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在培养条件下用2,3,7,8-四氯二苯并对二恶英处理的小鼠肝癌细胞中芳烃受体的下调。

Downregulation of the Ah receptor in mouse hepatoma cells treated in culture with 2,3,7,8-tetrachlorodibenzo-p-dioxin.

作者信息

Prokipcak R D, Okey A B

机构信息

Department of Pediatrics, Hospital for Sick Children, Toronto, Ont., Canada.

出版信息

Can J Physiol Pharmacol. 1991 Aug;69(8):1204-10. doi: 10.1139/y91-176.

Abstract

The aromatic hydrocarbon (Ah) receptor behaves as a ligand-dependent transcription factor in the induction of cytochrome P450IA1. In cells exposed to the Ah receptor ligand 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD), the Ah receptor undergoes a transformation from a form with low affinity for nucleic acids (cytosolic receptor) into a form that preferentially associates with the cell nucleus (nuclear receptor). We followed the fate of the Ah receptor in mouse hepatoma cells during short-term exposure to [3H]TCDD by analyzing both cytosolic and nuclear fractions for specific binding. Nuclear Ah receptor levels increased over the first 2 h of treatment and then decreased to about 50% of maximal concentrations by 5 h after start of treatment. The decrease in nuclear receptor was not accompanied by a reappearance of detectable Ah receptor in the cytosolic fraction; further incubation with [3H]TCDD in cytosols from lysed cells did not label any additional receptor sites in cytosolic extract. By the 6th h of incubation, the total receptor population in the cell was only about 15-20% of that detected at the start of the incubation. The levels of specific binding detected were unaffected by up to 20 h of incubation with the vehicle DMSO, confirming that the presence of TCDD is required for the observed downregulation to occur. These results indicate that there is a substantial ligand-dependent loss in total Ah receptor during short-term exposure of cells to TCDD in culture.

摘要

芳烃(Ah)受体在细胞色素P450IA1的诱导过程中作为一种配体依赖性转录因子发挥作用。在暴露于Ah受体配体2,3,7,8-四氯二苯并对二恶英(TCDD)的细胞中,Ah受体经历了从对核酸亲和力低的形式(胞质受体)转变为优先与细胞核结合的形式(核受体)的过程。我们通过分析胞质和核组分中的特异性结合,追踪了小鼠肝癌细胞在短期暴露于[3H]TCDD期间Ah受体的命运。在处理的最初2小时内,核Ah受体水平升高,然后在处理开始后5小时降至最大浓度的约50%。核受体的减少并未伴随着胞质组分中可检测到的Ah受体的重新出现;用裂解细胞的胞质溶胶与[3H]TCDD进一步孵育并未标记胞质提取物中的任何额外受体位点。到孵育的第6小时,细胞中的总受体数量仅为孵育开始时检测到的数量的约15 - 20%。在与溶剂二甲基亚砜(DMSO)孵育长达20小时的情况下,检测到的特异性结合水平未受影响,这证实了观察到的下调需要TCDD的存在。这些结果表明,在培养的细胞短期暴露于TCDD期间,总Ah受体会出现大量的配体依赖性损失。

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