Feline calicivirus (FCV)

  • 文章类型: Journal Article
    城市流浪猫是没有主人的猫,可以在野外长时间生存。它们是城市中最常见的流浪动物之一,因此,监测城市流浪猫携带的病原体是城市流行病学监测的重要组成部分。为了解上海市城市流浪猫呼吸道疾病的患病情况,为制定有针对性的流浪猫呼吸道疾病防控策略提供科学依据,我们收集了374眼,鼻部,2022年1月至2022年12月,上海城市流浪猫的口咽拭子。RNA提取后,我们使用实时PCR检测了六种呼吸道病原体,包括甲型流感病毒,猫杯状病毒,猫疱疹病毒1型支原体,衣原体,和支气管败血杆菌.结果表明,在374个样本中,146检测呈阳性,阳性率为39.04%。观察到最高的阳性率为18.72%(70/374),其次是衣原体,占11.76%(44/374),猫杯状病毒为3.74%(14/374),猫疱疹病毒1型,占3.48%(13/374),支气管败血波氏杆菌占1.34%(5/374),未检测到甲型流感病毒。非支原体阳性率最高的是闵行区,为31.94%(23/72),而嘉定区非衣原体和支气管败血波氏杆菌的阳性率最高,分别为23.53%(8/34)和5.88%(2/34),分别。青浦区猫杯状病毒和猫疱疹病毒1型阳性率均最高,分别为14.46%(12/83)和9.64%(8/83),分别。共有36份样本显示两种或两种以上病原体混合感染,在这些混合感染中,有32种由非支原体感染引起,在25个样本中,费氏衣原体的混合感染数量最高。全年检测到呼吸道病原体阳性,夏季和冬季的峰值检测率。不同季节猫呼吸道病原体阳性率差异有统计学意义(χ2=27.73,p<0.01)。不同性别猫呼吸道病原体阳性率差异无统计学意义(χ2=0.92,p>0.05)。不同年龄组猫呼吸道病原体阳性率差异有统计学意义(χ2=44.41,p<0.01)。非氏支原体和衣原体是导致流浪猫呼吸道感染的主要病原体,与其他呼吸道病原体相比,猫支原体显示出更高的阳性率,并且通常与猫衣原体和猫杯状病毒共同感染。夏季,白花支原体阳性率较高,秋天,冬天,季节之间没有统计学差异。这些结果表明,上海地区城市流浪猫的呼吸道病原体总体流行严重,表现出季节性趋势和与其他病原体的混合感染。这些发现表明,需要采取综合预防和控制措施来解决上海地区城市流浪猫的呼吸道病原体感染。
    Urban stray cats are cats without owners that survive in the wild for extended periods of time. They are one of the most common stray animals in cities, and as such, monitoring the pathogens carried by urban stray cats is an important component of urban epidemiological surveillance. In order to understand the prevalence of respiratory diseases in urban stray cats in Shanghai and provide scientific evidence for the development of targeted prevention and control strategies for respiratory diseases in stray cats, we collected 374 ocular, nasal, and oropharyngeal swabs from urban stray cats in Shanghai from January 2022 to December 2022. After RNA extraction, we used real-time PCR to detect six respiratory pathogens, including influenza A virus, feline calicivirus, feline herpesvirus type 1, Mycoplasma, Chlamydia, and Bordetella bronchiseptica. The results showed that among the 374 samples, 146 tested positive, with a positivity rate of 39.04%. The highest positivity rate was observed for Mycoplasma felis at 18.72% (70/374), followed by Chlamydia felis at 11.76% (44/374), feline calicivirus at 3.74% (14/374), feline herpesvirus 1 at 3.48% (13/374), Bordetella bronchiseptica at 1.34% (5/374), and influenza A virus was not detected. The highest positivity rate for Mycoplasma felis was in Minhang District at 31.94% (23/72), while Chlamydia felis and Bordetella bronchiseptica had the highest positivity rates in Jiading District at 23.53% (8/34) and 5.88% (2/34), respectively. The highest positivity rates for feline calicivirus and feline herpesvirus 1 were both observed in Qingpu District, at 14.46% (12/83) and 9.64% (8/83), respectively. A total of 36 samples showed mixed infections with two or more pathogens, with Mycoplasma felis being involved in 32 of these mixed infections, with the highest number of mixed infections being with Chlamydia felis at 25 samples. Respiratory pathogen positivity was detected throughout the year, with peak detection rates in summer and winter. The positivity rates of cat respiratory pathogens in different seasons showed statistical differences (χ2 = 27.73, p < 0.01). There was no statistical difference in the positivity rates of respiratory pathogens between cats of different genders (χ2 = 0.92, p > 0.05). The positivity rates of respiratory pathogens in cats of different age groups showed statistical differences (χ2 = 44.41, p < 0.01). Mycoplasma felis and Chlamydia felis were the main pathogens causing respiratory infections in stray cats, with Mycoplasma felis showing a much higher positivity rate than other respiratory pathogens and often co-infecting with Chlamydia felis and feline calicivirus. The positivity rate of Mycoplasma felis was high in summer, autumn, and winter, with no statistical difference between seasons. These results indicate a serious overall prevalence of respiratory pathogens in urban stray cats in the Shanghai area, showing seasonal trends and mixed infections with other pathogens. These findings suggest the need for comprehensive prevention and control measures to address respiratory pathogen infections in urban stray cats in the Shanghai area.
