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林丹处理的大鼠肝上皮细胞中缝隙连接通透性、缝隙连接数量和连接蛋白43表达的变化。

Changes in gap junction permeability, gap junction number, and connexin43 expression in lindane-treated rat liver epithelial cells.

作者信息

Guan X, Bonney W J, Ruch R J

机构信息

Department of Pathology, Medical College of Ohio, Toledo 43614.

出版信息

Toxicol Appl Pharmacol. 1995 Jan;130(1):79-86. doi: 10.1006/taap.1995.1011.

DOI:10.1006/taap.1995.1011
PMID:7530866
Abstract

The pesticide lindane (gamma-hexachlorocyclohexane) is a mammalian neurotoxin and hepatocarcinogen. Lindane can inhibit gap junctional intercellular communication (GJIC) and this effect may contribute to its toxic properties. The mechanism of inhibition of GJIC by lindane in WB-F344 rat liver epithelial cells was studied to determine if altered gap junction permeability, gap junction number, and/or gap junction protein (connexin43) expression were involved. GJIC was monitored by fluorescent Lucifer Yellow CH dye microinjection (dye-coupling). Gap junction number was quantified visually after indirect immunostaining of gap junctions using an anti-connexin43 monoclonal antibody. Connexin43 mRNA and protein levels were determined by Northern and Western blotting, respectively. Short-term treatment (10-30 min) with lindane (50 microM) resulted in the rapid (within 10 min), nearly complete loss of dye-coupling but no changes in gap junction number of connexin43 mRNA or protein levels. Medium-term treatment (1-4 hr) resulted in the loss of dye-coupling, gap junctions, and phosphorylated connexin43 proteins. Long-term treatment (1-14 days) led to reductions in dye-coupling, total connexin43 protein, and connexin43 mRNA. Nuclear run-on assays indicated that transcription of the connexin43 gene was reduced nonspecifically by lindane. These data indicate that reductions in gap junction permeability, number, and expression may be involved in the inhibition of GJIC depending on pesticide treatment duration.

摘要

农药林丹(γ-六氯环己烷)是一种哺乳动物神经毒素和肝致癌物。林丹可抑制间隙连接细胞间通讯(GJIC),这种作用可能与其毒性特性有关。研究了林丹在WB-F344大鼠肝上皮细胞中抑制GJIC的机制,以确定间隙连接通透性、间隙连接数量和/或间隙连接蛋白(连接蛋白43)表达是否发生改变。通过荧光鲁米诺黄CH染料显微注射(染料偶联)监测GJIC。使用抗连接蛋白43单克隆抗体对间隙连接进行间接免疫染色后,通过视觉定量间隙连接数量。分别通过Northern印迹和Western印迹测定连接蛋白43 mRNA和蛋白水平。用林丹(50微摩尔)进行短期处理(10 - 30分钟)导致快速(10分钟内)、几乎完全丧失染料偶联,但间隙连接数量、连接蛋白43 mRNA或蛋白水平没有变化。中期处理(1 - 4小时)导致染料偶联、间隙连接和磷酸化连接蛋白43蛋白丧失。长期处理(1 - 14天)导致染料偶联、总连接蛋白43蛋白和连接蛋白43 mRNA减少。核转录分析表明,林丹非特异性地降低了连接蛋白43基因的转录。这些数据表明,间隙连接通透性、数量和表达的降低可能参与了GJIC的抑制,这取决于农药处理的持续时间。

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