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一种新型转录起始因子(TIF),即TIF-IE,是棘阿米巴(Acanthamoeba castellanii)TIF-IB(SL1)形成稳定复合物所必需的。

A novel transcription initiation factor (TIF), TIF-IE, is required for homogeneous Acanthamoeba castellanii TIF-IB (SL1) to form a committed complex.

作者信息

Radebaugh C A, Kubaska W M, Hoffman L H, Stiffler K, Paule M R

机构信息

Department of Biochemistry and Molecular Biology, Colorado State University, Fort Collins, Colorado 80523-1870, USA.

出版信息

J Biol Chem. 1998 Oct 16;273(42):27708-15. doi: 10.1074/jbc.273.42.27708.

Abstract

The fundamental transcription initiation factor (TIF) for ribosomal RNA expression by eukaryotic RNA polymerase I, TIF-IB, has been purified to near homogeneity from Acanthamoeba castellanii using standard techniques. The purified factor consists of the TATA-binding protein and four TATA-binding protein-associated factors with relative molecular weights of 145,000, 99,000, 96,000, and 91,000. This yields a calculated native molecular weight of 460, 000, which compares well with its mass determined by scanning transmission electron microscopy (493,000) and its sedimentation rate, which is close to RNA polymerase I (515,000). Both impure and nearly homogeneous TIF-IB exhibit an apparent equilibrium dissociation constant of 56 +/- 3 pM. However, although impure TIF-IB can form a promoter-DNA complex resistant to challenge by other promoter-containing DNAs, near homogeneous TIF-IB cannot do so. An additional transcription factor, dubbed TIF-IE, restores the ability of near homogeneous TIF-IB to sequester DNA into a committed complex.

摘要

真核生物RNA聚合酶I用于核糖体RNA表达的基本转录起始因子(TIF),即TIF-IB,已使用标准技术从卡氏棘阿米巴中纯化至接近均一状态。纯化后的因子由TATA结合蛋白和四个TATA结合蛋白相关因子组成,其相对分子质量分别为145,000、99,000、96,000和91,000。由此计算出的天然分子量为460,000,与通过扫描透射电子显微镜测定的质量(493,000)以及其沉降速率(接近RNA聚合酶I的515,000)相当。不纯的和接近均一的TIF-IB都表现出56±3 pM的表观平衡解离常数。然而,尽管不纯的TIF-IB能够形成对其他含启动子的DNA的挑战具有抗性的启动子-DNA复合物,但接近均一的TIF-IB却不能。另一种转录因子,称为TIF-IE,可恢复接近均一的TIF-IB将DNA隔离到稳定复合物中的能力。

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