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Institut für Physiologie, Medizinische Fakultät Carl Gustav Carus, Technische Universität Dresden, 01307 Dresden, Germany
A detailed understanding of adenosine metabolism of vascular
smooth muscle cells (VSMC) is highly desirable to critically evaluate
possible autocrine effects of adenosine in this cell species.
Therefore, this study quantified intra- and extracellular adenosine
flux rates, the transmembrane concentration gradient, and the adenosine
surface concentration in porcine VSMC and, for comparison, aortic
endothelial cells (PAEC). Cell-covered microcarrier beads packed in a
chromatography column were superfused with a HEPES buffer. With the use
of specific inhibitors of adenosine kinase (iodotubericidine, 10 µM),
adenosine deaminase [erythro-9-(2-hydroxy-3-nonyl)-adenine, 5 µM], ecto-5'-nucleotidase (
,
-methylene-adenosine
5'-diphosphate, 50 µM), and adenosine membrane transport
(n-nitrobenzylthioinosine, 1 µM), total production rates
of 12.3 ± 2.7 and 7.5 ± 1.3 pmol · min
1 · µl cell
volume
1 were obtained for VSMC and PAEC, respectively.
Despite prevailing intracellular adenosine production (76 and 70% of
total production, respectively), transmembrane concentration gradients
under control conditions were directed toward the cytosol as a result
of rapid intracellular adenosine rephosphorylation and continuous
extracellular hydrolysis from 5'-AMP. Surface concentrations were ~18
nM in VSMC and PAEC under control conditions and increased to ~60 nM during partial inhibition of adenosine metabolism. Simultaneously, the
transmembrane adenosine concentration gradient was reversed. We
conclude that adenosine flux rates in VSMC and PAEC are quantitatively similar and that VSMC may influence the interstitial adenosine concentration under basal steady-state conditions.
acetate; adenosine membrane transport; cell superfusion model; dipyridamole; flow regulation; flux rate analysis
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