Your search keyword '"Frelinger, Andrew L."' showing total 424 results

151. Plasma Immunoreactive Calcitonin in Lung Cancer*

Author

ROOS, BERNARD A., primary, LINDALL, ARNOLD W., additional, BAYLIN, STEPHEN B., additional, O'NEIL, JUNE A., additional, FRELINGER, ANDREW L., additional, BIRNBAUM, ROGER S., additional, and LAMBERT, PHILLIP W., additional

Published

1980

152. Clopidogrel Linking Evaluation of Platelet Response Variability to Mechanism of Action⁎⁎Editorials published in the Journal of the American College of Cardiologyreflect the views of the authors and do not necessarily represent the views of JACCor the American College of Cardiology

Author

Frelinger, Andrew L. and Michelson, Alan D.

Subjects

cardiovascular diseases, circulatory and respiratory physiology

153. GLS-409, an Antagonist of Both P2Y1 and P2Y12, Potently Inhibits Canine Coronary Artery Thrombosis and Reversibly Inhibits Human Platelet Activation.

Author

Koganov, Elena Smolensky, Michelson, Alan D., Yanachkov, Ivan B., Yanachkova, Milka I., Wright, George E., Przyklenk, Karin, and Frelinger, Andrew L.

Abstract

Dual antiplatelet therapy with aspirin and an adenosine diphosphate (ADP) P2Y12 receptor antagonist reduces ischemic events in patients with acute coronary syndrome. Previous evidence from our group, obtained in a preclinical model of recurrent platelet-mediated thrombosis, demonstrated that GLS-409, a diadenosine tetraphosphate derivative that inhibits both P2Y1 and P2Y12 ADP receptors, may be a novel and promising antiplatelet drug candidate. However, the salutary antiplatelet effects of GLS-409 were accompanied by a trend toward an unfavorable increase in bleeding. The goals of this study were to: 1) provide proof-of-concept that the efficacy of GLS-409 may be maintained at lower dose(s), not accompanied by an increased propensity to bleeding; and 2) establish the extent and kinetics of the reversibility of human platelet inhibition by the agent. Lower doses of GLS-409 were identified that inhibited in vivo recurrent coronary thrombosis with no increase in bleeding time. Human platelet inhibition by GLS-409 was reversible, with rapid recovery of platelet reactivity to ADP, as measured by platelet surface activated GPIIb-IIIa and platelet surface P-selectin. These data support the concept that GLS-409 warrants further, larger-scale investigation as a novel, potential therapy in acute coronary syndromes. [ABSTRACT FROM AUTHOR]

Published

2018

154. Clopidogrel: Linking Evaluation of Platelet Response Variability to Mechanism of Action ⁎ [⁎] Editorials published in the Journal of the American College of Cardiology reflect the views of the authors and do not necessarily represent the views of JACC or the American College of Cardiology.

Author

Frelinger, Andrew L. and Michelson, Alan D.

Published

2005

155. GLS-409, a Synergistic Inhibitor of Both P2Y1and P2Y12: Efficacy in a Canine Model of Recurrent Coronary Thrombosis and Reversibility of Human Platelet Inhibition

Author

Smolensky Koganov, Elena, Michelson, Alan D, Yanachkov, Ivan B, Yanachkova, Milka I, Wright, George E, Przyklenk, Karin, and Frelinger, Andrew L

Abstract

Introduction.Dual antiplatelet therapy with aspirin and an adenosine diphosphate (ADP) P2Y12receptor inhibitor is a mainstay of pharmacological therapy in acute coronary syndromes. GLS-409 is a novel diadenosine tetraphosphate derivative that inhibits both P2Y1and P2Y12platelet ADP receptors.

Published

2017

156. Current Options in Platelet Function Testing

Author

Michelson, Alan D., Frelinger, Andrew L., and Furman, Mark I.

Subjects

*BLOOD platelets, *NONINVASIVE diagnostic tests, *DRUG interactions, *CARDIOVASCULAR diseases

Abstract

The variable response to antiplatelet therapy has led to the use of platelet function tests to monitor the effects of antiplatelet drugs in cardiovascular diseases. The goal is to guide antiplatelet therapy to the optimal dose for the prevention or treatment of thrombosis while minimizing hemorrhagic side effects. The bleeding time is no longer recommended for use because of its nonspecificity and lack of clinical correlations. The current de facto “gold standard” test of platelet function is turbidometric platelet aggregometry. Although this method has been successful in measuring the aggregation of platelets in a glycoprotein (GP) IIb/IIIa (integrin αIIbβ3)–dependent manner, it has several limitations, including poor reproducibility, high sample volume, requirement for sample preparation, length of assay time, requirement for a skilled technician, and cost. Therefore, new options for platelet function testing have been developed to address these disadvantages and to meet the need for point-of-care testing that can be performed at or near a patient’s bedside without requiring a high degree of technical expertise. The new tests include VerifyNow (Accumetrics, San Diego, CA); Plateletworks (Helena Laboratories, Beaumont, TX); Thrombelastograph PlateletMapping System (Haemoscope Corporation, Niles, IL); Impact cone and plate(let) analyzer (DiaMed, Cressier, Switzerland); and Platelet Function Analyzer 100 (PFA-100; Dade Behring, Newark, DE). In patients treated with antiplatelet drugs, the degree of platelet inhibition, as determined by several of these new platelet function assays, has been shown to predict major adverse cardiac events. [Copyright &y& Elsevier]

Published

2006

157. Progress in point-of-care laboratory testing for assessing platelet function

Author

Berkowitz, Scott D., Frelinger, Andrew L., III, and Hillman, Robert S.

Published

1998

158. In VivoPlatelet Activation and Its In VitroInhibition by Prasugrel's Active Metabolite In Adolescents with Sickle Cell Disease

Author

Frelinger, Andrew L., Jakubowski, Joseph A., Brooks, Julie K., Nigam, Anu, Berny-Lang, Michelle A., Barnard, Marc R., Heeney, Matthew M., and Michelson, Alan D.

Abstract

Abstract 2141

Published

2011

159. A Phase 1 Study of Prasugrel in Subjects with Sickle Cell Disease: Impact on Ex VivoPlatelet Reactivity

Author

Jakubowski, Joseph A., Zhou, Chunmei, Small, David S., Winters, Kenneth J., Lachno, D. Richard, Frelinger, Andrew L., Howard, Jo, Jurcevic, Stipo, and Payne, Christopher D.

Abstract

Abstract 1053

Published

2011

160. A Phase 1 Study of Prasugrel in Subjects with Sickle Cell Disease: Effects on In VivoMarkers of Platelet Activation and of Coagulation

Author

Jakubowski, Joseph A., Zhou, Chunmei, Small, David S., Winters, Kenneth J., Lachno, D. Richard, Frelinger, Andrew L., Howard, Jo, Jurcevic, Stipo, and Payne, Christopher D.

Abstract

Abstract 1049This icon denotes a clinically relevant abstract

Published

2011

161. Agonist and Antagonist Effects of Diadenosine Tetraphosphate, a Platelet Dense Granule Constituent, on Platelet P2Y1, P2Y12and P2X1Receptors

Author

Chang, Hung, Yanachkov, Ivan B, Michelson, Alan D, Li, YouFu, Barnard, Marc R, Wright, George E, and Frelinger, Andrew L

Abstract

Introduction:Diadenosine 5′,5‴-P1,P4- tetraphosphate (Ap4A) is stored in platelet dense granules, but its effects on platelet function are not well understood. In the current study, we examined the effects of Ap4A on signaling through the human platelet purinergic receptors P2Y1, P2Y12and P2X1.

Published

2008

162. A double-blind, randomized, multicenter phase 2 study of prasugrel versus placebo in adult patients with sickle cell disease.

Author

Wun, Ted, Soulieres, Denis, Frelinger, Andrew L., Krishnamurti, Lakshmanan, Novelli, Enrico M., Kutlar, Abdullah, Ataga, Kenneth I., Knupp, Charles L., McMahon, Lillian E., Strouse, John J., Zhou, Chunmei, Heath, Lori E., Nwachuku, Chuke E., Jakubowski, Joseph A., Riesmeyer, Jeffrey S., and Winters, Kenneth J.

Subjects

*SICKLE cell anemia treatment, *BLOOD platelet activation, *PRASUGREL, *PLATELET aggregation inhibitors, *HEMORRHAGIC diseases, *PLATELET function tests, *VASODILATOR-stimulated phosphoprotein, *PLACEBOS

Abstract

Background: Platelet activation has been implicated in the pathogenesis of sickle cell disease (SCD) suggesting antiplatelet agents may be therapeutic. To evaluate the safety of prasugrel, a thienopyridine antiplatelet agent, in adult patients with SCD, we conducted a double-blind, randomized, placebo-controlled study. Methods: The primary endpoint, safety, was measured by hemorrhagic events requiring medical intervention. Patients were randomized to prasugrel 5 mg daily (n = 41) or placebo (n = 21) for 30 days. Platelet function by VerifyNowW P2Y12 and vasodilator-stimulated phosphoprotein assays at days 10 and 30 were significantly inhibited in prasugrel- compared with placebo-treated SCD patients. Results: There were no hemorrhagic events requiring medical intervention in either study arm. Mean pain rate (percentage of days with pain) and intensity in the prasugrel arm were decreased compared with placebo. However, these decreases did not reach statistical significance. Platelet surface P-selectin and plasma soluble P-selectin, biomarkers of in vivo platelet activation, were significantly reduced in SCD patients receiving prasugrel compared with placebo. In sum, prasugrel was well tolerated and not associated with serious hemorrhagic events. Conclusions: Despite the small size and short duration of this study, there was a decrease in platelet activation biomarkers and a trend toward decreased pain. [ABSTRACT FROM AUTHOR]

Published

2013

163. Platelet surface GPIbα, activated GPIIb-IIIa, and P-selectin levels in adult veno-arterial extracorporeal membrane oxygenation patients.

