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Granulocytes enhance LPS‐induced tissue factor activity in monocytes via an interaction with platelets
Author(s) -
Halvorsen Hanne,
Olsen Jan Ole,
Osterud Bjarne
Publication year - 1993
Publication title -
journal of leukocyte biology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.819
H-Index - 191
eISSN - 1938-3673
pISSN - 0741-5400
DOI - 10.1002/jlb.54.4.275
Subject(s) - platelet , tumor necrosis factor alpha , lipopolysaccharide , biology , endocrinology , medicine , stimulation , tissue factor , monocyte , phorbol , granulocyte , platelet activating factor , microbiology and biotechnology , immunology , biochemistry , protein kinase c , coagulation , signal transduction
In the present study we have investigated the effect of platelets and granulocytes on bacterial lipopoly‐ saccharide (LPS)‐induced tissue factor (TF) activity in monocytes. Experiments were performed on freshly isolated cells resuspended in heparinized plasma and recombined with platelet‐poor or platelet‐rich plasma. In a platelet‐dependent reaction the granulocytes enhanced LPS‐induced TF activity by an average of 100%. The effect was dose dependent with regard to the number of both granulocytes and platelets, respectively. Granulocytes and/or platelets did not affect LPS‐induced tumor necrosis factor (TNF) secretion from monocytes. Phorbol myristate acetate (PMA) per se was not able to induce TF activity in our system. In contrast, the agonist caused a substantial increase in TF activity induced by LPS. The effect was totally dependent on the presence of platelets and was shown to be due to stimulation of both granulocytes and monocytes (the activity rose from 30 ± 7 to 83 ± 12 mU/10 6 cells in the presence of platelets and from 69 ± 8 to 143 ± 22 mU/10 6 cells in the presence of platelets and granulocytes). Effects similar to those observed with PMA were obtained with physiological concentrations (10 ng/ml) of TNF. A combination of these two agonists gave no further amplification of LPS‐induced TF activity compared with the effect of the agonists separately. Low concentrations of a monoclonal anti‐ CD15 antibody abolished the stimulatory effects of platelets and granulocytes. Furthermore, the anti‐GDI 5 antibody neutralized the effect of TNF, whereas the PMA effect was reduced by almost 75%. These results were confirmed in a whole‐blood system. The inhibitory effect of the antibody may be associated with CD15's role as a complementary ligand for PADGEM. Our study indicates that a close interaction between granulocytes, platelets, and monocytes is essential for optimal TF activity induced by LPS. It is hypothesized that the effect of granulocytes is related to their ability to activate platelets. We propose that upon activation granulocytes secrete a product that enhances the capacity of platelets to stimulate TF activity in monocytes.

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