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应激诱导表皮斑蛋白募集到角蛋白网络,增强了其对过度磷酸化诱导破坏的抗性。

Stress-induced recruitment of epiplakin to keratin networks increases their resistance to hyperphosphorylation-induced disruption.

作者信息

Spazierer Daniel, Raberger Julia, Gross Karin, Fuchs Peter, Wiche Gerhard

机构信息

Department of Molecular Cell Biology, Max F. Perutz Laboratories, University of Vienna, A-1030 Vienna, Austria.

出版信息

J Cell Sci. 2008 Mar 15;121(Pt 6):825-33. doi: 10.1242/jcs.013755. Epub 2008 Feb 19.

DOI:10.1242/jcs.013755
PMID:18285451
Abstract

Epiplakin is a large (>725 kDa) cytoskeletal protein exclusively expressed in epithelial tissues. It has a unique structure, consisting entirely of plakin repeat domains (PRDs), one of the hallmarks of spectraplakin protein family members. Previous studies, including the phenotypic analyses of knockout mice, failed to reveal the biological function of epiplakin. Using in vitro binding assays, we show here that all but one of the 16 PRDs of mouse epiplakin bind to keratins of basal keratinocytes. Nevertheless, in primary keratinocyte cell cultures, epiplakin only partially colocalized with keratin intermediate filament networks. However, upon application of cellular stress in the form of keratin hyperphosphorylation, osmotic shock or UV irradiation, the entire cytoplasmic epiplakin pool became associated with keratin. In response to such types of stress, epiplakin initially translocated to the still-intact keratin filament network and remained associated with keratin after its disruption and transformation into granular aggregates. Time-course experiments revealed that serine/threonine (okadaic acid) and tyrosine (orthovanadate) phosphatase inhibitor-induced filament disruption in differentiated keratinocytes proceeded faster in epiplakin-deficient cells compared with wild-type cells. Our data suggest that epiplakin plays a role in keratin filament reorganization in response to stress, probably by protecting keratin filaments against disruption in a chaperone-like fashion.

摘要

表皮 plak 蛋白是一种仅在上皮组织中表达的大型(>725 kDa)细胞骨架蛋白。它具有独特的结构,完全由 plak 重复结构域(PRD)组成,这是光谱 plak 蛋白家族成员的标志之一。包括基因敲除小鼠的表型分析在内的先前研究未能揭示表皮 plak 蛋白的生物学功能。通过体外结合试验,我们在此表明,小鼠表皮 plak 蛋白的 16 个 PRD 中除一个外均与基底角质形成细胞的角蛋白结合。然而,在原代角质形成细胞培养物中,表皮 plak 蛋白仅部分与角蛋白中间丝网络共定位。然而,当以角蛋白过度磷酸化、渗透休克或紫外线照射的形式施加细胞应激时,整个细胞质中的表皮 plak 蛋白池与角蛋白结合。针对此类应激,表皮 plak 蛋白最初转移至仍完整的角蛋白丝网络,并在其破坏并转化为颗粒聚集体后仍与角蛋白结合。时间进程实验表明,与野生型细胞相比,在表皮 plak 蛋白缺陷细胞中,丝氨酸/苏氨酸(冈田酸)和酪氨酸(原钒酸钠)磷酸酶抑制剂诱导的分化角质形成细胞中的丝断裂进行得更快。我们的数据表明,表皮 plak 蛋白可能通过以伴侣样方式保护角蛋白丝免受破坏,在应激反应中对角蛋白丝重组起作用。

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