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Enzyme Linked Immunosorbent Assay Video Lecture | Crash Course for CSIR NET Life Sciences

FAQs on Enzyme Linked Immunosorbent Assay Video Lecture - Crash Course for CSIR NET Life Sciences

1. What is the principle behind Indirect ELISA?
Ans. Indirect ELISA is based on the principle of antigen-antibody interaction. In this assay, an antigen is coated onto a microplate. When a sample containing antibodies is added, these antibodies bind to the antigen. After washing, a secondary antibody, which is linked to an enzyme, is introduced. This secondary antibody binds to the primary antibodies. A substrate is then added, which the enzyme converts into a detectable signal, usually a color change, indicating the presence and quantity of antibodies in the sample.
2. What are the main components involved in an Indirect ELISA?
Ans. The main components of an Indirect ELISA include: 1. <b>Coated Antigen</b>: The specific antigen that is immobilized on the plate. 2. <b>Sample</b>: The test serum or fluid that may contain antibodies against the antigen. 3. <b>Primary Antibody</b>: An antibody that binds specifically to the antigen. 4. <b>Secondary Antibody</b>: An enzyme-linked antibody that binds to the primary antibody. 5. <b>Substrate</b>: A chemical that the enzyme acts upon to produce a measurable signal, usually a color change.
3. What are the advantages of using Indirect ELISA compared to Direct ELISA?
Ans. Indirect ELISA has several advantages over Direct ELISA, including: 1. <b>Increased Sensitivity</b>: The use of a secondary antibody that can bind multiple primary antibodies increases signal amplification. 2. <b>Flexibility</b>: Multiple primary antibodies can be detected using the same secondary antibody, allowing for the simultaneous analysis of different targets. 3. <b>Cost-Effectiveness</b>: Fewer labeled antibodies are required, as one labeled secondary antibody can be used for various primary antibodies.
4. What are some common applications of Indirect ELISA?
Ans. Indirect ELISA is widely used in various fields, including: 1. <b>Diagnostic Testing</b>: For the detection of antibodies against pathogens such as viruses and bacteria. 2. <b>Vaccine Development</b>: To evaluate immune responses in clinical trials. 3. <b>Research</b>: For quantifying specific antibodies in serum or other biological samples. 4. <b>Quality Control</b>: In the manufacturing of vaccines and therapeutic antibodies to ensure consistency and efficacy.
5. What are the steps involved in performing an Indirect ELISA?
Ans. The steps of performing an Indirect ELISA include: 1. <b>Coating the Plate</b>: Add the antigen to the wells of a microplate and incubate to allow binding. 2. <b>Blocking</b>: Add a blocking solution to prevent non-specific binding. 3. <b>Sample Addition</b>: Introduce the test sample containing antibodies and incubate. 4. <b>Washing</b>: Remove unbound antibodies through washing steps. 5. <b>Secondary Antibody Addition</b>: Add an enzyme-linked secondary antibody and incubate. 6. <b>Washing Again</b>: Wash to remove unbound secondary antibodies. 7. <b>Substrate Addition</b>: Add substrate to allow the enzyme to react and generate a measurable signal. 8. <b>Signal Measurement</b>: Measure the signal using a spectrophotometer to determine the concentration of antibodies in the sample.
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