Your search keyword '"Meyer, Sheryl L."' showing total 8 results

1. Time-Resolved Fluorescence Resonance Energy Transfer as a Versatile Tool in the Development of Homogeneous Cellular Kinase Assays.

Author

Saville, Lisa, Spais, Chrysanthe, Mason, Jennifer L., Albom, Mark S., Murthy, Seetha, Meyer, Sheryl L., Ator, Mark A., Angeles, Thelma S., and Husten, Jean

Subjects

FLUORESCENCE resonance energy transfer, DRUG development, PROTEIN-tyrosine kinase inhibitors, FLUORESCENT proteins, FOCAL adhesion kinase, CELL lines

Abstract

Homogeneous cellular assays can streamline product detection in the drug discovery process. One commercially available assay employing time-resolved fluorescence resonance energy transfer (TR-FRET) that detects phosphorylated products was used to evaluate inhibitors of the receptor tyrosine kinase AXL in a cell line expressing an AXL-green fluorescent protein fusion protein. This TR-FRET assay was modified to evaluate the phosphorylation state of the AXL family member MER in a cell line expressing MER with a V5 tag by adding a fluorescein-labeled anti-V5 antibody. This homogeneous cellular assay was further modified to evaluate the nonreceptor tyrosine kinase focal adhesion kinase (FAK) in cell lines that expressed an untagged kinase by the inclusion of a commercially available anti-FAK antibody conjugated with an acceptor dye. The methods described here can be further adapted for TR-FRET detection of other cellular kinase activities. [ABSTRACT FROM AUTHOR]

Published

2012

2. Comparison of LanthaScreen Eu Kinase Binding Assay and Surface Plasmon Resonance Method in Elucidating the Binding Kinetics of Focal Adhesion Kinase Inhibitors.

Author

Mason, Jennifer L., Spais, Chrysanthe, Husten, Jean, Prouty, Eric, Albom, Mark S., Meyer, Sheryl L., Ator, Mark A., and Angeles, Thelma S.

Subjects

PHARMACEUTICAL research, EUROPIUM, BIOLOGICAL assay, SURFACE plasmon resonance, PHARMACOKINETICS, FOCAL adhesion kinase, ENZYME inhibitors, TARGETED drug delivery, DRUG interactions, COMPARATIVE studies

Abstract

An understanding of the dynamics of drug-target interactions is important in the drug discovery process. Information related to the binding kinetics of a drug toward its target or off-target aids in determining the efficacy or toxicity of a drug. Biophysical techniques such as surface plasmon resonance (SPR) have been available for over 20 years, but have been predominantly utilized to characterize protein-protein interactions. With improvements in instrument sensitivity and data analysis software, interactions between proteins (such as kinases) and small molecules have been successfully evaluated. More recently, the LanthaScreen Eu kinase binding assay for characterizing kinase inhibitors has been described. This assay monitors displacement of an Alexa Fluor 647-labeled tracer from the ATP-binding site of an epitope-tagged kinase by a test compound. Such behavior results in a decrease in time-resolved fluorescence energy transfer signal. In this report, a side-by-side comparison of the LanthaScreen Eu kinase binding assay and the SPR method was performed using inhibitors of focal adhesion kinase. The two methods yielded comparable results and identified compounds with time-dependent inhibition and relatively slow dissociation. [ABSTRACT FROM AUTHOR]

Published

2012

3. Improvement of Inhibitor Identification for Heat Shock Protein 90α by Utilizing a Red-Shifted Fluorescence Polarization Probe.

Author

Qian, Jie, Holskin, Beverly P., Theroff, Jay, Underiner, Ted, Meyer, Sheryl L., and Angeles, Thelma S.

