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Measurement of platelet aggregation functions using whole blood migration ratio in a microfluidic chip

Authors
Seo, Hong SeogChoi, Sung HyukHan, MiranKim, Kyeong AhCho, Chi HyunAn, Seong Soo A.Lim, Chae SeungShin, Sehyun
Issue Date
2016
Publisher
IOS PRESS
Keywords
Platelet; ADP; Collagen; PFA-100
Citation
CLINICAL HEMORHEOLOGY AND MICROCIRCULATION, v.62, no.2, pp.151 - 163
Journal Title
CLINICAL HEMORHEOLOGY AND MICROCIRCULATION
Volume
62
Number
2
Start Page
151
End Page
163
URI
https://scholarworks.bwise.kr/gachon/handle/2020.sw.gachon/9684
DOI
10.3233/CH-151961
ISSN
1386-0291
Abstract
Platelets play a major role in maintaining endothelial integrity and hemostasis. Of the various soluble agonists, ADP is an important in vivo stimulus for inducing platelet aggregation. In this study, a simple, rapid, and affordable method was designed for testing bleeding time (BT) and platelet aggregation with a two-channel microfluidic chip. Whole blood migration ratio (MR) from a microchip system was evaluated in comparison to the closure time (CT) from PFA-100 assays (Siemens, Germany) and CD62P expression on platelets. To induce platelet aggregation, a combination of collagen (1.84 mg/ml) and ADP (37.5 mg/ml) were used as agonists. After adding the agonists to samples, whole blood MR from the microchip system was measured. The outcome of the assessment depended on reaction time and agonist concentration. MR of whole blood from the microchip system was significantly correlated with CT from PFA-100 (r = 0.61, p < 0.05, n = 60). In addition, MR was negatively correlated with CD62P expression (r =-0.95, p < 0.05, n = 60). These results suggest that the measurement of MR using agonists is an easy, simple and efficient method for monitoring platelet aggregation in normal and ADP-receptors defective samples, along with the BT test. Thus, usage of the current microfluidic method could expand to diverse applications, including efficacy assessments in platelet therapy.
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