Author

Mazzeffi, Michael, Tanaka, Kenichi, Wu, Yi-Feng, Zhang, Aijun, Kareddy, Niharika, Tadjou Tito, Emmanuel, Rock, Peter, Michelson, Alan D., and Frelinger, Andrew L.

Subjects

*EXTRACORPOREAL membrane oxygenation, *THROMBIN receptors, *BLOOD platelets, *ADENOSINE diphosphate, *CARDIOGENIC shock

Abstract

Our objective was to characterize platelet surface glycoprotein (GP)Ibα, activated GPIIb-IIIa, and P-selectin levels during and after extracorporeal membrane oxygenation (ECMO). We performed a single center cohort study of 10 adult patients on ECMO for cardiogenic shock. Patients had blood samples drawn on ECMO day 1 or 2, day 3, day 5, and 48–72 hours after ECMO decannulation. Platelets from untreated blood samples and samples treated with either adenosine diphosphate (ADP) or thrombin receptor agonist peptide (TRAP) had surface GPIbα, activated GPIIb-IIIa, and P-selectin levels measured using flow cytometry. Platelet surface GPIbα levels varied significantly by time on ECMO (p =.002) and were significantly higher on ECMO day 5 compared to ECMO day 1 (p =.01). GPIbα levels during ECMO did not differ significantly from levels after ECMO decannulation (p =.14). Activated GPIIb-IIIa levels did not change significantly during ECMO, but were significantly higher after ECMO decannulation (p =.04). There were no significant differences in P-selectin levels during ECMO (p =.87) or after ECMO decannulation (p =.41). Platelet surface GPIbα and P-selectin levels were similar during and after ECMO whereas activated GPIIb-IIIa levels were lower during ECMO, particularly in response to TRAP stimulation, potentially contributing to ECMO-induced coagulopathy. [ABSTRACT FROM AUTHOR]

Published

2022

164. Reply: Collapse of the Aspirin Empire: Is it Diabetic Gastroparesis or Cardioprotective Paresis?

Author

Bhatt, Deepak L., Grosser, Tilo, Dong, Jing-fei, Logan, Douglas, Jeske, Walter, Angiolillo, Dominick J., Frelinger, Andrew L., Liang, Juan, Cryer, Byron, Marathi, Upendra, and Frelinger, Andrew L 3rd

Subjects

*GASTROPARESIS, *DIABETES complications, *ASPIRIN, *THERAPEUTICS, *COMPARATIVE studies, *DIABETIC neuropathies, *HEMIPLEGIA, *RESEARCH methodology, *MEDICAL cooperation, *RESEARCH, *EVALUATION research

Published

2017

165. A phase 1 study of prasugrel in patients with sickle cell disease: Effects on biomarkers of platelet activation and coagulation.

Author

Jakubowski, Joseph A., Zhou, Chunmei, Jurcevic, Stipo, Winters, Kenneth J., Lachno, D. Richard, Frelinger, Andrew L., Gupta, Neehar, Howard, Jo, Payne, Christopher D., and Mant, Timothy G.

Subjects

*PRASUGREL, *SICKLE cell anemia, *BIOMARKERS, *BLOOD platelets, *ADENOSINE diphosphate, *BLOOD coagulation, *PATIENTS

Abstract

Abstract: Introduction: Prasugrel, a P2Y12 adenosine diphosphate (ADP) receptor antagonist effectively inhibits ADP-mediated platelet activation and aggregation, and may be useful in reducing vaso-occlusive crises in sickle cell disease (SCD). In this study, we assess the effect of prasugrel on biomarkers of platelet activation and coagulation in patients with SCD. Materials and Methods: Twelve adult patients with SCD and 13 healthy subjects were examined before and after 12±2days of 5.0 or 7.5mg/day oral prasugrel. Assessed cellular biomarkers included monocyte- and neutrophil-platelet aggregates, activated glycoprotein IIb-IIIa (GPIIbIIIa), P-selectin, CD40 ligand (CD40L), tissue factor (TF) expression on circulating platelets and on monocyte-platelet aggregates, and platelet-erythrocyte aggregates. Soluble biomarkers included CD40L, prothrombin fragment 1.2 (F1.2), thromboxane B2 (TXB2), P-selectin, and TF. Results: Patients with SCD had increased platelet baseline activation compared to healthy subjects, as measured by percentages of monocyte-platelet aggregates, neutrophil-platelet aggregates, and platelets expressing CD40L. Likewise, baseline levels of soluble F1.2 and TXB2 were elevated in patients with SCD compared to healthy subjects. After 12days of prasugrel, patients with SCD had a significant reduction in platelet-monocyte aggregates that was not observed in healthy subjects. Following prasugrel administration, those with SCD maintained higher levels of monocyte-platelet aggregates and soluble F1.2, but had lower levels of platelet-erythrocyte aggregates and soluble TF compared to healthy subjects. Conclusions: These results provide evidence for chronic platelet activation in the SCD steady state, activation that was in part attenuated by prasugrel, thereby suggesting that ADP may mediate platelet activation in SCD. [Copyright &y& Elsevier]

Published

2014

166. The aryl hydrocarbon receptor directs hematopoietic progenitor cell expansion and differentiation.

Author

Smith, Brenden W., Rozelle, Sarah S., Leung, Amy, Ubellacker, Jessalyn, Parks, Ashley, Nah, Shirley K., French, Deborah, Gadue, Paul, Monti, Stefano, Chui, David H. K., Steinberg, Martin H., Frelinger, Andrew L., Michelson, Alan D., Theberge, Roger, McComb, Mark E., Costello, Catherine E., Kotton, Darrell N., Mostoslavsky, Gustavo, Sherr, David H., and Murphy, George J.

Subjects

*ARYL hydrocarbon receptors, *PROGENITOR cells, *IMMUNE system, *MEGAKARYOCYTES, *CELL growth

Abstract

The evolutionarily conserved aryl hydrocarbon receptor (AhR) has been studied for its role in environmental chemical-induced toxicity. However, recent studies have demonstrated that the AhR may regulate the hematopoietic and immune systems during development in a cell-specific manner. These results, together with the absence of an in vitro model system enabling production of large numbers of primary human hematopoietic progenitor cells (HPs) capable of differentiating into megakaryocyte- and erythroid-lineage cells, motivated us to determine if AhR modulation could facilitate both progenitor cell expansion and megakaryocyte and erythroid cell differentiation. Using a novel, pluripotent stem cell-based, chemically-defined, serum and feeder cell-free culture system, we show that the AhR is expressed in HPs and that, remarkably, AhR activation drives an unprecedented expansion of HPs, megakaryocyte-lineage cells, and erythroid-llneage cells'. Further AhR modulation within rapidly expanding progenitor cell populations directs cell fate, with chronic AhR agonism permissive to erythroid differentiation and acute antagonism favoring megakaryocyte specification. These results highlight the development of a new Good Manufacturing Practice-compliant platform for generating virtually unlimited numbers of human HPs with which to scrutinize red blood cell and platelet development, including the assessment of the role of the AhR critical cell fate decisions during hematopoiesis. [ABSTRACT FROM AUTHOR]

Published

2013

167. A phase 1 study of prasugrel in patients with sickle cell disease: pharmacokinetics and effects on ex vivo platelet reactivity.

Author

Jakubowski, Joseph A., Zhou, Chunmei, Small, David S., Winters, Kenneth J., Lachno, D. Richard, Frelinger, Andrew L., Howard, Jo, Mant, Timothy G., Jurcevic, Stipo, and Payne, Christopher D.

Subjects

*PRASUGREL, *SICKLE cell anemia in children, *PHARMACOKINETICS, *BLOOD platelets, *VASODILATOR-stimulated phosphoprotein, *ENZYME-linked immunosorbent assay, *THERAPEUTICS

Abstract

Aims Prasugrel is a novel thienopyridine P2Y12 adenosine diphosphate ( ADP) receptor antagonist that inhibits ADP-mediated platelet activation and aggregation. Accordingly, it may be useful in reducing platelet-related ischaemia in sickle cell disease ( SCD). Exposure to prasugrel's active metabolite ( Pras- AM) and its antiplatelet activity in SCD have not been investigated. Methods Thirteen adult patients with SCD and an equal number of matched healthy control subjects were studied before and after 12 days of 5.0 or 7.5 mg day−1 prasugrel treatment. Platelet reactivity was assessed by light transmission aggregometry ( LTA), impedance aggregometry ( MEA), Verify Now® P2Y12, vasodilator-stimulated phosphoprotein ( VASP) phosphorylation and Plateletworks. Exposure to Pras- AM was also assessed. Results At baseline, patients with SCD showed increased platelet reactivity vs. healthy control subjects with Verify Now (408 vs. 323 P2Y12 reaction units ( PRU), respectively, P = 0.003) and MEA (106 vs. 77 area under the aggregation curve ( AU.min), P = 0.002); lower platelet reactivity index with VASP flow cytometry (59 vs. 79% platelet reactivity index ( PRI), P = 0.018); and no significant differences with LTA, VASP enzyme-linked immunosorbent assay or Plateletworks. Relative to baseline, prasugrel significantly reduced platelet reactivity by all assays in both populations (all P < 0.05). Prasugrel was well tolerated, with no bleeding-related events in patients with SCD. The mean concentration-time profiles of Pras- AM were comparable between healthy subjects and patients with SCD following a single 10 mg prasugrel dose and following the 12th dose of 7.5 or 5 mg prasugrel. Conclusions Results demonstrate that in response to prasugrel, patients with SCD and healthy subjects have similar degrees of platelet inhibition and exposure to Pras- AM, and provide a basis for further study of prasugrel in patients with SCD. [ABSTRACT FROM AUTHOR]

Published

2013

168. In vivo effects of eltrombopag on platelet function in immune thrombocytopenia: no evidence of platelet activation.

Author

Psaila, Bethan, Bussel, James B., Linden, Matthew D., Babula, Bracken, Youfu Li, Barnard, Marc R., Tate, Chinara, Mathur, Kanika, Frelinger, Andrew L., and Michelson, Alan D.

