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对驱动VESA1表达并与牛巴贝斯虫抗原变异相关的异常双向ves启动子的表征。

Characterization of the unusual bidirectional ves promoters driving VESA1 expression and associated with antigenic variation in Babesia bovis.

作者信息

Wang Xinyi, Xiao Yu-Ping, Bouchut Anne, Al-Khedery Basima, Wang Hongbin, Allred David R

机构信息

Department of Infectious Diseases and Pathology, University of Florida, Gainesville, FL, USA.

出版信息

Eukaryot Cell. 2012 Mar;11(3):260-9. doi: 10.1128/EC.05318-11. Epub 2012 Jan 27.

Abstract

Rapid clonal antigenic variation in Babesia bovis involves the variant erythrocyte surface antigen-1 (VESA1) protein expressed on the infected-erythrocyte surface. Because of the significance of this heterodimeric protein for demonstrated mechanisms of parasite survival and virulence, there is a need to understand how expression of the ves multigene family encoding this protein is controlled. As an initial step toward this goal, we present here initial characterization of the ves promoter driving transcription of VESA1a and -1b subunits. A series of transfection constructs containing various sequence elements from the in vivo locus of active ves transcription (LAT) were used to drive expression of the firefly luciferase gene in a dual luciferase-normalized assay. The results of this approach reveal the presence of two bidirectional promoter activities within the 434-bp intergenic region (IGr), influenced by putative regulatory sequences embedded within the flanking ves1α and ves1β genes. Repressor-like effects on the apposing gene were observed for intron 1 of both ves1α and ves1β. This effect is apparently not dependent upon intronic promoter activity and acts only in cis. The expression of genes within the ves family is likely modulated by local elements embedded within ves coding sequences outside the intergenic promoter region in concert with chromatin modifications. These results provide a framework to help us begin to understand gene regulation during antigenic variation in B. bovis.

摘要

牛巴贝斯虫的快速克隆抗原变异涉及感染红细胞表面表达的变异红细胞表面抗原-1(VESA1)蛋白。由于这种异二聚体蛋白对于已证实的寄生虫生存和毒力机制具有重要意义,因此有必要了解编码该蛋白的ves多基因家族的表达是如何受到调控的。作为实现这一目标的第一步,我们在此展示驱动VESA1a和-1b亚基转录的ves启动子的初步特征。一系列包含来自活跃ves转录体内位点(LAT)的各种序列元件的转染构建体,用于在双荧光素酶标准化测定中驱动萤火虫荧光素酶基因的表达。这种方法的结果揭示了在434 bp基因间隔区(IGr)内存在两种双向启动子活性,受侧翼ves1α和ves1β基因中嵌入的假定调控序列影响。观察到ves1α和ves1β的内含子1对相对基因有类似阻遏物的作用。这种效应显然不依赖于内含子启动子活性,且仅顺式作用。ves家族内基因的表达可能受基因间隔启动子区域外ves编码序列中嵌入的局部元件与染色质修饰协同调节。这些结果提供了一个框架,有助于我们开始了解牛巴贝斯虫抗原变异过程中的基因调控。

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