体外大分子的经内皮转移。

Federation proceedings Pub Date : 1987-06-01
D M Shasby, R L Roberts
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引用次数: 0

摘要

由于体内模型的复杂性,大分子的跨内皮转移一直是研究的难点。我们开发了一种可渗透支架上培养的内皮细胞模型,并用它来表征白蛋白的跨内皮转移。猪肺动脉内皮细胞在明胶浸渍聚碳酸酯微孔过滤器内形成单层细胞,细胞形成与体内内皮紧密连接相似的连接结构。这种单层膜能抵抗电流,而且这种电阻对细胞外钙浓度很敏感。白蛋白在培养的单层细胞间的转移是不对称的,从间质到管腔的转移速率大于从管腔到间质的转移速率。不对称转移发生在浓度梯度上,并通过NaCN处理单层来消除。增加白蛋白浓度增加了间质向腔内转移的速度,并且在间质白蛋白浓度为725微米时,该过程表现出饱和。这些数据指出,体外制备在鉴定体内难以检测的跨内皮转运的潜在重要方面是有用的。
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Transendothelial transfer of macromolecules in vitro.

The transendothelial transfer of macromolecules has been difficult to study because of the complexities of the in vivo models. We have developed a model of an endothelium cultured on a permeable support and used it to characterize the transendothelial transfer of albumin. Porcine pulmonary artery endothelial cells form a single layer of cells lining the gelatin-impregnated polycarbonate micropore filters, and the cells develop junctional structures similar to endothelial tight junctions observed in vivo. The monolayer resists the flow of electrical current, and the resistance is sensitive to extracellular calcium concentrations. Albumin transfer across the cultured monolayers was found to be asymmetric, and the rate of transfer from interstitium to lumen was greater than that from lumen to interstitium. The asymmetric transfer occurred against a concentration gradient and was abolished by treating the monolayer with NaCN. Increasing albumin concentrations increased the rate of interstitial to luminal transfer, and the process demonstrated saturation at an interstitial albumin concentration of 725 microM. These data point out the usefulness of the in vitro preparation to identify potentially important aspects of transendothelial transport that would be difficult to detect in vivo.

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