Subjects

*PLATELET function tests, *ELTROMBOPAG, *THROMBOCYTOPENIA, *BLOOD platelet activation, *ADENOSINE diphosphate, *GENE expression, *DRUG dosage

Abstract

The effects of eltrombopag, a thrombopoi-etin-receptor agonist, on platelet function in immune thrombocytopenia (ITP) are not fully characterized. This study used whole blood flow cytometry to examine platelet function in 20 patients receiving eltrombopag treatment at days 0, 7, and 28. Platelet surface expression of activated GPIIb/IIIa, P-selectin, and GPIb was measured with and without low and high adenosine diphosphate (ADP) and thrombin receptor activating peptide (TRAP) concentrations. Before eltrombopag treatment with no ex vivo agonist, platelet activation was higher in ITP patients than controls. Platelet GPIb and activated GPIIb/IIIa expression without added agonist was unchanged following eltrombopag treatment, whereas a slight increase in P-selectin was observed. Expression of P-selectin and activated GPIIb/IIIa in response to high-dose ADP was lower during eltrombopag treatment than at baseline. Eltrombopag led to a slight increase in platelet reactivity to TRAP only in responders to eltrombopag but not to levels above those in controls; whole blood experiments demonstrated that this increase was probably because of higher platelet counts rather than higher platelet reactivity. In conclusion, although thrombocytopenic ITP patients have higher baseline platelet activation than controls, eltrombopag did not cause platelet activation or hyper-reactivity, irrespective of whether the platelet count increased. [ABSTRACT FROM AUTHOR]

Published

2012

169. Agonist and antagonist effects of diadenosine tetraphosphate, a platelet dense granule constituent, on platelet P2Y1, P2Y12 and P2X1 receptors

Author

Chang, Hung, Yanachkov, Ivan B., Michelson, Alan D., Li, YouFu, Barnard, M.R., Wright, George E., and Frelinger, Andrew L.

Subjects

*ADENINE nucleotides, *BLOOD platelets, *BLOOD platelet aggregation, *PURINERGIC receptors, *PHOSPHOPROTEINS, *PHOSPHORYLATION, *ADENOSINE diphosphate

Abstract

Abstract: Introduction: Diadenosine 5'',5''''''-P1,P4- tetraphosphate (Ap4A) is stored in platelet dense granules, but its effects on platelet function are not well understood. Methods and Results: We examined the effects of Ap4A on platelet purinergic receptors P2Y1, P2Y12 and P2X1. Flow cytometry was used to measure the effects of Ap4A in the presence or absence of ADP on: a) P2Y12-mediated decrease in intraplatelet phosphorylated vasodilator stimulated phosphoprotein (VASP), b) P2Y1-mediated increase in platelet cytosolic Ca2+, and c) P2X1-mediated intraplatelet entry of extracellular Ca2+. ADP-stimulated platelet shape change (P2Y1-mediated) and aggregation (P2Y1- and P2Y12-mediated) were measured optically. Ap4A inhibited 3μM ADP-induced: a) platelet aggregation (IC50 9.8±2.8μM), b) P2Y1-mediated shape change, c) P2Y1-mediated increase in platelet cytosolic Ca2+ (IC50 40.8±12.3μM), and d) P2Y12-mediated decrease in VASP phosphorylation (IC50 >250μM). In the absence of added ADP, Ap4A had agonist effects on platelet P2X1 and P2Y12, but not P2Y1, receptors. Conclusion: Ap4A, a constituent of platelet dense granules, is a) an antagonist of platelet P2Y1 and P2Y12 receptors, where it inhibits the effects of ADP, and b) an agonist of platelet P2X1 and P2Y12 receptors. [Copyright &y& Elsevier]

Published

2010

170. Protocol for assessing and visualizing cell microaggregate formation in whole blood by imaging flow cytometry.

Author

Krell J, Javarappa KK, Wenedy A, Frelinger AL 3rd, Renia L, Prazeres da Costa C, Schlegel M, Knolle P, Schneider G, and Hayden O

Abstract

Blood cell aggregates are clinically useful biomarkers in a number of medical disorders. This protocol provides accurate and quantitative analysis of cell aggregates using a small volume of whole blood and imaging flow cytometry. We describe steps for sample collection, staining, and measurement. We then detail gating procedures and analysis of cell morphology. Sample preparation artifacts, activation, and morphological changes of cells are mitigated by omitting erythrocyte lysis and leukocyte isolation while maintaining high-throughput accurate imaging of leukocytes and platelets., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2025 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2025

171. Platelet Physiology.

Author

Gremmel T, Frelinger AL 3rd, and Michelson AD

Subjects

Humans, Platelet Activation physiology, Hemostasis physiology, Thrombosis, Blood Platelets metabolism, Blood Platelets physiology

Abstract

Platelets are the smallest blood cells, numbering 150 to 350 × 10 9 /L in healthy individuals. The ability of activated platelets to adhere to an injured vessel wall and form aggregates was first described in the 19th century. Besides their long-established roles in thrombosis and hemostasis, platelets are increasingly recognized as pivotal players in numerous other pathophysiological processes including inflammation and atherogenesis, antimicrobial host defense, and tumor growth and metastasis. Consequently, profound knowledge of platelet structure and function is becoming more important in research and in many fields of modern medicine. This review provides an overview of platelet physiology focusing particularly on the structure, granules, surface glycoproteins, and activation pathways of platelets., Competing Interests: None declared., (Thieme. All rights reserved.)

Published

2024

172. Flow Cytometry and Platelets.

Author

Frelinger AL 3rd

Subjects

Humans, Platelet Function Tests, Blood Platelet Disorders diagnosis, Blood Platelet Disorders blood, Biomarkers blood, Flow Cytometry, Blood Platelets, Platelet Activation

Abstract

Clinical assessment of platelet activation by flow cytometry is useful in the characterization and diagnosis of platelet-specific disorders and as a measure of risk for thrombosis or bleeding. Platelets circulate in a resting, "unactivated" state, but when activated they undergo alterations in surface glycoprotein function and/or expression level, exposure of granule membrane proteins, and exposure of procoagulant phospholipids. Flow cytometry provides the means to detect these changes and, unlike other platelet tests, is appropriate for measuring platelet function in samples from patients with low platelet counts. The present review will focus on flow cytometric tests for platelet activation markers., Competing Interests: Disclosure The author has nothing to disclose., (Copyright © 2024 Elsevier Inc. All rights reserved.)

Published

2024

173. Dysregulation of platelet serotonin, 14-3-3, and GPIX in sudden infant death syndrome.

Author

Frelinger AL 3rd, Haynes RL, Goldstein RD, Berny-Lang MA, Gerrits AJ, Riehs M, Haas EA, Paunovic B, Mena OJ, Campman SC, Milne GL, Sleeper LA, Kinney HC, and Michelson AD

Subjects

Female, Humans, Infant, Infant, Newborn, Male, 14-3-3 Proteins blood, 14-3-3 Proteins metabolism, Blood Platelets metabolism, Serotonin blood, Serotonin metabolism, Sudden Infant Death etiology, Sudden Infant Death blood, Platelet Glycoprotein GPIb-IX Complex analysis, Platelet Glycoprotein GPIb-IX Complex metabolism

Abstract

Sudden infant death syndrome (SIDS) is the leading cause of post-neonatal infant mortality, but the underlying cause(s) are unclear. A subset of SIDS infants has abnormalities in the neurotransmitter, serotonin (5-hydroxytryptamine [5-HT]) and the adaptor molecule, 14-3-3 pathways in regions of the brain involved in gasping, response to hypoxia, and arousal. To evaluate our hypothesis that SIDS is, at least in part, a multi-organ dysregulation of 5-HT, we examined whether blood platelets, which have 5-HT and 14-3-3 signaling pathways similar to brain neurons, are abnormal in SIDS. We also studied platelet surface glycoprotein IX (GPIX), a cell adhesion receptor which is physically linked to 14-3-3. In infants dying of SIDS compared to infants dying of known causes, we found significantly higher intra-platelet 5-HT and 14-3-3 and lower platelet surface GPIX. Serum and plasma 5-HT were also elevated in SIDS compared to controls. The presence in SIDS of both platelet and brainstem 5-HT and 14-3-3 abnormalities suggests a global dysregulation of these pathways and the potential for platelets to be used as a model system to study 5-HT and 14-3-3 interactions in SIDS. Platelet and serum biomarkers may aid in the forensic determination of SIDS and have the potential to be predictive of SIDS risk in living infants., (© 2024. The Author(s).)

Published

2024

174. OMIP-097: High-parameter phenotyping of human platelets by spectral flow cytometry.

Author

Spurgeon BEJ and Frelinger AL 3rd

Subjects

Humans, Flow Cytometry methods, Platelet Activation, Blood Platelets, CD40 Ligand

Abstract

Using spectral flow cytometry, we developed a 16-color panel for analysis of platelet phenotype and function in human whole blood. The panel contains markers of clinical relevance and follows an optimized protocol for the high-parameter phenotyping of (phosphatidylserine positive) procoagulant platelets. Inclusion of established markers, such as CD62P and PAC-1, allows the subsetting of classic (proinflammatory and proaggregatory) phenotypes, while addition of novel markers, such as TLR9, allows the resolution of platelets with nonclassic functions. Multiple inducible (C3b, CD63, CD107a, CD154, and TLT-1) and constitutive (CD29, CD31, CD32, CD36, CD42a, CD61, and GPVI) markers are also measurable, and we demonstrate the use of automatic gating for platelet analysis. The panel is widely applicable to research and clinical settings and can be readily modified, should users wish to tailor the panel to more specific needs., (© 2023 International Society for Advancement of Cytometry.)

