirect Elisa
– Sandwich Elisa
– Competitive Elisa
Indirect Elisa
Sandwich ELISA
• Antigens such as tumor markers, hormones and serum proteins may be determined
• Antigen in the sample binds with the capture antibody on the microwell and becomes immobilized.
• The antibody of the enzyme conjugate binds with the immobilized antigen to form a sandwich of antibody-antigen-antibody/enzyme bound to the microwell.
Enzyme reaction product is directly proportional to concentration of standard or analytical antigen 21
ELISA SANDWICH FORMAT
Y Y Y
Y Y Y
Y
YY
Y Y Y
Y Y Y
2nd antibody with enzyme
Antibody/Antigen
Antibody
Y Y YY Y Y
enzyme produces colour
Primary antibody (unlabeled) is incubated with sample antigen.
Antibody-antigen complexes are then added to 96-well plates which are pre-coated with the same antigen.
Unbound antibody is removed by washing the plate. (The more antigen in the sample, the less antibody will be able to bind to the antigen in the well, hence "competition.")
The secondary antibody that is specific to the primary antibody and conjugated with an enzyme is added.
A substrate is added, and remaining enzymes elicit a chromogenic or fluorescent signal.
Competitive Elisa
Competitive Elisa
• Increased serum antigen results in reduced binding of the antigen-enzyme conjugate with the capture antibody producing less enzyme activity and color (yellow) formation
Substrate product concentration is inversely proportional to the concentration of standard or test antigen added
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Comparison between Indirect Sandwich & Competitive ELISA
to detect Ab (HIV, HCV)
to detect Ag ( Tumor Markers, Hormones )
to detect Ag ( Free Testosterone)
Results
Importance of incubation step
During the test performance incubation time and mentioned temperature is must required For the proper binding between antigen and antibody and also binding with conjugate and color development of substrate.
Importance of Washing :- For the removal of any unbound Antibody/Antigen proper washing and taping is required other wise we get the incorrect result.
So incubation & washing is much important for good results.
Elisa Plate
Microtitre wells.Generally 96 wells.Marked on one side alphabetically.Numerically on the other side.Comes with the kit.
Using a clean Pipette , add 100 µL of diluted serum sample (Dilute the sera to be tested 1:100 in the sample diluents) to each well. Incubate 1 hour at 37°C .
TEST PERFORMANCE
Measures the absorbance at 450 nm With the help of ELISA READER.
Calculate the absorbance for each sample and reference.
We used Ascent Software for Calculation of the result
ELISA PLATE READY FOR READING
Reagents have a long shelf life. ELISA is highly specific and sensitive.No radiation hazards occur during labelling or disposal
of waste.Easy to perform and quick procedures. Equipment can be inexpensive and widely available.ELISA can be used to a variety of infections.
Advantages of ELISA
Measurement of enzyme activity can be more complex than measurement of activity of some type of radioisotopes.
Enzyme activity may be affected by plasma constituents.
Kits are commercially available, but not cheapVery specific to a particular antigen. Won’t
recognize any other antigen.False positives/negatives possible, especially with
mutated/altered antigen.
Disadvantages of ELISA
Results may not be absolute.
Antibody must be available.
Concentration may be unclear.
False positive possible.
False negative possible.
Limitations
APPLICATIONS OF ELISA
1) Detection of Mycobacterium antibodies in tuberculosis.
2 )Detection of rotavirus in feces.3 )Detection of hepatitis B markers in serum.
4 )Detection of HIV antibodies in blood samples
5) It has also found applications in the food industry in detecting potential food allergens, such as milk, peanuts , walnuts, almonds, and eggs.
APPLICATIONS OF ELISA
1- Hormones 7- Vaccine Quality Control
2- Proteins 8- FOR GMO (Genetically modified organism)
3- Infectious Agent ( Viral, Bacterial, Parasitic, Fungal )
9- For Rapid Test
4- Drug Markers 10- IgG, IgM, IgA
5- Tumor Markers 11- In New Born Screening
6- Serum Proteins 12- In Clinical Research
Equipments for performing the ELISA test
PipettesIncubator
ELISA reader
ELISA READER
THERMOLAB SYSTEM (USA)
Radioimmunoassay
Radioimmunoassay (RIA) is a very sensitive in vitro assay technique used to measure concentrations of antigens (for example, hormone levels in the blood) by use of antibodies.
The RAST test (radioallergosorbent test) is an example of radioimmunoassay. It is used to detect the causative allergen for an allergy.
To perform a radioimmunoassay, a known quantity of an antigen is made radioactive, frequently by labeling it with gamma-radioactive isotopes of iodine attached to tyrosine .
INTRODUCTION
This radiolabeled antigen is then mixed with a known amount of antibody for that antigen, and as a result, the two specifically bind to one another.
Then, a sample of serum from a patient containing an unknown quantity of that same antigen is added.
• This causes the unlabeled (or "cold") antigen from the serum to compete with the radiolabeled antigen ("hot") for antibody binding sites. As the concentration of "cold" antigen is increased, more of it binds to the antibody, displacing the radiolabeled variant, and reducing the ratio of antibody-bound radiolabeled antigen to free radiolabeled antigen. The bound antigens are then separated from the unbound ones, and the radioactivity of the free antigen remaining in the supernatant is measured using a gamma counter.
Principle of Radioimmunoassay
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]
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.
-Radio-isotopes,- Enzymes
FluorescentChemi-luminescent probesMetal tags
Antibodies: types of labelling
Radioimmunoassay(RIA)
• Advantages– Flexibility– Sensitivity– Size
• Disadvantages– Toxicity– Shelf life– Disposal costs
INSTRUMENTATION
Incubate tissue withradioactive ligand
Expose to filmor emulsion
Isotope will emitradiation (usually beta)
Radiation will hit silver grains in emulsion and expose them
Autoradiography
INSTRUMENTATION
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