钙对镉诱导大鼠肝细胞毒性的改善作用。

In Vitro Pub Date : 1984-10-01 DOI:10.1007/BF02618293
E M Sorensen, N K Smith, C S Boecker, D Acosta
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引用次数: 4

摘要

分离新生大鼠的肝细胞,培养约24小时,暴露于含钙或不含钙的镉中,并进行扫描电镜处理。为了评估镉诱导变化的严重程度,根据形态学损伤的程度对暴露的肝细胞进行分类。表面起泡的差异、微绒毛的改变、肿胀程度的变化和细胞形状的变化被用来分类细胞损伤的严重程度。对每次暴露时间和镉浓度在钙存在或不存在情况下的细胞变化进行了双盲形态计量学分析(二维数据的几何统计学处理以收集三维信息)。在缺乏钙的情况下,将正常扁平细胞暴露于50或100微米镉环境30分钟,其相对体积百分比显著下降。相比之下,暴露于含有50或100微米镉和缺钙的溶液后,严重受损的球形细胞的相对体积百分比显着增加。在没有钙的情况下,暴露于所有镉浓度30分钟后,中间细胞的相对体积百分比(轻微肿胀并显示微绒毛数量变化)显着增加。对暴露60分钟的肝细胞的检查显示,在缺乏钙的情况下,镉诱导的细胞毒性程度比暴露30分钟的肝细胞更严重。如果培养物在无钙条件下暴露60分钟,与暴露30分钟的培养物相比,球形细胞的数量增加了约30%,扁平细胞的数量减少了30%。在无钙条件下,在所有镉浓度下,起泡的程度都明显更大。因此,钙的存在降低了大鼠肝细胞原代培养中镉诱导的细胞毒性,这些细胞在扫描电镜后进行形态计量学分析。
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Calcium amelioration of cadmium-induced cytotoxicity in cultured rat hepatocytes.

Parenchymal hepatocytes from neonatal rats were isolated, cultured about 24 h, exposed to cadmium with or without calcium, and processed for scanning electron microscopy. To assess the severity of cadmium-induced changes, exposed hepatocytes were categorized based upon the extent of morphological damage. Differences in surface blebbing, alterations in microvilli, variations in the degree of swelling, and changes in cell shape were used to categorize the severity of cell damage. A double-blind morphometric analysis (a geometricostatistical processing of two-dimensional data for the collection of three-dimensional information) of cellular changes was conducted for each exposure time and for each concentration of cadmium in the presence or absence of calcium. Significant decreases occurred in the percent relative volume of normal, flattened cells present in cultures exposed for 30 min to 50 or 100 microM cadmium in the absence of calcium. In contrast, the percent relative volume of severely damaged spherical cells was significantly increased after exposure to solutions containing 50 or 100 microM cadmium and lacking calcium. Percent relative volume of intermediate cells (which were slightly swollen and showed changes in microvillar number) was significantly increased following a 30 min exposure to all cadmium concentrations in the absence of calcium. The examination of hepatocytes exposed for 60 min showed that the degree of cadmium-induced cytotoxicity was more severe in the absence of calcium than was the case for the hepatocyte cultures exposed for 30 min: approximately 30% more spherical cells and 30% fewer flattened cells were present if cultures were exposed in the absence of calcium for 60 min compared to those exposed for 30 min. The degree of blebbing was significantly greater at all cadmium concentrations in the absence of calcium. The presence of calcium, therefore, reduced cadmium-induced cytotoxicity in primary cultures of rat hepatocytes subjected to morphometric analysis after scanning electron microscopy.

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