Published

2023

175. Outcomes of hematopoietic stem cell gene therapy for Wiskott-Aldrich syndrome.

Author

Labrosse R, Chu JI, Armant MA, Everett JK, Pellin D, Kareddy N, Frelinger AL, Henderson LA, O'Connell AE, Biswas A, Coenen-van der Spek J, Miggelbrink A, Fiorini C, Adhikari H, Berry CC, Cantu VA, Fong J, Jaroslavsky J, Karadeniz DF, Li QZ, Reddy S, Roche AM, Zhu C, Whangbo JS, Dansereau C, Mackinnon B, Morris E, Koo SM, London WB, Baris S, Ozen A, Karakoc-Aydiner E, Despotovic JM, Forbes Satter LR, Saitoh A, Aizawa Y, King A, Nguyen MAT, Vu VDU, Snapper SB, Galy A, Notarangelo LD, Bushman FD, Williams DA, and Pai SY

Subjects

Humans, Wiskott-Aldrich Syndrome Protein genetics, Hematopoietic Stem Cells metabolism, Genetic Therapy methods, Wiskott-Aldrich Syndrome genetics, Wiskott-Aldrich Syndrome therapy, Hematopoietic Stem Cell Transplantation adverse effects, Eczema etiology, Eczema metabolism, Eczema therapy

Abstract

Wiskott-Aldrich syndrome (WAS) is a rare X-linked disorder characterized by combined immunodeficiency, eczema, microthrombocytopenia, autoimmunity, and lymphoid malignancies. Gene therapy (GT) to modify autologous CD34+ cells is an emerging alternative treatment with advantages over standard allogeneic hematopoietic stem cell transplantation for patients who lack well-matched donors, avoiding graft-versus-host-disease. We report the outcomes of a phase 1/2 clinical trial in which 5 patients with severe WAS underwent GT using a self-inactivating lentiviral vector expressing the human WAS complementary DNA under the control of a 1.6-kB fragment of the autologous promoter after busulfan and fludarabine conditioning. All patients were alive and well with sustained multilineage vector gene marking (median follow-up: 7.6 years). Clinical improvement of eczema, infections, and bleeding diathesis was universal. Immune function was consistently improved despite subphysiologic levels of transgenic WAS protein expression. Improvements in platelet count and cytoskeletal function in myeloid cells were most prominent in patients with high vector copy number in the transduced product. Two patients with a history of autoimmunity had flares of autoimmunity after GT, despite similar percentages of WAS protein-expressing cells and gene marking to those without autoimmunity. Patients with flares of autoimmunity demonstrated poor numerical recovery of T cells and regulatory T cells (Tregs), interleukin-10-producing regulatory B cells (Bregs), and transitional B cells. Thus, recovery of the Breg compartment, along with Tregs appears to be protective against development of autoimmunity after GT. These results indicate that clinical and laboratory manifestations of WAS are improved with GT with an acceptable safety profile. This trial is registered at clinicaltrials.gov as #NCT01410825.

Published

2023

176. Clinical Cytometry for Platelets and Platelet Disorders.

Author

Frelinger AL 3rd and Spurgeon BEJ

Subjects

Humans, Antibodies, Flow Cytometry methods, Immunophenotyping, Blood Platelets physiology, Blood Platelet Disorders diagnosis

Abstract

Clinical flow cytometry tests for inherited and acquired platelet disorders are useful diagnostic tools but are not widely available. Flow cytometric methods are available to detect inherited glycoprotein deficiencies, granule release (secretion defects), drug-induced thrombocytopenias, presence of antiplatelet antibodies, and pharmacodynamic inhibition by antiplatelet agents. New tests take advantage of advanced multicolor cytometers and allow identification of novel platelet subsets by high-dimensional immunophenotyping. Studies are needed to evaluate the value of these new tests for diagnosis and monitoring of therapy in patients with platelet disorders., (Copyright © 2023 Elsevier Inc. All rights reserved.)

Published

2023

177. Platelet Phenotyping by Full Spectrum Flow Cytometry.

Author

Spurgeon BEJ and Frelinger AL 3rd

Subjects

Flow Cytometry methods, Phenotype, Biomarkers, Blood Platelets, Hemostasis

Abstract

Platelets play key roles in hemostasis, immunity, and inflammation, and tests of platelet phenotype and function are useful in studies of disease biology and pathology. Full spectrum flow cytometry offers distinct advantages over standard tests and enables the sensitive and simultaneous detection of many biomarkers. A typical assay provides a wealth of information on platelet biology and allows the assessment of in vivo activation and in vitro reactivity, as well as the discovery of novel phenotypes. Here, we describe the analysis of platelets by full spectrum flow cytometry and discuss a range of controls and methods for interpreting results. © 2023 Wiley Periodicals LLC. Basic Protocol: Platelet phenotyping by full spectrum flow cytometry Support Protocol 1: Spectral unmixing Support Protocol 2: Data preprocessing., (© 2023 Wiley Periodicals LLC.)

Published

2023

178. Expert opinion on the use of platelet secretion assay for the diagnosis of inherited platelet function disorders: Communication from the ISTH SSC Subcommittee on Platelet Physiology.

Author

Mezzano D, Harrison P, Frelinger AL 3rd, Mumford AD, Noris P, Lordkipanidzé M, and Gresele P

Subjects

Blood Platelets metabolism, Communication, Hemostasis, Humans, Multicenter Studies as Topic, Platelet Function Tests methods, Blood Platelet Disorders diagnosis, Blood Platelet Disorders metabolism, Thrombasthenia

Abstract

Assessment of platelet secretion is crucial for diagnosing suspected inherited platelet function disorders (IPFD). A previous survey of the SSC on Platelet Physiology of the ISTH and a comprehensive review highlighted that most of the platelet secretion assays (PSAs) lack standardization and validation. The aim of this study was to provide expert consensus guidance on the use of PSAs for IPFD diagnosis. We surveyed 26 experts from 10 different countries using the RAND/UCLA methodology, to attain a consensus on sensitivity, specificity, feasibility, time to readout, and cost of most PSAs. Answers were then graded in three categories: appropriate, uncertain, and inappropriate. Equivocal or misinterpretable statements required a second and third round survey involving 14 of the original 26 experts. We report here the consolidated results of the entire procedure. There was uniform agreement on several general statements, including that PSAs should be performed in hemostasis laboratories as first line diagnostic tests even in patients with normal platelet aggregation, and should include a δ-granule secretion marker. Among the specific assays examined, lumiaggregometry, other luciferin/luciferase-based assays, high-performance liquid chromatography methods, radiolabeled-serotonin based assays, and whole-mount transmission electron microscopy were rated as appropriate for the measurement of δ-granule release, and platelet P-selectin expression by flow cytometry and released proteins by ELISA for α-granule release. For most of the other PSAs, the expert opinions were widely dispersed. Lack of expert consensus on many PSAs clearly indicates an unmet need for rigorous standardization, multicenter comparison of results, and validation of PSAs for clinical laboratory practice., (© 2022 International Society on Thrombosis and Haemostasis.)

Published

2022

179. Comprehensive phenotyping of human platelets by single-cell cytometry.

Author

Spurgeon BEJ and Frelinger AL 3rd

Subjects

Biomarkers metabolism, Flow Cytometry, Hemostasis, Humans, Immunophenotyping, Platelet Activation genetics, Blood Platelets, Megakaryocytes

Abstract

Platelets are small anucleate blood cells that contribute to hemostasis, immunity, and inflammation. Circulating platelets are heterogeneous in size, age, receptor expression, and reactivity. They inherit many features from megakaryocytes and are further modified on exposure to bioactive substances in the bloodstream. Among these substances, prothrombotic agonists, vasodilators, and bloodborne pathogens modulate platelet phenotypes via distinct signaling cascades. The ability of platelets to respond to (patho)physiologic signals is incompletely understood but likely depends on their repertoire of surface receptors, which may partition them into discrete subsets with specialized functions and divergent abilities. The single-cell resolution of flow and mass cytometry is ideal for immunophenotyping and allows the identification of platelet subsets in remarkable detail. In this report, we describe the surface markers and gating strategies needed for the comprehensive characterization of platelets., (© 2022 International Society for Advancement of Cytometry.)

Published

2022

180. Inhibition of transcription factor NFAT activity in activated platelets enhances their aggregation and exacerbates gram-negative bacterial septicemia.

Author

Poli V, Di Gioia M, Sola-Visner M, Granucci F, Frelinger AL 3rd, Michelson AD, and Zanoni I

Subjects

Animals, Blood Coagulation drug effects, Blood Platelets metabolism, Cell Communication drug effects, Cytoplasmic Granules metabolism, Disease Models, Animal, Extracellular Traps metabolism, Humans, Inflammation, Mice, NFATC Transcription Factors metabolism, Neutrophils metabolism, Receptors, Thrombin metabolism, Sepsis metabolism, Blood Platelets drug effects, NFATC Transcription Factors antagonists & inhibitors, Platelet Aggregation drug effects, Sepsis pathology

Abstract

During gram-negative septicemia, interactions between platelets and neutrophils initiate a detrimental feedback loop that sustains neutrophil extracellular trap (NET) induction, disseminated intravascular coagulation, and inflammation. Understanding intracellular pathways that control platelet-neutrophil interactions is essential for identifying new therapeutic targets. Here, we found that thrombin signaling induced activation of the transcription factor NFAT in platelets. Using genetic and pharmacologic approaches, as well as iNFATuation, a newly developed mouse model in which NFAT activation can be abrogated in a cell-specific manner, we demonstrated that NFAT inhibition in activated murine and human platelets enhanced their activation and aggregation, as well as their interactions with neutrophils and NET induction. During gram-negative septicemia, NFAT inhibition in platelets promoted disease severity by increasing disseminated coagulation and NETosis. NFAT inhibition also partially restored coagulation ex vivo in patients with hypoactive platelets. Our results define non-transcriptional roles for NFAT that could be harnessed to address pressing clinical needs., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2021 Elsevier Inc. All rights reserved.)

