Effects of ex vivo blood anticoagulation and preanalytical processing time on the proteome content of platelets

Samuel Tassi Yunga; Austin J. Gower; Alexander R. Melrose; Meghan K. Fitzgerald; Ashmitha Rajendran; Theresa A. Lusardi; Randall J. Armstrong; Jessica Minnier; Kelley R. Jordan; Owen J.T. McCarty; Larry L. David; Phillip A. Wilmarth; Ashok P. Reddy; Joseph E. Aslan

doi:10.1111/jth.15694

Effects of ex vivo blood anticoagulation and preanalytical processing time on the proteome content of platelets

Samuel Tassi Yunga, Austin J. Gower, Alexander R. Melrose, Meghan K. Fitzgerald, Ashmitha Rajendran, Theresa A. Lusardi, Randall J. Armstrong, Jessica Minnier, Kelley R. Jordan, Owen J.T. McCarty, Larry L. David, Phillip A. Wilmarth, Ashok P. Reddy, Joseph E. Aslan

Research output: Contribution to journal › Article › peer-review

12 Scopus citations

Abstract

Background: Ex vivo assays of platelet function critically inform mechanistic and clinical hematology studies, where effects of divergent blood processing methods on platelet composition are apparent, but unspecified. Objective: Here, we evaluate how different blood anticoagulation options and processing times affect platelet function and protein content ex vivo. Methods: Parallel blood samples were collected from healthy human donors into sodium citrate, acid citrate dextrose, EDTA or heparin, and processed over an extended time course for functional and biochemical experiments, including platelet proteome quantification with multiplexed tandem mass tag (TMT) labeling and triple quadrupole mass spectrometry (MS). Results: Each anticoagulant had time-dependent effects on platelet function in whole blood. For instance, heparin enhanced platelet agonist reactivity, platelet-monocyte aggregate formation and platelet extracellular vesicle release, while EDTA increased platelet α-granule secretion. Following platelet isolation, TMT-MS quantified 3357 proteins amongst all prepared platelet samples. Altogether, >400 proteins were differentially abundant in platelets isolated from blood processed at 24 h versus 1 h post-phlebotomy, including proteins pertinent to membrane trafficking and exocytosis. Anticoagulant-specific effects on platelet proteomes included increased complement system and decreased α-granule proteins in platelets from EDTA-anticoagulated blood. Platelets prepared from heparinized blood had higher levels of histone and neutrophil-associated proteins in a manner related to neutrophil extracellular trap (NET) formation and platelet:NET interactions in whole blood ex vivo. Conclusion: Our results demonstrate that different anticoagulants routinely used for blood collection have varying effects on platelets ex vivo, where methodology-associated alterations in platelet proteome may influence mechanistic, translational and biomarker studies.

Original language	English (US)
Pages (from-to)	1437-1450
Number of pages	14
Journal	Journal of Thrombosis and Haemostasis
Volume	20
Issue number	6
DOIs	https://doi.org/10.1111/jth.15694
State	Published - Jun 2022

Keywords

anticoagulants
biomarkers
blood platelets
platelet function tests
proteomics

ASJC Scopus subject areas

Hematology

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10.1111/jth.15694

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Tassi Yunga, S., Gower, A. J., Melrose, A. R., Fitzgerald, M. K., Rajendran, A., Lusardi, T. A., Armstrong, R. J., Minnier, J., Jordan, K. R., McCarty, O. J. T., David, L. L., Wilmarth, P. A., Reddy, A. P., & Aslan, J. E. (2022). Effects of ex vivo blood anticoagulation and preanalytical processing time on the proteome content of platelets. Journal of Thrombosis and Haemostasis, 20(6), 1437-1450. https://doi.org/10.1111/jth.15694

Tassi Yunga, S, Gower, AJ, Melrose, AR, Fitzgerald, MK, Rajendran, A, Lusardi, TA, Armstrong, RJ, Minnier, J, Jordan, KR, McCarty, OJT , David, LL, Wilmarth, PA, Reddy, AP & Aslan, JE 2022, 'Effects of ex vivo blood anticoagulation and preanalytical processing time on the proteome content of platelets', Journal of Thrombosis and Haemostasis, vol. 20, no. 6, pp. 1437-1450. https://doi.org/10.1111/jth.15694

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title = "Effects of ex vivo blood anticoagulation and preanalytical processing time on the proteome content of platelets",

abstract = "Background: Ex vivo assays of platelet function critically inform mechanistic and clinical hematology studies, where effects of divergent blood processing methods on platelet composition are apparent, but unspecified. Objective: Here, we evaluate how different blood anticoagulation options and processing times affect platelet function and protein content ex vivo. Methods: Parallel blood samples were collected from healthy human donors into sodium citrate, acid citrate dextrose, EDTA or heparin, and processed over an extended time course for functional and biochemical experiments, including platelet proteome quantification with multiplexed tandem mass tag (TMT) labeling and triple quadrupole mass spectrometry (MS). Results: Each anticoagulant had time-dependent effects on platelet function in whole blood. For instance, heparin enhanced platelet agonist reactivity, platelet-monocyte aggregate formation and platelet extracellular vesicle release, while EDTA increased platelet α-granule secretion. Following platelet isolation, TMT-MS quantified 3357 proteins amongst all prepared platelet samples. Altogether, >400 proteins were differentially abundant in platelets isolated from blood processed at 24 h versus 1 h post-phlebotomy, including proteins pertinent to membrane trafficking and exocytosis. Anticoagulant-specific effects on platelet proteomes included increased complement system and decreased α-granule proteins in platelets from EDTA-anticoagulated blood. Platelets prepared from heparinized blood had higher levels of histone and neutrophil-associated proteins in a manner related to neutrophil extracellular trap (NET) formation and platelet:NET interactions in whole blood ex vivo. Conclusion: Our results demonstrate that different anticoagulants routinely used for blood collection have varying effects on platelets ex vivo, where methodology-associated alterations in platelet proteome may influence mechanistic, translational and biomarker studies.",

