The cAMP-producing agonist beraprost inhibits human vascular smooth muscle cell migration via exchange protein directly activated by cAMP

JS McKean, F Murray, G Gibson… - Cardiovascular …, 2015 - academic.oup.com
JS McKean, F Murray, G Gibson, DA Shewan, SJ Tucker, GF Nixon
Cardiovascular research, 2015academic.oup.com
Aims During restenosis, vascular smooth muscle cells (VSMCs) migrate from the vascular
media to the developing neointima. Preventing VSMC migration is therefore a therapeutic
target for restenosis. Drugs, such as prostacyclin analogues, that increase the intracellular
concentration of cyclic adenosine monophosphate (cAMP) can inhibit VSMC migration, but
the mechanisms via which this occurs are unknown. Two main downstream mediators of
cAMP are protein kinase A (PKA) and exchange protein directly activated by cAMP (Epac) …
Aims
During restenosis, vascular smooth muscle cells (VSMCs) migrate from the vascular media to the developing neointima. Preventing VSMC migration is therefore a therapeutic target for restenosis. Drugs, such as prostacyclin analogues, that increase the intracellular concentration of cyclic adenosine monophosphate (cAMP) can inhibit VSMC migration, but the mechanisms via which this occurs are unknown. Two main downstream mediators of cAMP are protein kinase A (PKA) and exchange protein directly activated by cAMP (Epac). This study has examined the effects of the prostacyclin analogue beraprost on VSMC migration and investigated the intracellular pathways involved.
Methods and results
In a chemotaxis chamber, human saphenous vein VSMC migrated towards a platelet-derived growth-factor-BB (PDGF) chemogradient. Incubation with therapeutically relevant concentrations of cAMP-producing agonist beraprost significantly decreased PDGF-induced migration. Direct activation of either PKA or Epac inhibited migration whereas inhibition of PKA did not prevent the anti-migratory effect of beraprost. Direct activation of Epac also prevented hyperplasia in ex vivo serum-treated human veins. Using fluorescence resonance energy transfer, we demonstrated that beraprost activated Epac but not PKA. The mechanisms of this Epac-mediated effect involved activation of Rap1 with subsequent inhibition of RhoA. Cytoskeletal rearrangement at the leading edge of the cell was consequently inhibited. Interestingly, Epac1 was localized to the leading edge of migrating VSMC.
Conclusions
These results indicate that therapeutically relevant concentrations of beraprost can inhibit VSMC migration via a previously unknown mechanism involving the cAMP mediator Epac. This may provide a novel target that could blunt neointimal formation.
Oxford University Press