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A new blood-brain barrier model using primary rat brain endothelial cells, pericytes and astrocytes.

机译:一种新的血脑屏障模型,使用原代大鼠脑内皮细胞,周细胞和星形胶质细胞。

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摘要

Blood-brain barrier (BBB) characteristics are induced and maintained by cross-talk between brain microvessel endothelial cells and neighbouring elements of the neurovascular unit. While pericytes are the cells situated closest to brain endothelial cells morphologically and share a common basement membrane, they have not been used in co-culture BBB models for testing drug permeability. We have developed and characterized a new syngeneic BBB model using primary cultures of the three main cell types of cerebral microvessels. The co-culture of endothelial cells, pericytes and astrocytes mimick the anatomical situation in vivo. In the presence of both pericytes and astrocytes rat brain endothelial cells expressed enhanced levels of tight junction (TJ) proteins occludin, claudin-5 and ZO-1 with a typical localization at the cell borders. Further morphological evidence of the presence of interendothelial TJs was provided by electron microscopy. The transendothelial electrical resistance (TEER) of brain endothelial monolayers in triple co-culture, indicating the tightness of TJs reached 400Omegacm(2) on average, while the endothelial permeability coefficients (P(e)) for fluorescein was in the range of 3x10(-6)cm/s. Brain endothelial cells in the new model expressed glucose transporter-1, efflux transporters P-glycoprotein and multidrug resistance protein-1, and showed a polarized transport of rhodamine 123, a ligand for P-glycoprotein. To further characterize the model, drug permeability assays were performed using a set of 19 compounds with known in vivo BBB permeability. Good correlation (R(2)=0.89) was found between in vitroP(e) values obtained from measurements on the BBB model and in vivo BBB permeability data. The new BBB model, which is the first model to incorporate pericytes in a triple co-culture setting, can be a useful tool for research on BBB physiology and pathology and to test candidate compounds for centrally acting drugs.
机译:脑微血管内皮细胞与神经血管单位的相邻元件之间的串扰可诱导并维持血脑屏障(BBB)特性。尽管周细胞是形态上最接近大脑内皮细胞并共享共同基底膜的细胞,但它们尚未用于共培养BBB模型中以测试药物的渗透性。我们已经开发和表征了一种新的同源BBB模型,使用了脑微血管的三种主要细胞类型的原代培养物。内皮细胞,周细胞和星形胶质细胞的共培养模仿体内的解剖学情况。在周细胞和星形胶质细胞均存在的情况下,大鼠脑内皮细胞表达的紧密连接(TJ)蛋白occludin,claudin-5和ZO-1的水平增强,典型的定位在细胞边界。电子显微术提供了存在内皮间TJs的进一步形态学证据。三联共培养中脑内皮单层的跨内皮电阻(TEER),表明TJ的紧密度平均达到400Omegacm(2),而荧光素的内皮通透性系数(P(e))在3x10( -6)cm / s。新模型中的脑内皮细胞表达葡萄糖转运蛋白-1,外排转运蛋白P-糖蛋白和多药耐药蛋白-1,并显示若丹明123(P-糖蛋白的配体)的极化转运。为了进一步表征模型,使用一组19种已知体内BBB渗透性的化合物进行了药物渗透性测定。从BBB模型的测量值和体内BBB通透性数据获得的体外P(e)值之间发现了良好的相关性(R(2)= 0.89)。新的BBB模型是第一个在三重共培养条件下结合周细胞的模型,可以成为研究BBB生理学和病理学并测试中枢作用药物候选化合物的有用工具。

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