Comparative Analysis of Microfluidics Thrombus Formation in Multiple Genetically Modified Mice: Link to Thrombosis and Hemostasis

Magdolna Nagy; Johanna P. van Geffen; David Stegner; David J. Adams; Attila Braun; Susanne M. de Witt; Margitta Elvers; Mitchell J. Geer; Marijke J. E. Kuijpers; Karl Kunzelmann; Jun Mori; Ccile Oury; Joachim Pircher; Irina Pleines; Alastair W. Poole; Yotis A. Senis; Remco Verdoold; Christian Weber; Bernhard Nieswandt; Johan W. M. Heemskerk; Constance C. F. M. J. Baaten

doi:10.3389/fcvm.2019.00099

Comparative Analysis of Microfluidics Thrombus Formation in Multiple Genetically Modified Mice: Link to Thrombosis and Hemostasis

Magdolna Nagy, Johanna P. van Geffen, David Stegner, David J. Adams, Attila Braun, Susanne M. de Witt, Margitta Elvers, Mitchell J. Geer, Marijke J. E. Kuijpers, Karl Kunzelmann, Jun Mori, Ccile Oury, Joachim Pircher, Irina Pleines, Alastair W. Poole, Yotis A. Senis, Remco Verdoold, Christian Weber, Bernhard Nieswandt, Johan W. M. Heemskerk^*Constance C. F. M. J. Baaten^*

^*Corresponding author for this work

Research output: Contribution to journal › Article › Academic › peer-review

Abstract

Genetically modified mice are indispensable for establishing the roles of platelets in arterial thrombosis and hemostasis. Microfluidics assays using anticoagulated whole blood are commonly used as integrative proxy tests for platelet function in mice. In the present study, we quantified the changes in collagen-dependent thrombus formation for 38 different strains of (genetically) modified mice, all measured with the same microfluidics chamber. The mice included were deficient in platelet receptors, protein kinases or phosphatases, small GTPases or other signaling or scaffold proteins. By standardized re-analysis of high-resolution microscopic images, detailed information was obtained on altered platelet adhesion, aggregation and/or activation. For a subset of 11 mouse strains, these platelet functions were further evaluated in rhodocytin- and laminin-dependent thrombus formation, thus allowing a comparison of glycoprotein VI (GPVI), C-type lectin-like receptor 2 (CLEC2) and integrin alpha(6)beta(1) pathways. High homogeneity was found between wild-type mice datasets concerning adhesion and aggregation parameters. Quantitative comparison for the 38 modified mouse strains resulted in a matrix visualizing the impact of the respective (genetic) deficiency on thrombus formation with detailed insight into the type and extent of altered thrombus signatures. Network analysis revealed strong clusters of genes involved in GPVI signaling and Ca2+ homeostasis. The majority of mice demonstrating an antithrombotic phenotype in vivo displayed with a larger or smaller reduction in multi-parameter analysis of collagen-dependent thrombus formation in vitro. Remarkably, in only approximately half of the mouse strains that displayed reduced arterial thrombosis in vivo, this was accompanied by impaired hemostasis. This was also reflected by comparing in vitro thrombus formation (by microfluidics) with alterations in in vivo bleeding time. In conclusion, the presently developed multi-parameter analysis of thrombus formation using microfluidics can be used to: (i) determine the severity of platelet abnormalities; (ii) distinguish between altered platelet adhesion, aggregation and activation; and (iii) elucidate both collagen and non-collagen dependent alterations of thrombus formation. This approach may thereby aid in the better understanding and better assessment of genetic variation that affect in vivo arterial thrombosis and hemostasis.

Original language	English
Article number	99
Number of pages	15
Journal	Frontiers in Cardiovascular Medicine
Volume	6
DOIs	https://doi.org/10.3389/fcvm.2019.00099
Publication status	Published - 30 Jul 2019

Keywords

arterial thrombus formation
bleeding
collagen
glycoprotein VI
platelets
microfluidics
DEFECTIVE PLATELET ACTIVATION
PROTEIN-INTERACTION NETWORKS
IN-VIVO DEPLETION
GLYCOPROTEIN-VI
ARTERIAL THROMBOSIS
ADHESION MECHANISMS
RECEPTOR CLEC-2
INTEGRIN
COLLAGEN
ROLES

