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植物bZIP转录激活因子中一个新型二聚体稳定区域的鉴定。

Identification of a novel dimer stabilization region in a plant bZIP transcription activator.

作者信息

Katagiri F, Seipel K, Chua N H

机构信息

Laboratory of Plant Molecular Biology, Rockefeller University, New York, New York 10021.

出版信息

Mol Cell Biol. 1992 Nov;12(11):4809-16. doi: 10.1128/mcb.12.11.4809-4816.1992.

Abstract

We have carried out deletion analyses of a tobacco transcription activator, TGA1a, in order to define its functional domains. TGA1a belongs to the basic-region-leucine zipper (bZIP) class of DNA-binding proteins. Like other proteins of this class, it binds to its target DNA as a dimer, and its bZIP domain is necessary and sufficient for specific DNA binding. A mutant polypeptide containing the bZIP domain alone, however, shows a lower DNA-binding affinity than the full-length TGA1a. The C-terminal portion of TGA1a, which is essential for the higher DNA-binding affinity, contains a polypeptide region that can stabilize dimeric forms of the protein. This polypeptide region is designated the dimer stabilization (DS) region. Under our in vitro conditions, TGA1a derivatives with the DS region and those without the region do not form a detectable mixed dimer. This result indicates that in addition to the leucine zipper, the DS region can serve as another determinant of the dimerization specificity of TGA1a. In fact, the DS region, when fused to another bZIP protein, C/EBP, can inhibit dimer formation between the fusion protein and native C/EBP, whereas each of these can form homodimers. Such a portable determinant of dimerization specificity has potential application in studies of DNA-binding proteins as well as in biotechnology.

摘要

为了确定烟草转录激活因子TGA1a的功能结构域,我们对其进行了缺失分析。TGA1a属于DNA结合蛋白的碱性区域-亮氨酸拉链(bZIP)家族。与该家族的其他蛋白一样,它以二聚体形式与其靶DNA结合,其bZIP结构域对于特异性DNA结合是必需且足够的。然而,仅包含bZIP结构域的突变多肽与全长TGA1a相比,显示出较低的DNA结合亲和力。TGA1a的C末端部分对于较高的DNA结合亲和力至关重要,它包含一个能够稳定该蛋白二聚体形式的多肽区域。这个多肽区域被命名为二聚体稳定(DS)区域。在我们的体外条件下,具有DS区域和不具有该区域的TGA1a衍生物不会形成可检测到的混合二聚体。这一结果表明,除了亮氨酸拉链外,DS区域还可以作为TGA1a二聚化特异性的另一个决定因素。事实上,当DS区域与另一个bZIP蛋白C/EBP融合时,它可以抑制融合蛋白与天然C/EBP之间的二聚体形成,而它们各自都能形成同二聚体。这种可移植的二聚化特异性决定因素在DNA结合蛋白的研究以及生物技术中具有潜在应用价值。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f66e/360413/f787ad7bd735/molcellb00134-0013-a.jpg

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