[Study on the translocation of cytosolic dihydrotestosterone-androgen binding protein complex to the nuclei in rat submandibular gland].

A Matsubayashi
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引用次数: 0

Abstract

The low molecular weight inhibitor (LMWI) and the translocation of dihydrotestosterone (DHT)-androgen binding protein (ABP) complex of the cytosol to the nuclei in rat submandibular gland (SMG) was studied by dialysis, ultrafiltration and glycerol linear gradient centrifugation procedures. Prebound cytosol was obtained by the incubation with 3H-DHT at 4 degrees C for 3hr in the presence or absence of 100 fold excess of unlabeled DHT prior to contact to nuclei. When prebound cytosol was dialyzed or ultrafiltrated, the binding ability of 3H-DHT-ABP complex to nuclei was increased up to 3 times of the control (nontreated prebound cytosol). The sedimentation rate of 3H-DHT-ABP complex by glycerol linear gradient centrifugation was 4S for dialyzed or ultrafiltrated prebound cytosol and 8S for control. These transformation of 8S to 4S and activation to the nuclear binding of 3H-DHT-ABP complex by dialysis or ultrafiltration were inhibited by molybdate in the prebound medium. The similar transformation of 8S to 4S and activation to the nuclear binding of 3H-DHT-ABP complex was shown in heated prebound cytosol. These results indicate that the LMWI regulate activation of 3H-DHT-ABP complex. The molecular weight of the dialyzed LMWI were estimated as 7,000 by dialysis or ultrafiltration membrane and SDS-PAGE. From the in vitro two step binding assay, it was revealed that rat SMG contained the low molecular weight protein (M. W. 7,000) in cytosol having a inhibitory effect on the translocation to the nuclei of 3H-DHT-ABP complex.

[大鼠颌下腺胞质双氢睾酮-雄激素结合蛋白复合物向细胞核易位的研究]。
采用透析、超滤和甘油线性梯度离心等方法研究了大鼠颌下腺(SMG)低分子量抑制剂(LMWI)和胞浆中二氢睾酮(DHT)-雄激素结合蛋白(ABP)复合物向细胞核的转运。在与细胞核接触之前,与3H-DHT在4℃下孵育3小时,在存在或不存在超过100倍的未标记DHT的情况下,获得预结合细胞质。预结合细胞质透析或超滤后,3H-DHT-ABP复合物对细胞核的结合能力增加到对照(未处理的预结合细胞质)的3倍。甘油线性梯度离心沉淀3H-DHT-ABP复合物,透析或超滤前结合胞浆沉淀速率为4S,对照沉淀速率为8S。通过透析或超滤将8S转化为4S并激活3H-DHT-ABP复合物的核结合,这些都被预结合介质中的钼酸盐所抑制。在加热的预结合细胞质中,8S转化为4S并激活3H-DHT-ABP复合物的核结合。这些结果表明LMWI调节3H-DHT-ABP复合物的活化。通过透析或超滤膜和SDS-PAGE测定透析后的LMWI分子量为7000。体外两步结合实验表明,大鼠SMG细胞质中含有低分子量蛋白(m.w . 7000),对3H-DHT-ABP复合体的核转运具有抑制作用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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