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  • 文章类型: Journal Article
    强烈建议所有猫的猫核心疫苗是针对猫泛白细胞减少症病毒(FPV),Felid疱疹病毒1型(FeHV-1),和猫杯状病毒(FCV),但是根据猫的生活方式,猫可以分为低风险和高风险。这项研究的目的是确定针对FPV的实际血清保护,通过使用VacciCheck测试,在一大群意大利猫中的FeHV-1和FCV。分析总共740只猫(567只拥有和173只流浪猫;435只接种疫苗和305只未接种疫苗)的保护性抗体滴度(PAT)。与原产地有关的差异,性别,年龄,品种,FIV/FeLV状态,健康状况,和自上次疫苗接种以来经过的时间进行了评估。整个队列中不到一半(36.4%)同时患有所有三种疾病的PAT,如果还考虑弱正值,则增加到48.6%,仅考虑435只接种疫苗的猫时增加到50.3%。特别是,检测到针对FCV的抗体,FPV,和FeHV-1在保护滴度(PAT)为78.6%,68.1和49.1%的猫,分别。总的来说,拥有,中性,成年FIV和/或FeLV阴性猫是最受保护的类别,即使不总是这三种病毒。大多数猫在接种FPV和FCV后3年或更长时间保持高PAT,但不是FeHV-1。在最后一次疫苗接种后,持久的保护性免疫力持续了很多年(在最古老的猫中超过18年)。然而,因为并不是所有的猫在这么多年后都受到了保护,所有的病原体,通过抗体滴定检查保护可能是防止免疫故障的最佳选择。讨论还重点讨论了两种URTD(上呼吸道疾病)病毒的抗体滴定的可靠性,与FPV不同,没有被广泛接受为有效的保护指标。
    Feline core vaccines strongly recommended for all cats are against Feline panleukopenia virus (FPV), Felid herpesvirus type 1 (FeHV-1), and Feline calicivirus (FCV), but cats can be classified as low- and high-risk based on their lifestyle. The aim of this study was to determine the actual seroprotection against FPV, FeHV-1, and FCV in a large cohort of Italian cats by using the VacciCheck test. A total of 740 cats (567 owned and 173 stray cats; 435 vaccinated and 305 unvaccinated) were analyzed for Protective Antibody Titers (PATs). Differences related to origin, sex, age, breed, FIV/FeLV status, health status, and time elapsed since last vaccination were evaluated. Less than half of the entire cohort (36.4%) had PATs for all three diseases simultaneously, increasing to 48.6% if weak positive values were also considered and 50.3% when considering only the 435 vaccinated cats. Particularly, antibodies were detected against FCV, FPV, and FeHV-1 at protective titers (PATs) in 78.6%, 68.1, and 49.1% of the cats, respectively. In general, owned, neutered, and adult FIV- and/or FeLV-negative cats were the most protected categories, even if not always for the three viruses. Most cats maintained high PATs for 3 years or longer after vaccination against FPV and FCV but not FeHV-1. Long-lasting protective immunity persisted for many years after the last vaccination (more than 18 years in the oldest cats). Nevertheless, since not all cats were protected after so many years and for all pathogens, checking protection via antibody titration could be the best choice to prevent immunity breakdowns. The discussion also focuses on the reliability of antibody titration for the two URTD (upper respiratory tract disease) viruses which, unlike for FPV, is not widely accepted as a valid index of protection.
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  • 文章类型: Journal Article
    猫杯状病毒(FCV)具有单链,正义RNA基因组,它是猫的许多传染性呼吸道疾病的原因。此外,更令人担忧的是,FCV的高毒力菌株可导致猫科动物的高死亡率。因此,快速可靠的诊断工具在控制FCV爆发中起着重要作用.在这项研究中,酶促重组酶扩增(ERA)结合侧流试纸(LFD)检测FCV,靶向FCV-ORF1的相对转换位置。结果表明,最佳反应条件为40℃反应30min。ERA-LFD方法灵敏度高,每个反应的FCVRNA的检出限低至3.2TCID50。特异性分析表明与猫细小病毒(FPV)没有交叉反应,猫疱疹病毒(FHV)和猫传染性腹膜炎病毒(FIPV)。ERA-LFD具有高度可重复性和可重复性,该方法的测定内和测定间变异系数均小于7%。一般测试表明,本实验室保存的所有具有已知突变位点的重组质粒和具有不同突变位点的FCV菌株均通过该方法检测到。在23个样本中,14份样本通过ERA-LFD和RT-qPCR检测为FCV阳性,分别。总之,ERA-LFD检测是一种快速的,准确,方便的诊断工具,用于FCV的检测。关键点:•介绍了ERA-LFD的检测原理。•几乎所有目前已知的FCV菌株都可以被检测到。•ERA-LFD易于操作,可用于现场检测。
    Feline calicivirus (FCV) has a single-stranded, positive-sense RNA genome, and it is responsible for many infectious respiratory diseases in cats. In addition, more worryingly, highly virulent strains of FCV can cause high mortality in felines. Therefore, a rapid and reliable diagnosis tool plays an important role in controlling the outbreak of FCV. In this study, enzymatic recombinase amplification (ERA) assay combined with lateral flow dipstick (LFD) was developed for the detection of FCV, targeting a relatively conversed position of FCV-ORF1. The results showed that the optimal reaction condition was at 40 °C for 30 min. ERA-LFD method was highly sensitive with the detection limit as low as 3.2 TCID50 of FCV RNA per reaction. The specificity analysis demonstrated no cross-reactivity with feline parvovirus (FPV), feline herpesvirus (FHV) and feline infectious peritonitis virus (FIPV). ERA-LFD was highly repeatable and reproducible, with the intra-assay and inter-assay coefficients of variation for this method both less than 7%. The general test showed that all the recombinant plasmids with known mutant sites and FCV strains with different mutant sites stored in our laboratory were all detected by this method. Of the 23 samples, 14 samples were tested positive for FCV by ERA-LFD and RT-qPCR, respectively. In summary, ERA-LFD assay was a fast, accurate and convenient diagnosis tool for the detection of FCV. KEY POINTS: • The detection principle of ERA-LFD was introduced. • Almost all the currently known FCV strains can be detected. • ERA-LFD is easy to operate and can be used for field detection.
