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Eliza (mutaib)

UNIVERSITY OF KASHMIR
UNIVERSITY OF KASHMIR

The document discusses Enzyme-Linked Immunosorbent Assay (ELISA), a common immunoassay technique used to detect antigens in biological samples. It describes the basic ELISA principles including immobilizing the antigen and using a detection antibody conjugated to an enzyme. The document outlines the advantages of ELISA including high sensitivity and specificity, high throughput, and ability to test various sample types. It also discusses the different types of ELISA - direct, indirect, sandwich, and competitive/inhibition - and compares their features in a table. The key information provided is an overview of the ELISA technique and a comparison of the different types of ELISA assays.

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MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 1 Enzyme-Linked Immunosorbent Assay (ELISA) Enzyme-Linked Immunosorbent Assay (ELISA) is a common immunoassay, in which antibodies, peptides, proteins, and small molecules can be detected and quantified using a multi-well plate. It is a technique to detect the presence of antigens in biological samples. An ELISA, like other types of immunoassays, relies on antibodies to detect a target antigen using highly specific antibody-antigen interactions. Basic ELISA principle: In an ELISA assay, the antigen is immobilized to a solid surface. This is done either directly or via the use of a capture antibody itself immobilized on the surface. The antigen is then complexed to a detection antibody conjugated with a molecule amenable for detection such as an enzyme or a fluorophore. An ELISA assay is typically performed in a multi-well plate (96- or 384-wells), which provides the solid surface to immobilize the antigen. Immobilization of the analytes facilitates the separation of the antigen from the rest of the components in the sample. This characteristic makes ELISA one of the easiest assays to perform on multiple samples simultaneously. Advantages ➢ High sensitivity and specificity: it is common for ELISAs to detect antigens at the picogram level in a very specific manner due to the use of antibodies. ➢ High throughput: commercial ELISA kits are normally available in a 96-well plate format. But the assay can be easily adapted to 384-well plates.
MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 2 ➢ Easy to perform: protocols are easy to follow and involve little hands-on time. ➢ Quantitative: it can determine the concentration of antigen in a sample. ➢ Possibility to test various sample types: serum, plasma, cellular and tissue extracts, urine, and saliva among others. Disadvantages ➢ Temporary readouts: detection is based on enzyme/substrate reactions and therefore readout must be obtained in a short time span. ➢ Limited antigen information: information limited to the amount or presence of the antigen in the sample. TYPES OF ELISA 1.Direct ELISA:It is the simplest configuration in which the antigen is bound by passive adsorption to the solid phase, washed to remove any unbound molecules and then directly incubated with a conjugated antibody. Following the incubation period and additional washing, substrate is added to produce signal that is allowed to develop. After certain time, the substrate
MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 3 reaction is stopped and the resulting signal quantified. It is commonly used for tittering conjugated secondary antibodies and very useful to estimate antigen cross-reactivity. 2. Indirect ELISA :In this system, initial antigen binding and washing steps are the same as the direct method. The main difference in this case is the use of unconjugated antibody to bind the immobilized antigen upon incubation. Following a washing step to remove unbound antibodies, the remaining antigen-bound antibodies are targeted by a conjugated secondary antibody that will generate the readout signal as described for direct ELISA. This system allows multiple sample evaluations using different primary antibodies to be screened with a single conjugated secondary antibody.
MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 4 3.Sandwich ELISA:This assay requires a compatible antibody pair that recognize different antigenic targets (epitopes) on the same antigen. The first antibody, called the capture antibody, is coated on the plate and used to immobilize the antigen upon binding during incubation with the sample. Free antigen is removed by a washing step and then a detection antibody is added to bind the captured antigen and enable subsequent detection. Sandwich ELISA is divided into two main systems: I. Direct Sandwich :It uses a detection antibody conjugated to an enzyme or fluorescence tag. Following incubation with the antibody-antigen complex immobilized on the plate well, signal detection is performed upon successive addition of substrate and stopping solution or appropriate excitation/emission of the fluorescent tag. II. Indirect Sandwich : uses an unconjugated antibody bound to the antibody-antigen complex on the well. Following a washing step to remove unbound antibodies, the remaining antigen-bound antibodies are targeted by a conjugated secondary detection antibody. Signal detection is performed upon successive addition of substrate and stopping solution or appropriate excitation/emission of the fluorescent tag.
MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 5 4. Competitive and Inhibition ELISA:Each of the core systems described above can be further modified to measure molecules based on their ability to interfere with a well- known pre-titrated assay. Such assays can be used to study either antigens or antibodies and they can be competitive or inhibitory based on the specific conditions of each assay. In both types of assays, a pre-titrated system is challenged with the presence of the testing sample whose binding activity is then determined from the degree of the resulting interference in the established system.
MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 6 ELISA COMPARSIONS TABULATED FORMAT Direct Indirect Sandwich Direct Sandwich Indirect Coating (adsorption to solid phase) Antigen Antigen Capture antibody Capture antibody Blocking Addition of blocking agent to prevent non-specific binding Wash Separate bound/unbound analytes Analyte (addition of testing sample) Enzyme- or fluorescence- conjugated antibody Unconjugated antibody Antigen sample Antigen sample Wash Separate bound/unbound analytes Secondary reagent N/A Enzyme- or fluorescence- conjugated antibody Enzyme- or fluorescence- conjugated detection antibody Biotin- conjugated or unconjugated detection antibody Wash Separate bound/unbound analytes Additional reagent N/A N/A N/A Enzyme- or fluorescence- conjugated streptavidin or secondary antibody Wash Separate bound/unbound analytes Signal development Addition of substrate for enzyme-conjugated antibodies Stop signal development For end-point reading of enzyme-based detection systems Signal Detection Colorimetric, fluorescent, or chemiluminescent detection
MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 7 Which type of ELISA should I use? Advantages Disadvantages Direct ELISA Short protocol: saves time and reagents. No cross-reactivity from secondary antibody. Potential high background: all proteins in the sample bind to the surface. No signal amplification. Low flexibility: the primary antibody must be conjugated. Indirect ELISA Signal amplification: several secondary antibodies will bind to the primary antibody. High flexibility: the same secondary antibody may be used for several primary antibodies. Long protocol if compared to direct ELISA. Potential cross-reactivity from secondary antibody. Sandwich ELISA High specificity: involves two antibodies detecting different epitopes on the same antigen. Suitable for complex samples. High flexibility and sensitivity: both direct and indirect methods can be used. Demanding design: finding two antibodies against the same target that recognize different epitopes and work well together can be challenging at times. Competitive ELISA Depends on base ELISA selected. Suitable for small antigens. Depends on base ELISA selected THANK YOU

