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HTRF Human IL-1β High Performance Detection Kit, 96 Assay Points

The HTRF High Performance Human IL-1β kit is designed for the quantification of human IL-1β release in cell supernatant. It replaces the existing HTRF human IL-1β kit.

For research use only. Not for use in diagnostic procedures. All products to be used in accordance with applicable laws and regulations including without limitation, consumption and disposal requirements under European REACH regulations (EC 1907/2006).

Feature Specification
Application Protein Quantification
Sample Volume 16 µL

The HTRF High Performance Human IL-1β kit is designed for the quantification of human IL-1β release in cell supernatant. It replaces the existing HTRF human IL-1β kit.

For research use only. Not for use in diagnostic procedures. All products to be used in accordance with applicable laws and regulations including without limitation, consumption and disposal requirements under European REACH regulations (EC 1907/2006).

Overview

IL-1β, also known as leukocytic pyrogen or mononuclear cell factor, is a pro-inflammatory cytokine of the IL1 family. IL1 beta is considered to be a major endogenous pyrogen and induces prostaglandin synthesis, T cell activation, B cell activation, and subsequent antibody production. It is also a known promoter of T cell differentiation into Th17.

Assessment of serum samples often requires enhanced sensitivity. In some cases, AlphaLISA assays may have sufficient sensitivity to enable the detection of low levels of analytes in serum or plasma. Check out the Human IL-1β AlphaLISA kit's analytical performances for more information, or learn more about AlphaLISA. When assaying, always follow the recommended protocol and avoid highly haemolyzed samples.

Specifications

Application
Protein Quantification
Brand
HTRF
Detection Modality
HTRF
Product Group
Kit
Sample Volume
16 µL
Shipping Conditions
Shipped in Dry Ice
Target Class
Cytokines
Target Species
Human
Technology
TR-FRET
Unit Size
96 Assay Points

Video gallery

How it works

Assay principle

Cell supernatant, sample, or standard is dispensed directly into the assay plate for the detection by HTRF® reagents (384-well low-volume white plate or Revvity low-volume 96-well plate in 20 µl). The antibodies labeled with the HTRF donor and acceptor are pre-mixed and added in a single dispensing step to further streamline the assay procedure. The assay can be run up to a 1536-well format by simply resizing each addition volume proportionally.

 

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Assay data analysis

The 4 Parameter Logistic (4PL) curve is commonly recommended for fitting an ELISA standard curve. This regression enables the accurate measurement of an unknown sample across a wider range of concentrations than linear analysis, making it ideally suited to the analysis of biological systems like cytokine releases.

To fully understand how to deal with HTRF data processing and also 4PL 1/y² fitting, 

Revvity also worked with Myassays.com to help you in your data analyses. You’ll be able to access a free online software to run your IL1 beta analysis.

 

Assay details

Human IL-1β standard curve

The IL-1β standard curve is generated in the assay Diluent 5 provided in the kit.

 


 

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Human IL-1β Assay Specifications

 

Sample size 16 µL
Final assay volume 20 µL
Kit components Lyophilized standard, frozen detection antibodies, buffers & protocol
LOD & LOQ (in Diluent) 8.3 pg/mL & 18.8 pg/mL
LOD & LOQ (in DMEM+10%FCS) 11.3 & 26.7 pg/mL
LOD & LOQ (in RPMI+10%FCS) 15.3 & 28.5 pg/mL
Range 75.8 – 6 500 pg/mL
Time to result 4h at RT
Correspondance to I.S. NIBSC (86/680) value (IU/mL) = 0,07 x HTRF hIL1ß value (pg/mL)
Species Human only

 

 

Analytical performance

Intra and inter assay

Intra-assay (n=24)

Sample Mean [IL-1ß] (pg/mL) CV
1 73.7 7%
2 714.4 2%
3 3406.8 2%
  Mean CV 4%

Each of the 3 samples was measured 24 times, and the % CV was calculated for each sample.

 

Inter-assay (n=4)

Sample Mean [IL-1ß] (pg/mL) CV
1 76 9%
2 702 8%
3 3095 4%

 
Mean CV 7%

Each of the samples was measured in 4 different experiments, and the % CV was calculated for each sample.

 

Dilutional linearity

The excellent % of recovery obtained from these experiments show the good dilution linearity of the assay. Samples are PBMC supernatants serially diluted with the kit DIL5 diluent.

Dilution Factor [IL-1β] Expected (pg/mL) [IL-1β] Measured (pg/mL) Dilution Recovery
Neat - 951  
1.5 655 610 93%
2.25 436 442 101%
3.37 291 287 99%
5.07 194 202 104%
  Mean CV   99%

 

 

Antigen Spike and Recovery

Recombinant cytokine was added to PBMC supernatant samples, and the measured response was compared to the calculated expected values. The 100% of recovery indicates similar measurements of cytokine from a sample and the kit standard.

Sample [IL-1β] Spiked Sample (pg/mL) [IL-1β] Standard (pg/mL) Expected (pg/mL) Measured (pg/mL) Recovery
1 982 3095 2039 1972 97%
334 658 637 97%
2 574 3095 1835 1720 94%
334 454 384 84%
Mean CV       93%

 

 

Cross reactivities

Cross reactivities were assessed using recombinant proteins from the IL-1 cytokine family. Proteins were tested up to 6 500 pg/mL, and standard curves were generated for each. Signals were interpolated on the assay standard curve to interpolate concentrations. The assay is human specific, as mouse IL-1β cytokines were not detected.

Tested Protein Cross Reactivity
Human IL-1β 100%
Human IL-1α 0%
Mouse IL-1β 0%

 

Assay validation

Modulation of secretion of human IL-1β in THP1 cell line

THP1 cells plated at 25, 50, and 100 kcells/well were stimulated for 18h with PMA and LPS, respectively used at 50 ng/mL and 1 µg/mL. 16 µL of supernatants were then transferred into a white detection plate (384 low volume) to be analyzed with the Human IL-1ß Assay.

 

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IL-1ß secretion in PBMC stimulated with LPS

PBMC plated at 50, 100, and 200 kcells/well were stimulated for 18 h with increasing concentrations of LPS ranging from 0.02 to 2 µg/mL. Then 16 µL of supernatants were transferred into a white detection plate (384 low volume) to be analyzed using the Human IL-1ß assay kit.

 

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Effect of dexamethasone on PBMC induced IL-1ß release

PBMC plated at 50 and 100 kcells/well were stimulated for 18h with 0.2 µg/mL of LPS and a co-treatment of increasing concentrations of dexamethasone, ranging from 0.05 to 50 µg/mL. Then 16 µL of supernatants were transferred into a white detection plate (384 low volume) to be analyzed using the Human IL-1ß Assay Kit.

 

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Resources

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