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利用绿色荧光蛋白进行体内氧成像。

In vivo oxygen imaging using green fluorescent protein.

作者信息

Takahashi Eiji, Takano Tomohiro, Nomura Yasutomo, Okano Satoshi, Nakajima Osamu, Sato Michihiko

机构信息

Department of Physiology, Yamagata University School of Medicine, Yamagata, Japan.

出版信息

Am J Physiol Cell Physiol. 2006 Oct;291(4):C781-7. doi: 10.1152/ajpcell.00067.2006. Epub 2006 May 31.

DOI:10.1152/ajpcell.00067.2006
PMID:16738007
Abstract

In vivo oxygen measurement is the key to understanding how biological systems dynamically adapt to reductions in oxygen supply. High spatial resolution oxygen imaging is of particular importance because recent studies address the significance of within-tissue and within-cell heterogeneities in oxygen concentration in health and disease. Here, we report a new technique for in vivo molecular imaging of oxygen in organs using green fluorescent protein (GFP). GFP-expressing COS-7 cells were briefly photoactivated with a strong blue light while lowering the oxygen concentration from 10% to <0.001%. Red fluorescence (excitation 520-550 nm, emission >580 nm) appeared after photoactivation at <2% oxygen (the red shift of GFP fluorescence). The red shift disappeared after reoxygenation of the cell, indicating that the red shift is stable as long as the cell is hypoxic. The red shift of GFP fluorescence was also demonstrated in single cardiomyocytes isolated from the GFP knock-in mouse (green mouse) heart. Then, we tried in vivo molecular imaging of hypoxia in organs. The red shift could be imaged in the ischemic liver and kidney in the green mouse using macroscopic optics provided that oxygen diffusion from the atmospheric air was prevented. In crystalloid-perfused beating heart isolated from the green mouse, significant spatial heterogeneities in the red shift were demonstrated in the epicardium distal to the coronary artery ligation. We conclude that the present technique using GFP as an oxygen indicator may allow in vivo molecular imaging of oxygen in organs.

摘要

体内氧测量是理解生物系统如何动态适应氧供应减少的关键。高空间分辨率氧成像尤为重要,因为最近的研究探讨了健康和疾病状态下组织内和细胞内氧浓度异质性的意义。在此,我们报告一种使用绿色荧光蛋白(GFP)对器官内氧进行体内分子成像的新技术。表达GFP的COS-7细胞在将氧浓度从10%降至<0.001%的同时,用强蓝光短暂光激活。在氧含量<2%时光激活后出现红色荧光(激发波长520 - 550 nm,发射波长>580 nm)(GFP荧光的红移)。细胞复氧后红移消失,表明只要细胞处于缺氧状态,红移就是稳定的。从GFP基因敲入小鼠(绿色小鼠)心脏分离的单个心肌细胞中也证实了GFP荧光的红移。然后,我们尝试对器官内的缺氧进行体内分子成像。在绿色小鼠中,如果防止大气中的氧扩散,使用宏观光学方法可以在缺血的肝脏和肾脏中成像红移。在从绿色小鼠分离的晶体灌注跳动心脏中,在冠状动脉结扎远端的心外膜中显示出红移存在显著的空间异质性。我们得出结论,目前使用GFP作为氧指示剂的技术可能允许对器官内的氧进行体内分子成像。

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