Influence of Preparative Procedures on Assay of Platelet Function and Apparent Effects of Antiplatelet Agents

Previous studies have shown that anticoagulants alter platelet reactivity and the apparent effects of antiplatelet agents. This study was conducted to identify the impact of methods of preparation of blood samples on an assay of platelet function and the effects of antiplatelet agents. The activatio...

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Published inThe American journal of cardiology Vol. 100; no. 4; pp. 722 - 727
Main Authors Madsen, Nathaniel J., MD, Holmes, Chris E., MD, PhD, Serrano, Feliciano A., MD, Sobel, Burton E., MD, Schneider, David J., MD
Format Journal Article
LanguageEnglish
Published New York, NY Elsevier Inc 15.08.2007
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Abstract Previous studies have shown that anticoagulants alter platelet reactivity and the apparent effects of antiplatelet agents. This study was conducted to identify the impact of methods of preparation of blood samples on an assay of platelet function and the effects of antiplatelet agents. The activation of platelets was identified with the use of flow cytometry in response to thrombin (1 and 10 nmol/L), adenosine diphosphate (0.2 and 1 μmol/L), platelet activating factor (1 nmol/L), and convulxin (1 and 10 ng/ml). Antiplatelet effects were assessed after the addition in vitro of tirofiban (50 ng/ml) and cangrelor (10 nmol/L). Results were compared in whole blood and platelet-rich plasma (PRP) anticoagulated with corn trypsin inhibitor (32 μg/ml, a specific inhibitor of factor XIIa). The fraction of young platelets was quantified with thiazole orange, which identifies ribonucleic acid. The activation of platelets was consistently less in PRP compared with whole blood. Activation in PRP was 23 ± 15% that in whole blood for thrombin, 65 ± 26% for adenosine diphosphate, 40 ± 20% for platelet activating factor, and 49 ± 25% for convulxin (p <0.01 for each comparison). The fraction of young platelets in PRP was 39 ± 11% that in whole blood (p <0.001). The effects of antiplatelet agents varied with agonist and antiplatelet agent but were generally greater in PRP compared with whole blood (p <0.05). In conclusion, platelet reactivity is lower and the effects of antiplatelet agents are greater and potentially misleading in PRP compared with whole blood. The accuracy of platelet function testing may be improved by performance in whole blood.
AbstractList Previous studies have shown that anticoagulants alter platelet reactivity and the apparent effects of antiplatelet agents. This study was conducted to identify the impact of methods of preparation of blood samples on an assay of platelet function and the effects of antiplatelet agents. The activation of platelets was identified with the use of flow cytometry in response to thrombin (1 and 10 nmol/L), adenosine diphosphate (0.2 and 1 μmol/L), platelet activating factor (1 nmol/L), and convulxin (1 and 10 ng/ml). Antiplatelet effects were assessed after the addition in vitro of tirofiban (50 ng/ml) and cangrelor (10 nmol/L). Results were compared in whole blood and platelet-rich plasma (PRP) anticoagulated with corn trypsin inhibitor (32 μg/ml, a specific inhibitor of factor XIIa). The fraction of young platelets was quantified with thiazole orange, which identifies ribonucleic acid. The activation of platelets was consistently less in PRP compared with whole blood. Activation in PRP was 23 ± 15% that in whole blood for thrombin, 65 ± 26% for adenosine diphosphate, 40 ± 20% for platelet activating factor, and 49 ± 25% for convulxin (p <0.01 for each comparison). The fraction of young platelets in PRP was 39 ± 11% that in whole blood (p <0.001). The effects of antiplatelet agents varied with agonist and antiplatelet agent but were generally greater in PRP compared with whole blood (p <0.05). In conclusion, platelet reactivity is lower and the effects of antiplatelet agents are greater and potentially misleading in PRP compared with whole blood. The accuracy of platelet function testing may be improved by performance in whole blood.
Previous studies have shown that anticoagulants alter platelet reactivity and the apparent effects of antiplatelet agents. This study was conducted to identify the impact of methods of preparation of blood samples on an assay of platelet function and the effects of antiplatelet agents. The activation of platelets was identified with the use of flow cytometry in response to thrombin (1 and 10 nmol/L), adenosine diphosphate (0.2 and 1 micromol/L), platelet activating factor (1 nmol/L), and convulxin (1 and 10 ng/ml). Antiplatelet effects were assessed after the addition in vitro of tirofiban (50 ng/ml) and cangrelor (10 nmol/L). Results were compared in whole blood and platelet-rich plasma (PRP) anticoagulated with corn trypsin inhibitor (32 microg/ml, a specific inhibitor of factor XIIa). The fraction of young platelets was quantified with thiazole orange, which identifies ribonucleic acid. The activation of platelets was consistently less in PRP compared with whole blood. Activation in PRP was 23 +/- 15% that in whole blood for thrombin, 65 +/- 26% for adenosine diphosphate, 40 +/- 20% for platelet activating factor, and 49 +/- 25% for convulxin (p &lt;0.01 for each comparison). The fraction of young platelets in PRP was 39 +/- 11% that in whole blood (p &lt;0.001). The effects of antiplatelet agents varied with agonist and antiplatelet agent but were generally greater in PRP compared with whole blood (p &lt;0.05). In conclusion, platelet reactivity is lower and the effects of antiplatelet agents are greater and potentially misleading in PRP compared with whole blood. The accuracy of platelet function testing may be improved by performance in whole blood.