Published

2022

181. Consensus recommendations on flow cytometry for the assessment of inherited and acquired disorders of platelet number and function: Communication from the ISTH SSC Subcommittee on Platelet Physiology.

Author

Frelinger AL 3rd, Rivera J, Connor DE, Freson K, Greinacher A, Harrison P, Kunishima S, Lordkipanidzé M, Michelson AD, Ramström S, and Gresele P

Subjects

Consensus, Flow Cytometry, Humans, Platelet Count, Communication, Platelet Function Tests

Abstract

Flow cytometry is increasingly used in the study of platelets in inherited and acquired disorders of platelet number and function. However, wide variation exists in specific reagents, methods, and equipment used, making interpretation and comparison of results difficult. The goal of the present study was to provide expert consensus guidance on the use of flow cytometry for the evaluation of platelet disorders. A modified RAND/UCLA survey method was used to obtain a consensus among 11 experts from 10 countries across four continents, on the appropriateness of statements relating to clinical utility, pre-analytical variables, instrument and reagent standardization, methods, reporting, and quality control for platelet flow cytometry. Feedback from the initial survey revealed that uncertainty was sometimes due to lack of expertise with a particular test condition rather than unavailable or ambiguous data. To address this, the RAND method was modified to allow experts to self-identify statements for which they could not provide expert input. There was uniform agreement among experts in the areas of instrument and reagent standardization, methods, reporting, and quality control and this agreement is used to suggest best practices in these areas. However, 25.9% and 50% of statements related to pre-analytical variables and clinical utility, respectively, were rated as uncertain. Thus, while citrate is the preferred anticoagulant for many flow cytometric platelet tests, expert opinions differed on the acceptability of other anticoagulants, particularly heparin. Lack of expert consensus on the clinical utility of many flow cytometric platelet tests indicates the need for rigorous multicenter clinical outcome studies., (© 2021 International Society on Thrombosis and Haemostasis.)

Published

2021

182. Sex-specific platelet activation through protease-activated receptor-1 in patients undergoing cardiac catheterization.

Author

Gremmel T, Michelson AD, Wadowski PP, Pultar J, Weikert C, Tscharre M, Lee S, Panzer S, and Frelinger AL 3rd

Subjects

Blood Platelets, Cardiac Catheterization, Female, Humans, Male, Platelet Activation, Platelet Aggregation, Platelet Glycoprotein GPIIb-IIIa Complex pharmacology, Platelet Aggregation Inhibitors pharmacology, Receptor, PAR-1

Abstract

Background and Aims: Protease-activated receptor (PAR)-1-mediated platelet activation may vary according to sex and clinical situation. In order to investigate sex-specific platelet activation through PAR-1, we assessed platelet response to thrombin receptor-activating peptide (TRAP) in 562 patients undergoing cardiac catheterization without (Group 1A) and with (Group 1B) acute coronary syndrome (ACS). Subsequently, we sought to confirm our findings in 287 patients undergoing elective (Group 2A) or acute (Group 2B) percutaneous coronary intervention., Methods: TRAP-stimulated platelet surface expression of P-selectin and activated glycoprotein IIb/IIIa (GPIIb/IIIa) were measured by flow cytometry in Group 1. Light transmission aggregometry (LTA) and multiple electrode aggregometry (MEA) in response to TRAP were assessed in Group 2., Results: In Group 1A, platelet activation in response to TRAP was significantly higher in women compared to men (P-selectin: 511 MFI [443-597 MFI] vs. 471 MFI [393-552 MFI]; GPIIb/IIIa: 84 MFI [58-119 MFI] vs. 70 MFI [47-103 MFI]; both p ≤ 0.002). In contrast, in Group 1B, TRAP-stimulated P-selectin and activated GPIIb/IIIa were similar in men and women (both p ≥ 0.3). Likewise, TRAP-stimulated platelet aggregation was significantly higher in female patients in Group 2A (LTA: 66% [54-76%] vs. 51% [41-65%]; MEA: 78 AU [66-107 AU] vs. 62 AU [52-88 AU]; both p ≤ 0.02), whereas men and women in Group 2 B had similar platelet aggregation (p = 0.5). The occurrence of ischemic endpoints did not differ significantly between men and women in Group 1A and Group 1B., Conclusions: Platelet PAR-1 signaling is more pronounced in women than in men without ACS. In ACS, however, PAR-1-mediated platelet activation is similar in male and female patients., (Copyright © 2021 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2021

183. Immunophenotypic Analysis of Platelets by Flow Cytometry.

Author

Spurgeon BEJ, Linden MD, Michelson AD, and Frelinger AL 3rd

Subjects

Factor Va, Flow Cytometry, Immunophenotyping, Blood Platelets, Platelet Activation

Abstract

Platelets are small but very abundant blood cells that play a key role in hemostasis, contributing to thrombus formation at sites of injury. The ability of platelets to perform this function, as well as functions in immunity and inflammation, is dependent on the presence of cell surface glycoproteins and changes in their quantity and conformation after platelet stimulation. In this article, we describe the characterization of platelet surface markers and platelet function using platelet-specific fluorescent probes and flow cytometry. Unlike traditional platelet tests, immunophenotypic analysis of platelets by flow cytometry allows the analysis of platelet function in samples with very low platelet counts as often encountered in clinical situations. © 2021 Wiley Periodicals LLC. Basic Protocol 1: Immunophenotyping of platelet surface receptors Alternate Protocol: Fix-first method for immunophenotyping of platelet surface receptors Basic Protocol 2: Determination of platelet activation using P-selectin expression and/or PAC1 binding Basic Protocol 3: Determination of procoagulant platelets using annexin V binding or antibodies specific for coagulation factor V/Va or X/Xa Support Protocol: Preparation of isolated platelets., (© 2021 Wiley Periodicals LLC.)

Published

2021

184. Platelet Immunophenotyping by High-Dimensional Mass Cytometry.

Author

Spurgeon BEJ, Michelson AD, and Frelinger AL 3rd

Subjects

Biomarkers, Flow Cytometry, Humans, Immunophenotyping, Blood Platelet Disorders, Blood Platelets

Abstract

Platelets are small blood cells that contribute to hemostasis, immunity, and inflammation. Characterization of platelet surface markers allows for differentiation of activated platelets from resting platelets, diagnosis of platelet disorders, and investigation of platelet biology and pathology. In this article, we describe the use of mass cytometry or "CyTOF" (mass spectroscopy detection of metal-tagged antibodies on individual cells) to measure a large number of markers on each platelet and to identify platelet subsets based on the shared expression of multiple markers. This powerful new approach provides a vastly more detailed picture of platelet immunophenotypes than conventional flow cytometry and enables investigation of the roles of platelet subsets in health and disease. © 2021 Wiley Periodicals LLC. Basic Protocol: Platelet immunophenotyping by high-dimensional mass cytometry Support Protocol: Data preprocessing., (© 2021 Wiley Periodicals LLC.)

Published

2021

185. Activation of platelet-rich plasma by pulse electric fields: Voltage, pulse width and calcium concentration can be used to control and tune the release of growth factors, serotonin and hemoglobin.

Author

Neculaes B, Frelinger AL 3rd, Gerrits AJ, Gremmel T, Forde EE, Klopman S, Carmichael SL, and Michelson AD

Subjects

Blood Cell Count, Calcium chemistry, Calcium pharmacology, Enzyme-Linked Immunosorbent Assay, Epidermal Growth Factor metabolism, Hemoglobins metabolism, Humans, Platelet Activation drug effects, Platelet-Derived Growth Factor metabolism, Serotonin metabolism, Electricity, Epidermal Growth Factor analysis, Hemoglobins analysis, Platelet-Derived Growth Factor analysis, Platelet-Rich Plasma metabolism, Serotonin analysis

Abstract

Activated platelet-rich plasma (PRP) has been used in the clinical settings of wound healing and regenerative medicine, with activation typically induced by the addition of bovine thrombin. To eliminate issues with availability, cost and potential side effects associated with bovine thrombin, ex vivo PRP activation using pulse electric fields (PEF) has been proposed and demonstrated. The present study characterizes the effect of PEF voltage and pulse width, in combination with a range of calcium concentrations, on clot formation, growth factor release, and serotonin (5-HT) release from dense granules. The main findings are: 1) increasing calcium concentrations with most PEF conditions leads to increased levels of PDGF and 5-HT release; 2) whether EGF levels increase or decrease with increasing calcium concentration depends on the specific PEF parameters; 3) the pattern of PDGF and EGF levels in supernatants suggest that these molecules are localized differently within platelets; 4) significant levels of PDGF, EGF, and 5-HT can be released without inducing clot formation or hemoglobin release. In conclusion, voltage, pulse width and calcium concentration can be used to control and tune the release of growth factors, serotonin and hemoglobin from PEF-activated PRP. Because growth factor requirements vary for different types of wounds and for wounds at different stages of healing, the unique balance of factors in supernatants of PEF-activated PRP may provide more clinically advantageous than the current standard of bovine thrombin-activated PRP., Competing Interests: I have read the journal’s policy and the authors of this manuscript have the following competing interests: A.L. Frelinger and A. D. Michelson received research support from GE Research. B. Neculaes and S. Klopman are employees of GE Research. This does not alter the authors’ adherence to PLOS ONE policies on sharing data and materials. The remaining authors declare no competing interests.

