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胎猪颅骨细胞体外合成骨连接蛋白

Biosynthesis of osteonectin by fetal porcine calvarial cells in vitro.

作者信息

Otsuka K, Yao K L, Wasi S, Tung P S, Aubin J E, Sodek J, Termine J D

出版信息

J Biol Chem. 1984 Aug 10;259(15):9805-12.

PMID:6086651
Abstract

The biosynthesis of osteonectin, a major glycoprotein of bone, has been studied in vitro using bone cells from fetal porcine calvariae. The calvarial cells, which were shown to produce osteonectin by immunotransfer and immunocytochemical analysis, were pulse labeled with [35S]methionine and the radiolabeled osteonectin in the cell layers and in the chase-medium was isolated by specific immunoprecipitation. The osteonectin, representing 0.1% of the radiolabeled cell layer and 1% of the medium proteins, co-migrated with authentic bovine osteonectin on sodium dodecyl sulfate-polyacrylamide gel electrophoresis under reduced and nonreduced conditions (Mr approximately 40,000), and was bound selectively to hydroxyapatite in the presence of 4 M guanidine HCl. The co-migration of the osteonectins indicates that the tissue-extracted osteonectin represents an intact protein and that a pro- form of osteonectin is unlikely. However, a preosteonectin form (Mr approximately 46,000) could be immunoprecipitated from cell-free translation of calvarial mRNA. The minimal secretion time for osteonectin synthesized in serum-containing medium was found to be approximately 40 min but maximal accumulation did not occur until 2 h postlabeling. In serum-free media, extensive degradation of osteonectin, characterized by the presence of two immunoprecipitable fragments (Mr approximately 36,000 and 31,000), was evident.

摘要

利用来自胎猪颅骨的骨细胞在体外研究了骨粘连蛋白(一种主要的骨糖蛋白)的生物合成。通过免疫印迹和免疫细胞化学分析表明能产生骨粘连蛋白的颅骨细胞,用[35S]甲硫氨酸进行脉冲标记,然后通过特异性免疫沉淀分离细胞层和追踪培养基中的放射性标记骨粘连蛋白。骨粘连蛋白占放射性标记细胞层的0.1%,占培养基蛋白的1%,在还原和非还原条件下,在十二烷基硫酸钠-聚丙烯酰胺凝胶电泳上与纯牛骨粘连蛋白共迁移(分子量约40,000),并且在4M盐酸胍存在下选择性地结合到羟基磷灰石上。骨粘连蛋白的共迁移表明组织提取的骨粘连蛋白代表一种完整的蛋白质,并且不太可能存在骨粘连蛋白的前体形式。然而,从颅骨mRNA的无细胞翻译中可以免疫沉淀出一种前骨粘连蛋白形式(分子量约46,000)。发现在含血清培养基中合成的骨粘连蛋白的最短分泌时间约为40分钟,但直到标记后2小时才出现最大积累。在无血清培养基中,骨粘连蛋白广泛降解,其特征是存在两个可免疫沉淀的片段(分子量约36,000和31,000)。

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