ves1α 基因的表达是巴贝西亚布氏杆菌感染的红细胞细胞粘附到内皮细胞的主要决定因素

Hassan Hakimi, Junya Yamagishi, Miako Sakaguchi, Guilherme G. Verocai, Shin-ichiro Kawazu, Masahito Asada
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Variant Erythrocyte Surface Antigen 1 (VESA1) is one of those exported proteins by <em>B. bovis</em> which represents a major virulence factor due to its central role in immune evasion by antigenic variation and intravascular parasite sequestration. VESA1 is a heterodimer protein encoded by <em>ves1α</em> and <em>ves1β</em> multigene family and localized on the ridges, the focal point for cytoadhesion. To gain further insights into the molecular mechanisms of cytoadhesion of <em>B. bovis</em>, we panned the parasites with bovine brain microvasculature endothelial cells, which resulted in obtaining several clones with different cytoadherence abilities. The transcriptome analysis of 2 high and 2 low cytoadherent clones revealed that <em>ves1α</em> sequences were diversified, likely resulting from genomic recombination. On the other hand, <em>ves1β</em> sequences were almost identical among these 4 clones. 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摘要

牛巴贝斯虫是牛巴贝斯虫病中致病性最强的一种,会导致天真成年牛的高死亡率。这种寄生虫会侵入牛宿主体内的红细胞(RBC),并在其中繁殖和产生临床疾病。牛巴贝斯虫会向被感染的红细胞输出大量蛋白质,从而改变其特性。因此,受感染的红细胞(iRBC)能够在内脏和大脑的微血管中形成细胞粘附,导致呼吸困难、神经症状和死亡。变异红细胞表面抗原 1(VESA1)是牛海绵状芽孢杆菌输出的蛋白质之一,由于其在通过抗原变异和血管内寄生虫螯合逃避免疫方面的核心作用,因此是一种主要的致病因子。VESA1 是由 ves1α 和 ves1β 多基因家族编码的异源二聚体蛋白,定位于细胞粘附的焦点脊上。为了进一步了解牛海绵状芽孢杆菌细胞粘附的分子机制,我们将寄生虫与牛脑微血管内皮细胞进行了比对,从而获得了几个具有不同细胞粘附能力的克隆。对两个高细胞黏附性克隆和两个低细胞黏附性克隆的转录组分析表明,ves1α序列具有多样性,这可能是基因组重组的结果。另一方面,这 4 个克隆的 ves1β 序列几乎相同。将高结合率克隆的 ves1α 植入低结合率克隆的 ef-1α 基因座并表达,增加了细胞粘附性,这证实了转录组数据所显示的 ves1α 的作用。细胞粘附克隆的全基因组测序显示 ves1 的活性位点位于 2 号染色体上。这些结果表明,由 ves1α 基因编码的 VESA1a 蛋白决定了牛立克次体的细胞粘附特异性和/或细胞粘附强度,它们处于重组的活性位点。
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ves1α genes expression is the major determinant of Babesia bovis-infected erythrocytes cytoadhesion to endothelial cells
Babesia bovis causes the most pathogenic form of babesiosis in cattle, resulting in high mortality in naive adults. This parasite invades red blood cells (RBCs) within the bovine hosts where they multiply and produce clinical disease. Babesia bovis exports numerous proteins into invaded RBCs changing its properties. Thus, the infected RBCs (iRBCs) are capable to cytoadhere in the microvasculature of internal organs and brain, leading to respiratory distress, neurologic signs, and mortality. Variant Erythrocyte Surface Antigen 1 (VESA1) is one of those exported proteins by B. bovis which represents a major virulence factor due to its central role in immune evasion by antigenic variation and intravascular parasite sequestration. VESA1 is a heterodimer protein encoded by ves1α and ves1β multigene family and localized on the ridges, the focal point for cytoadhesion. To gain further insights into the molecular mechanisms of cytoadhesion of B. bovis, we panned the parasites with bovine brain microvasculature endothelial cells, which resulted in obtaining several clones with different cytoadherence abilities. The transcriptome analysis of 2 high and 2 low cytoadherent clones revealed that ves1α sequences were diversified, likely resulting from genomic recombination. On the other hand, ves1β sequences were almost identical among these 4 clones. Insertion and expression of ves1α of a clone with high binding into ef-1α locus of a low binging clone increased cytoadherence confirming the role of ves1α suggested by our transcriptome data. Whole genome sequencing of cytoadherent clones revealed active locus of ves1 on chromosome 2. These results suggest that VESA1a proteins encoded by ves1α genes determine the cytoadherence specificity and/or cytoadherence strength of B. bovis and they are in the active site for recombination.
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