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反式作用因子与布氏锥虫双链变异表面糖蛋白(VSG)表达位点启动子的结合。

Binding of trans-acting factors to the double-stranded variant surface glycoprotein (VSG) expression site promoter of Trypanosoma brucei.

作者信息

Pham V P, Rothman P B, Gottesdiener K M

机构信息

Department of Microbiology, Columbia College of Physicians and Surgeons, New York 10032, USA.

出版信息

Mol Biochem Parasitol. 1997 Oct;89(1):11-23. doi: 10.1016/s0166-6851(97)00094-7.

Abstract

Trypanosoma brucei evades its host's immune response by utilizing the system of antigenic variation, whereby the organism sequentially expresses antigenically distinct variant surface glycoproteins (VSGs). Actively expressed VSG genes are found in VSG expression sites (ESs), and transcription of these ESs is directed by a small promoter composed of two essential cis-acting elements, the VSG ES promoter upstream element (VUE) and VSG ES promoter downstream element (VDE). Using electrophoretic mobility shift assays, we have identified double-stranded DNA binding activity in bloodstream-form trypanosome nuclear extracts. This activity, the VEP complex, is specific for the VSG ES promoter, and requires the intact sequences of the VUE and VDE in the appropriate spacing. These requirements of VEP Complex formation parallel the requirements for promoter function, suggesting that the VEP complex may be composed of functionally significant trans-acting factors. Furthermore, the requirement of both elements suggests that the binding of factors to the promoter may be cooperative. However, subtly different binding characteristics were observed when we used nuclear extracts derived from procyclic trypanosomes.

摘要

布氏锥虫通过利用抗原变异系统来逃避宿主的免疫反应,在该系统中,这种生物体依次表达抗原性不同的变异表面糖蛋白(VSG)。活跃表达的VSG基因存在于VSG表达位点(ES)中,这些ES的转录由一个小启动子指导,该启动子由两个必需的顺式作用元件组成,即VSG ES启动子上游元件(VUE)和VSG ES启动子下游元件(VDE)。使用电泳迁移率变动分析,我们在血流形式的锥虫核提取物中鉴定出双链DNA结合活性。这种活性,即VEP复合物,对VSG ES启动子具有特异性,并且需要VUE和VDE的完整序列以适当的间距存在。VEP复合物形成的这些要求与启动子功能的要求相似,这表明VEP复合物可能由功能上重要的反式作用因子组成。此外,对两个元件的需求表明因子与启动子的结合可能是协同的。然而,当我们使用源自前循环锥虫的核提取物时,观察到了细微不同的结合特征。

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