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矿化基质中细胞外纤溶酶依赖性蛋白水解系统的证据。

Evidence for an extracellular plasmin-dependent proteolytic system in mineralizing matrices.

作者信息

Robinson R M, Taylor R E, Birkedal-Hansen H

出版信息

Calcif Tissue Int. 1984 Jan;36(1):31-8. doi: 10.1007/BF02405291.

Abstract

Plasminogen activator, which specifically catalyzes the extracellular conversion of plasminogen to plasmin, was identified in the cell-free mineralizing matrices of enamel, dentin, cementum, and bone by a fibrinolytic overlay technique. The spatial separation in developing teeth of successive stages of dentinogenesis allowed us to identify predentin as a major site of plasminogen activator activity. In addition, plasminogen, the natural substrate for the activator, was demonstrated in predentin by immunohistochemical techniques. Extraction of human dentin/predentin with neutral demineralizing buffers solubilized the activator along with inhibitory components capable of blocking the activation of plasminogen. When resolved by polyacrylamide electrophoresis under dissociative conditions, however, the activator emerged in active form as two closely spaced bands at Mr 66,000 and 62,000. In the mineralizing enamel matrix of continuously forming rodent incisors, activator activity was limited to a 3-5 mm wide segment which marks the transition between "soft" and "chalky" enamel, whereas the entire overlying enamel organ was rich in activator activity at all developmental stages. This suggests that the activator is transported to the enamel matrix only in a narrow zone which coincides with the most rapidly mineralizing site. The coincident expression of plasminogen activator activity and mineral accretion suggests that plasmin-dependent proteolysis may play a role in the extracellular regulation of matrix mineralization.

摘要

通过纤维蛋白溶解覆盖技术,在牙釉质、牙本质、牙骨质和骨的无细胞矿化基质中鉴定出了纤溶酶原激活剂,它能特异性催化纤溶酶原在细胞外转化为纤溶酶。牙本质形成连续阶段在发育中的牙齿中的空间分离,使我们能够确定前期牙本质是纤溶酶原激活剂活性的主要部位。此外,通过免疫组织化学技术在前期牙本质中证实了激活剂的天然底物——纤溶酶原。用中性脱矿缓冲液提取人牙本质/前期牙本质,可使激活剂与能够阻断纤溶酶原激活的抑制成分一起溶解。然而,在解离条件下通过聚丙烯酰胺电泳分离时,激活剂以活性形式出现,表现为两条紧密相邻的条带,分子量分别为66,000和62,000。在不断生长的啮齿动物切牙的矿化牙釉质基质中,激活剂活性仅限于一个3 - 5毫米宽的区域,该区域标志着“软”牙釉质和“白垩质”牙釉质之间的过渡,而整个覆盖的牙釉质器官在所有发育阶段都富含激活剂活性。这表明激活剂仅在与矿化最快部位重合的狭窄区域被转运到牙釉质基质中。纤溶酶原激活剂活性与矿物质沉积的同时表达表明,纤溶酶依赖性蛋白水解可能在基质矿化的细胞外调节中发挥作用。

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