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与十头持续感染牛病毒性腹泻病毒(BVDV)的牛混养的牛中短暂性BVDV感染的分子检测与特征分析

Molecular detection and characterization of transient bovine viral diarrhea virus (BVDV) infections in cattle commingled with ten BVDV persistently infected cattle.

作者信息

Peddireddi Lalitha, Foster Kelly A, Poulsen Elizabeth G, An Baoyan, Hoang Quoc Hung, O'Connell Catherine, Anderson Joseph W, Thomson Daniel U, Hanzlicek Gregg A, Bai Jianfa, Hesse Richard A, Oberst Richard D, Anderson Gary A, Leyva-Baca Ivan

机构信息

Kansas State Veterinary Diagnostic Laboratory (Peddireddi, An, Poulsen, JW Anderson, Hanzlicek, Bai, Oberst, GA Anderson), College of Veterinary Medicine, Kansas State University, Manhattan, KS.

Department of Diagnostic Medicine/Pathobiology (Foster, Thomson), College of Veterinary Medicine, Kansas State University, Manhattan, KS.

出版信息

J Vet Diagn Invest. 2018 May;30(3):413-422. doi: 10.1177/1040638717753962. Epub 2018 Jan 11.

Abstract

Fifty-three cattle of unknown serologic status that were not persistently infected (PI) with bovine viral diarrhea virus (BVDV) were commingled with 10 cattle that were PI with different strains of BVDV, and were monitored for an extended commingle period using a reverse-transcription real-time PCR (RT-rtPCR) BVDV assay on various sample types. Transient infections with BVDV were also assessed by virus isolation, virus neutralization (VN) assays, and direct buffy coat 5'-UTR sequencing. Infections were demonstrated in all cattle by RT-rtPCR; however, the detection rate was dependent on the type of sample. Buffy coat samples demonstrated a significantly greater number of positive results ( p ≤ 0.05) than either serum or nasal swab samples. Presence of elevated BVDV VN titers at the onset inversely correlated with the number of test days positive that an individual would be identified by RT-rtPCR from buffy coat samples, and directly correlated with the average Ct values accumulated over all RT-rtPCR test days from buffy coat samples. Both single and mixed genotype/subgenotype/strain infections were detected in individual cattle by direct sample 5'-UTR sequencing. A BVDV-2a strain from a PI animal was found to be the predominant strain infecting 64% of all non-PI cattle; BVDV-1b strains originating from 3 PI cattle were never detected in non-PI cattle. Although direct sample 5'-UTR sequencing was capable of demonstrating mixed BVDV infections, identifying all strains suspected was not always efficient or possible.

摘要

将53头血清学状态不明且未持续感染牛病毒性腹泻病毒(BVDV)的牛与10头持续感染不同毒株BVDV的牛混群,并在延长的混群期内,使用逆转录实时PCR(RT-rtPCR)BVDV检测法对各种样本类型进行监测。还通过病毒分离、病毒中和(VN)试验和直接血沉棕黄层5'-UTR测序评估BVDV的短暂感染。通过RT-rtPCR在所有牛中均检测到感染;然而,检出率取决于样本类型。血沉棕黄层样本的阳性结果数量显著多于血清或鼻拭子样本(p≤0.05)。开始时BVDV VN滴度升高与个体通过血沉棕黄层样本的RT-rtPCR检测出阳性的检测天数呈负相关,与血沉棕黄层样本所有RT-rtPCR检测天数积累的平均Ct值呈正相关。通过直接样本5'-UTR测序在个体牛中检测到单基因型/亚基因型/毒株感染和混合感染。发现来自一头持续感染动物的BVDV-2a毒株是感染所有非持续感染牛的64%的主要毒株;源自3头持续感染牛的BVDV-1b毒株在非持续感染牛中从未检测到。尽管直接样本5'-UTR测序能够证明BVDV混合感染,但识别所有疑似毒株并不总是有效或可行的。

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