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本文引用的文献

1
Rap1b facilitates NK cell functions via IQGAP1-mediated signalosomes.Rap1b 通过 IQGAP1 介导的信号小体促进 NK 细胞功能。
J Exp Med. 2010 Aug 30;207(9):1923-38. doi: 10.1084/jem.20100040. Epub 2010 Aug 23.
2
Cyclic AMP phosphodiesterase 4D (PDE4D) Tethers EPAC1 in a vascular endothelial cadherin (VE-Cad)-based signaling complex and controls cAMP-mediated vascular permeability.环腺苷酸磷酸二酯酶 4D (PDE4D) 将 EPAC1 固定在基于血管内皮钙黏蛋白 (VE-Cad) 的信号复合物中,并控制 cAMP 介导的血管通透性。
J Biol Chem. 2010 Oct 29;285(44):33614-22. doi: 10.1074/jbc.M110.140004. Epub 2010 Aug 23.
3
RhoL controls invasion and Rap1 localization during immune cell transmigration in Drosophila.RhoL 在果蝇免疫细胞迁移过程中控制侵袭和 Rap1 定位。
Nat Cell Biol. 2010 Jun;12(6):605-10. doi: 10.1038/ncb2063. Epub 2010 May 23.
4
Role of afadin in vascular endothelial growth factor- and sphingosine 1-phosphate-induced angiogenesis.Afadin 在血管内皮生长因子和鞘氨醇 1-磷酸诱导的血管生成中的作用。
Circ Res. 2010 Jun 11;106(11):1731-42. doi: 10.1161/CIRCRESAHA.110.216747. Epub 2010 Apr 22.
5
Control of endothelial barrier function by regulating vascular endothelial-cadherin.通过调节血管内皮钙黏蛋白来控制内皮屏障功能。
Curr Opin Hematol. 2010 May;17(3):230-6. doi: 10.1097/MOH.0b013e328338664b.
6
Regulation of angiogenesis by a small GTPase Rap1.Rap1 通过小 GTPase 调节血管生成。
Vascul Pharmacol. 2010 Jul-Aug;53(1-2):1-10. doi: 10.1016/j.vph.2010.03.003. Epub 2010 Mar 16.
7
Adherens junctions connect stress fibres between adjacent endothelial cells.黏着连接将相邻内皮细胞之间的应力纤维连接起来。
BMC Biol. 2010 Feb 2;8:11. doi: 10.1186/1741-7007-8-11.
8
Vascular endothelial-cadherin stabilizes at cell-cell junctions by anchoring to circumferential actin bundles through alpha- and beta-catenins in cyclic AMP-Epac-Rap1 signal-activated endothelial cells.血管内皮钙黏蛋白通过α-和β-连环蛋白将自身锚定于环化 AMP-Epac-Rap1 信号激活的内皮细胞中环状肌动蛋白束,从而稳定在细胞-细胞连接处。
Mol Biol Cell. 2010 Feb 15;21(4):584-96. doi: 10.1091/mbc.e09-07-0580. Epub 2009 Dec 23.
9
Control of cell adhesion dynamics by Rap1 signaling.通过Rap1信号传导控制细胞粘附动力学。
Curr Opin Cell Biol. 2009 Oct;21(5):684-93. doi: 10.1016/j.ceb.2009.06.004. Epub 2009 Jul 16.
10
JAM-C induces endothelial cell permeability through its association and regulation of {beta}3 integrins.JAM-C通过与β3整合素的结合及调控来诱导内皮细胞通透性。
Arterioscler Thromb Vasc Biol. 2009 Aug;29(8):1200-6. doi: 10.1161/ATVBAHA.109.189217. Epub 2009 May 21.

Rap1A和Rap1B小G蛋白在形成内皮细胞连接中的亚型特异性差异。

Isoform-specific differences between Rap1A and Rap1B GTPases in the formation of endothelial cell junctions.

作者信息

Wittchen Erika S, Aghajanian Amir, Burridge Keith

机构信息

Department of Cell and Developmental Biology; Chapel Hill, NC USA.

出版信息

Small GTPases. 2011 Mar;2(2):65-76. doi: 10.4161/sgtp.2.2.15735.

DOI:10.4161/sgtp.2.2.15735
PMID:21776404
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3136906/
Abstract

Rap1 is a Ras-like GTPase that has been studied with respect to its role in cadherin-based cell adhesion. Rap1 exists as two separate isoforms, Rap1A and Rap1B, which are 95% identical and yet the phenotype of the isoform-specific knockout mice is different. We and others have previously identified a role for Rap1 in regulating endothelial adhesion, junctional integrity and barrier function; however, these early studies did not distinguish a relative role for each isoform. To dissect the individual contribution of each isoform in regulating the endothelial barrier, we utilized an engineered microRNA-based approach to silence Rap1A, Rap1B or both, then analyzed barrier properties of the endothelium. Electrical impedance sensing experiments show that Rap1A is the predominant isoform involved in endothelial cell junction formation. Quantification of monolayer integrity by VE-cadherin staining revealed that knockdown of Rap1A, but not Rap1B, increased the number of gaps in the confluent monolayer. This loss of monolayer integrity could be rescued by re-expression of exogenous Rap1A protein. Expression of GFP-tagged Rap1A or 1B revealed quantifiable differences in localization of each isoform, with the junctional pool of Rap1A being greater. The junctional protein AF-6 also co-immunoprecipitates more strongly with expressed GFP-Rap1A. Our results show that Rap1A is the more critical isoform in the context of endothelial barrier function, indicating that some cellular processes differentially utilize Rap1A and 1B isoforms. Studying how Rap1 isoforms differentially regulate EC junctions may thus reveal new targets for developing therapeutic strategies during pathological situations where endothelial barrier disruption leads to disease.

摘要

Rap1是一种类Ras GTP酶,人们已对其在基于钙黏蛋白的细胞黏附中的作用进行了研究。Rap1以两种不同的亚型Rap1A和Rap1B形式存在,它们有95%的同源性,但亚型特异性敲除小鼠的表型却不同。我们和其他人之前已确定Rap1在调节内皮细胞黏附、连接完整性和屏障功能方面发挥作用;然而,这些早期研究并未区分每种亚型的相对作用。为了剖析每种亚型在调节内皮屏障中的个体贡献,我们采用了基于工程化微小RNA的方法来沉默Rap1A、Rap1B或两者,然后分析内皮细胞的屏障特性。电阻抗传感实验表明,Rap1A是参与内皮细胞连接形成的主要亚型。通过VE-钙黏蛋白染色对单层完整性进行定量分析发现,敲低Rap1A而非Rap1B会增加汇合单层中的间隙数量。这种单层完整性的丧失可通过重新表达外源性Rap1A蛋白来挽救。绿色荧光蛋白标记的Rap1A或1B的表达揭示了每种亚型在定位上的可量化差异,其中Rap1A的连接池更大。连接蛋白AF-6与表达的绿色荧光蛋白-Rap1A的共免疫沉淀也更强。我们的结果表明,在调节内皮屏障功能方面,Rap1A是更关键的亚型,这表明一些细胞过程以不同方式利用Rap1A和1B亚型。因此,研究Rap1亚型如何不同地调节内皮细胞连接可能会揭示在病理情况下开发治疗策略的新靶点,在内皮屏障破坏导致疾病的病理情况下。