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  • 文章类型: Journal Article
    Feline calicivirus (FCV) is a major pathogen of cats associated with either respiratory disease or systemic disease, but its possible role as an enteric pathogen is neglected. Using RT-PCR, the RNA of FCV was identified in 25.9% (62/239) of stools of cats with enteritis and in 0/58 (0%) of cats without diarrhoea or other clinical signs. Isolates of enteric origin were obtained and a large 3.2-kb portion of the genome was sequenced, encompassing the 3\' end of the RNA polymerase, the capsid protein precursor and the minor capsid protein. Also, the complete genome sequence of one such strain, the 160/2015/ITA, was determined. Upon sequence analysis, the enteric viruses were found to be genetically heterogeneous and to differ from each other and from isolates of respiratory origin. The enteric isolates were found to be more resistant to low pH conditions, to trypsin and to bile treatment than respiratory isolates. Overall, these findings are consistent with the hypothesis that some FCVs may acquire enteric tropism and eventually act as enteric pathogens. Whether this enteric tropism is maintained stably and whether it may affect, to some extent, the ability of the virus to trigger the classical and/or hypervirulent forms of disease should be assessed. Also, FCV should be included in the diagnostic algorithms of enteric diseases of cats to gain further information about FCV strains displaying enteric pathotype.
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  • 文章类型: Journal Article
    Human noroviruses (HuNoVs) cause foodborne and waterborne viral gastroenteritis worldwide. Because HuNoV culture systems have not been developed thus far, no available medicines or vaccines preventing infection with HuNoVs exist. Some herbal extracts were considered as phytomedicines because of their bioactive components. In this study, the inhibitory effects of 29 edible herbal extracts against the norovirus surrogates murine norovirus (MNV) and feline calicivirus (FCV) were examined. FCV was significantly inhibited to 86.89 ± 2.01 and 48.71 ± 7.38% by 100 μg/mL of Camellia sinensis and Ficus carica, respectively. Similarly, ribavirin at a concentration of 100 μM significantly reduced the titer of FCV by 77.69 ± 10.40%. Pleuropterus multiflorus (20 μg/mL) showed antiviral activity of 53.33 ± 5.77, and 50.00 ± 16.67% inhibition was observed after treatment with 20 μg/mL of Alnus japonica. MNV was inhibited with ribavirin by 59.22 ± 16.28% at a concentration of 100 μM. Interestingly, MNV was significantly inhibited with 150 µg/mL Inonotus obliquus and 50 μg/mL Crataegus pinnatifida by 91.67 ± 5.05 and 57.66 ± 3.36%, respectively. Treatment with 20 µg/mL Coriandrum sativum slightly reduced MNV by 45.24 ± 4.12%. The seven herbal extracts of C. sinensis, F. carica, P. multiflorus, A. japonica, I. obliquus, C. pinnatifida, and C. sativum may have the potential to control noroviruses without cytotoxicity.
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  • 文章类型: Journal Article
    Feline calicivirus (FCV) is an important veterinary pathogen that causes acute upper respiratory tract diseases and, occasionally, highly contagious febrile hemorrhagic syndrome in cats. Many viruses have adopted mechanisms for evading IFN-α/β signaling, particularly by directly or indirectly suppressing activation of IRF-3. In this study, we investigated whether nonstructural proteins of FCV possess these mechanisms. When p39, a nonstructural protein of FCV, was transiently expressed in 293T cells, it suppressed IFN-β and ISG15 mRNA production induced by dsRNA. Expression of p39 also suppressed phosphorylation and dimerization of IRF-3 induced by dsRNA. These results suggest that p39 suppresses type 1 IFN production by preventing IRF-3 activation. This may become an important factor in understanding the pathogenesis and virulence of FCV.
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