Using six-colour flow cytometry to analyse the activation and interaction of platelets and leukocytes – A new assay suitable for bench and bedside conditions

Abstract Introduction Platelets are main effector cells in haemostasis and also promote inflammation. Platelet-leukocyte complexes are key mediators in a variety of thromboinflammatory disorders and consecutive organ failure. Cell-specific epitopes and activation markers on platelets and leukocytes...

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Veröffentlicht in:Thrombosis research 2015-10, Vol.136 (4), p.786-796
Hauptverfasser: Granja, Tiago, Schad, Jessica, Schüssel, Patricia, Fischer, Claudius, Häberle, Helene, Rosenberger, Peter, Straub, Andreas
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container_end_page 796
container_issue 4
container_start_page 786
container_title Thrombosis research
container_volume 136
creator Granja, Tiago
Schad, Jessica
Schüssel, Patricia
Fischer, Claudius
Häberle, Helene
Rosenberger, Peter
Straub, Andreas
description Abstract Introduction Platelets are main effector cells in haemostasis and also promote inflammation. Platelet-leukocyte complexes are key mediators in a variety of thromboinflammatory disorders and consecutive organ failure. Cell-specific epitopes and activation markers on platelets and leukocytes can be measured using flow cytometry. However, until recently a major restriction has been a paucity in antibody combinations and lack of detection strategies. We aimed to develop a six-colour flow cytometry method which depicts multiple aspects of platelet and leukocyte interactions in human whole blood. Materials and Methods Platelets, including microparticles and aggregates, were detected in flow cytometry using a platelet-specific anti-CD41-FITC antibody and size-defined regions. The morphology of platelet-leukocyte complexes (including granulocyte and monocyte content) were depicted using anti-CD45-PerCP, anti-CD66b-PE-Cy7, and anti-CD14-APC antibodies in a single sample. Expression of platelet and leukocyte activation markers P-selectin and CD11b were detected using anti-CD62P-PE and anti-CD11b-BV421 antibodies, respectively. Results The sensitivity of this assay to detect the effects of various agonists (TRAP-6, ADP, collagen, epinephrine, TNF-α and LPS) is demonstrated. Furthermore, the assay is shown to detect platelet and leukocyte activation induced by extracorporeal circulation in vitro. The suitability of this assay for bedside analysis is demonstrated exemplarily in a patient treated with mechanical circulatory life support. Conclusions Using the concurrent assessment of multiple parameters, this method gives detailed insights into the complexity and dynamics of platelet-leukocyte interactions. This assay carries the potential to increase our understanding of the mechanisms and pathophysiology of platelet-leukocyte interaction in the research laboratory and clinical setting.
doi_str_mv 10.1016/j.thromres.2015.07.009
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Platelet-leukocyte complexes are key mediators in a variety of thromboinflammatory disorders and consecutive organ failure. Cell-specific epitopes and activation markers on platelets and leukocytes can be measured using flow cytometry. However, until recently a major restriction has been a paucity in antibody combinations and lack of detection strategies. We aimed to develop a six-colour flow cytometry method which depicts multiple aspects of platelet and leukocyte interactions in human whole blood. Materials and Methods Platelets, including microparticles and aggregates, were detected in flow cytometry using a platelet-specific anti-CD41-FITC antibody and size-defined regions. The morphology of platelet-leukocyte complexes (including granulocyte and monocyte content) were depicted using anti-CD45-PerCP, anti-CD66b-PE-Cy7, and anti-CD14-APC antibodies in a single sample. Expression of platelet and leukocyte activation markers P-selectin and CD11b were detected using anti-CD62P-PE and anti-CD11b-BV421 antibodies, respectively. Results The sensitivity of this assay to detect the effects of various agonists (TRAP-6, ADP, collagen, epinephrine, TNF-α and LPS) is demonstrated. Furthermore, the assay is shown to detect platelet and leukocyte activation induced by extracorporeal circulation in vitro. The suitability of this assay for bedside analysis is demonstrated exemplarily in a patient treated with mechanical circulatory life support. Conclusions Using the concurrent assessment of multiple parameters, this method gives detailed insights into the complexity and dynamics of platelet-leukocyte interactions. 