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使用新型分子报告基因对蛋白水解酶活性进行体内成像。

In vivo imaging of proteolytic enzyme activity using a novel molecular reporter.

作者信息

Tung C H, Mahmood U, Bredow S, Weissleder R

机构信息

Center for Molecular Imaging Research, Massachusetts General Hospital, Harvard Medical School, Charlestown 02129, USA.

出版信息

Cancer Res. 2000 Sep 1;60(17):4953-8.

PMID:10987312
Abstract

The single biggest challenge facing in vivo imaging techniques is to develop biocompatible molecular beacons that are capable of specifically and accurately measuring in vivo targets at the protein, RNA, or DNA level. Our efforts have focused on developing activatable imaging probes to measure specific enzyme activities in vivo. Using cathepsin D as a model target protease, we synthesized a long-circulating, synthetic graft copolymer bearing near-infrared (NIR) fluorochromes positioned on cleavable substrate sequences. In its native state, the reporter probe was essentially nonfluorescent at 700 nm due to energy resonance transfer among the bound fluorochromes (quenching) but became brightly fluorescent when the latter were released by cathepsin D. NIR fluorescence signal activation was linear over at least 4 orders of magnitude and specific when compared with scrambled nonsense substrates. Using matched rodent tumor models implanted into nude mice expressing or lacking the targeted protease, it could be shown that the former generated sufficient NIR signal to be directly detectable and that the signal was significantly different compared with negative control tumors. The developed probes should find widespread applications for real-time in vivo imaging of a variety of clinically relevant proteases, for example, to detect endogenous protease activity in disease, to monitor the efficacy of protease inhibitors, or to image transgene expression.

摘要

体内成像技术面临的最大挑战是开发生物相容性分子信标,这种信标能够在蛋白质、RNA或DNA水平上特异性且准确地测量体内靶点。我们的工作重点是开发可激活的成像探针,以测量体内特定的酶活性。以组织蛋白酶D作为模型靶蛋白酶,我们合成了一种长循环的合成接枝共聚物,其携带位于可裂解底物序列上的近红外(NIR)荧光染料。在其天然状态下,由于结合的荧光染料之间的能量共振转移(淬灭),报告探针在700nm处基本无荧光,但当后者被组织蛋白酶D释放时会变得明亮荧光。近红外荧光信号激活在至少4个数量级上呈线性,并且与随机无义底物相比具有特异性。使用植入表达或缺乏靶向蛋白酶的裸鼠体内的匹配啮齿动物肿瘤模型,可以证明前者产生足够的近红外信号以直接检测到,并且与阴性对照肿瘤相比信号有显著差异。所开发的探针应该会在多种临床相关蛋白酶的实时体内成像中得到广泛应用,例如,检测疾病中的内源性蛋白酶活性、监测蛋白酶抑制剂的疗效或对转基因表达进行成像。

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