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一种用于检测三种猫肠道病毒的多重聚合酶链反应检测方法的开发与应用

Development and utilization of a multiplex PCR assay for detecting three feline enteroviruses.

作者信息

Gao Shansong, Zhang Ruihua, Liu Gang, Yu Yongle, Han Xianjie

机构信息

College of Veterinary Medicine, Qingdao Agricultural University, Qingdao, 266109, PR China.

Liangshan County, Jining, 272600, PR China.

出版信息

Mol Biol Rep. 2025 Jan 28;52(1):170. doi: 10.1007/s11033-025-10283-y.

Abstract

BACKGROUND

Feline diarrhea is a common digestive tract disease in clinical practice, with watery feces as the main clinical manifestation. There are numerous pathogenic factors causing feline diarrhea, among which viral infections are prevalent, and feline panleukopenia virus (FPV) is the most common pathogen. In recent years, a variety of novel viruses have been detected in the intestines of cats with diarrhea. For example, feline kobuvirus (FKoV) and feline norovirus (FNoV) have been identified. These viruses may have a direct relationship with feline diarrhea or the connection has yet to be discovered. However, with the continuous emergence of these novel viruses and the frequent contact between pet cats and humans, it is prone to large-scale epidemics and outbreaks of viruses. Therefore, developing an accurate, rapid, and simple method to detect novel enteric viruses is of great significance for the early warning of emerging feline enteric viral infectious diseases.

METHODS AND RESULTS

A detailed comparison of the genome sequences of the three aforementioned feline enteroviruses was conducted. Subsequently, three pairs of specific primers were designed by selecting the conserved gene regions, and the single and multiplex PCR amplification reaction systems as well as reaction conditions were repeatedly optimized. The target fragment sizes detected by the multiplex PCR method were 650 bp for FPV, 500 bp for FKoV, and 340 bp for FNoV. Sensitivity tests demonstrated that the lower detection limit was one-tenth of that of single PCR. Meanwhile, the detection results for feline calicivirus (FCV), feline herpesvirus (FHV), and feline coronavirus (FCoV) were all negative. Testing of a total of 209 clinical samples from various regions in Shandong Province revealed that the detection rates of the three viruses were 13.4%, 4.8%, and 3.8%, respectively, and mixed infections were present.

CONCLUSIONS

In this study, an epidemiological investigation of the three feline enteroviruses was performed, and a sensitive, specific, and reproducible multiplex PCR assay was developed, which can be utilized for the detection of clinical samples.

摘要

背景

猫腹泻是临床常见的消化道疾病,主要临床表现为粪便稀溏。引起猫腹泻的致病因素众多,其中病毒感染较为普遍,猫泛白细胞减少症病毒(FPV)是最常见的病原体。近年来,在腹泻猫的肠道中检测到多种新型病毒。例如,已鉴定出猫杯状病毒(FKoV)和猫诺如病毒(FNoV)。这些病毒可能与猫腹泻有直接关系,也可能尚未被发现其联系。然而,随着这些新型病毒的不断出现以及宠物猫与人类的频繁接触,容易引发病毒的大规模流行和暴发。因此,开发一种准确、快速且简便的方法来检测新型肠道病毒,对于早期预警猫肠道病毒性传染病具有重要意义。

方法与结果

对上述三种猫肠道病毒的基因组序列进行了详细比较。随后,通过选择保守基因区域设计了三对特异性引物,并反复优化了单重和多重PCR扩增反应体系以及反应条件。多重PCR方法检测到的目标片段大小分别为:FPV为650 bp,FKoV为500 bp,FNoV为340 bp。敏感性试验表明,较低检测限是单重PCR的十分之一。同时,猫杯状病毒(FCV)、猫疱疹病毒(FHV)和猫冠状病毒(FCoV)的检测结果均为阴性。对山东省不同地区的209份临床样本进行检测发现,三种病毒的检出率分别为13.4%、4.8%和3.8%,且存在混合感染。

结论

本研究对三种猫肠道病毒进行了流行病学调查,并开发了一种灵敏、特异且可重复的多重PCR检测方法,可用于临床样本的检测。

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