Multiplexed phosphospecific flow cytometry enables large-scale signaling profiling and drug screening in blood platelets

B E J Spurgeon; A Aburima; N G Oberprieler; K Taskén; K M Naseem

doi:10.1111/jth.12670

Multiplexed phosphospecific flow cytometry enables large-scale signaling profiling and drug screening in blood platelets

J Thromb Haemost. 2014 Oct;12(10):1733-43. doi: 10.1111/jth.12670. Epub 2014 Sep 18.

Authors

B E J Spurgeon¹, A Aburima, N G Oberprieler, K Taskén, K M Naseem

Affiliation

¹ Centre for Cardiovascular and Metabolic Research, Hull York Medical School, University of Hull, Hull, UK.

PMID: 25056834
DOI: 10.1111/jth.12670

Abstract

Background: Dissecting the signaling events that contribute to platelet activation will increase our understanding of platelet function and aid in the development of new antiplatelet agents. However, high-throughput methodology for the quantitative analysis of platelet signaling events is still lacking.

Objective: To develop a high-throughput assay for the analysis of platelet signaling events in whole blood.

Methods and results: We developed a fluorescent barcoding protocol to facilitate multiplexing and enable large-scale signaling profiling in platelets in whole blood. The methodology allowed simultaneous staining and acquisition of 24-96 samples in a single analysis tube with a standard flow cytometer. This approach significantly reduced experimental numbers, data acquisition time, and antibody consumption, while providing automated statistically rich quantitative data on signaling events. Using vasodilator-stimulated phosphoprotein (VASP), an established marker of platelet inhibition and antiplatelet drug therapy, we demonstrated that the assay could detect subtle changes in phosphoVASP-Ser157/239 in response to cAMP-elevating agents of varying potency and known modulators of the cAMP signaling cascade. The assay could be used with washed platelets or whole blood, analyzed immediately or frozen, without any significant change in assay performance. To demonstrate the usefulness of the assay as a drug discovery platform, we examined a prostaglandin screening library. Our screen of 70 prostaglandin derivatives revealed three previously uncharacterized lipids that stimulated phosphorylation of VASP-Ser157. Follow-up analyses demonstrated that these agents elevated intraplatelet cAMP and inhibited collagen-induced platelet aggregation.

Conclusions: This novel method enables rapid, large-scale quantitative signaling profiling and compound screening in human platelets present in whole blood.

Keywords: flow cytometry; phosphorylation; platelets; protein kinase A; signal transduction.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Antibodies / chemistry
Blood Platelets / drug effects*
Cell Adhesion Molecules / metabolism
Cyclic AMP / metabolism
Cyclic AMP-Dependent Protein Kinases / metabolism
Drug Design
Drug Evaluation, Preclinical*
Electrophoresis
Flow Cytometry*
Fluorescent Dyes / chemistry
Humans
Mice
Microfilament Proteins / metabolism
Phosphoproteins / metabolism
Phosphorylation
Platelet Aggregation
Platelet Aggregation Inhibitors / chemistry
Prostaglandins / chemistry
Signal Transduction

Substances

Antibodies
Cell Adhesion Molecules
Fluorescent Dyes
Microfilament Proteins
Phosphoproteins
Platelet Aggregation Inhibitors
Prostaglandins
vasodilator-stimulated phosphoprotein
Cyclic AMP
Cyclic AMP-Dependent Protein Kinases