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外血视网膜屏障体外模型中的渗透压应激

Osmotic stress in an in vitro model of the outer blood-retinal barrier.

作者信息

Orgül S, Reuter U, Kain H L

机构信息

Universitäts-Augenklinik, Basel, Switzerland.

出版信息

Ger J Ophthalmol. 1993 Nov;2(6):436-43.

PMID:8312831
Abstract

Because of the difficulty involved in in vivo experimental manipulations of the outer blood-retinal barrier, we developed an in vitro model. Retinal pigment epithelium (RPE) from bovine eyes was grown on semipermeable membranes. A continuous monolayer of RPE developed a measurable transepithelial electrical resistance (TER). TER was used as a parameter of barrier function. The tightness of the cellular monolayer was also tested with fluorescein. The TER increased in confluent cultures by 60-70 ohms-cm2, and there was no fluorescein leakage. After exposure of the cultures to 0.2% trypsin or 1% ethylenediaminetetraacetic acid (ETDA), we detected a reversible breakdown of the epithelial barrier function. Under transmission electron microscopy, we detected no disassembly of the junctional components after breakdown of the barrier function with trypsin or EDTA. A hyperosmotic NaCl solution in the basal medium as well as a hypoosmotic NaCl solution in the apical medium induced a breakdown in the TER, whereas a hyperosmotic NaCl solution in the apical medium induced only a slight decrease in the TER. Under transmission electron microscopy, we detected an intracellular blistering and large intercellular widening. A hypo-osmolar NaCl solution in the basal medium induced a rise in the TER. With regard to these experiments, it seems, at least in vitro, that the function of occluding junctions in bovine RPE as permeability barriers depends on extracellular calcium. Furthermore, our results were such as if the outer blood-retinal barrier were designed to prevent subretinal inflow of free water.

摘要

由于对视网膜外血-视网膜屏障进行体内实验操作存在困难,我们开发了一种体外模型。将牛眼的视网膜色素上皮(RPE)培养在半透膜上。连续的RPE单层形成了可测量的跨上皮电阻(TER)。TER被用作屏障功能的参数。还用荧光素测试了细胞单层的紧密性。汇合培养物中的TER增加了60 - 70欧姆·平方厘米,且没有荧光素泄漏。在将培养物暴露于0.2%胰蛋白酶或1%乙二胺四乙酸(EDTA)后,我们检测到上皮屏障功能的可逆性破坏。在透射电子显微镜下,在用胰蛋白酶或EDTA破坏屏障功能后,我们未检测到连接成分的解体。基础培养基中的高渗NaCl溶液以及顶膜培养基中的低渗NaCl溶液会导致TER破坏,而顶膜培养基中的高渗NaCl溶液只会使TER略有下降。在透射电子显微镜下,我们检测到细胞内出现水泡和细胞间明显增宽。基础培养基中的低渗NaCl溶液会导致TER升高。关于这些实验,至少在体外,似乎牛RPE中封闭连接作为通透性屏障的功能取决于细胞外钙。此外,我们的结果表明,视网膜外血-视网膜屏障似乎是为了防止游离水进入视网膜下而设计的。

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