Previous studies have shown that anticoagulants alter platelet reactivity and the apparent effects of antiplatelet agents. This study was conducted to identify the impact of methods of preparation of blood samples on an assay of platelet function and the effects of antiplatelet agents. The activation of platelets was identified with the use of flow cytometry in response to thrombin (1 and 10 nmol/L), adenosine diphosphate (0.2 and 1 ...mol/L), platelet activating factor (1 nmol/L), and convulxin (1 and 10 ng/ml). Antiplatelet effects were assessed after the addition in vitro of tirofiban (50 ng/ml) and cangrelor (10 nmol/L). Results were compared in whole blood and platelet-rich plasma (PRP) anticoagulated with corn trypsin inhibitor (32 ...g/ml, a specific inhibitor of factor XIIa). The fraction of young platelets was quantified with thiazole orange, which identifies ribonucleic acid. The activation of platelets was consistently less in PRP compared with whole blood. Activation in PRP was 23 ± 15% that in whole blood for thrombin, 65 ± 26% for adenosine diphosphate, 40 ± 20% for platelet activating factor, and 49 ± 25% for convulxin (p < 0.01 for each comparison). The fraction of young platelets in PRP was 39 ± 11% that in whole blood (p < 0.001). The effects of antiplatelet agents varied with agonist and antiplatelet agent but were generally greater in PRP compared with whole blood (p < 0.05). In conclusion, platelet reactivity is lower and the effects of antiplatelet agents are greater and potentially misleading in PRP compared with whole blood. The accuracy of platelet function testing may be improved by performance in whole blood. (ProQuest: ... denotes formulae/symbols omitted.)
Previous studies have shown that anticoagulants alter platelet reactivity and the apparent effects of antiplatelet agents. This study was conducted to identify the impact of methods of preparation of blood samples on an assay of platelet function and the effects of antiplatelet agents. The activation of platelets was identified with the use of flow cytometry in response to thrombin (1 and 10 nmol/L), adenosine diphosphate (0.2 and 1 micromol/L), platelet activating factor (1 nmol/L), and convulxin (1 and 10 ng/ml). Antiplatelet effects were assessed after the addition in vitro of tirofiban (50 ng/ml) and cangrelor (10 nmol/L). Results were compared in whole blood and platelet-rich plasma (PRP) anticoagulated with corn trypsin inhibitor (32 microg/ml, a specific inhibitor of factor XIIa). The fraction of young platelets was quantified with thiazole orange, which identifies ribonucleic acid. The activation of platelets was consistently less in PRP compared with whole blood. Activation in PRP was 23 +/- 15% that in whole blood for thrombin, 65 +/- 26% for adenosine diphosphate, 40 +/- 20% for platelet activating factor, and 49 +/- 25% for convulxin (p <0.01 for each comparison). The fraction of young platelets in PRP was 39 +/- 11% that in whole blood (p <0.001). The effects of antiplatelet agents varied with agonist and antiplatelet agent but were generally greater in PRP compared with whole blood (p <0.05). In conclusion, platelet reactivity is lower and the effects of antiplatelet agents are greater and potentially misleading in PRP compared with whole blood. The accuracy of platelet function testing may be improved by performance in whole blood.
Author Schneider, David J., MD
Sobel, Burton E., MD
Madsen, Nathaniel J., MD
Holmes, Chris E., MD, PhD
Serrano, Feliciano A., MD
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Keywords Assay
Platelet function
Procedure
Circulatory system
Cardiology
Phlebology
Antiplatelet agent
Language English
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Snippet Previous studies have shown that anticoagulants alter platelet reactivity and the apparent effects of antiplatelet agents. This study was conducted to identify...
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SubjectTerms Adenosine Diphosphate - pharmacology
Adenosine Monophosphate - analogs & derivatives
Adenosine Monophosphate - pharmacology
Benzothiazoles
Biological and medical sciences
Blood Platelets - drug effects
Blood Platelets - physiology
Cardiology. Vascular system
Cardiovascular
Coagulation
Comparative analysis
Coronary Disease - blood
Coronary Disease - drug therapy
Crotalid Venoms - pharmacology
Effects
Flow Cytometry
Fluorescent Dyes
Hemostatics - pharmacology
Humans
Lectins, C-Type
Leukocytes
Medical sciences
Plasma
Platelet Activating Factor - pharmacology
Platelet Activation - drug effects
Platelet Aggregation Inhibitors - pharmacology
Platelet Count
Platelet Glycoprotein GPIIb-IIIa Complex - antagonists & inhibitors
Quinolines
Studies
Thrombin - pharmacology
Tyrosine - analogs & derivatives
Tyrosine - pharmacology
Title Influence of Preparative Procedures on Assay of Platelet Function and Apparent Effects of Antiplatelet Agents
URI https://www.clinicalkey.es/playcontent/1-s2.0-S0002914907009666
https://dx.doi.org/10.1016/j.amjcard.2007.03.091
https://www.ncbi.nlm.nih.gov/pubmed/17697836
https://www.proquest.com/docview/230389306
https://search.proquest.com/docview/68169690
Volume 100
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