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鸡骨细胞的原代培养物在骨细胞之间以及骨细胞与成骨细胞之间保留了功能性缝隙连接。

Primary cultures of chick osteocytes retain functional gap junctions between osteocytes and between osteocytes and osteoblasts.

作者信息

Kamioka Hiroshi, Ishihara Yoshihito, Ris Hans, Murshid Sakhr A, Sugawara Yasuyo, Takano-Yamamoto Teruko, Lim Soo-Siang

机构信息

Department of Orthodontics and Dentofacial Orthopedics, Okayama University Graduate School of Medicine, Dentistry, and Pharmaceutical Sciences, Okayama, Japan.

出版信息

Microsc Microanal. 2007 Apr;13(2):108-17. doi: 10.1017/S143192760707016X.

Abstract

The inaccessibility of osteocytes due to their embedment in the calcified bone matrix in vivo has precluded direct demonstration that osteocytes use gap junctions as a means of intercellular communication. In this article, we report successfully isolating primary cultures of osteocytes from chick calvaria, and, using anti-connexin 43 immunocytochemistry, demonstrate gap junction distribution to be comparable to that found in vivo. Next, we demonstrate the functionality of the gap junctions by (1) dye coupling studies that showed the spread of microinjected Lucifer Yellow from osteoblast to osteocyte and between adjacent osteocytes and (2) analysis of fluorescence replacement after photobleaching (FRAP), in which photobleaching of cells loaded with a membrane-permeable dye resulted in rapid recovery of fluorescence into the photobleached osteocyte, within 5 min postbleaching. This FRAP effect did not occur when cells were treated with a gap junction blocker (18alpha-glycyrrhetinic acid), but replacement of fluorescence into the photobleached cell resumed when it was removed. These studies demonstrate that gap junctions are responsible for intercellular communication between adjacent osteocytes and between osteoblasts and osteocytes. This role is consistent with the ability of osteocytes to respond to and transmit signals over long distances while embedded in a calcified matrix.

摘要

由于骨细胞在体内嵌入钙化的骨基质中,难以接近,这使得无法直接证明骨细胞利用缝隙连接作为细胞间通讯的一种方式。在本文中,我们报告了成功从鸡颅盖骨中分离出骨细胞原代培养物,并使用抗连接蛋白43免疫细胞化学方法,证明缝隙连接的分布与体内发现的分布相当。接下来,我们通过以下方式证明缝隙连接的功能:(1)染料偶联研究,显示微注射的荧光素黄从成骨细胞扩散到骨细胞以及相邻骨细胞之间;(2)光漂白后荧光恢复分析(FRAP),其中用膜通透性染料加载的细胞进行光漂白后,在漂白后5分钟内荧光迅速恢复到被光漂白的骨细胞中。当细胞用缝隙连接阻滞剂(18α-甘草次酸)处理时,这种FRAP效应不会发生,但当去除阻滞剂时,荧光又会恢复到被光漂白的细胞中。这些研究表明,缝隙连接负责相邻骨细胞之间以及成骨细胞与骨细胞之间的细胞间通讯。这一作用与骨细胞在嵌入钙化基质时能够对信号做出反应并进行长距离信号传递的能力相一致。

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