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使用图像分析仪的定量免疫细胞化学。II. 递质免疫细胞化学的浓度标准。

Quantitative immunocytochemistry using an image analyzer. II. Concentration standards for transmitter immunocytochemistry.

作者信息

Nabors L B, Songu-Mize E, Mize R R

机构信息

Department of Anatomy and Neurobiology, College of Medicine, University of Tennessee Health Science Center, Memphis 38163.

出版信息

J Neurosci Methods. 1988 Nov;26(1):25-34. doi: 10.1016/0165-0270(88)90126-4.

Abstract

Image analyzers can measure both the optical density and geometry of immunocytochemically labeled cells and fibers, as reviewed in a companion paper (Mize et al., 1988). In this paper, we report a procedure which allows us to estimate the concentration of a neurotransmitter based upon the optical density of antibody labeling produced by immunocytochemistry. To accomplish this, we developed a standard which binds conjugated neurotransmitters. Several artificial media for the standard were compared, including agar, gelatin, and agar-gelatin. A 3% agar matrix was found to be most suitable because it cut well and was nearly transparent. The agar sections were activated with cyanogen bromide/acetonitrile to promote coupling to the antigen. To test the standard, we used gamma-aminobutyric acid (GABA) conjugated to bovine serum albumin (BSA) as the antigen. The antibody was directed against this conjugate. Activated agar sections were incubated in serial dilutions of the tritium-labeled GABA/BSA conjugate. The radioactivity of some of these sections was measured to estimate the amount of coupled antigen. The remaining sections were incubated in the GABA antibody and processed for immunocytochemistry. The optical density of these sections was measured with an image analyzer. A linear relationship was found between GABA concentration and optical density over a range of at least 0.01 to 1 nmol/mg of agar. These results show that the concentration of bound GABA can be estimated from the optical density of sections labeled by antibody immunocytochemistry. The applicability of this technique to fixed brain tissue is discussed.

摘要

图像分析仪可以测量免疫细胞化学标记的细胞和纤维的光密度及几何形状,如在一篇相关论文中所综述的那样(米泽等人,1988年)。在本文中,我们报告了一种方法,该方法使我们能够根据免疫细胞化学产生的抗体标记的光密度来估计神经递质的浓度。为实现这一点,我们开发了一种能结合结合型神经递质的标准物。比较了几种用于该标准物的人工介质,包括琼脂、明胶和琼脂 - 明胶。发现3%的琼脂基质最为合适,因为它切割良好且几乎透明。用溴化氰/乙腈激活琼脂切片以促进与抗原的偶联。为了测试该标准物,我们使用与牛血清白蛋白(BSA)偶联的γ-氨基丁酸(GABA)作为抗原。抗体针对这种偶联物。将激活的琼脂切片在氚标记的GABA/BSA偶联物的系列稀释液中孵育。测量其中一些切片的放射性以估计偶联抗原的量。其余切片在GABA抗体中孵育并进行免疫细胞化学处理。用图像分析仪测量这些切片的光密度。在至少0.01至1 nmol/mg琼脂的范围内,发现GABA浓度与光密度之间存在线性关系。这些结果表明,可以从抗体免疫细胞化学标记的切片的光密度估计结合的GABA的浓度。讨论了该技术在固定脑组织中的适用性。

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