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组织蛋白酶K介导的荧光的非侵入性光学检测揭示了体外和体内破骨细胞的活性。

Non-invasive optical detection of cathepsin K-mediated fluorescence reveals osteoclast activity in vitro and in vivo.

作者信息

Kozloff Kenneth M, Quinti Luisa, Patntirapong Somying, Hauschka Peter V, Tung Ching-Hsuan, Weissleder Ralph, Mahmood Umar

机构信息

Center for Molecular Imaging Research, Harvard Medical School, Massachusetts General Hospital, 149 13th Street, Room 5406, Charlestown, MA 02129-2060, USA.

出版信息

Bone. 2009 Feb;44(2):190-8. doi: 10.1016/j.bone.2008.10.036. Epub 2008 Oct 22.

Abstract

Osteoclasts degrade bone matrix by demineralization followed by degradation of type I collagen through secretion of the cysteine protease, cathepsin K. Current imaging modalities are insufficient for sensitive observation of osteoclast activity, and in vivo live imaging of osteoclast resorption of bone has yet to be demonstrated. Here, we describe a near-infrared fluorescence reporter probe whose activation by cathepsin K is shown in live osteoclast cells and in mouse models of development and osteoclast upregulation. Cathepsin K probe activity was monitored in live osteoclast cultures and correlates with cathepsin K gene expression. In ovariectomized mice, cathepsin K probe upregulation precedes detection of bone loss by micro-computed tomography. These results are the first to demonstrate non-invasive visualization of bone degrading enzymes in models of accelerated bone loss, and may provide a means for early diagnosis of upregulated resorption and rapid feedback on efficacy of treatment protocols prior to significant loss of bone in the patient.

摘要

破骨细胞通过脱矿质作用降解骨基质,随后通过分泌半胱氨酸蛋白酶组织蛋白酶K来降解I型胶原蛋白。目前的成像方式不足以灵敏地观察破骨细胞的活性,并且破骨细胞对骨的吸收在体内的实时成像尚未得到证实。在此,我们描述了一种近红外荧光报告探针,其在活破骨细胞以及发育和破骨细胞上调的小鼠模型中显示出被组织蛋白酶K激活。在活破骨细胞培养物中监测组织蛋白酶K探针的活性,并且其与组织蛋白酶K基因表达相关。在去卵巢小鼠中,组织蛋白酶K探针上调先于通过微型计算机断层扫描检测到骨质流失。这些结果首次证明了在骨质加速流失模型中骨降解酶的非侵入性可视化,并且可能为早期诊断吸收上调以及在患者出现明显骨质流失之前对治疗方案的疗效提供快速反馈提供一种手段。

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