Hexose transport in normal and SV40‐transformed human endothelial cells in culture

The mechanism of glucose entry into human vascular endothelial cells was studied in monolayer cultures of normal (primary) and virally (SV40) transformed umbilical vein endothelium. Radioisotopic uptake studies with the glucose analogues 2‐deoxy‐D‐glucose, and 3‐O‐methyl‐D‐glucose, and the nonmetabolizable stereoisomer L‐glucose, indicated the presence of a saturable, stereospecific hexose carrier mechanism in both cell types. In other experiments with D‐glucose and 3‐O‐methyl‐D‐glucose, the phenomenon of countertransport was demonstrable. Hexose transport was not affected by KCN, dinitrophenol, or ouabain, but was inhibited by phloretin and phlorizin in a pattern consistent with facilitated diffusion. Kinetic constants were obtained for both 2‐deoxy‐D‐glucose and 3‐O‐methyl‐D‐glucose uptake. Similar Km values (range, 3.3–4.7 mM) were noted with normal and transformed cells, whereas the apparent Vmax was 0.56 nmol/μ1 cytosol/minute for primary cells and 1.7–2.5 nmol/μ cytosol/minute for transformed cells. Under standard culture conditions, as well as following 18 hours of serum deprivation, insulin at concentrations up to 10−5 M did not appear to influence hexose uptake in either cell type. Metabolism of 14C(U)‐D‐glucose to 14CO2 also was not stimulated by insulin. The presence of an insulin‐insensitive, facilitated transport system for glucose in vascular endothelium has relevance for glucose metabolism in this tissue, and potentially for the association of certain vascular diseases (e.g., diabetic microangiopathy, atherosclerosis) with altered glucose homeostasis.

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