Blood platelets and vascular walls generate prostaglandin (PG) derivatives with oppening
effects. Since aspirin (ASA) inhibits synthesis of common precursors of these derivatives,
the rationale for its clinical use in thrombosis prevention trials has been questioned.
This is an experimental approach to this important therapeutic dilemma. Male CD rats
(250-350g) were given a single i.p. dose of ASA (0.5-200mg/kg) and killed from 1 to
120 h thereafter. Platelet PG production was measured by a thiobarbiturate assay of
malondialdehyde (MDA) under thrombin (25u/ml) stimulation. Vascular PG activity released
from rings of abdominal aorta and inferior vena cava was determined as platelet aggregation
inhibitory potency and characterized as PGI2 by standard criteria. The inhibitory effect of ASA lasted longer in platelets (96-120
h) than in venous (24-48 h) or arterial tissues (<24 h). Platelets were more sensitive
to ASA (ID50=3.6mg/kg) than arterial tissues (ID50=25mg/kg) but as sensitive as venous tissues (ID50=2.3mg/kg) when PG synthesis was measured 1 h after treatment. The proposed unique
sensitivity of platelet cyclo-oxygenase to ASA therefore needs reconsidering. ASA’s
effect on various systems might be better dissociated based on the different duration
of inhibition. We suggest that the lowest single dose of ASA totally inhibiting platelet
PG synthesis should be given at the longest possible intervals.
