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使用扫描积分显微密度测定法对兔主动脉平滑肌细胞进行福尔根脱氧核糖核酸分析。

Feulgen-deoxyribonucleic acid analysis of rabbit aortic smooth muscle cells using scanning- integrating microdensitometry.

作者信息

Anthony A, Hollis T M, Penman J A, Zerweck C, Doebler J A

出版信息

J Histochem Cytochem. 1981 Oct;29(10):1164-70. doi: 10.1177/29.10.7299105.

Abstract

A procedure entailing the use of the Feulgen reaction is described for precise quantification of nuclear DNA levels in smooth muscle cells (SMC) of paraffin-processed microtome sections of the rabbit aorta. It was established that maximal, stable, and reproducible Feulgen-DNA (F-DNA) staining of SMC nuclei is achieved using 3.5 N HCl hydrolysis of 30-50 min prior to staining of aortic sections in Schiff reagent for 60 min at 22 degrees C. Scanning-integrating microdensitometry of Feulgen-stained SMC revealed that the tunica media is comprised of a relatively homogeneous population of cells with between 0.3 and 1% of the SMC nuclei yielding 3C or 4C (tetraploid) F-DNA levels, depending on location within the aortic wall. The nuclear chromatin in inner medial SMC was found to be in a more dispersed state than that of outer SMC (using nuclear area and nuclear susceptibility to acid hydrolysis as indices of chromatin dispersion). A linear correspondence was evidenced between nuclear area and nuclear F-DNA stainability throughout the tunica media. The observation that the lumenal portion of the tunica media contains a greater abundance of SMC with large, vesicular nuclei is interpreted as reflecting a greater metabolic reactivity of this compartment relative to that of SMC bordering the tunica adventitia.

摘要

本文描述了一种使用福尔根反应的方法,用于精确量化兔主动脉石蜡切片平滑肌细胞(SMC)中的核DNA水平。研究发现,在22℃下,将主动脉切片在席夫试剂中染色60分钟之前,先用3.5N盐酸水解30 - 50分钟,可实现SMC细胞核最大程度、稳定且可重复的福尔根-DNA(F-DNA)染色。对福尔根染色的SMC进行扫描积分显微密度测定显示,中膜由相对均匀的细胞群体组成,根据主动脉壁内的位置不同,0.3%至1%的SMC细胞核产生3C或4C(四倍体)F-DNA水平。发现内侧SMC的核染色质比外侧SMC更分散(以核面积和核对酸水解的敏感性作为染色质分散的指标)。在整个中膜中,核面积与核F-DNA可染性之间存在线性对应关系。中膜腔面部分含有大量具有大泡状核的SMC,这一观察结果被解释为反映了该区域相对于与外膜相邻的SMC具有更高的代谢活性。

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