Thromb Haemost 2012; 108(02): 328-337
DOI: 10.1160/TH12-02-0064
Platelets and Blood Cells
Schattauer GmbH

Platelets selectively enhance lymphocyte adhesion on subendothelial matrix under arterial flow conditions

Galia Spectre*
1   Department of Medicine-Solna, Clinical Pharmacology Unit, Karolinska Institute, Karolinska University Hospital-Solna, Stockholm, Sweden
2   Department of Hematology, Hadassah Hebrew University Medical Center, Jerusalem, Israel
,
Linjing Zhu*
1   Department of Medicine-Solna, Clinical Pharmacology Unit, Karolinska Institute, Karolinska University Hospital-Solna, Stockholm, Sweden
,
Maria Ersoy
1   Department of Medicine-Solna, Clinical Pharmacology Unit, Karolinska Institute, Karolinska University Hospital-Solna, Stockholm, Sweden
,
Paul Hjemdahl
1   Department of Medicine-Solna, Clinical Pharmacology Unit, Karolinska Institute, Karolinska University Hospital-Solna, Stockholm, Sweden
,
Naphtali Savion
3   Goldschleger Eye Research Institute, Tel Aviv University, Tel Hashomer, Israel
,
David Varon
2   Department of Hematology, Hadassah Hebrew University Medical Center, Jerusalem, Israel
,
Nailin Li
1   Department of Medicine-Solna, Clinical Pharmacology Unit, Karolinska Institute, Karolinska University Hospital-Solna, Stockholm, Sweden
› Author Affiliations
Financial support: This work was supported by grants from the Swedish Research Council, the Swedish Heart-Lung Foundation, the Karolinska Institute, the Swedish Society of Medicine, and the Stockholm County Council.
Further Information

Publication History

Received: 06 February 2012

Accepted after major revision: 03 May 2012

Publication Date:
25 November 2017 (online)

Summary

Platelet adhesion at sites of cardiovascular injury may facilitate leukocyte deposition. We asked if and how platelets enhance lymphocyte adhesion on different subendothelial matrix protein (SEMP)-coated surface at arterial shear stress. Hirudinised whole blood was subjected to an arterial shear rate (500 s−1) in a Cone and Plate(let) analyser (CPA) for 5 minutes using plates coated with bovine serum albumin (BSA), collagen, fibrinogen, von Willebrand factor (vWF), or fibronectin. Platelet and lymphocyte adhesion were monitored by CPA and flow cytometry. Exposure of blood to collagen, fibrinogen, and vWF-coated surfaces induced platelet activation. The most marked effect was seen with collagen-coating, which markedly enhanced the adhesion of all lymphocyte subpopulations compared to BSA-coating. Fibrinogen-coating supported both T and NK cell adhesion, while vWF-coated surface only enhanced NK cell deposition. In contrast, fibronectin enhanced neither platelet activation nor lymphocyte adhesion. Moreover, platelets preferentially facilitated adhesion of large CD4+ and CD8+ T cells and NK cells, and of small B cells. Enhanced cell adhesion of larger lymphocytes was associated with elevated platelet conjugation and higher lymphocyte expression of PSGL-1, Mac-1, and CD40L. The enhancement of lymphocyte adhesion was totally platelet-dependent, and was abolished in platelet-depleted blood. Moreover, blockade of the platelet adhesion molecules P-selectin, GPIIb/IIIa, and CD40L attenuated platelet-dependent lymphocyte deposition. In conclusion, platelets support lymphocyte adhesion on SEMP-coated surfaces under arterial shear. The enhancement is selective for large T and NK cells and small B cells.

* These authors contributed equally to the study.


 
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