多药耐药 1 型-EGFP 转染大鼠与人脑微血管内皮细胞系中 P-糖蛋白的定位、转运和功能的相似性和差异。
Similarities and differences in the localization, trafficking, and function of P-glycoprotein in MDR1-EGFP-transduced rat versus human brain capillary endothelial cell lines.
机构信息
Department of Pharmacology, Toxicology, and Pharmacy, University of Veterinary Medicine Hannover, Bünteweg 17, 30559, Hannover, Germany.
Center for Systems Neuroscience, Hannover, Germany.
出版信息
Fluids Barriers CNS. 2021 Aug 3;18(1):36. doi: 10.1186/s12987-021-00266-z.
BACKGROUND
In vitro models based on brain capillary endothelial cells (BCECs) are among the most versatile tools in blood-brain barrier research for testing drug penetration into the brain and how this is affected by efflux transporters such as P-glycoprotein (Pgp). However, compared to freshly isolated brain capillaries or primary BCECs, the expression of Pgp in immortalized BCEC lines is markedly lower, which prompted us previously to transduce the widely used human BCEC line hCMEC/D3 with a doxycycline-inducible MDR1-EGFP fusion plasmid. The EGFP-labeled Pgp in these cells allows studying the localization and trafficking of the transporter and how these processes are affected by drug exposure. Here we used this strategy for the rat BCEC line RBE4 and performed a face-to-face comparison of RBE4 and hCMEC/D3 wild-type (WT) and MDR1-EGFP transduced cells.
METHODS
MDR1-EGFP-transduced variants were derived from WT cells by lentiviral transduction, using an MDR1-linker-EGFP vector. Localization, trafficking, and function of Pgp were compared in WT and MDR1-EGFP transduced cell lines. Primary cultures of rat BCECs and freshly isolated rat brain capillaries were used for comparison.
RESULTS
All cells exhibited typical BCEC morphology. However, significant differences were observed in the localization of Pgp in that RBE4-MDR1-EGFP cells expressed Pgp primarily at the plasma membrane, whereas in hCMEC/D3 cells, the Pgp-EGFP fusion protein was visible both at the plasma membrane and in endolysosomal vesicles. Exposure to doxorubicin increased the number of Pgp-EGFP-positive endolysosomes, indicating a lysosomotropic effect. Furthermore, lysosomal trapping of doxorubicin was observed, likely contributing to the protection of the cell nucleus from damage. In cocultures of WT and MDR1-EGFP transduced cells, intercellular Pgp-EGFP trafficking was observed in RBE4 cells as previously reported for hCMEC/D3 cells. Compared to WT cells, the MDR1-EGFP transduced cells exhibited a significantly higher expression and function of Pgp. However, the junctional tightness of WT and MDR1-EGFP transduced RBE4 and hCMEC/D3 cells was markedly lower than that of primary BCECs, excluding the use of the cell lines for studying vectorial drug transport.
CONCLUSIONS
The present data indicate that MDR1-EGFP transduced RBE4 cells are an interesting tool to study the biogenesis of lysosomes and Pgp-mediated lysosomal drug trapping in response to chemotherapeutic agents and other compounds at the level of the blood-brain barrier.
背景
基于脑毛细血管内皮细胞(BCEC)的体外模型是血脑屏障研究中最通用的工具之一,可用于测试药物穿透大脑的能力,以及这种穿透能力如何受到 P-糖蛋白(Pgp)等外排转运蛋白的影响。然而,与新鲜分离的脑毛细血管或原代 BCEC 相比,永生化 BCEC 系中的 Pgp 表达明显较低,这促使我们之前使用广泛使用的人 BCEC 系 hCMEC/D3 转导了一种强力霉素诱导的 MDR1-EGFP 融合质粒。这些细胞中的 EGFP 标记的 Pgp 可用于研究转运蛋白的定位和运输,以及这些过程如何受到药物暴露的影响。在这里,我们使用这种策略对大鼠 BCEC 系 RBE4 进行了研究,并对 RBE4 和 hCMEC/D3 野生型(WT)和 MDR1-EGFP 转导细胞进行了面对面比较。
方法
通过慢病毒转导,使用 MDR1-连接子-EGFP 载体,从 WT 细胞中衍生出 MDR1-EGFP 转导变体。比较 WT 和 MDR1-EGFP 转导细胞系中 Pgp 的定位、运输和功能。还比较了大鼠 BCEC 的原代培养物和新鲜分离的大鼠脑毛细血管。
结果
所有细胞均表现出典型的 BCEC 形态。然而,在 Pgp 的定位上观察到了显著差异,即 RBE4-MDR1-EGFP 细胞主要在质膜上表达 Pgp,而在 hCMEC/D3 细胞中,Pgp-EGFP 融合蛋白可见于质膜和内溶酶体小泡中。阿霉素的暴露增加了 Pgp-EGFP 阳性内溶酶体的数量,表明其具有溶酶体趋向性。此外,观察到阿霉素的溶酶体捕获,这可能有助于保护细胞核免受损伤。在 WT 和 MDR1-EGFP 转导细胞的共培养物中,如先前在 hCMEC/D3 细胞中所报道的,观察到细胞间 Pgp-EGFP 的运输。与 WT 细胞相比,MDR1-EGFP 转导的细胞表现出 Pgp 的表达和功能显著增加。然而,WT 和 MDR1-EGFP 转导的 RBE4 和 hCMEC/D3 细胞的细胞间紧密连接明显低于原代 BCEC,排除了使用细胞系来研究载体药物转运。
结论
本研究数据表明,MDR1-EGFP 转导的 RBE4 细胞是研究化疗药物和其他化合物引起的血脑屏障中溶酶体生物发生和 Pgp 介导的溶酶体药物捕获的一个有趣工具。
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