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通过有限蛋白酶解鉴定出与闭合蛋白细胞骨架锚定结构域形成的体外蛋白质复合物。

In vitro protein complex formation with cytoskeleton-anchoring domain of occludin identified by limited proteolysis.

作者信息

Peng Bi-Hung, Lee J Ching, Campbell Gerald A

机构信息

Department of Pathology, The University of Texas Medical Branch, Galveston, Texas 77555-0750, USA.

出版信息

J Biol Chem. 2003 Dec 5;278(49):49644-51. doi: 10.1074/jbc.M302782200. Epub 2003 Sep 25.

DOI:10.1074/jbc.M302782200
PMID:14512431
Abstract

Occludin is an essential membrane protein component of cellular tight junctions, participating in both cell-cell adhesion in the paracellular space and anchoring of the junctional complex to the cytoskeleton. The latter function is accomplished through binding of the C-terminal cytoplasmic region to scaffolding proteins that mediate binding to cytoskeletal actin. We isolated a structural domain from both the bacterial-expressed C-terminal cytoplasmic region of human occludin and native cellular occludin, extracted from epithelial (Madin-Darby canine kidney) or endothelial (human brain) cells, by limited proteolysis with trypsin. This human occludin domain contains the last 119 amino acids as identified by N-terminal sequencing and peptide mass fingerprinting using matrix-assisted laser desorption ionization-time of flight mass spectrometry. Based on the sequence and secondary structure prediction, this domain contains 4 of 5 alpha-helices in the C-terminal region and is linked to the fourth membrane-spanning region by a loosely structured tethering polypeptide. Comparison of circular dichroism spectra of recombinant proteins corresponding to the entire C-terminal region versus only the binding domain region also supports the interpretation that the helical structural elements are concentrated in that domain. Co-immunoprecipitation of this domain with ZO-2 demonstrated preservation of the specificity of the scaffolding protein-binding function, and binding studies with immobilized ZO-2 suggest the presence of multiple ZO-2 binding sites in this domain. These results provide a basis for development of a structural model of the ZO-binding site that can be used to investigate regulation of tight junction anchoring by intracellular signaling events.

摘要

闭合蛋白是细胞紧密连接的一种重要膜蛋白成分,参与细胞旁间隙的细胞间黏附以及连接复合体与细胞骨架的锚定。后一种功能是通过C末端胞质区域与介导细胞骨架肌动蛋白结合的支架蛋白结合来实现的。我们通过用胰蛋白酶进行有限蛋白水解,从人闭合蛋白的细菌表达C末端胞质区域以及从上皮细胞(马-达二氏犬肾细胞)或内皮细胞(人脑细胞)中提取的天然细胞闭合蛋白中分离出一个结构域。通过N末端测序和使用基质辅助激光解吸电离飞行时间质谱的肽质量指纹图谱鉴定,这个人闭合蛋白结构域包含最后119个氨基酸。基于序列和二级结构预测,该结构域在C末端区域包含5个α螺旋中的4个,并通过一个结构松散的连接多肽与第四个跨膜区域相连。对应于整个C末端区域与仅结合结构域区域的重组蛋白的圆二色光谱比较也支持这样的解释,即螺旋结构元件集中在该结构域中。该结构域与ZO-2的共免疫沉淀证明了支架蛋白结合功能的特异性得以保留,并且与固定化ZO-2的结合研究表明该结构域中存在多个ZO-2结合位点。这些结果为开发ZO结合位点的结构模型提供了基础,该模型可用于研究细胞内信号事件对紧密连接锚定的调节。

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