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雄激素受体向脱氧核糖核酸结合状态的转变:匀浆和完整细胞中的研究。

Transformation of the androgen receptor to the deoxyribonucleic acid-binding state: studies in homogenates and intact cells.

作者信息

Grino P B, Griffin J E, Wilson J D

出版信息

Endocrinology. 1987 May;120(5):1914-20. doi: 10.1210/endo-120-5-1914.

Abstract

Transformation of the [3H]dihydrotestosterone-receptor complex to the DNA-binding state was studied in intact monolayers and in homogenates of cultured human fibroblasts and mouse L-cells. When homogenates of either cell type were prepared in low salt buffer, incubated at 0 C with [3H]dihydrotestosterone, chromatographed on DNA-Sepharose, and eluted with a NaCl gradient, the receptor complex was eluted at 25 mM NaCl (peak A). After incubation of the homogenate at 25 C for 20 min, peak A decreased in amplitude. The major peak of the receptor from human fibroblasts eluted at 100 mM NaCl, while that from L-cells eluted at 170 mM NaCl (peak B). Flow-through fractions contained only minimal amounts of transformable dihydrotestosterone-receptor complex under the same conditions. Furthermore, isolated peak A could be converted to peak B by the same warming process. The appearance of peak B was prevented when 10 mM, but not 1 mM, sodium molybdate was present during the homogenization process. Unoccupied receptor was recovered exclusively in peak A both at 0 C and after incubation at 25 C. When intact fibroblast and L-cell monolayers were incubated with [3H]dihydrotestosterone at 37 C, all receptor in both cytosol and nuclear extract was recovered in peak B. In sucrose density gradient centrifugation, peak A was 6-8S in size, and peak B was 4.6S. These findings suggest that peak A corresponds to the nontransformed and peak B to the transformed states of the androgen receptor; the transformation reaction may be the consequence of a dissociation of a macromolecular complex into subunits; and sodium molybdate acts to stabilize the macromolecular complex.

摘要

在完整的单层细胞以及培养的人成纤维细胞和小鼠L细胞的匀浆中,研究了[³H]双氢睾酮受体复合物向DNA结合状态的转变。当在低盐缓冲液中制备任一细胞类型的匀浆,在0℃下与[³H]双氢睾酮孵育,在DNA琼脂糖上进行层析,并用NaCl梯度洗脱时,受体复合物在25 mM NaCl处洗脱(峰A)。将匀浆在25℃孵育20分钟后,峰A的幅度降低。人成纤维细胞受体的主要峰在100 mM NaCl处洗脱,而L细胞的主要峰在170 mM NaCl处洗脱(峰B)。在相同条件下,流穿组分仅含有极少量可转化的双氢睾酮受体复合物。此外,分离的峰A可通过相同的升温过程转化为峰B。当在匀浆过程中存在10 mM(而非1 mM)钼酸钠时,峰B的出现受到抑制。在0℃以及25℃孵育后,未结合的受体仅在峰A中回收。当完整的成纤维细胞和L细胞单层在37℃下与[³H]双氢睾酮孵育时,细胞质和核提取物中的所有受体均在峰B中回收。在蔗糖密度梯度离心中,峰A的大小为6 - 8S,峰B的大小为4.6S。这些发现表明,峰A对应于雄激素受体的未转化状态,峰B对应于转化状态;转化反应可能是大分子复合物解离为亚基的结果;钼酸钠起到稳定大分子复合物的作用。

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