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本文引用的文献

1
High-throughput molecular detection of hemorrhagic fever virus threats with applications for outbreak settings.用于疫情爆发场景的出血热病毒威胁的高通量分子检测
J Infect Dis. 2007 Nov 15;196 Suppl 2:S205-12. doi: 10.1086/520601.
2
Complete genome analysis of 33 ecologically and biologically diverse Rift Valley fever virus strains reveals widespread virus movement and low genetic diversity due to recent common ancestry.对33种生态和生物学特性各异的裂谷热病毒株进行的全基因组分析显示,由于近期存在共同祖先,该病毒出现了广泛传播且遗传多样性较低。
J Virol. 2007 Mar;81(6):2805-16. doi: 10.1128/JVI.02095-06. Epub 2006 Dec 27.
3
Rift Valley fever epidemic in Saudi Arabia: epidemiological, clinical, and laboratory characteristics.沙特阿拉伯的裂谷热疫情:流行病学、临床及实验室特征
Clin Infect Dis. 2003 Oct 15;37(8):1084-92. doi: 10.1086/378747. Epub 2003 Sep 23.
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The pathogenesis of Rift Valley fever in lambs.羔羊裂谷热的发病机制。
Am J Vet Res. 1962 May;23:470-9.
5
Genetic analysis of viruses associated with emergence of Rift Valley fever in Saudi Arabia and Yemen, 2000-01.2000 - 2001年沙特阿拉伯和也门与裂谷热出现相关病毒的基因分析
Emerg Infect Dis. 2002 Dec;8(12):1415-20. doi: 10.3201/eid0812.020195.
6
Rapid detection and quantification of RNA of Ebola and Marburg viruses, Lassa virus, Crimean-Congo hemorrhagic fever virus, Rift Valley fever virus, dengue virus, and yellow fever virus by real-time reverse transcription-PCR.通过实时逆转录聚合酶链反应快速检测和定量埃博拉病毒、马尔堡病毒、拉沙病毒、克里米亚-刚果出血热病毒、裂谷热病毒、登革病毒和黄热病病毒的RNA
J Clin Microbiol. 2002 Jul;40(7):2323-30. doi: 10.1128/JCM.40.7.2323-2330.2002.
7
Quantitative real-time PCR detection of Rift Valley fever virus and its application to evaluation of antiviral compounds.裂谷热病毒的定量实时聚合酶链反应检测及其在抗病毒化合物评价中的应用。
J Clin Microbiol. 2001 Dec;39(12):4456-61. doi: 10.1128/JCM.39.12.4456-4461.2001.
8
Update: outbreak of Rift Valley Fever--Saudi Arabia, August-November 2000.最新消息:裂谷热疫情——沙特阿拉伯,2000年8月至11月
MMWR Morb Mortal Wkly Rep. 2000 Nov 3;49(43):982-5.
9
Climate and satellite indicators to forecast Rift Valley fever epidemics in Kenya.用于预测肯尼亚裂谷热疫情的气候和卫星指标
Science. 1999 Jul 16;285(5426):397-400. doi: 10.1126/science.285.5426.397.
10
Rift Valley fever in humans in South Africa.南非人类中的裂谷热
S Afr Med J. 1980 Nov 15;58(20):803-6.

用于高通量检测裂谷热病毒的高灵敏度和广泛反应性定量逆转录-PCR检测法

Highly sensitive and broadly reactive quantitative reverse transcription-PCR assay for high-throughput detection of Rift Valley fever virus.

作者信息

Bird Brian H, Bawiec Darcy A, Ksiazek Thomas G, Shoemaker Trevor R, Nichol Stuart T

机构信息

Special Pathogens Branch, Division of Viral and Rickettsial Diseases, National Center for Zoonotic, Vector-Borne and Enteric Diseases, Centers for Disease Control and Prevention, Atlanta, GA 30329, USA.

出版信息

J Clin Microbiol. 2007 Nov;45(11):3506-13. doi: 10.1128/JCM.00936-07. Epub 2007 Sep 5.

DOI:10.1128/JCM.00936-07
PMID:17804663
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2168471/
Abstract

Rift Valley fever (RVF) virus is a mosquito-borne virus associated with large-scale epizootics/epidemics throughout Africa and the Arabian peninsula. Virus infection can result in economically disastrous "abortion storms" and high newborn mortality in livestock. Human infections result in a flu-like illness, with 1 to 2% of patients developing severe complications, including encephalitis or hemorrhagic fever with high fatality rates. There is a critical need for a highly sensitive and specific molecular diagnostic assay capable of detecting the natural genetic spectrum of RVF viruses. We report here the establishment of a pan-RVF virus quantitative real-time reverse transcription-PCR assay with high analytical sensitivity (approximately 5 RNA copies of in vitro-transcribed RNA/reaction or approximately 0.1 PFU of infectious virus/reaction) and efficiency (standard curve slope = -3.66). Based on the alignments of the complete genome sequences of 40 ecologically and biologically diverse virus isolates collected over 56 years (1944 to 2000), the primer and probe annealing sites targeted in this assay are known to be located in highly conserved genomic regions. The performance of this assay relative to serologic assays is illustrated by testing of known RVF case materials obtained during the Saudi Arabia outbreak in 2000. Furthermore, analysis of acute-phase blood samples collected from human patients (25 nonfatal, 8 fatal) during that outbreak revealed that patient viremia at time of presentation at hospital may be a useful prognostic tool in determining patient outcome.

摘要

裂谷热(RVF)病毒是一种由蚊子传播的病毒,与非洲和阿拉伯半岛各地的大规模动物疫情/流行病有关。病毒感染可导致牲畜出现经济损失惨重的“流产风暴”和高新生死亡率。人类感染会引发类似流感的疾病,1%至2%的患者会出现严重并发症,包括脑炎或出血热,病死率很高。迫切需要一种能够检测RVF病毒自然遗传谱的高度灵敏且特异的分子诊断检测方法。我们在此报告建立了一种泛RVF病毒定量实时逆转录PCR检测方法,该方法具有高分析灵敏度(约5个体外转录RNA拷贝/反应或约0.1个感染性病毒PFU/反应)和效率(标准曲线斜率=-3.66)。基于对56年(1944年至2000年)收集的40株生态和生物学特性各异的病毒分离株完整基因组序列的比对,已知该检测方法中引物和探针的退火位点位于高度保守的基因组区域。通过对2000年沙特阿拉伯疫情期间获得的已知RVF病例材料进行检测,说明了该检测方法相对于血清学检测方法的性能。此外,对该疫情期间从人类患者(25例非致命、8例致命)采集的急性期血样进行分析发现,患者入院时的病毒血症可能是确定患者预后的有用预后工具。