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对表达基因编码钙传感器的犁鼻器脑片标本中的神经元反应进行成像。

Imaging neuronal responses in slice preparations of vomeronasal organ expressing a genetically encoded calcium sensor.

作者信息

Ma Limei, Haga-Yamanaka Sachiko, Yu Qingfeng Elden, Qiu Qiang, Kim Sangseong, Yu C Ron

机构信息

Stowers Institute for Medical Research, USA.

出版信息

J Vis Exp. 2011 Dec 6(58):3404. doi: 10.3791/3404.

Abstract

The vomeronasal organ (VNO) detects chemosensory signals that carry information about the social, sexual and reproductive status of the individuals within the same species. These intraspecies signals, the pheromones, as well as signals from some predators, activate the vomeronasal sensory neurons (VSNs) with high levels of specificity and sensitivity. At least three distinct families of G-protein coupled receptors, V1R, V2R and FPR, are expressed in VNO neurons to mediate the detection of the chemosensory cues. To understand how pheromone information is encoded by the VNO, it is critical to analyze the response profiles of individual VSNs to various stimuli and identify the specific receptors that mediate these responses. The neuroepithelia of VNO are enclosed in a pair of vomer bones. The semi-blind tubular structure of VNO has one open end (the vomeronasal duct) connecting to the nasal cavity. VSNs extend their dendrites to the lumen part of the VNO, where the pheromone cues are in contact with the receptors expressed at the dendritic knobs. The cell bodies of the VSNs form pseudo-stratified layers with V1R and V2R expressed in the apical and basal layers respectively. Several techniques have been utilized to monitor responses of VSNs to sensory stimuli. Among these techniques, acute slice preparation offers several advantages. First, compared to dissociated VSNs, slice preparations maintain the neurons in their native morphology and the dendrites of the cells stay relatively intact. Second, the cell bodies of the VSNs are easily accessible in coronal slice of the VNO to allow electrophysiology studies and imaging experiments as compared to whole epithelium and whole-mount preparations. Third, this method can be combined with molecular cloning techniques to allow receptor identification. Sensory stimulation elicits strong Ca2+ influx in VSNs that is indicative of receptor activation. We thus develop transgenic mice that express G-CaMP2 in the olfactory sensory neurons, including the VSNs. The sensitivity and the genetic nature of the probe greatly facilitate Ca2+ imaging experiments. This method has eliminated the dye loading process used in previous studies. We also employ a ligand delivery system that enables application of various stimuli to the VNO slices. The combination of the two techniques allows us to monitor multiple neurons simultaneously in response to large numbers of stimuli. Finally, we have established a semi-automated analysis pipeline to assist image processing.

摘要

犁鼻器(VNO)可检测化学感应信号,这些信号携带有关同一物种内个体的社会、性和生殖状态的信息。这些种内信号,即信息素,以及来自一些捕食者的信号,以高度的特异性和敏感性激活犁鼻感觉神经元(VSN)。犁鼻器神经元中至少表达三种不同的G蛋白偶联受体家族,即V1R、V2R和FPR,以介导对化学感应线索的检测。为了了解犁鼻器如何编码信息素信息,分析单个犁鼻器感觉神经元对各种刺激的反应谱并确定介导这些反应的特定受体至关重要。犁鼻器的神经上皮包裹在一对犁骨中。犁鼻器的半盲管状结构有一个开口端(犁鼻管)与鼻腔相连。犁鼻器感觉神经元将其树突延伸至犁鼻器的管腔部分,信息素线索在此处与树突小体上表达的受体接触。犁鼻器感觉神经元的细胞体形成假复层,V1R和V2R分别在顶端层和基底层表达。已经使用了几种技术来监测犁鼻器感觉神经元对感觉刺激的反应。在这些技术中,急性切片制备具有几个优点。首先,与解离的犁鼻器感觉神经元相比,切片制备能使神经元保持其天然形态,细胞的树突相对完整。其次,与全上皮和整装制备相比,在犁鼻器的冠状切片中很容易接近犁鼻器感觉神经元的细胞体,以进行电生理研究和成像实验。第三,该方法可以与分子克隆技术相结合以进行受体鉴定。感觉刺激会在犁鼻器感觉神经元中引发强烈的Ca2+内流,这表明受体被激活。因此,我们培育了在包括犁鼻器感觉神经元在内的嗅觉感觉神经元中表达G-CaMP2的转基因小鼠。该探针的敏感性和遗传特性极大地促进了Ca2+成像实验。这种方法省去了先前研究中使用的染料加载过程。我们还采用了一种配体递送系统,能够将各种刺激应用于犁鼻器切片。这两种技术的结合使我们能够同时监测多个神经元对大量刺激的反应。最后,我们建立了一个半自动分析流程来辅助图像处理。

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