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HTRF MAb Anti 6HIS-Eu cryptate Kinase Binding Kit, 1,000 Assay Points

​​This anti 6HIS-Eu cryptate is used in the HTRF® Kinase Binding format, in combination with a 6HIS-tagged Kinase and red-fluorescent tracers.

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Feature Specification
Application Biochemical Enzymatic Assay
Sample Volume 5 µL

​​This anti 6HIS-Eu cryptate is used in the HTRF® Kinase Binding format, in combination with a 6HIS-tagged Kinase and red-fluorescent tracers.

Click to copy promo code to clipboard.
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SAVE 10% on your first Revvity.com order. Use promo code below.

HELLO10

Terms and conditions apply.

Product Variants
Unit Size: 1,000 assay points
Part #:
62KBHISKAF
List Price
USD 277.46
Your online price:
Unit Size: 20,000 assay points
Part #:
62KBHISKAB
List Price
USD 2,021.84
Your online price:
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

MAb Anti-6HIS-Eu cryptate Kinase Binding is an IgG2a raised against a polyhistidine tagged fusion protein labeled with Eu. It has been shown to react with 6HIS-tagged kinases.

This reagent is intended for use in the biochemical HTRF Kinase Binding platform.​

Specifications

Application
Biochemical Enzymatic Assay
Brand
HTRF
Detection Modality
HTRF
Product Group
Fluorescent Reagent
Sample Volume
5 µL
Shipping Conditions
Shipped in Dry Ice
Target Class
Kinases
Technology
TR-FRET
Therapeutic Area
Metabolism/Diabetes
Neuroscience
Oncology & Inflammation
Unit Size
1,000 assay points

Video gallery

How it works

Kd determination assay principal

​The binding of the tracers is detected in a sandwich assay format using the Anti 6HIS antibody labeled with Europium Cryptate (donor), which binds to the 6HIS-tagged Kinase, and a red fluorescent tracer labelled with d2 (acceptor). The detection principle is based on HTRF® technology. The HTRF ratio (665/620) will increase upon the addition of more of the tracer, and will saturate depending on the dissociation constant (Kd) of the tracer to the 6HIS-tagged kinase.

1kinase-binding-how-it-works-assay-principal-saturation-staurosporine-red-62kb01redc-62kb01rede.svg

 

Kd determination assay protocol

Saturation binding experiments on the three tracers (i.e. Staurosporine-Red, Dasatinib-Red, and Sunitinib-Red) can be run in 96- or 384-well plates (20 µL final volume). First, a dilution series of tracer ranging between 0 and 1 µM in the Kinase Binding Buffer is prepared in a 96-well non-binding plate. Next, 5 µL of Kinase Binding Buffer are dispensed into the final 96- or 384-well plate. Then 5 µL of 6HIS tagged-Kinase are added, followed by 5 µL of Anti-6HIS Eu-cryptate. Finally, 5 µL of the red tracer solution are added. The HTRF ratio is measured after 1 H of incubation.

2kinase-binding-how-it-works-assay-protocol-saturation-staurosporine-red-62kb01redc-62kb01rede.svg

 

IC50/Ki determination assay principle

Principle of HTRF® Kinase binding assay (IC50/Ki-determination). The binding of the tracers is detected in a sandwich assay format using the Anti-6HIS labeled with Europium Cryptate (donor), which binds to the tagged Kinase, and a red fluorescent tracer labelled with d2 (acceptor). The detection principle is based on HTRF® technology. The HTRF ratio (665/620) will increase upon the addition of more of the tracer, and will saturate depending on the dissociation constant (Kd ) of the tracer to the tagged kinase. When an inhibitor of the kinase is added, the tracer will be displaced and the HTRF signal will disappear, depending on the dose.

10kinase-binding-how-it-works-assay-principal-inhibition-anti-gst-eu-62kbgstkab-62kbgstkaf.svg

 

IC50/Ki determination assay protocol

​​Pharmacological evaluation of inhibitors of interest can be run in 96- or 384-well plates. First a dilution series ranging between 40 µM and 0.23 nM of inhibitor is prepared, and 5 µL of each concentration are dispensed into the plate. Next, 5 µL of tagged-Kinase are added, followed by 5 µL of anti-6HIS Eu-cryptate. Finally, 5 µL of tracer solution are added, prepared at 4x the final concentration. The HTRF ratio is measured after 1H of incubation. Analyses of the data give typical dose response curves ranging between 10 µM and 56 pM, enabling an evaluation of the IC50/Ki values for the inhibitor of interest.

2kinase-binding-how-it-works-assay-protocol-saturation-staurosporine-red-62kb01redc-62kb01rede.svg

 

Assay validation

Saturation Binding FGFR1-6HIS

​​​A typical saturation binding experiment is performed using final tracer concentrations between 0 and 250 nM, and measuring total- and non-specific binding signals. Subtracting the non-specific from the total binding signal gives the specific signal, which can be analysed to give the Kd. Here an example is shown where the best tracer for inhibitor studies proved to be Staurosporine-Red, with a Kd of 22 nM on 5 nM FGFR1-6HIS.

 

1assay-validation-kinase-binding-6his-discovery-1.svg

 

Competitive Binding PDGFRb-6HIS

D​ose response curves of various known kinase inhibitors (Staurosporine, Dasatinib, PP2, Imatinib, Tozasertib, Sunitinib, Gefitinib, and Sorafenib) were measured using Sunitinib-Red at its Kd (45 nM) on 5 nM PDGFRb-6HIS. Staurosporine, Dasatinib, Sunitinib, and Imatinib show showed high potencies, in good correlation with literature values.

2assay-validation-kinase-binding-6his-discovery-2.svg

 

Resources

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