This work was supported by a grant from The National Natural Science Foundation of China(39970631).
啮齿目动物的睾丸较肝脏对镉毒性更为敏感.为阐明不同组织细胞的镉毒性分子机制,对镉暴露大鼠睾丸支持细胞与肝脏金属硫蛋白基因(MT)的表达及镉蓄积进行了时相研究.成年雄性SD大鼠低剂量镉(4.0 μmol/kg)皮下注射后,立即进行睾丸支持细胞和肝脏组织的分离.采用RT-PCR技术分析mRNA,并用光密度扫描作半定量分析,蛋白质定量用ELISA方法,原子分光光度吸收法测定镉浓度.结果显示:镉暴露1 h后肝脏MT mRNA即有明显的诱导表达,3 h达高峰;支持细胞也有明显的诱导表达, 6 h达高峰.镉暴露后肝脏MT有明显的诱导表达,但睾丸支持细胞不但未见MT增加而且还稍有下降.提示:a.镉对MTmRNA的诱导表达具有时间依赖性和组织特异性.b.镉虽然能诱导睾丸MT的转录,但没有促进其MT的合成,这可能是睾丸对镉毒性与致癌作用较肝脏更敏感的重要原因.
The rodent testes are generally more susceptible to cadmium(Cd)-induced toxicity than the liver. In order to clarify the molecular mechanism underlying tissue and cell differences in Cd sensitivity, metallothionein(MT) gene expression, MT protein accumulation, and Cd retention were compared under different time in freshly isolated testicular sertoli cells and liver of rats treated with Cd. Adult male Sprague-Dawley rats received a s.c. injection of 4.0 μmol/kg and 0 h(control), 1 h, 3 h, 6 h, or 24 h later, tissue were sampled and testicular sertoli cells were isolated. MT1 and MT2 mRNA levels were determined by semi-quantitative RT-PCR analysis followed by densitometry scanning, and MT was estimated by the enzyme-linked immunosorbent assay (ELISA) method. Cadmium content was determined by atomic absorption spectrophotometry. The results demonstrated that both isoform mRNA: MT1 and MT2 were increased after Cd treatment in liver and peaked at 3h, followed by a decline, in contrast, the mRNA levels in sertoli cells peaked at 6h. Cd exposure substantially increased hepatic MT, but did not increase MT translation in sertoli cells. These results indicate that: (1)metallothionein mRNA expression is tissue- and time-dependent; (2) the inability to induce the metal-detoxicating MT-protein in response to Cd, might account for higher susceptibility of testes to Cd toxicity and carcinogenesis relative to liver.
任绪义,周雍,张建鹏,仲燕,冯伟华,焦炳华.镉暴露大鼠睾丸支持细胞金属硫蛋白表达的时相研究[J].生物化学与生物物理进展,2003,30(6):965-968
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