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Nagy, M., van Geffen, J. P., Stegner, D., Adams, D. J., Braun, A., de Witt, S. M., Elvers, M., Geer, M. J., Kuijpers, M. J. E., Kunzelmann, K., Mori, J., Oury, C., Pircher, J., Pleines, I., Poole, A. W., Senis, Y. A., Verdoold, R., Weber, C., Nieswandt, B., ... Baaten, C. C. F. M. J. (2019). Comparative Analysis of Microfluidics Thrombus Formation in Multiple Genetically Modified Mice: Link to Thrombosis and Hemostasis. Frontiers in Cardiovascular Medicine, 6, Article 99. https://doi.org/10.3389/fcvm.2019.00099

@article{2aad39025737416f99a51d5d1a3f80be,

title = "Comparative Analysis of Microfluidics Thrombus Formation in Multiple Genetically Modified Mice: Link to Thrombosis and Hemostasis",

abstract = "Genetically modified mice are indispensable for establishing the roles of platelets in arterial thrombosis and hemostasis. Microfluidics assays using anticoagulated whole blood are commonly used as integrative proxy tests for platelet function in mice. In the present study, we quantified the changes in collagen-dependent thrombus formation for 38 different strains of (genetically) modified mice, all measured with the same microfluidics chamber. The mice included were deficient in platelet receptors, protein kinases or phosphatases, small GTPases or other signaling or scaffold proteins. By standardized re-analysis of high-resolution microscopic images, detailed information was obtained on altered platelet adhesion, aggregation and/or activation. For a subset of 11 mouse strains, these platelet functions were further evaluated in rhodocytin- and laminin-dependent thrombus formation, thus allowing a comparison of glycoprotein VI (GPVI), C-type lectin-like receptor 2 (CLEC2) and integrin alpha(6)beta(1) pathways. High homogeneity was found between wild-type mice datasets concerning adhesion and aggregation parameters. Quantitative comparison for the 38 modified mouse strains resulted in a matrix visualizing the impact of the respective (genetic) deficiency on thrombus formation with detailed insight into the type and extent of altered thrombus signatures. Network analysis revealed strong clusters of genes involved in GPVI signaling and Ca2+ homeostasis. The majority of mice demonstrating an antithrombotic phenotype in vivo displayed with a larger or smaller reduction in multi-parameter analysis of collagen-dependent thrombus formation in vitro. Remarkably, in only approximately half of the mouse strains that displayed reduced arterial thrombosis in vivo, this was accompanied by impaired hemostasis. This was also reflected by comparing in vitro thrombus formation (by microfluidics) with alterations in in vivo bleeding time. In conclusion, the presently developed multi-parameter analysis of thrombus formation using microfluidics can be used to: (i) determine the severity of platelet abnormalities; (ii) distinguish between altered platelet adhesion, aggregation and activation; and (iii) elucidate both collagen and non-collagen dependent alterations of thrombus formation. This approach may thereby aid in the better understanding and better assessment of genetic variation that affect in vivo arterial thrombosis and hemostasis.",

keywords = "arterial thrombus formation, bleeding, collagen, glycoprotein VI, platelets, microfluidics, DEFECTIVE PLATELET ACTIVATION, PROTEIN-INTERACTION NETWORKS, IN-VIVO DEPLETION, GLYCOPROTEIN-VI, ARTERIAL THROMBOSIS, ADHESION MECHANISMS, RECEPTOR CLEC-2, INTEGRIN, COLLAGEN, ROLES",

author = "Magdolna Nagy and {van Geffen}, {Johanna P.} and David Stegner and Adams, {David J.} and Attila Braun and {de Witt}, {Susanne M.} and Margitta Elvers and Geer, {Mitchell J.} and Kuijpers, {Marijke J. E.} and Karl Kunzelmann and Jun Mori and Ccile Oury and Joachim Pircher and Irina Pleines and Poole, {Alastair W.} and Senis, {Yotis A.} and Remco Verdoold and Christian Weber and Bernhard Nieswandt and Heemskerk, {Johan W. M.} and Baaten, {Constance C. F. M. J.}",

note = "Funding Information: MN, MK, and JH have received funding from the Cardiovascular Centre (HVC) MUMC+ Maastricht, the Interreg V Euregio Meuse-Rhine program (Poly-Valve). DS, AB, IP, and BN were supported by the Deutsche Forschungsgemeinschaft (project-number 374031971 – TRR240). CO is Senior Research Associate at the Belgian Fund for Scientific Research (F.R.S.-FNRS). YS received founding from a BHF Fellowship (FS/13/1/29894 and a Programme Grant RG/15/13/31673. CB is supported by the Alexander von Humboldt Foundation. Funding Information: Funding. MN, MK, and JH have received funding from the Cardiovascular Centre (HVC) MUMC+ Maastricht, the Interreg V Euregio Meuse-Rhine program (Poly-Valve). DS, AB, IP, and BN were supported by the Deutsche Forschungsgemeinschaft (project-number 374031971 ? TRR240). CO is Senior Research Associate at the Belgian Fund for Scientific Research (F.R.S.-FNRS). YS received founding from a BHF Fellowship (FS/13/1/29894 and a Programme Grant RG/15/13/31673. CB is supported by the Alexander von Humboldt Foundation. Publisher Copyright: {\textcopyright} Copyright {\textcopyright} 2019 Nagy, van Geffen, Stegner, Adams, Braun, de Witt, Elvers, Geer, Kuijpers, Kunzelmann, Mori, Oury, Pircher, Pleines, Poole, Senis, Verdoold, Weber, Nieswandt, Heemskerk and Baaten.",