Published

2021

186. Evaluation of Longitudinal Pain Study in Sickle Cell Disease (ELIPSIS) by patient-reported outcomes, actigraphy, and biomarkers.

Author

Pittman DD, Hines PC, Beidler D, Rybin D, Frelinger AL, Michelson AD, Liu K, Gao X, White J, Zaidi AU, Charnigo RJ, and Callaghan MU

Subjects

Actigraphy, Adolescent, Adult, Anemia, Sickle Cell diagnosis, Anemia, Sickle Cell drug therapy, Antisickling Agents therapeutic use, Biomarkers analysis, Female, Humans, Hydroxyurea therapeutic use, Longitudinal Studies, Male, Middle Aged, Pain diagnosis, Patient Reported Outcome Measures, Young Adult, Anemia, Sickle Cell complications, Pain etiology

Abstract

Clinical trials in sickle cell disease (SCD) often focus on health care utilization for painful vaso-occlusive crises (VOCs). However, no objective, quantifiable pain biomarkers exist, pain is not specific to VOCs, health care utilization varies between patients, unreported at-home VOCs likely contribute to long-term outcomes, and patient-reported outcomes are seldom considered. This noninterventional, longitudinal, 6-month study aimed to develop tools to identify VOCs in SCD patients with or without health care utilization. Participants wore an actigraph device, tracking sleep and activity. Patients with SCD used an electronic patient-reported outcome (ePRO) tool to collect data on pain, medication, fatigue, and daily function. Patients self-reported when they experienced VOC pain (VOC day). Biomarkers were collected every 3 weeks (non-VOC). Self-reported VOCs triggered at-home or in-hospital blood collection. The study enrolled 37 participants with SCD; 35 completed the study. Participants reported 114 VOC events and 346 VOC days, of which 62.3% and 78.3%, respectively, were self-treated at home. The ePRO and actigraphy captured end points of pain, functionality, fatigue, activity, and sleep; each was significantly altered on VOC days compared with non-VOC days. Biomarkers collected at home or in the hospital on VOC days were significantly altered compared with non-VOC baseline values, including leukocyte-platelet aggregates, microfluidic-based blood cell adhesion, interleukin-6, C-reactive protein, interleukin-10, tumor necrosis factor-α, and thrombin-antithrombin. The Evaluation of Longitudinal Pain Study in Sickle Cell Disease (ELIPSIS) trial shows the feasibility of accurately monitoring out-of-hospital pain by using patient-reported VOC days as potential end points for clinical trials in SCD; it describes the changes in biomarkers and activity measured by actigraphy that may enable improved identification and assessment of VOCs., (© 2021 by The American Society of Hematology.)

Published

2021

187. Decreased platelet surface phosphatidylserine predicts increased bleeding in patients with severe factor VIII deficiency.

Author

Croteau SE, Frelinger AL 3rd, Gerrits AJ, and Michelson AD

Subjects

Blood Platelets, Factor VIII, Humans, Phosphatidylserines, Platelet Activation, Thrombin, Cell-Derived Microparticles, Hemophilia A diagnosis

Abstract

Background: Bleeding phenotypes among individuals with severe factor VIII (FVIII) deficiency are variable, even with routine prophylactic FVIII administration. Activated platelets, in addition to their role in primary hemostasis, play a major role in coagulation by providing a phospholipid surface to which coagulation factors bind., Objectives: The aim of this study was to determine whether platelet function is associated with past and/or future bleeding in patients with severe FVIII deficiency on prophylaxis., Patients/methods: Platelet function quantified by platelet surface expression of phosphatidylserine, platelet surface glycoprotein (GP) VI, platelet surface activated GPIIb-IIIa, platelet surface P-selectin, the percentage of coated platelets, and the percentage of platelet-derived microparticles in the presence or absence of in vitro activation by various agonists was assessed in 34 patients., Results: Decreased platelet surface phosphatidylserine expression (identified by annexin V binding), both in the presence and absence of ADP/thrombin receptor activating peptide, demonstrated a significant association with both prior and subsequent bleeding in any location and specifically with hemarthrosis. No significant difference between patients with and without bleeding was observed in any of the other platelet activity markers., Conclusions: Decreased platelet surface phosphatidylserine expression measured by annexin V binding predicts increased bleeding in severe FVIII deficient patients on prophylaxis., (© 2021 International Society on Thrombosis and Haemostasis.)

Published

2021

188. Biomarkers of platelet activation and cardiovascular risk in the DAPT trial.

Author

Berg DD, Yeh RW, Mauri L, Morrow DA, Kereiakes DJ, Cutlip DE, Gao Q, Jarolim P, Michelson AD, Frelinger AL 3rd, Cange AL, Sabatine MS, and O'Donoghue ML

Subjects

Biomarkers blood, CD40 Ligand blood, Drug Monitoring methods, Dual Anti-Platelet Therapy adverse effects, Dual Anti-Platelet Therapy methods, Duration of Therapy, Female, Humans, Male, Middle Aged, Percutaneous Coronary Intervention instrumentation, Percutaneous Coronary Intervention methods, Platelet Function Tests methods, Reproducibility of Results, Risk Assessment methods, Calgranulin A blood, Calgranulin B blood, Coronary Restenosis blood, Coronary Restenosis etiology, Coronary Restenosis prevention & control, Hemorrhage blood, Hemorrhage chemically induced, Hemorrhage prevention & control, P-Selectin blood, Percutaneous Coronary Intervention adverse effects

Abstract

Prolonged use of dual antiplatelet therapy (DAPT) post-percutaneous coronary intervention (PCI) has been shown to reduce the risk of major adverse cardiovascular events (MACE), but with increased bleeding. It remains unknown whether biomarkers of platelet activation may be useful for identifying patients at increased risk of MACE. The DAPT study was a randomized trial of 12 versus 30 months of DAPT in patients who underwent PCI. Serum biomarkers [myeloid-related protein (MRP)-8/14, P-selectin, soluble CD-40 ligand (sCD40L)] were assessed in 1399 patients early post-PCI. On-treatment platelet reactivity index (PRI) using VASP phosphorylation was assessed in 443 patients randomized to continued DAPT at 1 year. MACE was defined as CV death, MI, or ischemic stroke. Multivariable models were adjusted for baseline characteristics, index event, and stent type. A stepwise increase in the risk of MACE was observed with increasing tertiles of both MRP-8/14 and P-selectin (p-trend = 0.04 for both). After multivariable adjustment, the adjusted HR (95% CI) for MACE in patients in the top tertile was 1.94 (1.14-3.30) for MRP-8/14 and 1.62 (0.99-2.64) for P-selectin. In contrast, baseline sCD40L was not associated with CV risk. Among patients randomized to continued DAPT, higher on-treatment platelet reactivity was not significantly associated with risk of MACE (p-trend = 0.32; adj-HR T3 vs. T1 1.54, 95% CI 0.20-12.18) or bleeding (P-trend = 0.17; adj-HR 0.25, 95% CI 0.05-1.21). MRP-8/14 and soluble P-selectin may be useful for identifying patients at increased risk of MACE after PCI. The utility of on-treatment platelet function testing requires further study.Clinical Trial Registration https://www.clinicaltrials.gov . Unique identifier NCT00977938.

Published

2021

189. Platelet mass cytometry: Optimization of sample, reagent, and analysis parameters.

Author

Spurgeon BEJ, Michelson AD, and Frelinger AL 3rd

Subjects

Flow Cytometry, Humans, Indicators and Reagents, Platelet Activation, Reproducibility of Results, Blood Platelets, Hemostasis

Abstract

Platelets mediate key biological processes, including hemostasis, immunity, and inflammation. Although platelets are often treated as a homogeneous cell population, they are known to be heterogeneous in size, age, surface receptor expression, and response to agonist stimulation, raising the possibility that distinct platelet subsets perform specialized functions and that such subsets may be altered in disease settings. Attempts to identify platelet subsets by flow cytometry have had limited success due in part to limits on the number of probes that can be used at the same time and due to the challenges of compensating for probes that have large spectral overlap. We recently reported a method to identify platelet subsets by mass cytometry using a panel of 14 metal-tagged antibodies directed at platelet surface markers. Here, we describe the technical considerations and best practices for platelet sample preparation, processing, and analysis by mass cytometry. Specifically, we show that anticoagulant choice alters platelet phenotype and function and that antibody cocktail storage and sample processing are critical for reproducibility. Additionally, we optimize sample density and instrument setup for maximal platelet transmission. Lastly, we demonstrate the importance of panel design and compensation and the use of clustering and dimension reduction to map platelet heterogeneity across resting and stimulated samples., (© 2020 International Society for Advancement of Cytometry.)

Published

2021

190. Platelet count and disease - editorial policy.

Author

Harrison P, Lordkipanidzé M, Frelinger AL 3rd, Thomas MR, and Watson SP

Published

2020

191. Platelet surface marker analysis by mass cytometry.

Author

Blair TA and Frelinger AL 3rd

Subjects

Blood Platelets cytology, Humans, Blood Platelets metabolism, Flow Cytometry methods

Abstract

Mass cytometry is a next generation flow cytometry technology which analyzes cells one at a time (up to 1000/sec) using mass spectrometry to detect probes labeled with rare-earth metals. Rare-earth metals detected by mass spectrometry have extremely low backgrounds and can be identified with high resolution enabling the routine simultaneous detection of more than 45 probes on each cell without the need for complex compensation matrices. Here we describe a panel of 14 platelet-specific metal-conjugated antibodies (targeting cluster of differentiation [CD] 9, CD29, CD31, CD36, CD41, CD42a, CD42b, CD61, CD62P, CD63, CD107a, CD154, glycoprotein [GP] VI and activated integrin αIIbβ3) and methods for staining and analysis of platelets by mass cytometry. High dimensional clustering algorithms, which take into account the levels of all 14 markers detected by mass cytometry on each cell, allow identification of platelet subpopulations not previously appreciated. We previously reported that platelet heterogeneity identified by mass cytometry appears similar across healthy donors and consistent over time. High dimensional analysis revealed the presence of a platelet subpopulation with significantly higher levels of surface expression of activated GPIIb-IIIa and P -selectin suggesting this subpopulation may play a greater role in thrombus formation than other platelet subpopulations. Thus, analysis by mass cytometry of platelet heterogeneity and subpopulations may suggest distinct biological roles for different platelet subpopulations and may be useful in evaluating inherited or acquired platelet disorders and platelet function in health and disease.

