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商业肉鸡中强毒传染性法氏囊病病毒的持续临床病理和分子识别。

Continuous clinicopathological and molecular recognition of very virulent infectious bursal disease virus in commercial broiler chickens.

机构信息

Department of Poultry Diseases, Faculty of Veterinary Medicine, Cairo University, Giza 12211, Egypt; Ceva Sante Animale, Al Sheikh Zayed, Giza, Egypt.

Reference Laboratory for Veterinary Quality Control on Poultry Production, Animal Health Research Institute, Agriculture Research Center, Giza 12618, Egypt.

出版信息

Poult Sci. 2024 Feb;103(2):103306. doi: 10.1016/j.psj.2023.103306. Epub 2023 Nov 20.

Abstract

Gumboro virus is one of the most dangerous immunosuppressant viruses that infect chickens and causes massive financial losses worldwide. The current study aims to conduct a molecular characterization of chicken farms for the infectious bursal disease virus (IBDV). Based on postmortem (PM) lesions, 125 bursal samples from 25 farms were collected from clinically diseased commercial chicken farms with increased mortality and suspected Gumboro virus infection. Pooled bursal samples from suspected IBD-vaccinated flocks were tested for IBDV by reverse transcriptase polymerase chain reaction (RT-PCR). Fifteen out of 25 pooled specimens were found positive for IBDV, with a 60% detection rate, and confirmed positive for very virulent IBDV (vvIBDV) by sequence analysis. Nucleotide phylogenetic analysis of VP1 and VP2 genes was employed to compare the 5 chosen isolates with strains representing different governorates in Egypt during 2022. All strains were clustered with vvIBDV with no evidence of reassortment in the VP1 gene. The VP1 and VP2 genes are divided into groups (I, II). The strains in our study were related to group II, and it acquired a new mutation in the VP2 gene that clustered it into new subgroup B. By mutation analysis, the VP2 gene of all strains had a characteristic mutation to vvIBDV. It acquired new mutations in HVRs compared with HK46 in Y220F, A222T/V in all strains in our study, and Q221K that was found in IBD-EGY-AH5 and AH2 in the loop P in addition to G254S in all strains in our study and Q249k that found in IBD-EGY-AH1 and AH3 in the loop P These mutations are important in the virulency and antigenicity of the virus. The VP1 had 242E, 390M, and 393D which were characteristic of vvIBDV and KpnI restriction enzyme (GGTAC/C) in addition to a new mutation (F243Y and N383H) in IBD-EGY-AH1 and AH4 strains. According to the current study, the strains were distinct from the vaccinal strain; they could be responsible for the most recent IBDV outbreaks observed in flocks instead of received vaccinations. The current study highlighted the importance of molecular monitoring to keep up to date on the circulating IBDV for regular evaluation of commercial vaccination programs against circulating field viruses.

摘要

传染性法氏囊病病毒(IBDV)是一种感染鸡并导致全球巨大经济损失的最危险的免疫抑制病毒之一。本研究旨在对鸡场进行传染性法氏囊病病毒(IBDV)的分子特征分析。根据尸检(PM)病变,从临床患病的商业鸡场采集了 25 个农场的 125 个法氏囊样本,这些鸡场的死亡率增加,并疑似感染了传染性法氏囊病毒。对疑似 IBD 疫苗接种鸡群的混合法氏囊样本进行反转录聚合酶链反应(RT-PCR)检测 IBDV。25 个混合样本中有 15 个被检测出 IBDV 呈阳性,检出率为 60%,并通过序列分析证实为强毒传染性法氏囊病病毒(vvIBDV)。通过 VP1 和 VP2 基因的核苷酸系统进化分析,将所选的 5 株分离株与 2022 年埃及不同省份的代表株进行比较。所有分离株均与 vvIBDV 聚类,VP1 基因无重组证据。VP1 和 VP2 基因分为 I 组和 II 组。本研究中的分离株与 II 组相关,在 VP2 基因中获得了一个新的突变,使其聚类为新的亚组 B。通过突变分析,所有分离株的 VP2 基因均具有 vvIBDV 的特征性突变。与 HK46 相比,所有分离株的 Y220F、A222T/V 在 VP2 基因中的 HVR 区获得了新的突变,在所有分离株中均发现了 Q221K,在 IBD-EGY-AH5 和 AH2 中的环 P 中发现了 G254S,在所有分离株中均发现了 Q249k,在 IBD-EGY-AH1 和 AH3 中的环 P 中发现了新的突变。这些突变在病毒的毒力和抗原性中很重要。VP1 有 242E、390M 和 393D,这是 vvIBDV 的特征,除了在 IBD-EGY-AH1 和 AH4 株中发现的新突变(F243Y 和 N383H)外,还有 KpnI 限制酶(GGTAC/C)。根据目前的研究,这些分离株与疫苗株不同,它们可能是最近观察到的鸡群中 IBDV 暴发的原因,而不是接种疫苗所致。本研究强调了进行分子监测的重要性,以随时了解循环 IBDV 的情况,从而定期评估针对循环田间病毒的商业疫苗接种计划。

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