year = "2019",

month = jul,

day = "30",

doi = "10.3389/fcvm.2019.00099",

language = "English",

volume = "6",

journal = "Frontiers in Cardiovascular Medicine",

issn = "2297-055X",

publisher = "Frontiers Media S.A.",

}

Nagy, M, van Geffen, JP, Stegner, D, Adams, DJ, Braun, A, de Witt, SM, Elvers, M, Geer, MJ, Kuijpers, MJE, Kunzelmann, K, Mori, J, Oury, C, Pircher, J, Pleines, I, Poole, AW, Senis, YA, Verdoold, R, Weber, C, Nieswandt, B, Heemskerk, JWM & Baaten, CCFMJ 2019, 'Comparative Analysis of Microfluidics Thrombus Formation in Multiple Genetically Modified Mice: Link to Thrombosis and Hemostasis', Frontiers in Cardiovascular Medicine, vol. 6, 99. https://doi.org/10.3389/fcvm.2019.00099

TY - JOUR

T1 - Comparative Analysis of Microfluidics Thrombus Formation in Multiple Genetically Modified Mice

T2 - Link to Thrombosis and Hemostasis

AU - Nagy, Magdolna

AU - van Geffen, Johanna P.

AU - Stegner, David

AU - Adams, David J.

AU - Braun, Attila

AU - de Witt, Susanne M.

AU - Elvers, Margitta

AU - Geer, Mitchell J.

AU - Kuijpers, Marijke J. E.

AU - Kunzelmann, Karl

AU - Mori, Jun

AU - Oury, Ccile

AU - Pircher, Joachim

AU - Pleines, Irina

AU - Poole, Alastair W.

AU - Senis, Yotis A.

AU - Verdoold, Remco

AU - Weber, Christian

AU - Nieswandt, Bernhard

AU - Heemskerk, Johan W. M.

AU - Baaten, Constance C. F. M. J.

N1 - Funding Information: MN, MK, and JH have received funding from the Cardiovascular Centre (HVC) MUMC+ Maastricht, the Interreg V Euregio Meuse-Rhine program (Poly-Valve). DS, AB, IP, and BN were supported by the Deutsche Forschungsgemeinschaft (project-number 374031971 – TRR240). CO is Senior Research Associate at the Belgian Fund for Scientific Research (F.R.S.-FNRS). YS received founding from a BHF Fellowship (FS/13/1/29894 and a Programme Grant RG/15/13/31673. CB is supported by the Alexander von Humboldt Foundation. Funding Information: Funding. MN, MK, and JH have received funding from the Cardiovascular Centre (HVC) MUMC+ Maastricht, the Interreg V Euregio Meuse-Rhine program (Poly-Valve). DS, AB, IP, and BN were supported by the Deutsche Forschungsgemeinschaft (project-number 374031971 ? TRR240). CO is Senior Research Associate at the Belgian Fund for Scientific Research (F.R.S.-FNRS). YS received founding from a BHF Fellowship (FS/13/1/29894 and a Programme Grant RG/15/13/31673. CB is supported by the Alexander von Humboldt Foundation. Publisher Copyright: © Copyright © 2019 Nagy, van Geffen, Stegner, Adams, Braun, de Witt, Elvers, Geer, Kuijpers, Kunzelmann, Mori, Oury, Pircher, Pleines, Poole, Senis, Verdoold, Weber, Nieswandt, Heemskerk and Baaten.