Published

2020

192. An exploratory, randomised, placebo-controlled, 14 day trial of the soluble guanylate cyclase stimulator praliciguat in participants with type 2 diabetes and hypertension.

Author

Hanrahan JP, Seferovic JP, Wakefield JD, Wilson PJ, Chickering JG, Jung J, Carlson KE, Zimmer DP, Frelinger AL 3rd, Michelson AD, Morrow L, Hall M, Currie MG, Milne GT, and Profy AT

Subjects

Adult, Aged, Diabetes Mellitus, Type 2 complications, Diabetes Mellitus, Type 2 metabolism, Diabetic Nephropathies prevention & control, Double-Blind Method, Drug Therapy, Combination, Female, Guanylyl Cyclase C Agonists pharmacokinetics, Guanylyl Cyclase C Agonists therapeutic use, Humans, Hypertension complications, Hypertension metabolism, Hypoglycemic Agents pharmacokinetics, Hypoglycemic Agents therapeutic use, Insulin administration & dosage, Insulin adverse effects, Male, Middle Aged, Treatment Outcome, Diabetes Mellitus, Type 2 drug therapy, Hypertension drug therapy, Pyrazoles pharmacokinetics, Pyrazoles therapeutic use, Pyrimidines pharmacokinetics, Pyrimidines therapeutic use

Abstract

Aims/hypothesis: Praliciguat (IW-1973), a soluble guanylate cyclase stimulator, amplifies nitric oxide signalling. This exploratory trial investigated the safety, tolerability, pharmacokinetic profile and pharmacodynamic effects of praliciguat in individuals with type 2 diabetes and hypertension., Methods: This Phase IIA, double-blind, placebo-controlled trial investigated praliciguat in 26 participants with type 2 diabetes and hypertension on stable glucose- and BP-lowering therapies. Participants were randomly allocated in a 3:5:5 ratio to three groups: placebo (n = 6), praliciguat 40 mg once daily for days 1-14 (n = 10), or praliciguat 20 mg twice daily for days 1-7 then 40 mg once daily for days 8-14 (n = 10). Assessments were made in clinic and included treatment-emergent adverse events, pharmacokinetics, metabolic variables, 24 h BP and heart rate, platelet function, reactive hyperaemia index (RHI) and plasma biomarkers. Participants, the sponsor, the investigator and clinic study staff (except designated pharmacy personnel) were blinded to group assignment., Results: Participants treated for 14 days with praliciguat had least-square mean change-from-baseline differences vs placebo (95% CI) of -0.7 (-1.8, 0.4) mmol/l for fasting plasma glucose, -0.7 (-1.1, -0.2) mmol/l for total cholesterol, -0.5 (-1.0, -0.1) mmol/l for LDL-cholesterol, -23 (-56, 9) for HOMA-IR in those not being treated with insulin, and -5 (-10, 1) mmHg and 3 (-1, 6) beats/min for average 24 h mean arterial pressure and heart rate, respectively. Apart from one serious adverse event (SAE; upper gastrointestinal haemorrhage), praliciguat was well tolerated. Praliciguat did not affect platelet function or RHI. Among exploratory biomarkers, plasma levels of asymmetric dimethylarginine decreased in praliciguat vs placebo recipients., Conclusions/interpretation: In participants with type 2 diabetes and hypertension on standard therapies, over 14 days praliciguat was well tolerated, except for a single SAE, and showed positive trends in metabolic and BP variables. These results support further clinical investigation of praliciguat., Trial Registration: ClinicalTrials.gov NCT03091920., Funding: This trial was funded by Cyclerion Therapeutics.

Published

2020

193. Using extracellular calcium concentration and electric pulse conditions to tune platelet-rich plasma growth factor release and clotting.

Author

Garner AL, Frelinger AL 3rd, Gerrits AJ, Gremmel T, Forde EE, Carmichael SL, Michelson AD, and Neculaes VB

Subjects

Adolescent, Adult, Animals, Calcium metabolism, Cattle, Electricity, Healthy Volunteers, Humans, Pilot Projects, Platelet Activation, Platelet-Derived Growth Factor metabolism, Thrombin, Young Adult, Blood Coagulation, Intercellular Signaling Peptides and Proteins metabolism, Platelet-Rich Plasma metabolism

Abstract

Platelet-rich plasma (PRP) is an emerging autologous biologic method for wound healing. Clinicians apply PRP either topically (where it is activated ex-vivo before treatment by adding an external agent to trigger clotting and the release of growth factors that facilitate wound healing) or through injection (where it is activated in vivo at the injury site with no prior activation before injection). Because topical PRP activation typically utilizes bovine thrombin, which has significant potential side effects and high costs, recent studies have assessed the efficacy of combining extracellular calcium (EC) and electric pulses (EPs) to activate PRP. The potential to apply this novel technique to PRP both topically and internally via injection raises the question about the ability to tune the clotting time and growth factor release for a given application. While previous studies have assessed the impact of applying EPs of various durations either directly (conductive coupling) or indirectly (capacitive coupling) to PRP containing EC, no studies have assessed the tunability of this activation based on modifying EP parameters, EP delivery method (conductive or capacitive coupling), and the EC concentration. We hypothesize that tuning these parameters will modify intracellular calcium uptake to permit the control of growth factor release and clotting time, which are critical for optimizing PRP for either topical or internal clinical applications. A pilot study for a single donor demonstrates the potential for tunability as a function of the intensity of membrane manipulation and calcium concentration, which facilitate the increase of cytosolic calcium. This motivates future studies assessing EC and EP optimization and in vivo studies to determine the overall efficacy of this tunability for wound healing., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019

194. Publisher Correction: GLS-409, an Antagonist of Both P2Y 1 and P2Y 12 , Potently Inhibits Canine Coronary Artery Thrombosis and Reversibly Inhibits Human Platelet Activation.

Author

Smolensky Koganov E, Michelson AD, Yanachkov IB, Yanachkova MI, Wright GE, Przyklenk K, and Frelinger AL 3rd

Abstract

A correction to this article has been published and is linked from the HTML and PDF versions of this paper. The error has been fixed in the paper.

Published

2018

195. Novel aspects of antiplatelet therapy in cardiovascular disease.

Author

Gremmel T, Michelson AD, Frelinger AL III, and Bhatt DL

Abstract

Antiplatelet therapy is a cornerstone in the secondary prophylaxis of adverse cardiovascular events such as myocardial infarction and stroke. The cyclooxygenase inhibitor aspirin remains the most frequently prescribed antiplatelet drug, followed by adenosine diphosphate P2Y 12 receptor blockers. Glycoprotein IIb-IIIa antagonists are intravenously available antiplatelet agents preventing platelet-to-platelet aggregation via the fibrinogen receptor. The thrombin receptor inhibitor vorapaxar allows the targeting of yet a third pathway of platelet activation. Despite the advent of novel agents and major advances in antiplatelet treatment over the last decade, atherothrombotic events still impair the prognosis of many patients with cardiovascular disease. Consequently, antiplatelet therapy remains a field of intense research and a large number of studies on its various aspects are published each year. This review article summarizes recent developments in antiplatelet therapy in cardiovascular disease focusing particularly on the duration of dual antiplatelet therapy, new treatment regimens, the role of platelet function testing, and potential future targets of antiplatelet agents.

Published

2018

196. Calpain-1 regulates platelet function in a humanized mouse model of sickle cell disease.

Author

Nwankwo JO, Gremmel T, Gerrits AJ, Mithila FJ, Warburton RR, Hill NS, Lu Y, Richey LJ, Jakubowski JA, Frelinger AL 3rd, and Chishti AH

Subjects

Animals, Disease Models, Animal, Female, Humans, Hypoxia blood, Male, Mice, Mice, Inbred C57BL, Mice, Knockout, Anemia, Sickle Cell blood, Blood Coagulation drug effects, Blood Platelets metabolism, Calpain blood, Platelet Activation drug effects

Abstract

One of the major contributors to sickle cell disease (SCD) pathobiology is the hemolysis of sickle red blood cells (RBCs), which release free hemoglobin and platelet agonists including adenosine 5'-diphosphate (ADP) into the plasma. While platelet activation/aggregation may promote tissue ischemia and pulmonary hypertension in SCD, modulation of sickle platelet dysfunction remains poorly understood. Calpain-1, a ubiquitous calcium-activated cysteine protease expressed in hematopoietic cells, mediates aggregation of platelets in healthy mice. We generated calpain-1 knockout Townes sickle (SSCKO) mice to investigate the role of calpain-1 in steady state and hypoxia/reoxygenation (H/R)-induced sickle platelet activation and aggregation, clot retraction, and pulmonary arterial hypertension. Using multi-electrode aggregometry, which measures platelet adhesion and aggregation in whole blood, we determined that steady state SSCKO mice exhibit significantly impaired PAR4-TRAP-stimulated platelet aggregation as compared to Townes sickle (SS) and humanized control (AA) mice. Interestingly, the H/R injury induced platelet hyperactivity in SS and SSCKO, but not AA mice, and partially rescued the aggregation defect in SSCKO mice. The PAR4-TRAP-stimulated GPIIb-IIIa (α IIb β 3 ) integrin activation was normal in SSCKO platelets suggesting that an alternate mechanism mediates the impaired platelet aggregation in steady state SSCKO mice. Taken together, we provide the first evidence that calpain-1 regulates platelet hyperactivity in sickle mice, and may offer a viable pharmacological target to reduce platelet hyperactivity in SCD., (Copyright © 2017 Elsevier Ltd. All rights reserved.)

