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一种新型半胱氨酸交联方法揭示了紧密连接蛋白-1与四跨膜蛋白CD9之间的直接关联。

A novel cysteine cross-linking method reveals a direct association between claudin-1 and tetraspanin CD9.

作者信息

Kovalenko Oleg V, Yang Xiuwei H, Hemler Martin E

机构信息

Department of Cancer Immunology and AIDS, Dana-Farber Cancer Institute, Harvard Medical School, Boston, Massachusetts 02115, USA.

出版信息

Mol Cell Proteomics. 2007 Nov;6(11):1855-67. doi: 10.1074/mcp.M700183-MCP200. Epub 2007 Jul 20.

DOI:10.1074/mcp.M700183-MCP200
PMID:17644758
Abstract

Tetraspanins serve as molecular organizers of multiprotein microdomains in cell membranes. Hence to understand functions of tetraspanin proteins, it is critical to identify laterally interacting partner proteins. Here we used a novel technical approach involving exposure and cross-linking of membrane-proximal cysteines coupled with LC-MS/MS protein identification. In this manner we identified nine potential tetraspanin CD9 partners, including claudin-1. Chemical cross-linking yielded a CD9-claudin-1 heterodimer, thus confirming direct association and adding claudin-1 to the short list of proteins that can directly associate with CD9. Interaction of CD9 (and other tetraspanins) with claudin-1 was supported by subcellular colocalization and was confirmed in multiple cell lines, although other claudins (claudin-2, -3, -4, -5, and -7) associated to a much lesser extent. Moreover claudin-1 was distributed very similarly to CD9 in sucrose gradients and, like CD9, was released from A431 and A549 cells upon cholesterol depletion. These biochemical features of claudin-1 are characteristic of tetraspanin microdomain proteins. Although claudins are major structural components of intercellular tight junctions, CD9-claudin-1 complexes did not reside in tight junctions, and depletion of key tetraspanins (CD9 and CD151) by small interfering RNA had no effect on paracellular permeability. However, tetraspanin depletion did cause a marked decrease in the stability of newly synthesized claudin-1. In conclusion, these results (a) validate a technical approach that appears to be particularly well suited for identifying protein partners directly associated with tetraspanins or with other proteins that contain membrane-proximal cysteines and (b) provide insight into how non-junctional claudins may be regulated in the context of tetraspanin-enriched microdomains.

摘要

四跨膜蛋白作为细胞膜中多蛋白微结构域的分子组织者。因此,要了解四跨膜蛋白的功能,识别横向相互作用的伴侣蛋白至关重要。在这里,我们采用了一种新颖的技术方法,该方法涉及膜近端半胱氨酸的暴露和交联,并结合液相色谱-串联质谱(LC-MS/MS)蛋白质鉴定。通过这种方式,我们鉴定出了九个潜在的四跨膜蛋白CD9伴侣,包括紧密连接蛋白-1。化学交联产生了CD9-紧密连接蛋白-1异二聚体,从而证实了直接关联,并将紧密连接蛋白-1添加到可与CD9直接关联的蛋白质短名单中。CD9(和其他四跨膜蛋白)与紧密连接蛋白-1的相互作用得到亚细胞共定位的支持,并在多种细胞系中得到证实,尽管其他紧密连接蛋白(紧密连接蛋白-2、-3、-4、-5和-7)的关联程度要小得多。此外,紧密连接蛋白-1在蔗糖梯度中的分布与CD9非常相似,并且与CD9一样,在胆固醇耗竭时从A431和A549细胞中释放出来。紧密连接蛋白-1的这些生化特征是四跨膜蛋白微结构域蛋白的特征。尽管紧密连接蛋白是细胞间紧密连接的主要结构成分,但CD9-紧密连接蛋白-1复合物并不存在于紧密连接中,并且通过小干扰RNA耗尽关键四跨膜蛋白(CD9和CD151)对细胞旁通透性没有影响。然而,四跨膜蛋白的耗尽确实导致新合成的紧密连接蛋白-1的稳定性显著降低。总之,这些结果(a)验证了一种技术方法,该方法似乎特别适合于识别与四跨膜蛋白或其他含有膜近端半胱氨酸的蛋白质直接相关的蛋白质伴侣,并且(b)深入了解了在富含四跨膜蛋白的微结构域背景下非连接紧密连接蛋白可能如何受到调控。

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