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Platelet-leukocyte complexes are key mediators in a variety of thromboinflammatory disorders and consecutive organ failure. Cell-specific epitopes and activation markers on platelets and leukocytes can be measured using flow cytometry. However, until recently a major restriction has been a paucity in antibody combinations and lack of detection strategies. We aimed to develop a six-colour flow cytometry method which depicts multiple aspects of platelet and leukocyte interactions in human whole blood. Materials and Methods Platelets, including microparticles and aggregates, were detected in flow cytometry using a platelet-specific anti-CD41-FITC antibody and size-defined regions. The morphology of platelet-leukocyte complexes (including granulocyte and monocyte content) were depicted using anti-CD45-PerCP, anti-CD66b-PE-Cy7, and anti-CD14-APC antibodies in a single sample. Expression of platelet and leukocyte activation markers P-selectin and CD11b were detected using anti-CD62P-PE and anti-CD11b-BV421 antibodies, respectively. Results The sensitivity of this assay to detect the effects of various agonists (TRAP-6, ADP, collagen, epinephrine, TNF-α and LPS) is demonstrated. Furthermore, the assay is shown to detect platelet and leukocyte activation induced by extracorporeal circulation in vitro. The suitability of this assay for bedside analysis is demonstrated exemplarily in a patient treated with mechanical circulatory life support. Conclusions Using the concurrent assessment of multiple parameters, this method gives detailed insights into the complexity and dynamics of platelet-leukocyte interactions. This assay carries the potential to increase our understanding of the mechanisms and pathophysiology of platelet-leukocyte interaction in the research laboratory and clinical setting.</description><subject>20.130: Inflammation, leukocytes, and thrombosis</subject><subject>20.190: Platelets</subject><subject>20.210: Platelet agonists and adhesion receptors</subject><subject>20: Platelets and Cell Biology</subject><subject>Color</subject><subject>Flow Cytometry - methods</subject><subject>Hematology, Oncology and Palliative Medicine</subject><subject>Humans</subject><subject>Leukocytes - metabolism</subject><subject>Platelet Activation - physiology</subject><subject>Platelet Aggregation - physiology</subject><issn>0049-3848</issn><issn>1879-2472</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2015</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNqFks9u1DAQxiMEoqXwCpWPXLLYSRzbF0RVlT9SJQ5QiZvl2LOst9548TgtufEOPADvxpPgdFsOXDjZHn_zjWZ-U1WnjK4YZf2r7SpvUtwlwFVDGV9RsaJUPaqOmRSqbjrRPK6OKe1U3cpOHlXPELeUMsEUf1odNX0jy707rn5doR-_EvTfaxtDnBJZh3hL7JzjDnKaSY7EjCbMCCRvgBib_Y3JPo4l7IgfM6QlVt5xTfbBZAiQ8e4zwHQdixMg-f3jJzkjI9wSg2hmgpPPZghA1jGRAUa7ucsYwKF3QGwcnV9M8Xn1ZG0Cwov786S6envx-fx9ffnx3Yfzs8vadqrNtaGD6cAO0vVdSxunLBfQMmaU4aprpeVcGQMCeGeNA2mEBCOcbHsKTkrRnlQvD777FL9NgFnvPFoIwYwQJ9RlWrznSommSPuD1KaImGCt98nvTJo1o3qBo7f6AY5e4GgqdIFTEk_va0zDDtzftAcaRfDmIIDS6Y2HpNH6MhxwPoHN2kX__xqv_7GwwY_emnANM-C2EC40Sz8aG031p2VFlg1hvKWUyy_tH8envl0</recordid><startdate>20151001</startdate><enddate>20151001</enddate><creator>Granja, Tiago</creator><creator>Schad, Jessica</creator><creator>Schüssel, Patricia</creator><creator>Fischer, Claudius</creator><creator>Häberle, Helene</creator><creator>Rosenberger, Peter</creator><creator>Straub, Andreas</creator><general>Elsevier Ltd</general><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>7X8</scope><orcidid>https://orcid.org/0000-0002-8137-1449</orcidid></search><sort><creationdate>20151001</creationdate><title>Using six-colour flow cytometry to analyse the activation and interaction of platelets and leukocytes – A new assay suitable for bench and bedside conditions</title><author>Granja, Tiago ; Schad, Jessica ; Schüssel, Patricia ; Fischer, Claudius ; Häberle, Helene ; Rosenberger, Peter ; Straub, Andreas</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c493t-a0ba4ecb8d64302d9c57e311a9a59438c559aae7e54cade8a78ea7d8360ed8873</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2015</creationdate><topic>20.130: Inflammation, leukocytes, and thrombosis</topic><topic>20.190: Platelets</topic><topic>20.210: Platelet agonists and adhesion receptors</topic><topic>20: Platelets and Cell Biology</topic><topic>Color</topic><topic>Flow Cytometry - methods</topic><topic>Hematology, Oncology and Palliative Medicine</topic><topic>Humans</topic><topic>Leukocytes - metabolism</topic><topic>Platelet Activation - physiology</topic><topic>Platelet Aggregation - physiology</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Granja, Tiago</creatorcontrib><creatorcontrib>Schad, Jessica</creatorcontrib><creatorcontrib>Schüssel, Patricia</creatorcontrib><creatorcontrib>Fischer, Claudius</creatorcontrib><creatorcontrib>Häberle, Helene</creatorcontrib><creatorcontrib>Rosenberger, Peter</creatorcontrib><creatorcontrib>Straub, Andreas</creatorcontrib><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>CrossRef</collection><collection>MEDLINE - Academic</collection><jtitle>Thrombosis research</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Granja, Tiago</au><au>Schad, Jessica</au><au>Schüssel, Patricia</au><au>Fischer, Claudius</au><au>Häberle, Helene</au><au>Rosenberger, Peter</au><au>Straub, Andreas</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Using six-colour flow cytometry to analyse the activation and interaction of platelets and leukocytes – A new assay suitable for bench and bedside conditions</atitle><jtitle>Thrombosis research</jtitle><addtitle>Thromb Res</addtitle><date>2015-10-01</date><risdate>2015</risdate><volume>136</volume><issue>4</issue><spage>786</spage><epage>796</epage><pages>786-796</pages><issn>0049-3848</issn><eissn>1879-2472</eissn><abstract>Abstract Introduction Platelets are main effector cells in haemostasis and also promote inflammation. Platelet-leukocyte complexes are key mediators in a variety of thromboinflammatory disorders and consecutive organ failure. Cell-specific epitopes and activation markers on platelets and leukocytes can be measured using flow cytometry. However, until recently a major restriction has been a paucity in antibody combinations and lack of detection strategies. We aimed to develop a six-colour flow cytometry method which depicts multiple aspects of platelet and leukocyte interactions in human whole blood. Materials and Methods Platelets, including microparticles and aggregates, were detected in flow cytometry using a platelet-specific anti-CD41-FITC antibody and size-defined regions. The morphology of platelet-leukocyte complexes (including granulocyte and monocyte content) were depicted using anti-CD45-PerCP, anti-CD66b-PE-Cy7, and anti-CD14-APC antibodies in a single sample. Expression of platelet and leukocyte activation markers P-selectin and CD11b were detected using anti-CD62P-PE and anti-CD11b-BV421 antibodies, respectively. Results The sensitivity of this assay to detect the effects of various agonists (TRAP-6, ADP, collagen, epinephrine, TNF-α and LPS) is demonstrated. Furthermore, the assay is shown to detect platelet and leukocyte activation induced by extracorporeal circulation in vitro. The suitability of this assay for bedside analysis is demonstrated exemplarily in a patient treated with mechanical circulatory life support. Conclusions Using the concurrent assessment of multiple parameters, this method gives detailed insights into the complexity and dynamics of platelet-leukocyte interactions. 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subjects 20.130: Inflammation, leukocytes, and thrombosis
20.190: Platelets
20.210: Platelet agonists and adhesion receptors
20: Platelets and Cell Biology
Color
Flow Cytometry - methods
Hematology, Oncology and Palliative Medicine
Humans
Leukocytes - metabolism
Platelet Activation - physiology
Platelet Aggregation - physiology
title Using six-colour flow cytometry to analyse the activation and interaction of platelets and leukocytes – A new assay suitable for bench and bedside conditions
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