Published

2017

197. High serum serotonin in sudden infant death syndrome.

Author

Haynes RL, Frelinger AL 3rd, Giles EK, Goldstein RD, Tran H, Kozakewich HP, Haas EA, Gerrits AJ, Mena OJ, Trachtenberg FL, Paterson DS, Berry GT, Adeli K, Kinney HC, and Michelson AD

Subjects

Adult, Autopsy, Brain Stem metabolism, Case-Control Studies, Chromatography, High Pressure Liquid, Cohort Studies, Female, Genotype, Humans, Hydroxyindoleacetic Acid blood, Infant, Male, Polymorphism, Genetic, Risk Factors, Serotonin Plasma Membrane Transport Proteins genetics, Asphyxia blood, Biomarkers blood, Serotonin blood, Sudden Infant Death blood

Abstract

Sudden infant death syndrome (SIDS), the leading cause of postneonatal infant mortality, likely comprises heterogeneous disorders with the common phenotype of sudden death without explanation upon postmortem investigation. Previously, we reported that ∼40% of SIDS deaths are associated with abnormalities in serotonin (5-hydroxytryptamine, 5-HT) in regions of the brainstem critical in homeostatic regulation. Here we tested the hypothesis that SIDS is associated with an alteration in serum 5-HT levels. Serum 5-HT, adjusted for postconceptional age, was significantly elevated (95%) in SIDS infants ( n = 61) compared with autopsied controls ( n = 15) [SIDS, 177.2 ± 15.1 (mean ± SE) ng/mL versus controls, 91.1 ± 30.6 ng/mL] ( P = 0.014), as determined by ELISA. This increase was validated using high-performance liquid chromatography. Thirty-one percent (19/61) of SIDS cases had 5-HT levels greater than 2 SDs above the mean of the controls, thus defining a subset of SIDS cases with elevated 5-HT. There was no association between genotypes of the serotonin transporter promoter region polymorphism and serum 5-HT level. This study demonstrates that SIDS is associated with peripheral abnormalities in the 5-HT pathway. High serum 5-HT may serve as a potential forensic biomarker in autopsied infants with SIDS with serotonergic defects., Competing Interests: The authors declare no conflict of interest.

Published

2017

198. In Vivo and protease-activated receptor-1-mediated platelet activation in patients presenting for cardiac catheterization.

Author

Gremmel T, Michelson AD, and Frelinger AL 3rd

Subjects

Acute Coronary Syndrome diagnosis, Acute Coronary Syndrome metabolism, Acute Coronary Syndrome therapy, Aged, Biomarkers, Blood Platelets drug effects, Comorbidity, Coronary Angiography, Coronary Artery Disease diagnosis, Coronary Artery Disease metabolism, Coronary Artery Disease therapy, Female, Humans, Male, Middle Aged, Monocytes metabolism, Odds Ratio, P-Selectin metabolism, Platelet Aggregation drug effects, Platelet Glycoprotein GPIIb-IIIa Complex metabolism, Platelet Membrane Glycoproteins metabolism, ROC Curve, Receptors, Thrombin therapeutic use, Blood Platelets metabolism, Cardiac Catheterization adverse effects, Platelet Activation drug effects, Receptor, PAR-1 metabolism

Abstract

Pathways of platelet activation that are not targeted by current antithrombotic therapy may be crucial for the development of ischemic events in patients undergoing coronary angiography. We therefore investigated whether in vivo and thrombin receptor activating peptide (TRAP)-stimulated platelet activation and monocyte-platelet aggregate (MPA) levels can serve as independent risk markers for adverse outcomes in aspirin-treated patients presenting for cardiac catheterization. In vivo and TRAP-stimulated platelet surface P-selectin, activated glycoprotein IIb/IIIa (GPIIb/IIIa) and MPA levels were determined in 682 consecutive patients undergoing cardiac catheterization and in 47 healthy controls. Two-year follow-up data were obtained from 562 patients. In vivo platelet surface P-selectin, activated GPIIb/IIIa and MPA levels were significantly higher in patients with angiographically-proven coronary artery disease than in healthy controls (all p≤0.02). Patients with an acute coronary syndrome (ACS; n=125) had significantly higher levels of in vivo MPA than patients without ACS (n=437; p=0.01). In the overall study population (n=562) the surface expression of P-selectin and activated GPIIb/IIIa, and the levels of MPA in vivo and in response to TRAP were similar in patients without and with subsequent ischemic events (all p>0.05). Similar results were obtained when only patients with angiographically-proven coronary artery disease (n=459), stent implantation (n=205) or ACS (n=125) were analyzed. Receiver-operating characteristic curve analyses did not reveal cut-off values for P-selectin, activated GPIIb/IIIa, and MPA levels for the prediction of ischemic events. In conclusion, in vivo and TRAP-stimulated platelet activation and MPA levels did not predict adverse ischemic outcomes in aspirin-treated patients presenting for cardiac catheterization.

Published

2016

199. Platelet Physiology.

Author

Gremmel T, Frelinger AL 3rd, and Michelson AD

Subjects

Blood Platelets metabolism, Hemostasis physiology, Humans, Models, Biological, Platelet Membrane Glycoproteins metabolism, Signal Transduction physiology, Thrombosis physiopathology, Blood Platelets physiology, Platelet Activation physiology, Platelet Adhesiveness physiology, Platelet Aggregation physiology

Abstract

Platelets are the smallest blood cells, numbering 150 to 350 × 10(9)/L in healthy individuals. The ability of activated platelets to adhere to an injured vessel wall and form aggregates was first described in the 19th century. Besides their long-established roles in thrombosis and hemostasis, platelets are increasingly recognized as pivotal players in numerous other pathophysiological processes including inflammation and atherogenesis, antimicrobial host defense, and tumor growth and metastasis. Consequently, profound knowledge of platelet structure and function is becoming more important in research and in many fields of modern medicine. This review provides an overview of platelet physiology focusing particularly on the structure, granules, surface glycoproteins, and activation pathways of platelets., (Thieme Medical Publishers 333 Seventh Avenue, New York, NY 10001, USA.)

Published

2016

200. Synergistic Inhibition of Both P2Y1 and P2Y12 Adenosine Diphosphate Receptors As Novel Approach to Rapidly Attenuate Platelet-Mediated Thrombosis.

Author

Gremmel T, Yanachkov IB, Yanachkova MI, Wright GE, Wider J, Undyala VV, Michelson AD, Frelinger AL 3rd, and Przyklenk K

Subjects

Adenosine Diphosphate analogs & derivatives, Adenosine Diphosphate pharmacology, Adenosine Monophosphate analogs & derivatives, Adenosine Monophosphate pharmacology, Adult, Animals, Aspirin pharmacology, Blood Coagulation drug effects, Blood Platelets metabolism, Coronary Thrombosis blood, Disease Models, Animal, Dogs, Dose-Response Relationship, Drug, Female, Humans, Male, Platelet Function Tests, Rats, Sprague-Dawley, Receptors, Purinergic P2Y1 blood, Receptors, Purinergic P2Y12 blood, Time Factors, Young Adult, Blood Platelets drug effects, Coronary Thrombosis drug therapy, Dinucleoside Phosphates pharmacology, Fibrinolytic Agents pharmacology, Platelet Aggregation drug effects, Platelet Aggregation Inhibitors pharmacology, Purinergic P2Y Receptor Antagonists pharmacology, Receptors, Purinergic P2Y1 drug effects, Receptors, Purinergic P2Y12 drug effects

Abstract

Objective: Unlike currently approved adenosine diphosphate receptor antagonists, the new diadenosine tetraphosphate derivative GLS-409 targets not only P2Y12 but also the second human platelet adenosine diphosphate receptor P2Y1 and may, therefore, be a promising antiplatelet drug candidate. The current study is the first to investigate the in vivo antithrombotic effects of GLS-409., Approach and Results: We studied (1) the in vivo effects of GLS-409 on agonist-stimulated platelet aggregation in anesthetized rats, (2) the antithrombotic activity of GLS-409 and the associated effect on the bleeding time in a canine model of platelet-mediated coronary artery thrombosis, and (3) the inhibition of agonist-stimulated platelet aggregation by GLS-409 versus selective P2Y1 and P2Y12 inhibition in vitro in samples from healthy human subjects before and 2 hours after aspirin intake. In vivo treatment with GLS-409 significantly inhibited adenosine diphosphate- and collagen-stimulated platelet aggregation in rats. Further, GLS-409 attenuated cyclic flow variation, that is, platelet-mediated thrombosis, in vivo in our canine model of unstable angina. The improvement in coronary patency was accompanied by a nonsignificant 30% increase in bleeding time. Of note, GLS-409 exerted its effects without affecting rat and canine hemodynamics. Finally, in vitro treatment with GLS-409 showed effects similar to that of cangrelor and the combination of cangrelor with the selective P2Y1 inhibitor MRS 2179 on agonist-stimulated platelet aggregation in human platelet-rich plasma and whole blood before and 2 hours after aspirin intake., Conclusions: Synergistic inhibition of both P2Y1 and P2Y12 adenosine diphosphate receptors by GLS-409 immediately attenuates platelet-mediated thrombosis and effectively blocks agonist-stimulated platelet aggregation irrespective of concomitant aspirin therapy., (© 2016 American Heart Association, Inc.)

Published

2016