Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.

Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.

Microfluidic flow assays (MFA) that measure shear dependent platelet function have potential clinical applications in the diagnosis and treatment of bleeding and thrombotic disorders. As a step towards clinical application, the objective of this study was to measure how phenotypic and genetic factor...

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Main Authors: Keith B Neeves, Abimbola A Onasoga, Ryan R Hansen, Jessica J Lilly, Diana Venckunaite, Meghan B Sumner, Andrew T Irish, Gary Brodsky, Marilyn J Manco-Johnson, Jorge A Di Paola
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC3552855?pdf=render
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spelling doaj-50d4de22ce744995aa29005490b9542f2020-11-25T02:48:24ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-0181e5468010.1371/journal.pone.0054680Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.Keith B NeevesAbimbola A OnasogaRyan R HansenJessica J LillyDiana VenckunaiteMeghan B SumnerAndrew T IrishGary BrodskyMarilyn J Manco-JohnsonJorge A Di PaolaMicrofluidic flow assays (MFA) that measure shear dependent platelet function have potential clinical applications in the diagnosis and treatment of bleeding and thrombotic disorders. As a step towards clinical application, the objective of this study was to measure how phenotypic and genetic factors, as well as experimental conditions, affect the variability of platelet accumulation on type 1 collagen within a MFA. Whole blood was perfused over type 1 fibrillar collagen at wall shear rates of 150, 300, 750 and 1500 s⁻¹ through four independent channels with a height of 50 µm and a width of 500 µm. The accumulation of platelets was characterized by the lag time to 1% platelet surface coverage (Lag(T)), the rate of platelet accumulation (V(PLT)), and platelet surface coverage (SC). A cohort of normal donors was tested and the results were correlated to plasma von Willebrand factor (VWF) levels, platelet count, hematocrit, sex, and collagen receptors genotypes. VWF levels were the strongest determinant of platelet accumulation. VWF levels were positively correlated to V(PLT) and SC at all wall shear rates. A longer Lag(T) for platelet accumulation at arterial shear rates compared to venous shear rates was attributed to the time required for plasma proteins to adsorb to collagen. There was no association between platelet accumulation and hematocrit or platelet count. Individuals with the AG genotype of the GP6 gene had lower platelet accumulation than individuals with the AA genotype at 150 s⁻¹ and 300 s⁻¹. Recalcified blood collected into sodium citrate and corn trypsin inhibitor (CTI) resulted in diminished platelet accumulation compared to CTI alone, suggesting that citrate irreversibly diminishes platelet function. This study the largest association study of MFA in healthy donors (n = 104) and will likely set up the basis for the determination of the normal range of platelet responses in this type of assay.http://europepmc.org/articles/PMC3552855?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Keith B Neeves
Abimbola A Onasoga
Ryan R Hansen
Jessica J Lilly
Diana Venckunaite
Meghan B Sumner
Andrew T Irish
Gary Brodsky
Marilyn J Manco-Johnson
Jorge A Di Paola
spellingShingle Keith B Neeves
Abimbola A Onasoga
Ryan R Hansen
Jessica J Lilly
Diana Venckunaite
Meghan B Sumner
Andrew T Irish
Gary Brodsky
Marilyn J Manco-Johnson
Jorge A Di Paola
Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.
PLoS ONE
author_facet Keith B Neeves
Abimbola A Onasoga
Ryan R Hansen
Jessica J Lilly
Diana Venckunaite
Meghan B Sumner
Andrew T Irish
Gary Brodsky
Marilyn J Manco-Johnson
Jorge A Di Paola
author_sort Keith B Neeves
title Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.
title_short Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.
title_full Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.
title_fullStr Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.
title_full_unstemmed Sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.
title_sort sources of variability in platelet accumulation on type 1 fibrillar collagen in microfluidic flow assays.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description Microfluidic flow assays (MFA) that measure shear dependent platelet function have potential clinical applications in the diagnosis and treatment of bleeding and thrombotic disorders. As a step towards clinical application, the objective of this study was to measure how phenotypic and genetic factors, as well as experimental conditions, affect the variability of platelet accumulation on type 1 collagen within a MFA. Whole blood was perfused over type 1 fibrillar collagen at wall shear rates of 150, 300, 750 and 1500 s⁻¹ through four independent channels with a height of 50 µm and a width of 500 µm. The accumulation of platelets was characterized by the lag time to 1% platelet surface coverage (Lag(T)), the rate of platelet accumulation (V(PLT)), and platelet surface coverage (SC). A cohort of normal donors was tested and the results were correlated to plasma von Willebrand factor (VWF) levels, platelet count, hematocrit, sex, and collagen receptors genotypes. VWF levels were the strongest determinant of platelet accumulation. VWF levels were positively correlated to V(PLT) and SC at all wall shear rates. A longer Lag(T) for platelet accumulation at arterial shear rates compared to venous shear rates was attributed to the time required for plasma proteins to adsorb to collagen. There was no association between platelet accumulation and hematocrit or platelet count. Individuals with the AG genotype of the GP6 gene had lower platelet accumulation than individuals with the AA genotype at 150 s⁻¹ and 300 s⁻¹. Recalcified blood collected into sodium citrate and corn trypsin inhibitor (CTI) resulted in diminished platelet accumulation compared to CTI alone, suggesting that citrate irreversibly diminishes platelet function. This study the largest association study of MFA in healthy donors (n = 104) and will likely set up the basis for the determination of the normal range of platelet responses in this type of assay.
url http://europepmc.org/articles/PMC3552855?pdf=render
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