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一种用于研究软骨蛋白聚糖代谢的“耦合”软骨下骨-关节软骨组织培养系统。

A "coupled" subchondral bone-articular cartilage tissue culture system for the study of cartilage proteoglycan metabolism.

作者信息

Athanassiades A, Anastassiades T P

机构信息

Department of Medicine, Queen's University, Kingston, Ontario, Canada.

出版信息

In Vitro Cell Dev Biol Anim. 1994 Aug;30A(8):504-11.

PMID:7987538
Abstract

Current evidence suggests that interactions between the subchondral bone and the articular cartilage of mammalian diarthrodial joints may occur through the action of bone-associated peptide factors. However, there is no suitable organ culture model for studying these interactions. This study defines a long-term tissue culture system where the articular cartilage is coupled to the adjacent subchondral bone obtained from the proximal ends of bovine metacarpals. Autoradiography done over 3 mo., by utilizing [35S]SO4 incorporation into cartilage proteoglycan (PG) and a procedure for cutting non-decalcified bone, demonstrated similar numbers of silver grains over chondrocytes in all cartilage zones, including the bone-cartilage interface. Newly synthesized PG (NSPG) from the cartilage of the "coupled" system over a 3-wk period was primarily of large hydrodynamic size (Kav of 0.34). Comparable bovine articular and nasal cartilage slice systems, incubated for short periods of time, yielded similar and somewhat larger NSPG, respectively. Labeled chondroitin sulphate PG accumulating in the medium of primary chondrocyte monolayer cultures, derived from the cartilage of the coupled system at 0, 1, 2, and 3 wk, revealed two polydisperse subpopulations (Kav of 0.30 to 0.38 and 0.51 to 0.68). We conclude that this coupled bone-cartilage system is viable for prolonged periods, is suitable for studies on the metabolism of articular cartilage PGs, and seems to have some advantages over the cultured articular cartilage slice system.

摘要

目前的证据表明,哺乳动物动关节的软骨下骨与关节软骨之间的相互作用可能通过骨相关肽因子的作用发生。然而,尚无合适的器官培养模型来研究这些相互作用。本研究定义了一种长期组织培养系统,其中关节软骨与从牛掌骨近端获取的相邻软骨下骨相连。通过利用[35S]SO4掺入软骨蛋白聚糖(PG)并采用切割未脱钙骨的方法,在3个月内进行放射自显影,结果显示在所有软骨区域,包括骨-软骨界面,软骨细胞上的银粒数量相似。“相连”系统的软骨在3周内新合成的PG(NSPG)主要具有较大的流体力学尺寸(洗脱体积Kav为0.34)。较短时间孵育的可比牛关节软骨和鼻软骨切片系统分别产生了相似且稍大的NSPG。在0、1、2和3周时,从相连系统的软骨中获取的原代软骨细胞单层培养物的培养基中积累的标记硫酸软骨素PG显示出两个多分散亚群(洗脱体积Kav为0.30至0.38和0.51至0.68)。我们得出结论,这种骨-软骨相连系统在长时间内是有活力的,适用于关节软骨PG代谢的研究,并且似乎比培养的关节软骨切片系统具有一些优势。

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In Vitro Cell Dev Biol Anim. 1998 Jun;34(6):492-8. doi: 10.1007/s11626-998-0084-z.