Structural and Functional Comparison of HDL From Homologous Human Plasma and Follicular Fluid : A Model for Extravascular Fluid

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Arteriosclerosis, Thrombosis, and Vascular Biology. 1997;17:1605-1613

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(Arteriosclerosis, Thrombosis, and Vascular Biology. 1997;17:1605-1613.)
© 1997 American Heart Association, Inc.

Articles

Structural and Functional Comparison of HDL From Homologous Human Plasma and Follicular Fluid

A Model for Extravascular Fluid

Béatrice Jaspard; Nathalie Fournier; Gérard Vieitez; Véronique Atger; Ronald Barbaras; Claude Vieu; Jeanine Manent; Hugues Chap; Bertrand Perret; ; Xavier Collet

From the Institut National de la santé et de la Recherche Médicale, Unité 326, Phospholipides membranaires, Signalisation cellulaire et Lipoprotéines, Hôpital Purpan, Toulouse (B.J., R.B., C.V., J.M., H.C., B.P., X.C.); Hôpital Broussais, Paris (N.F., V.A.); and Laboratoire de Fécondation in vitro, Hôpital Lagrave, Toulouse, France (G.V.).

Correspondence to Dr X. Collet, Institut National de la santé et de la Recherche Médicale, Unité 326, Phospholipides membranaires, Signalisation cellulaire et Lipoprotéines, Hôpital Purpan, 31059, Toulouse, France. E-mail collet{at}cict.fr.

Abstract In the preovulatory period, follicular fluid containsonly HDL. Biochemical characterization of such lipoproteins showedthat follicular fluid HDLs were cholesterol-poor particles comparedwith serum HDLs, whereas the amount of phospholipids, expressedas percent weight, was significantly higher in follicular fluidHDLs (28.5%) than in serum HDLs (25.0%, P<.05). The amountof apolipoprotein (apo) A-IV per apo A-I was significantly higherin follicular fluid than in serum (0.77 versus 0.58 mg/g apoA-I, P<.02). To explore the role of HDLs as cholesterol acceptorsin physiological media, we compared the ability of either wholehuman follicular fluids or homologous sera to promote cellularcholesterol efflux using Fu5AH rat hepatoma cells. At equivalentconcentrations of HDL cholesterol in follicular fluid and inserum, t_1/2 values for cholesterol efflux were in the same range.In addition, estimated maximal efflux values were not significantlydifferent in follicular fluid and serum (45.9% and 49.6%, respectively),as were K_m values (0.064 and 0.071 mmol/L HDL cholesterol, respectively).In addition, isolated HDLs displayed the same capacity to promotecellular cholesterol efflux in both media. Thus, the kineticsand dose-response data between these two physiological mediashowed that HDLs play the major role in cellular cholesterolefflux. The rate of cholesterol esterification, as measuredin the presence of cells, was significantly higher in follicularfluid than in serum at constant HDL cholesterol concentrations,whereas the rate of esterified cholesterol transfer toward addedLDL was lower. In contrast, in a cell-free system, lecithin:cholesterolacyltransferase activity represented only 26% of that in serumHDL, whereas cholesterol ester transfer protein activities were comparable.In summary, in this particular model, we confirmed the essentialrole of HDLs as physiological acceptors in the removal of cellularcholesterol.

Key Words: cholesterol efflux • follicular fluidity • HDL

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