PY - 2019/7/30

Y1 - 2019/7/30

N2 - Genetically modified mice are indispensable for establishing the roles of platelets in arterial thrombosis and hemostasis. Microfluidics assays using anticoagulated whole blood are commonly used as integrative proxy tests for platelet function in mice. In the present study, we quantified the changes in collagen-dependent thrombus formation for 38 different strains of (genetically) modified mice, all measured with the same microfluidics chamber. The mice included were deficient in platelet receptors, protein kinases or phosphatases, small GTPases or other signaling or scaffold proteins. By standardized re-analysis of high-resolution microscopic images, detailed information was obtained on altered platelet adhesion, aggregation and/or activation. For a subset of 11 mouse strains, these platelet functions were further evaluated in rhodocytin- and laminin-dependent thrombus formation, thus allowing a comparison of glycoprotein VI (GPVI), C-type lectin-like receptor 2 (CLEC2) and integrin alpha(6)beta(1) pathways. High homogeneity was found between wild-type mice datasets concerning adhesion and aggregation parameters. Quantitative comparison for the 38 modified mouse strains resulted in a matrix visualizing the impact of the respective (genetic) deficiency on thrombus formation with detailed insight into the type and extent of altered thrombus signatures. Network analysis revealed strong clusters of genes involved in GPVI signaling and Ca2+ homeostasis. The majority of mice demonstrating an antithrombotic phenotype in vivo displayed with a larger or smaller reduction in multi-parameter analysis of collagen-dependent thrombus formation in vitro. Remarkably, in only approximately half of the mouse strains that displayed reduced arterial thrombosis in vivo, this was accompanied by impaired hemostasis. This was also reflected by comparing in vitro thrombus formation (by microfluidics) with alterations in in vivo bleeding time. In conclusion, the presently developed multi-parameter analysis of thrombus formation using microfluidics can be used to: (i) determine the severity of platelet abnormalities; (ii) distinguish between altered platelet adhesion, aggregation and activation; and (iii) elucidate both collagen and non-collagen dependent alterations of thrombus formation. This approach may thereby aid in the better understanding and better assessment of genetic variation that affect in vivo arterial thrombosis and hemostasis.

AB - Genetically modified mice are indispensable for establishing the roles of platelets in arterial thrombosis and hemostasis. Microfluidics assays using anticoagulated whole blood are commonly used as integrative proxy tests for platelet function in mice. In the present study, we quantified the changes in collagen-dependent thrombus formation for 38 different strains of (genetically) modified mice, all measured with the same microfluidics chamber. The mice included were deficient in platelet receptors, protein kinases or phosphatases, small GTPases or other signaling or scaffold proteins. By standardized re-analysis of high-resolution microscopic images, detailed information was obtained on altered platelet adhesion, aggregation and/or activation. For a subset of 11 mouse strains, these platelet functions were further evaluated in rhodocytin- and laminin-dependent thrombus formation, thus allowing a comparison of glycoprotein VI (GPVI), C-type lectin-like receptor 2 (CLEC2) and integrin alpha(6)beta(1) pathways. High homogeneity was found between wild-type mice datasets concerning adhesion and aggregation parameters. Quantitative comparison for the 38 modified mouse strains resulted in a matrix visualizing the impact of the respective (genetic) deficiency on thrombus formation with detailed insight into the type and extent of altered thrombus signatures. Network analysis revealed strong clusters of genes involved in GPVI signaling and Ca2+ homeostasis. The majority of mice demonstrating an antithrombotic phenotype in vivo displayed with a larger or smaller reduction in multi-parameter analysis of collagen-dependent thrombus formation in vitro. Remarkably, in only approximately half of the mouse strains that displayed reduced arterial thrombosis in vivo, this was accompanied by impaired hemostasis. This was also reflected by comparing in vitro thrombus formation (by microfluidics) with alterations in in vivo bleeding time. In conclusion, the presently developed multi-parameter analysis of thrombus formation using microfluidics can be used to: (i) determine the severity of platelet abnormalities; (ii) distinguish between altered platelet adhesion, aggregation and activation; and (iii) elucidate both collagen and non-collagen dependent alterations of thrombus formation. This approach may thereby aid in the better understanding and better assessment of genetic variation that affect in vivo arterial thrombosis and hemostasis.

KW - arterial thrombus formation

KW - bleeding

KW - collagen

KW - glycoprotein VI

KW - platelets

KW - microfluidics

KW - DEFECTIVE PLATELET ACTIVATION

KW - PROTEIN-INTERACTION NETWORKS

KW - IN-VIVO DEPLETION

KW - GLYCOPROTEIN-VI

KW - ARTERIAL THROMBOSIS

KW - ADHESION MECHANISMS

KW - RECEPTOR CLEC-2

KW - INTEGRIN

KW - COLLAGEN

KW - ROLES

U2 - 10.3389/fcvm.2019.00099

DO - 10.3389/fcvm.2019.00099

M3 - Article

C2 - 31417909

SN - 2297-055X

VL - 6

JO - Frontiers in Cardiovascular Medicine

JF - Frontiers in Cardiovascular Medicine

M1 - 99

ER -