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本文引用的文献

1
Tropical Q Fever.热带Q热
Am J Trop Med Hyg. 2022 Jul 11;107(2):219-220. doi: 10.4269/ajtmh.22-0372. Print 2022 Aug 17.
2
Incidence Estimates of Acute Q Fever and Spotted Fever Group Rickettsioses, Kilimanjaro, Tanzania, from 2007 to 2008 and from 2012 to 2014.2007 年至 2008 年和 2012 年至 2014 年坦桑尼亚乞力马扎罗急性 Q 热和斑点热群立克次体病的发病率估计。
Am J Trop Med Hyg. 2021 Dec 20;106(2):494-503. doi: 10.4269/ajtmh.20-1036.
3
Pediatric Q Fever.小儿Q热
Curr Infect Dis Rep. 2020 Mar 18;22(4). doi: 10.1007/s11908-020-0719-0.
4
Ten years of monitoring malaria trend and factors associated with malaria test positivity rates in Lower Moshi.洛莫希低地疟疾趋势监测及与疟疾检测阳性率相关因素十年分析
Malar J. 2021 Apr 20;20(1):193. doi: 10.1186/s12936-021-03730-1.
5
Diagnosis of Acute Q Fever by Detection of DNA using Real-Time PCR, Employing a Commercial Genesig Easy Kit.使用商业Genesig简易试剂盒通过实时PCR检测DNA诊断急性Q热
J Clin Diagn Res. 2017 Sep;11(9):DC10-DC13. doi: 10.7860/JCDR/2017/31005.10606. Epub 2017 Sep 1.
6
Influence of Antibiotics on the Detection of Bacteria by Culture-Based and Culture-Independent Diagnostic Tests in Patients Hospitalized With Community-Acquired Pneumonia.抗生素对社区获得性肺炎住院患者基于培养和非培养诊断检测细菌的影响
Open Forum Infect Dis. 2017 Feb 10;4(1):ofx014. doi: 10.1093/ofid/ofx014. eCollection 2017 Winter.
7
From Q Fever to Coxiella burnetii Infection: a Paradigm Change.从Q热到伯氏考克斯氏体感染:范式转变
Clin Microbiol Rev. 2017 Jan;30(1):115-190. doi: 10.1128/CMR.00045-16.
8
Lyophilization to improve the sensitivity of qPCR for bacterial DNA detection in serum: the Q fever paradigm.冻干法提高血清中细菌DNA检测的qPCR敏感性:Q热范例
J Med Microbiol. 2016 Jun;65(6):462-467. doi: 10.1099/jmm.0.000253. Epub 2016 Mar 23.
9
Epidemiology of Coxiella burnetii infection in Africa: a OneHealth systematic review.非洲贝氏柯克斯体感染的流行病学:一项 OneHealth 系统综述。
PLoS Negl Trop Dis. 2014 Apr 10;8(4):e2787. doi: 10.1371/journal.pntd.0002787. eCollection 2014 Apr.
10
High Coxiella burnetii DNA load in serum during acute Q fever is associated with progression to a serologic profile indicative of chronic Q fever.血清中高浓度的柯克斯体 DNA 负荷与急性 Q 热进展为提示慢性 Q 热的血清学特征相关。
J Clin Microbiol. 2013 Oct;51(10):3192-8. doi: 10.1128/JCM.00993-13. Epub 2013 Jul 17.

2012 - 2014年坦桑尼亚乞力马扎罗山地区发热患者中配对免疫荧光抗体血清学检测与实时聚合酶链反应检测用于急性Q热诊断的比较

Comparison of Paired Immunofluorescent Antibody Serology and Real-Time Polymerase Chain Reaction Testing for the Detection of Acute Q Fever among Febrile Patients in Kilimanjaro, Tanzania, 2012-2014.

作者信息

Rolfe Robert J, Crump John A, Maro Venance P, Mmbaga Blandina T, Saganda Wilbrod, Lwezaula Bingileki F, Couturier Marc Roger, Hymas Weston C, Perniciaro Jamie L, Nicholson William L, Kersh Gilbert J, Rubach Matthew P

机构信息

Division of Infectious Diseases and International Health, Department of Medicine, Duke University, Durham, North Carolina.

Duke University Global Health Institute, Durham, North Carolina.

出版信息

Am J Trop Med Hyg. 2024 Dec 31;112(3):533-538. doi: 10.4269/ajtmh.23-0860. Print 2025 Mar 5.

DOI:10.4269/ajtmh.23-0860
PMID:39742524
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11884282/
Abstract

Acute Q fever diagnosis via paired serology is problematic because it requires follow-up for convalescent sample collection; as such, it cannot provide a diagnosis to inform a treatment decision at the time of acute presentation. Real-time polymerase chain reaction (PCR) may be a useful approach for the diagnosis of acute Q fever in endemic settings. Among febrile patients enrolled in a sentinel surveillance study for Q fever at two referral hospitals in Moshi, Tanzania, from 2012 to 2014, we analyzed those with paired sera for IgG to Coxiella burnetii (C. burnetii) phase II antigens using immunofluorescent antibody (IFA) testing, and acute serum was tested for C. burnetii with PCR. Acute Q fever was defined as a fourfold or greater rise from the acute to convalescent sample in IFA reciprocal titer or PCR detection that was confirmed through repeat testing. Test characteristics were tabulated. Among 496 participants tested using both paired IFA and PCR testing, 463 (93.3%) tested negative on both IFA and PCR, five (1.0%) tested positive for Q fever on both IFA and PCR, and 28 (5.6%) tested positive for Q fever on IFA alone. The sensitivity of PCR testing using paired IFA testing as an index was 0.15 (5/33), and the specificity was 1 (463/463). C. burnetii PCR testing provides a clinically specific method that may aid in timely diagnosis in settings in which acute Q fever is a common cause of febrile illness. However, we found a low clinical sensitivity of PCR testing on serum when compared with paired IFA serology.

摘要

通过双份血清学检测诊断急性Q热存在问题,因为这需要在恢复期采集样本进行后续检测;因此,在急性发病时,它无法为治疗决策提供诊断依据。实时聚合酶链反应(PCR)可能是在流行地区诊断急性Q热的一种有用方法。在2012年至2014年期间,于坦桑尼亚莫希的两家转诊医院参加Q热哨点监测研究的发热患者中,我们使用免疫荧光抗体(IFA)检测分析了那些双份血清针对伯纳特柯克斯体(C. burnetii)II期抗原的IgG情况,并对急性期血清进行了C. burnetii的PCR检测。急性Q热定义为IFA效价或PCR检测结果从急性期到恢复期样本呈四倍或更高倍数升高,且通过重复检测得以确认。列出了检测特征。在496名同时接受双份IFA和PCR检测的参与者中,463人(93.3%)在IFA和PCR检测中均呈阴性,5人(1.0%)在IFA和PCR检测中均呈Q热阳性,28人(5.6%)仅在IFA检测中呈Q热阳性。以双份IFA检测为指标时,PCR检测的敏感性为0.15(5/33),特异性为1(463/463)。C. burnetii的PCR检测提供了一种临床特异性方法,在急性Q热是发热性疾病常见病因的情况下,可能有助于及时诊断。然而,与双份IFA血清学检测相比,我们发现血清PCR检测的临床敏感性较低。