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通过胰蛋白酶肽段分析证实表皮前丝聚合蛋白中存在多个磷酸化丝聚合蛋白拷贝。

Multiple copies of phosphorylated filaggrin in epidermal profilaggrin demonstrated by analysis of tryptic peptides.

作者信息

Resing K A, Dale B A, Walsh K A

出版信息

Biochemistry. 1985 Jul 16;24(15):4167-75. doi: 10.1021/bi00336a053.

DOI:10.1021/bi00336a053
PMID:4052387
Abstract

The precursor of mouse (c57/B16) epidermal filaggrin (profilaggrin) is a very large (ca. 500 000 daltons), highly phosphorylated protein containing multiple copies of filaggrin (26 000 daltons). The conversion of profilaggrin to filaggrin late in epidermal cell differentiation involves dephosphorylation and proteolysis to yield the unphosphorylated filaggrin, which polymerizes with keratin filaments into macrofibrils. In order to gain insight in the nature of these processes, we compared tryptic digests of profilaggrin with those of filaggrin by reverse-phase liquid chromatography. Approximately 80% of the profilaggrin mass consists of multiple copies of filaggrin. Twenty peptides purified in good yield from both profilaggrin and filaggrin accounted for most of the filaggrin sequence. A detailed analysis of the yield of several peptides provided an estimate of the size and frequency of the repeat unit within profilaggrin. These data indicate that the repeating substructure of profilaggrin contains about 265 amino acids and that about 50 residues are removed per filaggrin domain as the precursor is processed to filaggrin. Assuming a molecular weight of 500 000 (as estimated from sodium dodecyl sulfate-polyacrylamide gel electrophoresis), this indicates there are 16 repeats. Analysis of phosphopeptides isolated from profilaggrin showed that 66% of the phosphate was located on peptides that are unphosphorylated in filaggrin. Analysis of peptide recoveries confirmed the repeat size and showed that every copy of filaggrin was phosphorylated in profilaggrin.

摘要

小鼠(C57/B16)表皮聚角蛋白微丝蛋白(前聚角蛋白微丝蛋白)的前体是一种非常大的(约500000道尔顿)、高度磷酸化的蛋白质,含有多个聚角蛋白微丝蛋白拷贝(26000道尔顿)。在表皮细胞分化后期,前聚角蛋白微丝蛋白转化为聚角蛋白微丝蛋白涉及去磷酸化和蛋白水解,以产生未磷酸化的聚角蛋白微丝蛋白,其与角蛋白丝聚合成大纤维。为了深入了解这些过程的本质,我们通过反相液相色谱法比较了前聚角蛋白微丝蛋白和聚角蛋白微丝蛋白的胰蛋白酶消化产物。前聚角蛋白微丝蛋白质量的约80%由多个聚角蛋白微丝蛋白拷贝组成。从前聚角蛋白微丝蛋白和聚角蛋白微丝蛋白中以高产率纯化的20种肽占了聚角蛋白微丝蛋白序列的大部分。对几种肽产量的详细分析提供了前聚角蛋白微丝蛋白中重复单元大小和频率的估计。这些数据表明,前聚角蛋白微丝蛋白的重复亚结构包含约265个氨基酸,并且在前体加工成聚角蛋白微丝蛋白时,每个聚角蛋白微丝蛋白结构域约有50个残基被去除。假设分子量为500000(如从十二烷基硫酸钠-聚丙烯酰胺凝胶电泳估计),这表明有16个重复。对从前聚角蛋白微丝蛋白中分离的磷酸肽的分析表明,66%的磷酸盐位于聚角蛋白微丝蛋白中未磷酸化的肽上。肽回收率的分析证实了重复大小,并表明聚角蛋白微丝蛋白的每个拷贝在前聚角蛋白微丝蛋白中都被磷酸化。

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