Chusacultanachai S, Glenn K A, Rodriguez A O, Read E K, Gardner J F, Katzenellenbogen B S, Shapiro D J
Department of Biochemistry, University of Illinois, Urbana, Illinois 61801, USA.
J Biol Chem. 1999 Aug 13;274(33):23591-8. doi: 10.1074/jbc.274.33.23591.
To analyze the role of amino acids in the steroid receptor DNA binding domain (DBD) recognition helix in binding of the receptor to the estrogen response element (ERE), we adapted the powerful P22 challenge phage selection system for use with a vertebrate protein. We used the progesterone receptor DNA binding domain and selected for mutants that gained the ability to bind to the ERE. We used a mutagenesis protocol based on degenerate oligonucleotides to create a large and diverse pool of mutants in which 10 nonconsensus amino acids in the DNA recognition helix of the progesterone receptor DNA binding domain were randomly mutated. After a single cycle of modified P22 challenge phage selection, 37 mutant proteins were identified, all of which lost the ability to bind to the progesterone response element. In gel mobility shift assays, approximately 70% of the genetically selected mutants bound to the consensus ERE with a >4-fold higher affinity than the naturally occurring estrogen receptor DBD. In the P-box region of the DNA recognition helix, the selected mutants contained the amino acids found in the wild-type estrogen receptor DBD, as well as other amino acid combinations seen in naturally occurring steroid/nuclear receptors that bind the aGGTCA half-site. We also obtained high affinity DBDs with Trp(585) as the first amino acid of the P-box, although this is not found in the known steroid/nuclear receptors. In the linker region between the two zinc fingers, G597R was by far the most common mutation. In transient transfections in mammalian cells using promoter interference assays, the mutants displayed enhanced affinity for the ERE. When linked to an activation domain, the transfected mutants activated transcription from ERE-containing reporter genes. We conclude that the P-box amino acids can display considerable variation and that the little studied linker amino acids play an important role in determining affinity for the ERE. This work also demonstrates that the P22 challenge phage genetic selection system, modified for use with a mammalian protein, provides a novel, single cycle selection for steroid/nuclear receptor DBDs with altered specificity and greatly enhanced affinity for their response elements.
为了分析氨基酸在类固醇受体DNA结合结构域(DBD)识别螺旋中对于受体与雌激素反应元件(ERE)结合的作用,我们对强大的P22攻击噬菌体选择系统进行了改造,使其适用于脊椎动物蛋白。我们使用孕酮受体DNA结合结构域,并筛选出获得与ERE结合能力的突变体。我们采用基于简并寡核苷酸的诱变方案,在孕酮受体DNA结合结构域的DNA识别螺旋中10个非保守氨基酸处随机诱变,创建了一个庞大且多样的突变体库。经过一轮改良的P22攻击噬菌体选择后,鉴定出37个突变蛋白,它们均丧失了与孕酮反应元件结合的能力。在凝胶迁移率变动分析中,约70%的经基因筛选的突变体与共有ERE结合,其亲和力比天然存在的雌激素受体DBD高4倍以上。在DNA识别螺旋的P盒区域,筛选出的突变体包含野生型雌激素受体DBD中的氨基酸,以及在天然存在的结合aGGTCA半位点的类固醇/核受体中出现的其他氨基酸组合。我们还获得了以Trp(585)作为P盒第一个氨基酸的高亲和力DBD,尽管在已知的类固醇/核受体中未发现这种情况。在两个锌指之间的连接区,G597R是迄今为止最常见的突变。在使用启动子干扰分析的哺乳动物细胞瞬时转染中,这些突变体对ERE表现出增强的亲和力。当与激活结构域相连时,转染的突变体激活了含ERE的报告基因的转录。我们得出结论,P盒氨基酸可以表现出相当大的变异性,而研究较少的连接区氨基酸在决定对ERE的亲和力方面起着重要作用。这项工作还表明,经过改造用于哺乳动物蛋白的P22攻击噬菌体遗传选择系统,为具有改变的特异性和对其反应元件大大增强的亲和力的类固醇/核受体DBD提供了一种新颖的单轮选择。
