Three Mechanistically Distinct Kinase Assays Compared: Measurement of Intrinsic ATPase Activity Identified the Most Comprehensive Set of ITK Inhibitors

Kashem, Mohammed A.; Nelson, Richard M.; Yingling, Jeffrey D.; Pullen, Steven S.; Prokopowicz, Anthony S.; Jones, Jessi Wildeson; Wolak, John P.; Rogers, George R.; Morelock, Maurice M.; Snow, Roger J.; Homon, Carol; Jakes, Scott

doi:10.1177/1087057106296047

Cited by 113 publications

(80 citation statements)

References 39 publications

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“…Decisions on whether to use a binding assay or measure phosphorylation, whether to use colorimetric, fluorescent, radiometric or luminescence endpoints and what format to use are all important. It has been noted that different assay formats can give different results, so one approach is to carry out a number of assay types in parallel to look for consistent patterns [78,107,128].…”

Section: Understanding the Limitations Of In Vitro Kinase Selectivitymentioning

confidence: 99%

Measuring and interpreting the selectivity of protein kinase inhibitors

2009

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Protein kinase inhibitors are a well-established class of clinically useful drugs, particularly for the treatment of cancer. Achieving inhibitor selectivity for particular protein kinases often remains a significant challenge in the development of new small molecules as drugs or as tools for chemical biology research. This review summarises the methodologies available for measuring kinase inhibitor selectivity, both in vitro and in cells. The interpretation of kinase inhibitor selectivity data is discussed, particularly with reference to the structural biology of the protein targets. Measurement and prediction of kinase inhibitor selectivity will be important for the development of new multi-targeted kinase inhibitors.

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Section: Understanding the Limitations Of In Vitro Kinase Selectivitymentioning

confidence: 99%

Measuring and interpreting the selectivity of protein kinase inhibitors

2009

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“…When the same assay was reconfigured in the TR-FRET format presented here, the observed IC 50 for staurosporine was reduced to 3 nM (data not shown). 37 The ability to use a sub-K d concentration of kinase, as well as a concentration of tracer that is close to the K d for the kinase⋅tracer interaction, is particularly advantageous when using tracers that have relatively low affinity for the kinase (>100 nM K d ) and is a distinguishing feature of the TR-FRET format that we have presented when compared to binding assays performed in FLT, 5 FP, 2 or EFC 7 formats. Although the convenience of using an epitope tag for the purification or visualization of a recombinant kinase is well established, such tags could potentially alter the activity of the kinase being studied.…”

Section: Discussionmentioning

confidence: 99%

“…Common requirements for all activity-based assays include a suitable substrate for phosphorylation, sufficient catalytic activity to generate an adequate amount of product for detection, and a direct or indirect means of detecting the phosphorylation event. There are exceptions to these requirements, such as the use of nonactivated kinases in "cascade" types of assays 1 or the use of water as a nonspecific phosphoacceptor substrate, 2 but these exceptions often come with their own caveats such as complications from nonlinear product formation or slower reaction rates. In contrast, the requirements for an assay to directly measure the affinity of a compound for a kinase are much less demanding.…”

Section: Introductionmentioning

confidence: 99%

Development and Applications of a Broad-Coverage, TR-FRET-Based Kinase Binding Assay Platform

Lebakken¹,

Riddle²,

Singh³

et al. 2009

SLAS Discovery

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The expansion of kinase assay technologies over the past decade has mirrored the growing interest in kinases as drug targets. As a result, there is no shortage of convenient, fluorescence-based methods available to assay targets that span the kinome. The authors recently reported on the development of a non-activity-based assay to characterize kinase inhibitors that depended on displacement of an Alexa Fluor  647 conjugate of staurosporine (a "tracer") from a particular kinase. Kinase inhibitors were characterized by a change in fluorescence lifetime of the tracer when it was bound to a kinase relative to when it was displaced by an inhibitor. Here, the authors report on improvements to this strategy by reconfiguring the assay in a time-resolved fluorescence resonance energy transfer (TR-FRET) format that simplifies instrumentation requirements and allows for the use of a substantially lower concentration of kinase than was required in the fluorescence-lifetime-based format. The authors use this new assay to demonstrate several aspects of the binding assay format that are advantageous relative to traditional activity-based assays. The TR-FRET binding format facilitates the assay of compounds against lowactivity kinases, allows for the characterization of type II kinase inhibitors either using nonactivated kinases or by monitoring compound potency over time, and ensures that the signal being detected is specific to the kinase of interest and not a contaminating kinase. (Journal of Biomolecular Screening 2009:924-935)

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“…Our data suggest that by altering signals coming from this kinase one can manipulate these T cell responses. A number of inhibitors have recently been developed that target the kinase activity of Itk, which completely inhibit T cell responses (17)(18)(19)(20)(21), but can potentially lead to immunosuppression. Our work in this study suggests that manipulation of the dose of these inhibitors to selectively alter T cell migration while maintaining normal systemic T cell responses may provide researchers with a better and more effective strategy to treat allergic asthma.…”

Section: Discussionmentioning

confidence: 99%

“…Because mice lacking Itk are resistant to developing allergic asthma (6,7), a number of inhibitors have recently been developed that target the kinase activity of Itk (17)(18)(19)(20)(21). However, the role of kinase activity of Itk in the induction of allergic asthma is still unknown.…”

mentioning

confidence: 99%

Differential Sensitivity to Itk Kinase Signals for T Helper 2 Cytokine Production and Chemokine-Mediated Migration

Sahu

Mueller

Fischer

et al. 2008

The Journal of Immunology

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Allergic asthma is dependent on chemokine-mediated Th2 cell migration and Th2 cytokine secretion into the lungs. The inducible T cell tyrosine kinase Itk regulates the production of Th2 cytokines as well as migration in response to chemokine gradients. Mice lacking Itk are resistant to developing allergic asthma. However, the role of kinase activity of Itk in the development of this disease is unclear. In addition, whether distinct Itk-derived signals lead to T cell migration and secretion of Th2 cytokines is also unknown. Using transgenic mice specifically lacking Itk kinase activity, we show that active kinase signaling is required for control of Th2 responses and development of allergic asthma. Moreover, dominant suppression of kinase Itk activity led to normal Th2 responses, but significantly reduced chemokine-mediated migration, resulting in prevention of allergic asthma. These observations indicate that signals required for Th2 responses and migration are differentially sensitive to Itk activity. Manipulation of Itk’s activity can thus provide a new strategy to treat allergic asthma by differentially affecting migration of T cells into the lungs, leaving Th2 responses intact.

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Three Mechanistically Distinct Kinase Assays Compared: Measurement of Intrinsic ATPase Activity Identified the Most Comprehensive Set of ITK Inhibitors

Cited by 113 publications

References 39 publications

Measuring and interpreting the selectivity of protein kinase inhibitors

Measuring and interpreting the selectivity of protein kinase inhibitors

Development and Applications of a Broad-Coverage, TR-FRET-Based Kinase Binding Assay Platform

Differential Sensitivity to Itk Kinase Signals for T Helper 2 Cytokine Production and Chemokine-Mediated Migration

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