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人类角蛋白丝聚集蛋白-2 的脱亚氨基作用促进钙蛋白酶 1 对其的蛋白水解。

Deimination of human filaggrin-2 promotes its proteolysis by calpain 1.

机构信息

UMR5165 CNRS, F-31059 Toulouse, France.

出版信息

J Biol Chem. 2011 Jul 1;286(26):23222-33. doi: 10.1074/jbc.M110.197400. Epub 2011 Apr 29.

Abstract

Filaggrin-2 (FLG2), a member of the S100-fused type protein family, shares numerous features with filaggrin (FLG), a key protein implicated in the epidermal barrier functions. Both display a related structural organization, an identical pattern of expression and localization in human epidermis, and proteolytic processing of a large precursor. Here, we tested whether FLG2 was a substrate of calpain 1, a calcium-dependent protease directly involved in FLG catabolism. In addition, deimination being critical for FLG degradation, we analyzed whether FLG2 deimination interfered with its proteolytic processing. With this aim, we first produced a recombinant form of FLG2 corresponding to subunits B7 to B10 fused to a COOH-terminal His tag. Incubation with calpain 1 in the presence of calcium induced a rapid degradation of the recombinant protein and the production of several peptides, as shown by Coomassie Blue-stained gels and Western blotting with anti-FLG2 or anti-His antibodies. MALDI-TOF mass spectrometry confirmed this result and further evidenced the production of non-immunoreactive smaller peptides. The degradation was not observed when a calpain 1-specific inhibitor was added. The calpain cleavage sites identified by Edman degradation were regularly present in the B-type repeats of FLG2. Moreover, immunohistochemical analysis of normal human skin revealed colocalization of FLG2 and calpain 1 in the upper epidermis. Finally, the FLG2 deiminated by human peptidylarginine deiminases was shown to be more susceptible to calpain 1 than the unmodified protein. Altogether, these data demonstrate that calpain 1 is essential for the proteolytic processing of FLG2 and that deimination accelerates this process.

摘要

丝聚合蛋白-2(FLG2)是 S100 融合型蛋白家族的成员,与丝聚合蛋白(FLG)有许多共同特征,FLG 是一种与表皮屏障功能有关的关键蛋白。两者均显示出相关的结构组织、在人表皮中相同的表达和定位模式以及大前体的蛋白水解加工。在这里,我们测试了 FLG2 是否是钙依赖性蛋白酶钙蛋白酶 1 的底物,钙蛋白酶 1 直接参与 FLG 的代谢。此外,脱亚氨基作用对于 FLG 的降解至关重要,我们分析了 FLG2 的脱亚氨基作用是否干扰其蛋白水解加工。为此,我们首先产生了一种对应于 B7 至 B10 亚基与 COOH 端 His 标签融合的重组 FLG2 形式。在存在钙的情况下用钙蛋白酶 1 孵育会导致重组蛋白的快速降解,并产生几种肽,如考马斯亮蓝染色凝胶和抗-FLG2 或抗-His 抗体的 Western 印迹所示。MALDI-TOF 质谱证实了这一结果,并进一步证明了产生非免疫反应性较小肽。当添加钙蛋白酶 1 的特异性抑制剂时,未观察到降解。通过 Edman 降解鉴定的钙蛋白酶切割位点通常存在于 FLG2 的 B 型重复序列中。此外,对正常人皮肤的免疫组织化学分析显示 FLG2 和钙蛋白酶 1 在表皮上层共定位。最后,人肽基精氨酸脱亚氨酶脱亚氨基的 FLG2 比未修饰的蛋白更容易受到钙蛋白酶 1 的影响。总之,这些数据表明钙蛋白酶 1 是 FLG2 蛋白水解加工所必需的,并且脱亚氨基作用加速了这一过程。

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