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从牙骨质中分离出一种成纤维细胞附着蛋白。

Isolation of a fibroblast attachment protein from cementum.

作者信息

McAllister B, Narayanan A S, Miki Y, Page R C

机构信息

Department of Periodontics, University of Texas Health Sciences Center, San Antonio.

出版信息

J Periodontal Res. 1990 Mar;25(2):99-105. doi: 10.1111/j.1600-0765.1990.tb00899.x.

Abstract

Cementum forms the interface through which soft connective tissue of the periodontium is attached to the root surface. The interactions between cementum and connective tissue are not completely understood and whether cementum influences periodontal connective tissue formation and regeneration is not clear. We have examined the effect of cementum components on the attachment of gingival fibroblasts. Cementum was harvested from healthy human and bovine teeth and extracted sequentially in 0.5 M CH3COOH, 4 M guanidine and bacterial collagenase. Fibroblast attachment was measured using 51Cr-labelled human gingival fibroblasts on tissue culture plates previously incubated with cementum components. Results showed that all three extracts mediated fibroblast attachment and attachment was dependent on concentration and incubation time. The attachment activity was not destroyed by digestion with bacterial collagenase or by antibodies to fibronectin and laminin. However, it was inhibited by a peptide containing the amino acid sequence RGD. By gel filtration or HPLC using a DEAE-cellulose column several proteins with attachment activity were fractionated. SDS-polyacrylamide gel electrophoresis revealed that HPLC fraction eluted by 0.2-0.3 M NaCl contained a protein with molecular weight 55 kDa as a major component. This protein was isolated and shown to promote fibroblast attachment, and optimal attachment occurred at a concentration of 2 micrograms/ml. We conclude that cementum contains substances capable of mediating fibroblast attachment and that these substances play an important role in periodontal connective tissue formation and regeneration by facilitating fibroblast attachment to root surfaces.

摘要

牙骨质形成了牙周膜的软结缔组织附着于牙根表面的界面。牙骨质与结缔组织之间的相互作用尚未完全明了,牙骨质是否影响牙周结缔组织的形成和再生也不清楚。我们研究了牙骨质成分对牙龈成纤维细胞附着的影响。从健康人牙和牛牙采集牙骨质,并依次用0.5M醋酸、4M胍和细菌胶原酶进行提取。使用51Cr标记的人牙龈成纤维细胞在预先用牙骨质成分孵育的组织培养板上测量成纤维细胞的附着。结果表明,所有三种提取物都介导成纤维细胞附着,且附着依赖于浓度和孵育时间。附着活性不会因用细菌胶原酶消化或用抗纤连蛋白和层粘连蛋白的抗体处理而被破坏。然而,它会被含有氨基酸序列RGD的肽抑制。通过凝胶过滤或使用DEAE-纤维素柱的高效液相色谱法,分离出了几种具有附着活性的蛋白质。十二烷基硫酸钠-聚丙烯酰胺凝胶电泳显示,用0.2-0.3M氯化钠洗脱的高效液相色谱级分含有一种分子量为55kDa的蛋白质作为主要成分。该蛋白质被分离出来并显示能促进成纤维细胞附着,最佳附着浓度为2微克/毫升。我们得出结论,牙骨质含有能够介导成纤维细胞附着的物质,并且这些物质通过促进成纤维细胞附着于牙根表面,在牙周结缔组织的形成和再生中发挥重要作用。

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