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红细胞衍生的鞘氨醇-1-磷酸稳定大鼠微血管的基础水力传导率和溶质通透性。

Erythrocyte-derived sphingosine-1-phosphate stabilizes basal hydraulic conductivity and solute permeability in rat microvessels.

机构信息

Department of Physiology and Membrane Biology, School of Medicine, University of California at Davis, Davis, CA 95616, USA.

出版信息

Am J Physiol Heart Circ Physiol. 2012 Oct 1;303(7):H825-34. doi: 10.1152/ajpheart.00181.2012. Epub 2012 Aug 3.

Abstract

Exogenous sphingosine-1-phosphate (S1P), a lipid mediator in blood, attenuates acute microvascular permeability increases via receptor S1P1 to stabilize the endothelium. To evaluate the contribution of erythrocytes as an endogenous source of S1P to the regulation of basal permeability, we measured permeability coefficients in intact individually perfused venular microvessels of rat mesentery. This strategy also enabled the contributions of other endogenous S1P sources to be evaluated. Apparent permeability coefficients (P(S)) to albumin and α-lactalbumin and the hydraulic conductivity of mesenteric microvessels were measured in the presence or absence of rat erythrocytes or rat erythrocyte-conditioned perfusate. Rat erythrocytes added to the perfusate were the principal source of S1P in these microvessels. Basal P(S) to albumin was stable and typical of blood-perfused microvessels (mean 0.5 × 10(-6) cm/s) when erythrocytes or erythrocyte-conditioned perfusates were present. When they were absent, P(S) to albumin or α-lactalbumin increased up to 40-fold (over 10 min). When exogenous S1P was added to perfusates, permeability returned to levels comparable with those seen in the presence of erythrocytes. Addition of SEW 2871, an agonist specific for S1P1, in the absence of red blood cells reduced P(S)(BSA) (40-fold reduction) toward basal. The specific S1P1 receptor antagonist (W-146) reversed the stabilizing action of erythrocytes and increased permeability (27-fold increase) in a manner similar to that seen in the absence of erythrocytes. Erythrocytes are a primary source of S1P that maintains normal venular microvessel permeability. Absence of erythrocytes or conditioned perfusate in in vivo and in vitro models of endothelial barriers elevates basal permeability.

摘要

外源性鞘氨醇-1-磷酸(S1P)是血液中的一种脂质介质,通过受体 S1P1 减轻急性微血管通透性增加,从而稳定内皮。为了评估红细胞作为 S1P 的内源性来源对基础通透性调节的贡献,我们测量了大鼠肠系膜完整单个灌注的小静脉微血管的通透性系数。这种策略还能够评估其他内源性 S1P 来源的贡献。在存在或不存在大鼠红细胞或大鼠红细胞条件培养液的情况下,测量白蛋白和α-乳白蛋白的表观渗透系数(P(S))和肠系膜微血管的水力传导率。添加到灌流液中的大鼠红细胞是这些微血管中 S1P 的主要来源。当存在红细胞或红细胞条件灌流液时,白蛋白的基础 P(S)是稳定的,且与血液灌注的微血管相似(平均值为 0.5×10(-6)cm/s)。当它们不存在时,白蛋白或α-乳白蛋白的 P(S)增加了高达 40 倍(超过 10 分钟)。当外源性 S1P 添加到灌流液中时,通透性恢复到与存在红细胞时相似的水平。在没有红细胞的情况下添加 SEW 2871,一种特异性针对 S1P1 的激动剂,可使 P(S)(BSA)(降低 40 倍)降低至基础水平。特异性 S1P1 受体拮抗剂(W-146)逆转了红细胞的稳定作用,并以类似于不存在红细胞的方式增加了通透性(增加 27 倍)。红细胞是维持正常静脉微血管通透性的 S1P 的主要来源。在体内和体外内皮屏障模型中,缺乏红细胞或条件灌流液会增加基础通透性。

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