Platelet Incorporation of Labelled Adenosine and Adenosine Diphosphate

E. W Salzman; T. P Ashford; D. A Chambers; Lena L. Neri

doi:10.1055/s-0038-1651356

Thrombosis and Haemostasis, Table of Contents

Thromb Haemost 1969; 22(02): 304-315
DOI: 10.1055/s-0038-1651356

Originalarbeiten-Original Articles-Travaux Originaux

Schattauer GmbH

Platelet Incorporation of Labelled Adenosine and Adenosine Diphosphate

E. W Salzman

¹Currently at Columbia University, New York, New York.

,

T. P Ashford

¹Currently at Columbia University, New York, New York.

,

D. A Chambers

¹Currently at Columbia University, New York, New York.

,

Lena L. Neri

¹Currently at Columbia University, New York, New York.

› Author Affiliations

Abstract

Summary

After incubation of platelet-rich plasma with labelled adenosine or ADP, platelet incorporation of radioactivity was assessed. Platelets were rapidly separated for counting by filtration through cellulose acetate Millipore. Inulin-H³ served as a plasma marker, and triple isotope techniques permitted simultaneous assessment of the behavior of the adenine and phosphate moieties of ADP without washing of platelets. In other experiments, electron microscopic radioautography was employed to trace the label after platelet incorporation.

The results were consistent with previous reports that ADP is dephosphorylated in plasma and is incorporated by platelets only as a dephosphorylated residue, probably adenosine. The label crossed the platelet membrane and entered the platelet, where it was distributed in platelet granules and the agranular cell sap. Concentration within granules occurred to a minor degree.

The results support the hypothesis that platelet aggregation by ADP occurs without a persistent bond of ADP to the platelet. Inhibition of aggregation by adenosine probably depends on a metabolic or transport process rather than on competition between adenosine and ADP for platelet binding sites.

Full Text

References

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