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有证据表明,猪表皮中主要的78 - 44kD伴刀豆球蛋白A结合糖多肽是在终末分化过程中桥粒糖蛋白降解产生的。

Evidence that major 78-44-kD concanavalin A-binding glycopolypeptides in pig epidermis arise from the degradation of desmosomal glycoproteins during terminal differentiation.

作者信息

King I A, Tabiowo A, Fryer P R

机构信息

Dermatology Research Group, Medical Research Council, Clinical Research Centre, Harrow, United Kingdom.

出版信息

J Cell Biol. 1987 Dec;105(6 Pt 2):3053-63. doi: 10.1083/jcb.105.6.3053.

Abstract

The major concanavalin A (Con A)-binding component in urea/deoxycholate/mercaptoethanol extracts from pig ear epidermis had an apparent Mr of 78 kD. In indirect immunofluorescence affinity-purified polyclonal antibodies against this glycopolypeptide strongly stained the surface of suprabasal cells in the epidermis of pig and human skin. Immunocytochemical labeling with gold-labeled second antibody localized this staining to externally disposed, trypsin-sensitive components of desmosomes. Western blotting showed that the 78-kD glycopolypeptide was immunologically related to several other Con A-binding components in pig epidermis. Immunoreactive components with Mr of 115 and 100 kD were membrane-bound, appeared to be susceptible to trypsin in intact epidermis, and were absent from the stratum corneum. Immunoreactive components of lower Mr (78-44 kD) were not membrane-bound, were resistant to trypsin in intact tissue, and were present predominantly in the keratinized layers of pig epidermis. The 115-44-kD glycopolypeptides were also recognized by antisera raised against desmoglein II/desmocollin glycoproteins isolated from bovine spinous layer desmosomes. In addition, these antisera reacted with 120- and 105-kD bands that were apparently not recognized by the anti-78-kD glycopolypeptide antiserum in immunoblotting. In immune precipitation the anti-78-kD glycopolypeptide and antidesmoglein II/desmocollin antisera precipitated comparable amounts of the radioiodinated 78-44-kD components. Both antisera also precipitated the 120- and 105-kD components although the anti-78-kD glycopolypeptide serum was less effective. Little reaction with the 115- and 105-kD components was observed in immune precipitation with either serum. Proteolytic peptide mapping confirmed that the various immunoreactive glycopolypeptides were biochemically as well as immunologically related. The results suggest that terminal differentiation in pig epidermis is accompanied by the orderly degradation of desmoglein II/desmocollin glycoproteins resulting in the accumulation of 78-44-kD glycopolypeptides in the stratum corneum. These glycopolypeptides may represent functionally important nonmembranous domains of cell-adhesion molecules in desmosomes.

摘要

猪耳表皮尿素/脱氧胆酸盐/巯基乙醇提取物中主要的伴刀豆球蛋白A(Con A)结合成分的表观分子量为78 kD。在间接免疫荧光实验中,针对这种糖多肽的亲和纯化多克隆抗体强烈地标记了猪和人类皮肤表皮中基底层以上细胞的表面。用金标二抗进行免疫细胞化学标记将这种标记定位到桥粒外部、对胰蛋白酶敏感的成分上。蛋白质印迹分析表明,78-kD糖多肽在免疫上与猪表皮中的其他几种Con A结合成分相关。分子量为115和100 kD的免疫反应性成分与膜结合,在完整表皮中似乎对胰蛋白酶敏感,且角质层中不存在。分子量较低(78 - 44 kD)的免疫反应性成分不与膜结合,在完整组织中对胰蛋白酶有抗性,且主要存在于猪表皮的角质化层中。115 - 44 kD的糖多肽也被针对从牛棘层桥粒中分离出的桥粒芯糖蛋白II/桥粒胶蛋白糖蛋白产生的抗血清所识别。此外,在蛋白质印迹分析中,这些抗血清与120和105 kD的条带发生反应,而抗78-kD糖多肽抗血清显然不识别这些条带。在免疫沉淀实验中,抗78-kD糖多肽抗血清和抗桥粒芯糖蛋白II/桥粒胶蛋白抗血清沉淀出等量的放射性碘化78 - 44 kD成分。两种抗血清也沉淀出120和105 kD成分,不过抗78-kD糖多肽血清的效果较差。用任何一种血清进行免疫沉淀时,与115和105 kD成分的反应都很弱。蛋白水解肽图谱分析证实,各种免疫反应性糖多肽在生化和免疫方面都相关。结果表明,猪表皮的终末分化伴随着桥粒芯糖蛋白II/桥粒胶蛋白糖蛋白的有序降解,导致角质层中积累78 - 44 kD的糖多肽。这些糖多肽可能代表桥粒中细胞粘附分子功能上重要的非膜结构域。

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本文引用的文献

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