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Eliza (mutaib)

  • 1. MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 1 Enzyme-Linked Immunosorbent Assay (ELISA) Enzyme-Linked Immunosorbent Assay (ELISA) is a common immunoassay, in which antibodies, peptides, proteins, and small molecules can be detected and quantified using a multi-well plate. It is a technique to detect the presence of antigens in biological samples. An ELISA, like other types of immunoassays, relies on antibodies to detect a target antigen using highly specific antibody-antigen interactions. Basic ELISA principle: In an ELISA assay, the antigen is immobilized to a solid surface. This is done either directly or via the use of a capture antibody itself immobilized on the surface. The antigen is then complexed to a detection antibody conjugated with a molecule amenable for detection such as an enzyme or a fluorophore. An ELISA assay is typically performed in a multi-well plate (96- or 384-wells), which provides the solid surface to immobilize the antigen. Immobilization of the analytes facilitates the separation of the antigen from the rest of the components in the sample. This characteristic makes ELISA one of the easiest assays to perform on multiple samples simultaneously. Advantages ➢ High sensitivity and specificity: it is common for ELISAs to detect antigens at the picogram level in a very specific manner due to the use of antibodies. ➢ High throughput: commercial ELISA kits are normally available in a 96-well plate format. But the assay can be easily adapted to 384-well plates.
  • 2. MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 2 ➢ Easy to perform: protocols are easy to follow and involve little hands-on time. ➢ Quantitative: it can determine the concentration of antigen in a sample. ➢ Possibility to test various sample types: serum, plasma, cellular and tissue extracts, urine, and saliva among others. Disadvantages ➢ Temporary readouts: detection is based on enzyme/substrate reactions and therefore readout must be obtained in a short time span. ➢ Limited antigen information: information limited to the amount or presence of the antigen in the sample. TYPES OF ELISA 1.Direct ELISA:It is the simplest configuration in which the antigen is bound by passive adsorption to the solid phase, washed to remove any unbound molecules and then directly incubated with a conjugated antibody. Following the incubation period and additional washing, substrate is added to produce signal that is allowed to develop. After certain time, the substrate
  • 3. MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 3 reaction is stopped and the resulting signal quantified. It is commonly used for tittering conjugated secondary antibodies and very useful to estimate antigen cross-reactivity. 2. Indirect ELISA :In this system, initial antigen binding and washing steps are the same as the direct method. The main difference in this case is the use of unconjugated antibody to bind the immobilized antigen upon incubation. Following a washing step to remove unbound antibodies, the remaining antigen-bound antibodies are targeted by a conjugated secondary antibody that will generate the readout signal as described for direct ELISA. This system allows multiple sample evaluations using different primary antibodies to be screened with a single conjugated secondary antibody.
  • 4. MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 4 3.Sandwich ELISA:This assay requires a compatible antibody pair that recognize different antigenic targets (epitopes) on the same antigen. The first antibody, called the capture antibody, is coated on the plate and used to immobilize the antigen upon binding during incubation with the sample. Free antigen is removed by a washing step and then a detection antibody is added to bind the captured antigen and enable subsequent detection. Sandwich ELISA is divided into two main systems: I. Direct Sandwich :It uses a detection antibody conjugated to an enzyme or fluorescence tag. Following incubation with the antibody-antigen complex immobilized on the plate well, signal detection is performed upon successive addition of substrate and stopping solution or appropriate excitation/emission of the fluorescent tag. II. Indirect Sandwich : uses an unconjugated antibody bound to the antibody-antigen complex on the well. Following a washing step to remove unbound antibodies, the remaining antigen-bound antibodies are targeted by a conjugated secondary detection antibody. Signal detection is performed upon successive addition of substrate and stopping solution or appropriate excitation/emission of the fluorescent tag.
  • 5. MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 5 4. Competitive and Inhibition ELISA:Each of the core systems described above can be further modified to measure molecules based on their ability to interfere with a well- known pre-titrated assay. Such assays can be used to study either antigens or antibodies and they can be competitive or inhibitory based on the specific conditions of each assay. In both types of assays, a pre-titrated system is challenged with the presence of the testing sample whose binding activity is then determined from the degree of the resulting interference in the established system.
  • 6. MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 6 ELISA COMPARSIONS TABULATED FORMAT Direct Indirect Sandwich Direct Sandwich Indirect Coating (adsorption to solid phase) Antigen Antigen Capture antibody Capture antibody Blocking Addition of blocking agent to prevent non-specific binding Wash Separate bound/unbound analytes Analyte (addition of testing sample) Enzyme- or fluorescence- conjugated antibody Unconjugated antibody Antigen sample Antigen sample Wash Separate bound/unbound analytes Secondary reagent N/A Enzyme- or fluorescence- conjugated antibody Enzyme- or fluorescence- conjugated detection antibody Biotin- conjugated or unconjugated detection antibody Wash Separate bound/unbound analytes Additional reagent N/A N/A N/A Enzyme- or fluorescence- conjugated streptavidin or secondary antibody Wash Separate bound/unbound analytes Signal development Addition of substrate for enzyme-conjugated antibodies Stop signal development For end-point reading of enzyme-based detection systems Signal Detection Colorimetric, fluorescent, or chemiluminescent detection
  • 7. MUTAIB SIDDIQUI MSC 4TH SEM UNIVERSITY OF KASHMIR 7 Which type of ELISA should I use? Advantages Disadvantages Direct ELISA Short protocol: saves time and reagents. No cross-reactivity from secondary antibody. Potential high background: all proteins in the sample bind to the surface. No signal amplification. Low flexibility: the primary antibody must be conjugated. Indirect ELISA Signal amplification: several secondary antibodies will bind to the primary antibody. High flexibility: the same secondary antibody may be used for several primary antibodies. Long protocol if compared to direct ELISA. Potential cross-reactivity from secondary antibody. Sandwich ELISA High specificity: involves two antibodies detecting different epitopes on the same antigen. Suitable for complex samples. High flexibility and sensitivity: both direct and indirect methods can be used. Demanding design: finding two antibodies against the same target that recognize different epitopes and work well together can be challenging at times. Competitive ELISA Depends on base ELISA selected. Suitable for small antigens. Depends on base ELISA selected THANK YOU