Publication year
2012Source
Thrombosis Research, 130, 1, (2012), pp. 92-8ISSN
Annotation
01 juli 2012
Publication type
Article / Letter to editor
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Organization
Laboratory of Hematology
Haematology
Cardiology
Journal title
Thrombosis Research
Volume
vol. 130
Issue
iss. 1
Page start
p. 92
Page end
p. 8
Subject
N4i 2: Invasive mycoses and compromised host ONCOL 3: Translational research; NCEBP 14: Cardiovascular diseases; Laboratory Medicine - Radboud University Medical CenterAbstract
INTRODUCTION: Flow cytometry allows the analysis of multiple antigens in a single tube at a single cell level. We present a rapid and sensitive two tube flow cytometric protocol for the detection of multiple platelet antigens and activation markers gated on a pure platelet population. MATERIALS AND METHODS: The presence of platelet specific antigens was analyzed in citrated whole blood of normal platelets and from patients diagnosed with platelet abnormalities. Quiescent platelets as well as stimulated platelets were analyzed using a gating strategy based on ubiquitously expressed platelet membrane markers. A ubiquitously expressed platelet marker was combined with antibodies against the activated alpha2b-beta3 (PAC-1), Lysosomal Activated Membrane Protein (CD63) and P-selectin (CD62P). RESULTS: We were able to detect the platelet antigens CD36, CD41, CD42a, CD42b and CD61 in one single tube. Our approach allowed the single tube determination of PAC-1, CD63 and CD62P after activation of platelets by thrombin, collagen, ADP and PAR-1, and determination of platelet abnormalities. CONCLUSIONS: Our two tube multi-parameter screening protocol is suited for the analysis of platelet antigens expressed on quiescent and activated platelets and allows the detection of aberrancies as found in blood of patients with thrombocytopathy such as Glanzmann Thrombasthenia, storage pool disease with diminished granule content and patients treated with clopidogrel and acetylsalicylic acid.
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- Faculty of Medical Sciences [92811]
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