Dellweg H G, Hotz A, Mugele K, Gehring U
EMBO J. 1982;1(3):285-9. doi: 10.1002/j.1460-2075.1982.tb01161.x.
[3H]Triamcinolone acetonide was used to tag covalently specific glucocorticoid receptors by photoaffinity labelling at lambda greater than or equal to 320 nm. Receptors of wild-type mouse lymphoma cells and two glucocorticoid resistant mutants of "nuclear transfer deficient" (nt-) and "increased nuclear transfer" (nti) phenotypes, respectively, were used. Wild-type and nt- receptors yielded radiolabelled polypeptide bands of mol. wt. 98 000 as revealed by gel electrophoresis under denaturing conditions and fluorography. In contrast, the nti receptor had a mol. wt. of 42 000. Partial proteolysis of the wild-type receptor with alpha-chymotrypsin resulted in a fragment of mol. wt. 39 000 which still contained the steroid binding site but had increased affinity for DNA indistinguishable from that of the nti receptor. Chymotrypsin thus removed a domain from the wild-type receptor polypeptide which is involved in modulating DNA binding. The same domain is missing from the nti receptor.
用[3H]曲安奈德通过在波长大于或等于320nm处进行光亲和标记来共价标记特异性糖皮质激素受体。分别使用野生型小鼠淋巴瘤细胞的受体以及两种具有“核转运缺陷”(nt-)和“核转运增加”(nti)表型的糖皮质激素抗性突变体的受体。野生型和nt-受体在变性条件下通过凝胶电泳和荧光自显影显示出分子量为98000的放射性标记多肽条带。相比之下,nti受体的分子量为42000。用α-胰凝乳蛋白酶对野生型受体进行部分蛋白酶解产生了一个分子量为39000的片段,该片段仍然含有类固醇结合位点,但对DNA的亲和力增加,与nti受体的亲和力无法区分。因此,胰凝乳蛋白酶从野生型受体多肽中去除了一个参与调节DNA结合的结构域。nti受体中缺少相同的结构域。
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