Viral Protein 1 (VP1) Sequence-Based Genetic Diversity of SAT 2 FMDV Circulating in Ethiopia from 1990 to 2015.

IF 1.7 Q2 VETERINARY SCIENCES
Fanos Woldemariyam, Jan Paeshuyse
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引用次数: 0

Abstract

Introduction: Pathogen molecular epidemiology determines the origin of specific outbreaks locality of foot-and-mouth disease virus serotype South African Territories-2 sequence-based analysis of highly variable Viral Protein 1 (VP1), which helps to identify the evolution of this virus through time and space. The objective of this study was to compare the differences between SAT-2 VP1 sequences of FMDV circulated in Ethiopia from 1990 to 2015 at the genetic level.

Methods: The nucleotide and amino acid sequences were analyzed using Basic Local Alignment Search Tools (BLAST), Multiple sequence alignment and sequence editing and Phylogenetic tree reconstruction. The nucleotide and amino acid sequences alignment, distance matrix, and phylogenetic tree constructions were done using the MEGA 6.0 software package.

Result and discussion: In this analysis, we found 76% nucleotide identities and amino acid similarities among the sequences. The overall group mean distance at nucleotide level was 19% with a mean intra-population diversity of 2%. The lowest sequence variation was observed among sequences obtained from the years 2007/09/10, 2014/15, and 1990/91 which was less than 5% among them. This analysis revealed that in the last 25 years, four different topotypes of the FMDV SAT-2 were circulating in Ethiopia. The Arg-Gly-Asp (RGD) amino acid (AA) motif at AA position 144-146 within the G-H loop of the VP1 protein of FMDV is conserved, but up- and downstream hyper-variable AA sequences are identified. In this study, it was observed that four topotypes (IV, XIV, XIII, and VII) were circulating in Ethiopia for 25 years. Further, compared with sequences from neighboring countries (Sudan, Kenya) confirmed the presence of these topotypes.

Conclusion: Pertinent to this genetic diversity control strategies in Ethiopia should be based on having regular antigenic and genetic vaccine matching tests with the circulating strain within a defined period, space, transboundary nature of the disease and applying biosecurity measures.

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基于病毒蛋白1 (VP1)序列的埃塞俄比亚1990 - 2015年流行的SAT 2 FMDV遗传多样性
病原体分子流行病学确定了口蹄疫病毒血清型南非地区特定暴发的起源-2基于序列的高可变病毒蛋白1 (VP1)分析,有助于确定该病毒的时空演变。本研究的目的是比较1990年至2015年在埃塞俄比亚流行的FMDV的SAT-2 VP1序列在遗传水平上的差异。方法:利用BLAST (Basic Local Alignment Search Tools)、多序列比对和序列编辑、系统发育树重建等工具对其核苷酸和氨基酸序列进行分析。利用MEGA 6.0软件包进行核苷酸和氨基酸序列比对、距离矩阵和系统发育树构建。结果与讨论:在本分析中,我们发现76%的序列具有核苷酸同源性和氨基酸相似性。整个群体在核苷酸水平上的平均距离为19%,平均种群内多样性为2%。2007/09/10年、2014/15年和1990/91年的序列变异最小,均小于5%。这一分析表明,在过去25年中,四种不同类型的FMDV SAT-2在埃塞俄比亚流行。FMDV VP1蛋白G-H环中位于144-146位的Arg-Gly-Asp (RGD)氨基酸(AA)基序是保守的,但发现了上下游高度可变的AA序列。在这项研究中,观察到四种类型(IV, XIV, XIII和VII)在埃塞俄比亚流行了25年。此外,与邻国(苏丹、肯尼亚)的序列比较证实了这些拓扑型的存在。结论:与此相关的埃塞俄比亚遗传多样性控制战略应基于在规定的时间、空间、疾病的跨界性质和应用生物安全措施内与流行毒株定期进行抗原和遗传疫苗匹配试验。
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