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暴露于氯化镉的巨噬细胞的超微结构与X射线微分析

Ultrastructure and x-ray microanalysis of macrophages exposed to cadmium chloride.

作者信息

Bell S W, Masters S K, Ingram P, Waters M, Shelburne J D

出版信息

Scan Electron Microsc. 1979(3):111-21.

PMID:523993
Abstract

Macrophages have a direct role in the inflammatory response to cadmium exposure. Cadmium is not only an important air pollutant, but is also one component of cigarette smoke. To study the effects of soluble cadmium on macrophages, two model systems were chosen:rabbit alveolar macrophages (RAMs) obtained by pulmonary lavage and peritoneal macrophages elicited by intraperitoneal injections of 10(7) viable M. bovis, bacillus Calmette Guérin (BCG MACs). Macrophages were maintained in standard tissue culture medium from 4 to 30 hours with concentrations of cadmium chloride (CdCl2) ranging from 0 to 1.0 mM. Attached macrophages and RAMs in suspension were studied by conventional transmission electron microscopy (TEM), scanning electron microscopy (SEM), and energy dispersive x-ray microanalysis (EDX). In addition to routine techniques for TEM and SEM, preparatory procedures included snap freezing in liquid propane, and either cryoultramicrotomy or freeze-substitution with 1% osmium tetroxide in acetone. By TEM many macrophages exhibited laminated nuclear inclusions at doses as low as 0.05 mM CdCl2) (at 20 hrs) and as early as 4 hrs (at 1.0 mM CdCl2). Sections of cells fixed by freezing exhibited the same nuclear inclusions as well as mitochondrial densities that were not visible with any other preparative technique. Cadmium was demonstrated in the nuclear inclusions and mitochondrial densities by EDX in snap frozen cells. Lesser amounts of cadmium were also detected diffusely in treated cell cytoplasm and nuclei. Cadmium was only detected by EDX in cells fixed by freezing. These studies document the localization of Cd in nuclear inclusions and mitochondria providing morphological support for the biochemical findings of other laboratories. In addition, the value of fixation by freezing over conventional chemical fixation is illustrated.

摘要

巨噬细胞在对镉暴露的炎症反应中起直接作用。镉不仅是一种重要的空气污染物,也是香烟烟雾的成分之一。为了研究可溶性镉对巨噬细胞的影响,选择了两个模型系统:通过肺灌洗获得的兔肺泡巨噬细胞(RAMs)和通过腹腔注射10(7) 活卡介苗(BCG)诱导产生的腹腔巨噬细胞(BCG MACs)。巨噬细胞在标准组织培养基中培养4至30小时,氯化镉(CdCl2)浓度范围为0至1.0 mM。通过传统透射电子显微镜(TEM)、扫描电子显微镜(SEM)和能量色散X射线微分析(EDX)研究贴壁巨噬细胞和悬浮的RAMs。除了TEM和SEM的常规技术外,制备程序还包括在液态丙烷中速冻,以及冷冻超薄切片术或用1%四氧化锇丙酮溶液进行冷冻置换。通过TEM观察,许多巨噬细胞在低至0.05 mM CdCl2(20小时时)以及早在4小时(1.0 mM CdCl2时)的剂量下就表现出层状核内包涵体。冷冻固定的细胞切片显示出相同的核内包涵体以及线粒体密度,而这些在任何其他制备技术下均不可见。通过EDX在速冻细胞的核内包涵体和线粒体密度中检测到镉。在处理过的细胞质和细胞核中也分散检测到少量镉。仅在冷冻固定的细胞中通过EDX检测到镉。这些研究记录了镉在核内包涵体和线粒体中的定位,为其他实验室的生化研究结果提供了形态学支持。此外,还说明了冷冻固定相对于传统化学固定的价值。

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