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2023 - 2024年埃塞俄比亚默克莱和比绍夫图商业养鸡场传染性支气管炎病毒的分离、分子鉴定及系统发育分析

Isolation, molecular identification, and phylogenetic analysis of infectious bronchitis virus from commercial chicken farms in Mekele and Bishoftu, Ethiopia, 2023-2024.

作者信息

Berhanu Nigusu, Hirpa Eyob, Mohammed Hawa, Legesse Abinet, Deresse Getaw, Assefa Eyob, Tesgera Takele, Akalu Mirtneh, Abayneh Takele, Bayissa Berecha, Tesfaw Liyuwork, Birhanu Kenaw, Gelaye Esayas

机构信息

Research and Development Directorate, National Veterinary Institute (NVI), P.O. Box 19, Bishoftu, Ethiopia.

College of Veterinary Medicine and Agriculture, Department of Microbiology, Immunology and Veterinary Public Health, Addis Ababa University, P.O. Box 34, Bishoftu, Ethiopia.

出版信息

Virol J. 2025 Apr 2;22(1):90. doi: 10.1186/s12985-025-02639-4.

Abstract

BACKGROUND

Avian infectious bronchitis (IB) is a highly contagious respiratory disease that affects the poultry industry globally. The disease is caused by avian infectious bronchitis virus (IBV), member of the genus Gammacoronavirus. In Ethiopia, IBV has been reported in both commercial and backyard chickens based on clinical observation. The objectives of this study were to isolate the virus, conduct molecular based identification, and phylogenetic analysis of the circulating IBV isolates.

METHODS AND MATERIALS

A cross-sectional study was conducted between November 2023 and May 2024 in Mekele and Bishoftu, Ethiopia. A total of 49 clinical samples were collected, comprising 12 tissue samples and 39 pooled swab samples. Of these, 6 samples-specifically, 5 swab samples and 1 tissue sample-tested positive for infectious bronchitis virus (IBV) through virus-specific conventional RT-PCR and real-time PCR. Nested PCR was performed using serotype-specific primers. The purified PCR products, which targeted the spike glycoprotein S1 subunit gene and the 3' UTR of the IBV, were sequenced, followed by phylogenetic tree analysis.

RESULTS

The six positive samples propagated into specific pathogen free embryonated eggs and exhibited characteristic IBV lesions and mortality observed over five consecutive passages. IBV isolates from Bishoftu (n = 4) and Mekele (n = 2) were amplified using one-step RT-PCR to target 466 bp of the S1 subunit gene and 433 bp of the 3'UTR. A BLAST search on the S1 partial gene and 3'UTR sequences, nested PCR, and phylogenetic analysis revealed that the present IBV isolates are genetically similar to the Massachusetts serotype. The S1 gene sequences of the five IBV isolates were deposited in GenBank with accession numbers PQ389500 to PQ389504.

CONCLUSIONS

This is the first detailed study on IB virus isolation, molecular detection, sequencing, and phylogenetic analysis in Ethiopia. The findings revealed that the outbreaks were caused by the IB virus, which created a serious health risk and economic losses in the chicken industry. To the author's knowledge, this is the first comprehensive study on the isolation and genetic analysis of IBV in Ethiopia. Further research on the economic impact of IBV in chicken production, farm biosecurity, serotyping of circulating IB virus, and vaccine development based on the local serotypes is recommended.

摘要

背景

禽传染性支气管炎(IB)是一种高度传染性的呼吸道疾病,影响着全球家禽业。该疾病由γ冠状病毒属的禽传染性支气管炎病毒(IBV)引起。在埃塞俄比亚,根据临床观察,商业鸡群和后院鸡群中均有IBV感染的报道。本研究的目的是分离病毒,进行基于分子的鉴定,并对循环中的IBV分离株进行系统发育分析。

方法和材料

2023年11月至2024年5月在埃塞俄比亚的梅克内和比绍夫图进行了一项横断面研究。共收集了49份临床样本,包括12份组织样本和39份混合拭子样本。其中,6份样本——具体为5份拭子样本和1份组织样本——通过病毒特异性常规RT-PCR和实时PCR检测出传染性支气管炎病毒(IBV)呈阳性。使用血清型特异性引物进行巢式PCR。对靶向IBV刺突糖蛋白S1亚基基因和3'UTR的纯化PCR产物进行测序,随后进行系统发育树分析。

结果

6份阳性样本在无特定病原体的鸡胚中传代,在连续5代中均表现出特征性的IBV病变和死亡率。使用一步RT-PCR对来自比绍夫图(n = 4)和梅克内(n = 2)的IBV分离株进行扩增,以靶向S1亚基基因的466 bp和3'UTR的433 bp。对S1部分基因和3'UTR序列进行BLAST搜索、巢式PCR和系统发育分析后发现,目前的IBV分离株在基因上与马萨诸塞血清型相似。5株IBV分离株的S1基因序列已存入GenBank,登录号为PQ389500至PQ389504。

结论

这是埃塞俄比亚首次关于IB病毒分离、分子检测、测序和系统发育分析的详细研究。研究结果表明,疫情是由IB病毒引起的,这给养鸡业带来了严重的健康风险和经济损失。据作者所知,这是埃塞俄比亚首次关于IBV分离和遗传分析的全面研究。建议进一步研究IBV对鸡肉生产的经济影响、农场生物安全、循环IB病毒的血清分型以及基于当地血清型的疫苗开发。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/925a/11963663/8cacedb8084a/12985_2025_2639_Fig1_HTML.jpg

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