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牙骨质蛋白的细胞附着活性及内毒素抑制机制。

Cell attachment activity of cementum proteins and mechanism of endotoxin inhibition.

作者信息

Olson S, Arzate H, Narayanan A S, Page R C

机构信息

Department of Pathology, University of Washington, Seattle 98195.

出版信息

J Dent Res. 1991 Sep;70(9):1272-7. doi: 10.1177/00220345910700090801.

Abstract

Cementum occupies a unique anatomical location where soft connective tissues of the periodontium are attached to root surfaces. Cell attachment properties of proteins present in cementum were studied. Human and bovine cementum were extracted with 0.5 mol/L CH3COOH followed by 4 mol/L guanidine, and proteins were separated by ion-exchange chromatography and SDS-polyacrylamide gel electrophoresis. Cells were labeled with radioactive amino acids and added to tissue-culture plastic plates incubated with cementum proteins, and attachment was measured. Results showed that cementum proteins promoted the attachment of smooth muscle cells, endothelial cells, and fibroblasts, but not epithelial cells. Fibroblasts attached more efficiently than other cell types, and they manifested spreading with re-organization of actin filaments. No attachment occurred to plates incubated with endotoxin from A. actinomycetemcomitans. Fewer fibroblasts attached to plates treated with cementum proteins in the presence of endotoxin, but cells pre-treated with endotoxin attached normally. Attachment was not inhibited when plates were incubated first with attachment proteins and then with endotoxin; however, it was decreased when endotoxin or bovine serum albumin preceded cementum proteins. Cementum proteins with Mr 68,000, 61,000, 55,000, and 36,000 (p68, p61, p55, and p36, respectively) manifested attachment activity, while protein(s) with Mr 23,000-24,000 did not. Western blots revealed that guanidine extracts contained three bands cross-reacting with anti-bovine sialoprotein-II antibody, but the p61, p55, and p36 were negative. We conclude that cementum contains bovine sialoprotein-II and at least four other fibroblast attachment proteins, and that they do not support epithelial cell attachment.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

牙骨质占据着牙周膜的软结缔组织附着于牙根表面的独特解剖位置。对牙骨质中存在的蛋白质的细胞附着特性进行了研究。用人和牛的牙骨质先后用0.5 mol/L的CH₃COOH和4 mol/L的胍进行提取,然后通过离子交换色谱法和十二烷基硫酸钠-聚丙烯酰胺凝胶电泳对蛋白质进行分离。用放射性氨基酸标记细胞,并将其添加到与牙骨质蛋白一起孵育的组织培养塑料平板中,然后测量细胞附着情况。结果表明,牙骨质蛋白能促进平滑肌细胞、内皮细胞和成纤维细胞的附着,但不能促进上皮细胞的附着。成纤维细胞比其他细胞类型更有效地附着,并且它们表现出肌动蛋白丝重新组织的铺展。与伴放线放线杆菌的内毒素一起孵育的平板未发生细胞附着。在内毒素存在的情况下,与牙骨质蛋白处理过的平板上附着的成纤维细胞较少,但预先用内毒素处理过的细胞能正常附着。当平板先与附着蛋白孵育然后再与内毒素孵育时,附着并未受到抑制;然而,当内毒素或牛血清白蛋白先于牙骨质蛋白时,附着则减少。分子量为68,000、61,000、55,000和36,000的牙骨质蛋白(分别为p68、p61、p55和p36)表现出附着活性,而分子量为23,000 - 24,000的蛋白质则没有。蛋白质免疫印迹显示,胍提取物中有三条带与抗牛唾液酸蛋白-II抗体发生交叉反应,但p61、p55和p36呈阴性。我们得出结论,牙骨质含有牛唾液酸蛋白-II和至少四种其他成纤维细胞附着蛋白,并且它们不支持上皮细胞附着。(摘要截短于250字)

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