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荧光成像技术追踪破骨细胞前体的全身循环和骨募集。

Systemic circulation and bone recruitment of osteoclast precursors tracked by using fluorescent imaging techniques.

机构信息

Laboratory of Cellular Dynamics, World Premier International Research Center Initiative-Immunology Frontier Research Center, Osaka University, Suita, Osaka 565-0871, Japan.

出版信息

J Immunol. 2013 Jan 15;190(2):605-12. doi: 10.4049/jimmunol.1201345. Epub 2012 Dec 14.


DOI:10.4049/jimmunol.1201345
PMID:23241888
Abstract

Osteoclasts are bone-resorbing polykaryons differentiated from monocyte/macrophage-lineage hematopoietic precursors. It remains unclear whether osteoclasts originate from circulating blood monocytes or from bone tissue-resident precursors. To address this question, we combined two different experimental procedures: 1) shared blood circulation "parabiosis" with fluorescently labeled osteoclast precursors, and 2) photoconversion-based cell tracking with a Kikume Green-Red protein (KikGR). In parabiosis, CX(3)CR1-EGFP knock-in mice in which osteoclast precursors were labeled with EGFP were surgically connected with wild-type mice to establish a shared circulation. Mature EGFP(+) osteoclasts were found in the bones of the wild-type mice, indicating the mobilization of EGFP(+) osteoclast precursors into bones from systemic circulation. Receptor activator for NF-κB ligand stimulation increased the number of EGFP(+) osteoclasts in wild-type mice, suggesting that this mobilization depends on the bone resorption state. Additionally, KikGR(+) monocytes (including osteoclast precursors) in the spleen were exposed to violet light, and 2 d later we detected photoconverted "red" KikGR(+) osteoclasts along the bone surfaces. These results indicate that circulating monocytes from the spleen entered the bone spaces and differentiated into mature osteoclasts during a certain period. The current study used fluorescence-based methods clearly to demonstrate that osteoclasts can be generated from circulating monocytes once they home to bone tissues.

摘要

破骨细胞是由单核细胞/巨噬细胞谱系造血前体细胞分化而来的具有多核的骨吸收细胞。目前仍不清楚破骨细胞是来源于循环血液中的单核细胞,还是来源于骨组织中的固有前体细胞。为了解决这个问题,我们结合了两种不同的实验程序:1)带有荧光标记的破骨细胞前体的共享血液循环“联体共生”,和 2)基于光转化的细胞追踪技术与 Kikume 绿-红蛋白(KikGR)。在联体共生中,用 EGFP 标记破骨细胞前体的 CX(3)CR1-EGFP 敲入小鼠与野生型小鼠进行手术连接,以建立共享循环。在野生型小鼠的骨骼中发现了成熟的 EGFP(+)破骨细胞,这表明 EGFP(+)破骨细胞前体从全身循环动员到骨骼中。核因子-κB 配体(receptor activator for NF-κB ligand,RANKL)刺激增加了野生型小鼠中 EGFP(+)破骨细胞的数量,这表明这种动员依赖于骨吸收状态。此外,脾脏中的 KikGR(+)单核细胞(包括破骨细胞前体)被暴露于紫光下,2 天后,我们在骨表面检测到光转化的“红色”KikGR(+)破骨细胞。这些结果表明,来自脾脏的循环单核细胞可以进入骨腔,并在一定时间内分化为成熟的破骨细胞。本研究使用荧光方法清楚地表明,破骨细胞可以从循环单核细胞中产生,一旦它们归巢到骨组织中。

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