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The Babesia bovis Merozoite Surface Antigen 2 Locus Contains Four Tandemly Arranged and Expressed Genes Encoding Immunologically Distinct Proteins

机译:牛巴贝斯菌裂殖子表面抗原2基因座包含四个串联排列并表达的编码免疫学上不同蛋白质的基因。

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摘要

Members of the variable merozoite surface antigen (vmsa) gene family of Babesia bovis encode membrane proteins involved in erythrocyte invasion. In this study, we have identified and sequenced the complete 8.3-kb genomic locus containing msa-2, a member of the vmsa family, in the biologically cloned Mexico Mo7 strain. Four tandemly arranged copies of msa-2-related genes were found in the locus. The four genes, designated msa-2a1 (which corresponds to the originally described msa-2 gene), msa-2a2, msa-2b, and msa-2c, were shown to be transcribed and expressed and encode proteins with open reading frames ranging in size from 266 (MSA-2c) to 317 (MSA-2a1) amino acids. MSA-2a1 and -2a2 are the most closely related of the four proteins (90% identity), differing by (i) the number of 24-amino-acid repeats that comprise a surface-exposed B-cell epitope and (ii) the presence of a 32-amino-acid area of recombination between MSA-2a2 and -2b. In contrast, msa-2c is most closely related to the previously described babr 0.8 gene in Australia strains of B. bovis. Comparison of MSA-2 proteins in the Argentina R1A strain of B. bovis with the Mexico Mo7 clone revealed a relatively high degree of conservation (83.6, 69.4, 79.1, and 88.7% amino acid identity for MSA-2a1, -2a2, -2b, and -2c, respectively), in contrast to the extensive MSA-1 sequence variation (52% identity) between the same two strains. Postinfection bovine immune serum contains antibodies that bound to each of the recombinant MSA-2 proteins. Blocking assays demonstrated the presence of unique B-cell epitopes in MSA-2a1, -2b, and -2c. The results support the evolution of the msa-2 locus through at least two gene duplications, with selection for multiple related but antigenically distinct merozoite surface proteins.
机译:牛巴贝斯虫的可变裂殖子表面抗原(vmsa)基因家族的成员编码参与红细胞入侵的膜蛋白。在这项研究中,我们已经鉴定并测序了在生物学上克隆的墨西哥Mo7菌株中包含mssa-2(vmsa家族成员)的完整8.3kb基因组座位。在基因座中发现了四个串联排列的msa-2相关基因拷贝。已显示四个基因,命名为msa-2a1(与最初描述的msa-2基因相对应),msa-2a2,msa-2b和msa-2c,可以被转录和表达,并以开放阅读框编码蛋白质。大小从266(MSA-2c)至317(MSA-2a1)个氨基酸。 MSA-2a1和-2a2是这四种蛋白中最紧密相关的(90%相同),区别在于(i)包含表面暴露的B细胞表位的24个氨基酸重复序列的数量和(ii) MSA-2a2和-2b之间存在32个氨基酸的重组区域。相比之下,msa-2c与澳大利亚牛分枝杆菌中先前描述的babr 0.8基因最密切相关。比较墨西哥牛Mo7克隆的阿根廷牛B.bovis R1A株中的MSA-2蛋白显示出相对较高的保守性(MSA-2a1,-2a2,-2b的氨基酸同一性为83.6、69.4、79.1和88.7%与分别在两个菌株之间产生的MSA-1序列变异较大(同一性为52%)相反。感染后牛免疫血清含有与每种重组MSA-2蛋白结合的抗体。阻断试验表明,MSA-2a1,-2b和-2c中存在独特的B细胞表位。结果支持通过至少两个基因重复来进行msa-2基因座的进化,并选择了多个相关但抗原性不同的裂殖子表面蛋白。

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