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原位杂交组织化学定量分析:数字图像中单个细胞的自动计数

In situ hybridization histochemistry quantification: automatic count on single cell in digital image.

作者信息

Masseroli M, Bollea A, Bendotti C, Forloni G

机构信息

Department of Geriatric Neuropsychiatry, Istituto di Ricerche Farmacologiche Mario Negri, Milan, Italy.

出版信息

J Neurosci Methods. 1993 Apr;47(1-2):93-103. doi: 10.1016/0165-0270(93)90025-m.

Abstract

It is extremely useful in investigations of the central nervous system (CNS) to measure mRNA expression in cells by in situ hybridization. However, this approach is limited by the difficulties of a reliable quantitative evaluation. In the present paper we describe a method for quantifying radioactive hybrids on individual cells by a silver grain count in digital images. Quantification is based on the real size and grey level of a single grain obtained by computerized microscope image analysis (IBAS 2, Kontron-Zeiss, PC 286). The program provides for automatic identification of cell area, the portion occupied by grains and their grey level. The number of grains per cell results from a mathematical function integrating these parameters with a 'density factor'. This factor is introduced to better estimate the number of grains when there is overlapping. The method was tested by measuring the expression of preproNPY (pp-NPY) mRNA in rat dentate gyrus and preproSomatostatin (pp-SOM) mRNA in frontal cerebral cortex of control and colchicine-treated rats. Colchicine did not modify the number of pp-SOM mRNA-positive cells but reduced the expression per cell. These results confirm the advantages of our method to quantify a wide range of silver grains (10-5000) and improves the sensitivity of in situ hybridization. With this support the in situ hybridization technique could be considered a real quantitative method for measuring small alterations in neuronal function.

摘要

通过原位杂交来测量细胞中的mRNA表达,在中枢神经系统(CNS)研究中极其有用。然而,这种方法因难以进行可靠的定量评估而受到限制。在本文中,我们描述了一种通过对数字图像中的银颗粒计数来量化单个细胞上放射性杂交体的方法。定量基于通过计算机显微镜图像分析(IBAS 2,康强 - 蔡司,PC 286)获得的单个颗粒的实际大小和灰度。该程序可自动识别细胞区域、颗粒所占部分及其灰度。每个细胞的颗粒数由一个将这些参数与“密度因子”整合的数学函数得出。引入这个因子是为了在存在重叠时更好地估计颗粒数。通过测量对照大鼠和秋水仙碱处理大鼠的齿状回中前神经肽Y原(pp - NPY)mRNA的表达以及额叶皮质中前生长抑素原(pp - SOM)mRNA的表达来测试该方法。秋水仙碱并未改变pp - SOM mRNA阳性细胞的数量,但降低了每个细胞的表达。这些结果证实了我们的方法在量化广泛范围的银颗粒(10 - 5000)方面的优势,并提高了原位杂交的灵敏度。有了这种支持,原位杂交技术可被视为一种用于测量神经元功能微小变化的真正定量方法。

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