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建立血视网膜外屏障的人体体外模型。

Establishment of a human in vitro model of the outer blood-retinal barrier.

作者信息

Hamilton R D, Foss A J, Leach L

机构信息

Centre for Integrated Systems Biology and Medicine, School of Biomedical Sciences, Faculty of Medicine, University of Nottingham, UK.

出版信息

J Anat. 2007 Dec;211(6):707-16. doi: 10.1111/j.1469-7580.2007.00812.x. Epub 2007 Oct 8.

Abstract

The outer blood-retinal barrier is composed of a monolayer of retinal pigment epithelium, Bruch's membrane and the choriocapillaris which is fenestrated. Endothelial proliferation and breaching of Bruch's membrane leads to the neovascular form of age-related macula degeneration (ARMD). The aim of this study was to generate an in vitro model that mimics more faithfully the phenotype of the choriocapillaris and the trilayer architecture in vitro. A trilayer culture model was generated with retinal pigment epithelium (ARPE-19) cell cultures on the epithelial surface of amniotic membrane and with human umbilical vein-derived endothelial cells on the other surface. A control model for the effect of retinal pigment epithelium on endothelial changes was generated with corneal epithelial cells replacing the ARPE-19. Both human umbilical vein-derived endothelial and ARPE-19 cells formed confluent monolayers on respective surfaces of the amnion. The human umbilical vein-derived endothelial cells in the trilayer became fenestrated when co-cultured with the ARPE-19 cells, but not with corneal epithelial cells, or when grown as monolayers on the amnion, showing a loss of fidelity of origin in the presence of ARPE-19 cells. These cells also revealed VE-cadherin and ZO-1 at cell-cell contacts from 24 h in the trilayer. The tight junctional molecules, occludin and ZO-1, were localized to cell-cell contact regions in the retinal pigment epithelium, both in the monolayer and in the trilayer system. Permeability of the trilayer was tested by using fluorescein and fluorescein-conjugated tracers under flow. At 72 h the trilayer severely restricted transfer of sodium fluorescein (NaF) (ten-fold reduction) whilst transfer of a 4 kDa FITC-conjugated dextran was virtually occluded, confirming a restrictive barrier. Ultrastructural studies showed the retinal pigment epithelium monolayer was polarized with microvilli present on the apical surface. Paracellular clefts showed numerous tight junctional-like appositions, similar to that seen on amnion alone. This study demonstrates that ARPE-19 and human umbilical vein-derived endothelial cells can be co-cultured on the amniotic membrane and that the resultant cross-talk leads to formation of a fenestrated endothelium, whilst maintaining a polarized restrictive epithelial layer. The fenestrated endothelial phenotype achieved in this human in vitro trilayer model is a first and offers an outer-retinal barrier which approaches the in vivo state and has potential for studies into induced junctional disruption, endothelial proliferation and migration: features of ARMD.

摘要

外血视网膜屏障由单层视网膜色素上皮、布鲁赫膜和有窗孔的脉络膜毛细血管组成。内皮细胞增殖和布鲁赫膜破裂会导致年龄相关性黄斑变性(ARMD)的新生血管形成。本研究的目的是建立一种体外模型,更忠实地模拟脉络膜毛细血管的表型和体外三层结构。通过在羊膜上皮表面培养视网膜色素上皮(ARPE - 19)细胞,并在另一表面培养人脐静脉来源的内皮细胞,建立了三层培养模型。用角膜上皮细胞替代ARPE - 19细胞,建立了视网膜色素上皮对内皮细胞变化影响的对照模型。人脐静脉来源的内皮细胞和ARPE - 19细胞在羊膜各自表面形成汇合的单层。三层培养中的人脐静脉来源的内皮细胞与ARPE - 19细胞共培养时会形成窗孔,但与角膜上皮细胞共培养时不会,或在羊膜上单层生长时也不会,这表明在有ARPE - 19细胞存在时,其来源的保真度有所丧失。这些细胞在三层培养中24小时后在细胞间接触处也显示出血管内皮钙黏蛋白和闭锁小带蛋白1。紧密连接分子闭合蛋白和闭锁小带蛋白1定位于视网膜色素上皮的细胞间接触区域,无论是在单层还是在三层系统中。在流动条件下,使用荧光素和荧光素偶联的示踪剂测试三层培养物的通透性。在72小时时,三层培养物严重限制了荧光素钠(NaF)的转运(降低了10倍),而4 kDa异硫氰酸荧光素偶联葡聚糖的转运几乎被阻断,证实了其具有限制性屏障。超微结构研究表明,视网膜色素上皮单层是极化的,顶端表面有微绒毛。细胞旁间隙显示出许多类似紧密连接的并列结构,类似于仅在羊膜上看到的情况。本研究表明,ARPE - 19细胞和人脐静脉来源的内皮细胞可以在羊膜上共培养,并且由此产生的相互作用导致形成有窗孔的内皮,同时维持极化的限制性上皮层。在这种人体体外三层模型中实现的有窗孔内皮表型尚属首次,它提供了一种接近体内状态的外视网膜屏障,具有研究诱导性连接破坏、内皮细胞增殖和迁移的潜力,这些都是ARMD的特征。

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