Subjects

HEAT shock proteins, FLUORESCENT probes, ADENOSINE triphosphatase, ENZYME inhibitors, ENZYME kinetics, CANCER treatment, GELDANAMYCIN, MOLECULAR chaperones

Abstract

Heat shock protein-90 (HSP90) is an ATP-dependent molecular chaperone with intrinsic ATPase activity. HSP90 is required for the stability and function of client proteins, many of which are involved in oncogenesis. Thus, identification of HSP90 inhibitors would potentially lead to the discovery of cancer therapeutics. Here, we present a high-throughput screening campaign utilizing two geldanamycin (GM)-labeled probes in a fluorescence polarization (FP) assay. For the primary screen, a previously reported green BODIPY-labeled GM (GM-BODIPY) was used to evaluate a library collection of about 400,000 compounds. From this screen, 3058 compounds showed >30% inhibition. To distinguish true positives from compound interference, a confirmatory screen was deemed necessary. Accordingly, a red-shifted FP binding assay was developed using GM labeled with red BODIPY. This tool enabled reliable identification of promising HSP90α inhibitors. [ABSTRACT FROM AUTHOR]

Published

2012

4. Comparison of Two Homogeneous Cell-Based Kinase Assays for JAK2 V617F: SureFire pSTAT5 and GeneBLAzer Fluorescence Resonance Energy Transfer Assays.

Author

Qian, Jie, Mason, Jennifer L., Holskin, Beverly P., Murray, Kristen A., Meyer, Sheryl L., Ator, Mark A., and Angeles, Thelma S.

Subjects

BIOLOGICAL assay, CELLULAR signal transduction, CYTOKINES, FLUORESCENCE resonance energy transfer, SOMATIC mutation, DRUG development, MYELOPROLIFERATIVE neoplasms

Abstract

The Janus kinase (JAK)/signal transducer and activator of transcription (STAT) signaling pathway plays an important role in cellular responses to cytokines and growth factors. Recent studies have identified a recurrent somatic activating mutation (JAK2 V617F) in majority of patients with myeloproliferative disorders (MPDs). Development of drugs that target JAK2 V617F is, therefore, of therapeutic relevance. To discover small molecule inhibitors for this target, robust and reliable cell-based assays are important. Here, we present a comparison of two homogeneous, 384-well plate-based cellular assays using Invitrogen's CellSensor® JAK2 V617F interferon regulatory factor-1 (irf1)-beta-lactamase (bla) human erythroleukemia line (HEL): (1) SureFire® pSTAT5 AlphaScreen® assay from PerkinElmer; and (2) GeneBLAzer® fluorescence resonance energy transfer assay from Invitrogen. HEL cells are growth factor-independent due to JAK2 V617F mutation that causes constitutive STAT5 activation. The SureFire assay measures levels of phosphorylated STAT5 downstream of JAKs, while the GeneBLAzer assay is a reporter assay that monitors bla activity further downstream of STAT5. Evaluation of a number of chemically diverse JAK2 inhibitors in the two cellular assays yielded comparable half-maximal inhibitory concentration (IC50) values, boding well for the utility of these assay formats in compound profiling. [ABSTRACT FROM AUTHOR]

Published

2012

5. BDNF and NT4/5 promote survival and neurite outgrowth of pontocerebellar mossy fiber neurons.

Author

Rabacchi, Sylvia A., Kruk, Barbara, Hamilton, Jason, Carney, Catrina, Hoffman, John R., Meyer, Sheryl L., Springer, Joe E., and Baird, Douglas H.

Published

1999

6. Production and Characterization of Recombinant Mouse Brain-Derived Neurotrophic Factor and Rat Neurotrophin-3 Expressed in Insect Cells.

Author

Meyer, Sheryl L., Lang, Diane M., Forbes, M. Elizabeth, Knight, Ernest, Hirsch, James D., Trusko, Stephen P., and Scott, Richard W.

Published

1994

7. K-252a and Staurosporine Promote Choline Acetyltransferase Activity in Rat Spinal Cord Cultures.

Author

Glicksman, Marcie A., Prantner, J. Eric, Meyer, Sheryl L., Forbes, M. Elizabeth, Dasgupta, Malini, Lewis, Michael E., and Neff, Nicola

Published

1993

8. Quantitative non-radioactive in situ hybridization of preproenkephalin mRNA with digoxigenin-labeled cRNA probes.

Author

Robbins, Elaine, Baldino, Frank, Roberts-Lewis, Jill M., Meyer, Sheryl L., Grega, Debra, and Lewis, Michael E.

Published

1991