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用于免疫组织化学和受体结合位点放射自显影的密度测定法的定量图像分析——方法学考量

Quantitative image analysis with densitometry for immunohistochemistry and autoradiography of receptor binding sites--methodological considerations.

作者信息

Peretti-Renucci R, Feuerstein C, Manier M, Lorimier P, Savasta M, Thibault J, Mons N, Geffard M

机构信息

Laboratoire de Physiologie Section Neurophysiologie (LAPSEN), INSERM U 318, Département des Neurosciences Cliniques et Biologiques, CHU de Grenoble, France.

出版信息

J Neurosci Res. 1991 Apr;28(4):583-600. doi: 10.1002/jnr.490280416.

Abstract

Major technical progress in the development of computer-based image analysis has made possible the entry of autoradiography and immunohistochemistry into a new era where quantification by densitometry has become easily accessible. Autoradiography could become quantitative and displayed adequate reproducibility with the help of emulsion-coated films and the use of scales of standards of known radioactivity exposed and analyzed in parallel to the tissue sections. Immunohistochemistry after revelation by a color-based enzymatic technique can also become quantitative, providing that standardization of the crucial steps of the procedure and calibration through a parallel treatment of a scale of antigen standards can be ensured. Such an approach is described here in the rat with reference to tyrosine hydroxylase (TH), the main synthesizing enzyme for catecholamines, and with dopamine (DA) itself, a catecholaminergic neurotransmitter. The different parts of the procedure, which can influence the results, such as the fixation of the animals by perfusion and the evaluation of the fluctuations via the calibration curve, are discussed in detail. Biological validation of the proposed procedure is described by reference to experiments already well documented biochemically, such as the induction effect of reserpine on TH in the rat locus coeruleus and the depleting effect of alpha-methyltyrosine (AMPT), a well-known blocker of TH activity, on rat striatal DA content. Finally the importance of restricting the measurements to the (pseudo)linear portion of the calibration curve is illustrated by the autoradiographic identification of the differential intrastriatal repartition of the dopaminergic D1 and D2 receptor sites, particularly the dual patch-matrix compartments.

摘要

基于计算机的图像分析技术的重大进展,使得放射自显影和免疫组织化学进入了一个新时代,在这个时代中,通过光密度测定进行定量变得轻而易举。借助涂有乳剂的胶片以及与组织切片平行曝光和分析的已知放射性标准刻度,放射自显影可以实现定量,并显示出足够的重现性。基于颜色的酶促技术显色后的免疫组织化学也可以实现定量,前提是能够确保该过程关键步骤的标准化以及通过对抗原标准刻度进行平行处理来进行校准。本文以大鼠为例,介绍了一种针对酪氨酸羟化酶(TH)(儿茶酚胺的主要合成酶)以及儿茶酚胺能神经递质多巴胺(DA)本身的方法。详细讨论了该过程中可能影响结果的不同部分,例如通过灌注固定动物以及通过校准曲线评估波动情况。通过参考已经有充分生化记录的实验,如利血平对大鼠蓝斑中TH的诱导作用以及α-甲基酪氨酸(AMPT)(一种众所周知的TH活性阻断剂)对大鼠纹状体DA含量的耗竭作用,描述了所提出方法的生物学验证。最后,通过放射自显影鉴定多巴胺能D1和D2受体位点在纹状体内的差异分布,特别是双斑-基质区室,说明了将测量限制在校准曲线(伪)线性部分的重要性。

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