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破骨细胞前体的动力学和细胞化学鉴定及其向多核破骨细胞的分化。

Kinetic and cytochemical identification of osteoclast precursors and their differentiation into multinucleated osteoclasts.

作者信息

Baron R, Neff L, Tran Van P, Nefussi J R, Vignery A

出版信息

Am J Pathol. 1986 Feb;122(2):363-78.

Abstract

Positive identification of osteoclast percursors has not yet been possible. The authors have, in the present report, used a model system in the rat in which it is possible to induce the formation of multinucleated osteoclasts at a predictable and reproducible site and time (Tran Van P, Vignery A, Baron R. Anat Rec 1982, 202:445-451; Cell Tissue Res 1982, 225:283-292). This system allowed the investigation of the cellular events occurring locally during the recruitment and differentiation of osteoclast precursors. Prior to the formation of multinucleated osteoclasts, mononuclear cells positive for fluoride-inhibitable nonspecific esterase and cells positive for tartrate-resistant acid phosphatase increase in number locally. Double staining procedures demonstrated the presence of both enzymes in a number of cells, thereby suggesting that they are steps in the differentiation of a single cell population. Ultrastructural studies show that lysosomal enzymes are present in every compartment of the biosynthetic pathway, in small primary lysosomes and various forms of storage granules. As these precursors arrive at the bone surface, the storage granule lysosomes are markedly depleted. It is concluded that mononuclear precursors of the osteoclast are members of the mononuclear-phagocyte lineage and differentiate early to synthesize, store, and later secrete large quantities of lysosomal enzymes. The mature osteoclast, which, as its precursor, is positive for the mononuclear-phagocyte marker enzyme nonspecific esterase, results from the fusion of these mononuclear precursors, which occurs only after their attachment to the bone surface to be resorbed.

摘要

目前尚未能够对破骨细胞前体进行确切鉴定。在本报告中,作者使用了大鼠模型系统,在此系统中能够在可预测且可重复的部位和时间诱导多核破骨细胞的形成(Tran Van P, Vignery A, Baron R.《解剖学记录》1982年,202:445 - 451;《细胞与组织研究》1982年,225:283 - 292)。该系统使得研究破骨细胞前体募集和分化过程中局部发生的细胞事件成为可能。在多核破骨细胞形成之前,氟化物抑制性非特异性酯酶阳性的单核细胞以及抗酒石酸酸性磷酸酶阳性的细胞在局部数量增加。双重染色程序显示许多细胞中同时存在这两种酶,从而表明它们是单个细胞群体分化过程中的步骤。超微结构研究表明,溶酶体酶存在于生物合成途径的每个区室、小的初级溶酶体和各种形式的储存颗粒中。当这些前体到达骨表面时,储存颗粒溶酶体明显减少。得出的结论是,破骨细胞的单核前体是单核吞噬细胞谱系的成员,并且早期分化以合成、储存并随后分泌大量溶酶体酶。成熟破骨细胞作为其前体,对单核吞噬细胞标记酶非特异性酯酶呈阳性,是由这些单核前体融合形成的,这种融合仅在它们附着于待吸收的骨表面后发生。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0e36/1888102/e5f88d2a64d8/amjpathol00161-0180-a.jpg

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