keywords = "anticoagulants, biomarkers, blood platelets, platelet function tests, proteomics",

author = "{Tassi Yunga}, Samuel and Gower, {Austin J.} and Melrose, {Alexander R.} and Fitzgerald, {Meghan K.} and Ashmitha Rajendran and Lusardi, {Theresa A.} and Armstrong, {Randall J.} and Jessica Minnier and Jordan, {Kelley R.} and McCarty, {Owen J.T.} and David, {Larry L.} and Wilmarth, {Phillip A.} and Reddy, {Ashok P.} and Aslan, {Joseph E.}",

note = "Publisher Copyright: {\textcopyright} 2022 International Society on Thrombosis and Haemostasis.",

year = "2022",

month = jun,

doi = "10.1111/jth.15694",

language = "English (US)",

volume = "20",

pages = "1437--1450",

journal = "Journal of Thrombosis and Haemostasis",

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T1 - Effects of ex vivo blood anticoagulation and preanalytical processing time on the proteome content of platelets

AU - Tassi Yunga, Samuel

AU - Gower, Austin J.

AU - Melrose, Alexander R.

AU - Fitzgerald, Meghan K.

AU - Rajendran, Ashmitha

AU - Lusardi, Theresa A.

AU - Armstrong, Randall J.

AU - Minnier, Jessica

AU - Jordan, Kelley R.

AU - McCarty, Owen J.T.

AU - David, Larry L.

AU - Wilmarth, Phillip A.

AU - Reddy, Ashok P.

AU - Aslan, Joseph E.

PY - 2022/6

Y1 - 2022/6

N2 - Background: Ex vivo assays of platelet function critically inform mechanistic and clinical hematology studies, where effects of divergent blood processing methods on platelet composition are apparent, but unspecified. Objective: Here, we evaluate how different blood anticoagulation options and processing times affect platelet function and protein content ex vivo. Methods: Parallel blood samples were collected from healthy human donors into sodium citrate, acid citrate dextrose, EDTA or heparin, and processed over an extended time course for functional and biochemical experiments, including platelet proteome quantification with multiplexed tandem mass tag (TMT) labeling and triple quadrupole mass spectrometry (MS). Results: Each anticoagulant had time-dependent effects on platelet function in whole blood. For instance, heparin enhanced platelet agonist reactivity, platelet-monocyte aggregate formation and platelet extracellular vesicle release, while EDTA increased platelet α-granule secretion. Following platelet isolation, TMT-MS quantified 3357 proteins amongst all prepared platelet samples. Altogether, >400 proteins were differentially abundant in platelets isolated from blood processed at 24 h versus 1 h post-phlebotomy, including proteins pertinent to membrane trafficking and exocytosis. Anticoagulant-specific effects on platelet proteomes included increased complement system and decreased α-granule proteins in platelets from EDTA-anticoagulated blood. Platelets prepared from heparinized blood had higher levels of histone and neutrophil-associated proteins in a manner related to neutrophil extracellular trap (NET) formation and platelet:NET interactions in whole blood ex vivo. Conclusion: Our results demonstrate that different anticoagulants routinely used for blood collection have varying effects on platelets ex vivo, where methodology-associated alterations in platelet proteome may influence mechanistic, translational and biomarker studies.

AB - Background: Ex vivo assays of platelet function critically inform mechanistic and clinical hematology studies, where effects of divergent blood processing methods on platelet composition are apparent, but unspecified. Objective: Here, we evaluate how different blood anticoagulation options and processing times affect platelet function and protein content ex vivo. Methods: Parallel blood samples were collected from healthy human donors into sodium citrate, acid citrate dextrose, EDTA or heparin, and processed over an extended time course for functional and biochemical experiments, including platelet proteome quantification with multiplexed tandem mass tag (TMT) labeling and triple quadrupole mass spectrometry (MS). Results: Each anticoagulant had time-dependent effects on platelet function in whole blood. For instance, heparin enhanced platelet agonist reactivity, platelet-monocyte aggregate formation and platelet extracellular vesicle release, while EDTA increased platelet α-granule secretion. Following platelet isolation, TMT-MS quantified 3357 proteins amongst all prepared platelet samples. Altogether, >400 proteins were differentially abundant in platelets isolated from blood processed at 24 h versus 1 h post-phlebotomy, including proteins pertinent to membrane trafficking and exocytosis. Anticoagulant-specific effects on platelet proteomes included increased complement system and decreased α-granule proteins in platelets from EDTA-anticoagulated blood. Platelets prepared from heparinized blood had higher levels of histone and neutrophil-associated proteins in a manner related to neutrophil extracellular trap (NET) formation and platelet:NET interactions in whole blood ex vivo. Conclusion: Our results demonstrate that different anticoagulants routinely used for blood collection have varying effects on platelets ex vivo, where methodology-associated alterations in platelet proteome may influence mechanistic, translational and biomarker studies.

KW - anticoagulants

KW - biomarkers

KW - blood platelets

KW - platelet function tests

KW - proteomics

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JO - Journal of Thrombosis and Haemostasis

JF - Journal of Thrombosis and Haemostasis

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Effects of ex vivo blood anticoagulation and preanalytical processing time on the proteome content of platelets

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