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Expression and purification of human full-length N Oct-3, a transcription factor involved in melanoma growth

机译:人全长N Oct-3的表达和纯化,N Oct-3是涉及黑色素瘤生长的转录因子

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This report describes the first purification procedure of the human full-length N Oct-3 protein in amounts suitable for structural studies and proteomic investigations. N Oct-3 is a transcription factor member of the POU protein family. It possesses a large N-terminal transactivation domain and a DNA-binding domain (DBD) which is composed of two subdomains, PCUs and POUh, which are joined by a linker peptide. N Oct-3 is a master gene for central nervous system development but also for melanoma progression. Previous structural studies have all been performed using N Oct-3 DBD only. In this study, the full-length N Oct-3 protein was bacterially expressed and purified to homogeneity. The purified protein gave a single band at approximately 53 kDa on SDS-PAGE, while cDNA sequence analysis revealed a calculated molecular mass of 47 kDa confirmed by mass spectroscopy. Size-exclusion chromatography experiments indicated that in solution, full-length N Oct-3 was a monomer. Circular dichroism and intrinsic tryptophan fluorescence showed that full-length N Oct-3 was folded, with a significant alpha-helix content probably located in its DBD. Comparison with the purified N Oct-3 DBD demonstrated that, at least in vitro, the affinity of the protein for its DNA targets was similar. This suggests that the transactivation domain of N Oct-3 was not involved in N Oct-3 DNA interaction. (C) 2008 Elsevier Inc. All rights reserved.
机译:该报告描述了适合结构研究和蛋白质组学研究的人全长N Oct-3蛋白的首次纯化程序。 N Oct-3是POU蛋白家族的转录因子成员。它具有一个大的N末端反式激活结构域和一个DNA结合结构域(DBD),该结构域由两个亚结构域PCU和POUh组成,这两个亚结构域通过连接肽连接。 N Oct-3是中枢神经系统发育以及黑色素瘤进展的主要基因。先前的结构研究全部仅使用N Oct-3 DBD进行。在这项研究中,全长N Oct-3蛋白被细菌表达并纯化至同质。纯化的蛋白质在SDS-PAGE上显示了一个约53 kDa的单条带,而cDNA序列分析表明,经质谱确认的计算分子量为47 kDa。尺寸排阻色谱实验表明,在溶液中,全长N Oct-3是单体。圆二色性和固有色氨酸荧光表明全长N Oct-3被折叠,其DBD中可能含有大量的α-螺旋。与纯化的N Oct-3 DBD的比较表明,至少在体外,蛋白质与其DNA靶标的亲和力相似。这表明N Oct-3的反式激活结构域不参与N Oct-3 DNA的相互作用。 (C)2008 Elsevier Inc.保留所有权利。

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