Development of an imaging system for in vivo real-time monitoring of neuronal activity in deep brain of free-moving rats

被引:3
|
作者
Iijima, Norio [1 ,4 ]
Miyamoto, Shinji [2 ,5 ]
Matsumoto, Keisuke [1 ]
Takumi, Ken [1 ,6 ]
Ueta, Yoichi [3 ]
Ozawa, Hitoshi [1 ]
机构
[1] Nippon Med Sch, Grad Sch Med, Dept Anat & Neurobiol, Bunkyo Ku, I-1-5 Sendagi, Tokyo 1138602, Japan
[2] Indeco Inc, Bunkyo Ku, 1-11-14 Kasuga, Tokyo 1120003, Japan
[3] Univ Occupat & Environm Hlth, Sch Med, Dept Physiol, Kitakyushu, Fukuoka 8078555, Japan
[4] Int Univ Hlth & Welf, Ctr Med Sci, 2600 1 Kitakanamaru, Ohtawara 3248501, Japan
[5] Activelase, 3-5-22 Imai, Oume Si, Tokyo, Japan
[6] Okayama Univ Sci, Dept Zool, 1-1 Ridai Cho, Okayama 7000005, Japan
基金
日本学术振兴会;
关键词
Optical fiber; Laser; Deep brain; Real-time monitoring; Free movement; GREEN FLUORESCENT PROTEIN; LONG-TERM POTENTIATION; SUPRACHIASMATIC NUCLEUS; OSMOTIC STIMULATION; CALCIUM SIGNALS; EXPRESSION; MICE; VISUALIZATION; DELIVERY; RELEASE;
D O I
10.1007/s00418-017-1576-2
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
We have newly developed a system that allows monitoring of the intensity of fluorescent signals from deep brains of rats transgenically modified to express enhanced green fluorescent protein (eGFP) via an optical fiber. One terminal of the optical fiber was connected to a blue semiconductor laser oscillator/green fluorescence detector. The other terminal was inserted into the vicinity of the eGFP-expressing neurons. Since the optical fiber was vulnerable to twisting stresses caused by animal movement, we also developed a cage in which the floor automatically turns, in response to the turning of the rat's head. This relieved the twisting stress on the optical fiber. The system then enabled real-time monitoring of fluorescence in awake and unrestrained rats over many hours. Using this system, we could continuously monitor eGFP-expression in arginine vasopressin-eGFP transgenic rats. Moreover, we observed an increase of eGFP-expression in the paraventricular nucleus under salt-loading conditions. We then performed in vivo imaging of eGFP-expressing GnRH neurons in the hypothalamus, via a bundle consisting of 3000 thin optical fibers. With the combination of the optical fiber bundle connection to the fluorescence microscope, and the special cage system, we were able to capture and retain images of eGFP-expressing neurons from free-moving rats. We believe that our newly developed method for monitoring and imaging eGFP-expression in deep brain neurons will be useful for analysis of neuronal functions in awake and unrestrained animals for long durations.
引用
收藏
页码:289 / 298
页数:10
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