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建立一种基于分子和组织培养的联合方法用于检测鸡潜伏传染性喉气管炎病毒(ILTV)。

Development and application of a combined molecular and tissue culture-based approach to detect latent infectious laryngotracheitis virus (ILTV) in chickens.

机构信息

Asia-Pacific Centre for Animal Health, Melbourne Veterinary School, The University of Melbourne, Parkville, Victoria, Australia.

Asia-Pacific Centre for Animal Health, Melbourne Veterinary School, The University of Melbourne, Parkville, Victoria, Australia.

出版信息

J Virol Methods. 2020 Mar;277:113797. doi: 10.1016/j.jviromet.2019.113797. Epub 2019 Dec 9.

Abstract

Infectious laryngotracheitis virus (ILTV) causes severe respiratory disease in chickens. ILTV can establish latency and reactivate later in life, but there have been few investigations of ILTV latency. This study aimed to contribute to the methodologies available to detect latent ILTV. A nested PCR was developed which was more sensitive than three other molecular methods investigated in this study. This nested PCR was then used in conjunction with in vitro reactivation culture methods that were optimized and applied to trigeminal ganglia (TG) and tracheal samples from ILTV-vaccinated commercial layer birds (n = 30). ILTV DNA was detected by nested PCR in the upper respiratory tract (URT) or eye of 22 birds. Of the remaining 8 birds, ILTV could be detected by co-culture in TG of 5 birds, with reactivated virus mostly detected 6 days post-explant (dpe). ILTV was also detected in tracheal cultures by 6 dpe. In the ILTV-positive URT samples, the virus could be characterised as vaccine strains SA2 (n = 9) or A20 (n = 5). This study provides evidence for reactivation and shedding of vaccine ILTV in commercial layer birds. Moreover, this study produced a molecular and in-vitro culture method to detect latent viral infection.

摘要

传染性喉气管炎病毒(ILTV)可引起鸡的严重呼吸道疾病。ILTV 可以潜伏并在以后的生活中重新激活,但对 ILTV 潜伏的研究很少。本研究旨在为检测潜伏性 ILTV 的现有方法提供帮助。本研究开发了一种巢式 PCR,比本研究中调查的其他三种分子方法更敏感。然后,使用这种巢式 PCR 结合体外再激活培养方法,对来自 ILTV 疫苗接种的商业蛋鸡的三叉神经节(TG)和气管样本进行优化和应用(n=30)。通过巢式 PCR 在 22 只鸟的上呼吸道(URT)或眼睛中检测到 ILTV DNA。在其余 8 只鸟中,通过 5 只 TG 的共培养可检测到 ILTV,再激活病毒大多在 6 天(dpe)后检测到。在 6 dpe 时也可通过气管培养检测到 ILTV。在 ILTV 阳性 URT 样本中,病毒可被鉴定为疫苗株 SA2(n=9)或 A20(n=5)。本研究为商业蛋鸡中疫苗 ILTV 的再激活和脱落提供了证据。此外,本研究还产生了一种分子和体外培养方法来检测潜伏性病毒感染。

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