Quantify Human IL-1 beta Levels with High Precision using the Human IL-1 beta ELISA Kit

Quantify Human IL-1 beta Levels with High Precision using the Human IL-1 beta ELISA Kit

The Human IL-1 beta ELISA Kit is a powerful tool for accurately measuring levels of interleukin-1 beta (IL-1 beta) in human samples. This technical article provides an in-depth exploration of the kit, including its components, principles, and applications. Additionally, a comprehensive lab protocol is included to guide researchers in obtaining reliable and reproducible results.

Principles of the Human IL-1 beta ELISA Kit: The Human IL-1 beta ELISA Kit utilizes a sandwich enzyme-linked immunosorbent assay (ELISA) technique. The kit includes specific antibodies that recognize and bind to IL-1 beta, allowing for its detection and quantification. This approach ensures high sensitivity, specificity, and accuracy in measuring IL-1 beta levels.

Components and Storage: The Human IL-1 beta ELISA Kit typically contains pre-coated microplate strips, standard solutions, detection antibodies, enzyme conjugate, substrate solution, stop solution, wash buffer, and a detailed user manual. Proper storage and handling of these components are crucial to maintain their stability and effectiveness.

Lab Protocol: The article presents a step-by-step lab protocol for using the Human IL-1 beta ELISA Kit. It covers sample preparation, plate setup, antibody incubation, washing steps, substrate addition, and measurement using a microplate reader. Adhering to the recommended protocol is essential to ensure accurate and reliable results.

Applications and Significance: The accurate measurement of IL-1 beta levels is vital for understanding the inflammatory response, immune system modulation, and various disease processes in humans. The Human IL-1 beta ELISA Kit offers researchers a valuable tool for investigating these areas, contributing to advancements in immunology, inflammatory disorders, and therapeutic development.

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The Human IL-1 beta ELISA Kit provides a robust and precise method for quantifying IL-1 beta levels in human samples. By following the detailed lab protocol and utilizing this kit, researchers can enhance their understanding of the role of IL-1 beta in various biological processes and diseases. Trust in the reliability and accuracy of the Human IL-1 beta ELISA Kit to facilitate impactful discoveries in the field of immunology and inflammation research.

1. Sample Preparation:

  • Collect human samples (serum, plasma, cell culture supernatant, etc.) and transfer them to clean tubes.
  • Centrifuge the samples at a suitable speed and duration to remove any debris or particles.
  • Transfer the clarified supernatant to new tubes and store on ice until ready for analysis.

2. Kit Preparation:

  • Allow the kit components to reach room temperature (RT) before use.
  • Prepare the necessary reagents, including the standard solutions and working dilutions of the detection antibody and enzyme conjugate as specified in the kit's user manual.
  • Dilute the samples if necessary according to the recommended range provided in the manual.

3. Plate Setup:

  • Remove the desired number of coated microplate strips from the kit, leaving the remaining strips in the provided resealable bag with desiccant to maintain their integrity.
  • Label the plate wells according to the sample and standard identification.
  • Add the diluted samples, standards, and appropriate controls to the designated wells in duplicate or triplicate, following the plate layout provided in the manual.
  • Cover the plate with an adhesive strip and gently shake or tap the plate to ensure thorough mixing.

4. Antibody Incubation:

  • Incubate the plate at a suitable temperature and duration, typically at RT or 37°C, as specified in the manual.
  • Add the detection antibody to each well and gently mix.
  • Incubate the plate while protected from light, allowing the antibody to bind to the captured IL-1 beta.

5. Washing:

  • Carefully remove the adhesive strip from the plate.
  • Wash the plate wells thoroughly with the provided wash buffer, following the recommended number of wash cycles and duration specified in the manual.
  • Completely remove the wash buffer from the wells by gently tapping the plate upside down on a clean absorbent material.

6. Substrate Addition and Measurement:

  • Add the enzyme conjugate to each well and gently mix.
  • Incubate the plate again while protected from light, allowing the conjugate to bind to the IL-1 beta-antibody complex.
  • Add the substrate solution to each well and incubate for a suitable duration to allow color development.
  • Stop the reaction by adding the stop solution to each well.
  • Measure the absorbance of each well using a microplate reader at the appropriate wavelength specified in the manual.

7. Data Analysis:

  • Use the absorbance values obtained from the standard curve to calculate the IL-1 beta concentrations in the samples, following the instructions provided in the manual.
  • Analyze the data statistically using appropriate software or methods.

This general protocol provides a broad overview of the steps involved in using the Human IL-1 beta ELISA Kit. It is crucial to consult the specific instructions and recommendations provided by the manufacturer to ensure accurate and reliable results.

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