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Comparison of the FDA-approved CDC DENV-1-4 real-time reverse transcription-PCR with a laboratory-developed assay for dengue virus detection and serotyping.比较美国食品药品监督管理局(FDA)批准的疾病预防控制中心(CDC)登革热病毒 1-4 型实时逆转录聚合酶链反应(RT-PCR)与实验室开发的登革热病毒检测和血清分型检测方法。
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Analytical and clinical performance of the CDC real time RT-PCR assay for detection and typing of dengue virus.疾病预防控制中心实时 RT-PCR 检测和分型登革热病毒的分析和临床性能。
PLoS Negl Trop Dis. 2013 Jul 11;7(7):e2311. doi: 10.1371/journal.pntd.0002311. Print 2013.
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Single-reaction, multiplex, real-time rt-PCR for the detection, quantitation, and serotyping of dengue viruses.用于登革热病毒的检测、定量和血清分型的单反应、多重、实时 RT-PCR。
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Development of an internally controlled real-time reverse transcriptase PCR assay for pan-dengue virus detection and comparison of four molecular dengue virus detection assays.建立一种内对照实时逆转录聚合酶链反应检测方法用于泛 dengue 病毒检测,并比较四种分子 dengue 病毒检测方法。
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Comparison of real-time SYBR green dengue assay with real-time taqman RT-PCR dengue assay and the conventional nested PCR for diagnosis of primary and secondary dengue infection.实时SYBR Green登革热检测法与实时TaqMan RT-PCR登革热检测法及传统巢式PCR用于诊断原发性和继发性登革热感染的比较。
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Clinical presentation of dengue among patients admitted to the adult emergency department of a tertiary care hospital in Martinique: implications for triage, management, and reporting.法属马提尼克岛一家三级护理医院成人急诊收治的登革热患者的临床表现:分诊、治疗和报告的意义。
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Validation of an internally controlled one-step real-time multiplex RT-PCR assay for the detection and quantitation of dengue virus RNA in plasma.验证一种内部对照的一步法实时多重 RT-PCR 检测方法,用于检测和定量血浆中的登革病毒 RNA。
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Prospective evaluation of nonstructural 1 enzyme-linked immunosorbent assay and rapid immunochromatographic tests to detect dengue virus in patients with acute febrile illness.前瞻性评估非结构蛋白 1 酶联免疫吸附试验和快速免疫层析试验在急性发热患者中检测登革热病毒的效果。
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评估四种用于检测临床样本中登革病毒的商用实时逆转录聚合酶链反应试剂盒。

Evaluation of four commercial real-time RT-PCR kits for the detection of dengue viruses in clinical samples.

作者信息

Najioullah Fatiha, Viron Florent, Césaire Raymond

机构信息

Laboratoire de Virologie, Centre Hospitalier Universitaire de Fort-de-France, and EA 4537, Université des Antilles et de la Guyane, Martinique, France.

出版信息

Virol J. 2014 Sep 15;11:164. doi: 10.1186/1743-422X-11-164.

DOI:10.1186/1743-422X-11-164
PMID:25219286
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4177702/
Abstract

BACKGROUND

Dengue is the most frequent arthropod-borne viral disease worldwide. Because dengue manifestations are similar to those of many other febrile syndromes, the availability of dengue-specific laboratory tests is useful for the differential diagnosis. Timely and accurate diagnosis of dengue virus (DENV) infection is important for appropriate management of complications, pathophysiological studies, epidemiological investigations and optimization of vector-control measures. Several "in-house" reverse transcriptase-polymerase chain reaction (RT-PCR) methods have been developed to detect, type and/or quantify DENV. Standardized dengue RT-PCR kits with internal controls have been recently introduced, but need clinical evaluation. We assessed the performances of 4 commercial DENV real-time RT-PCR kits.

FINDINGS

The 4 kits were evaluated using a panel of 162 samples positive with an existing in-place hemi-nested RT-PCR used for routine DENV-infection diagnosis in patients with acute-febrile disease. The panel included 46 DENV-1, 37 DENV-2, 33 DENV-3, and 46 DENV-4. Also, 70 negative serum specimens were used to determine specificity. Geno-Sen's Dengue 1-4 Real-Time RT-PCR kit was the only assay to provide quantification using standards, but lacked sensitivity for DENV-4 detection. The SimplexaTM Dengue RT-PCR assay, with 151 (93.2% [95% confidence interval, 89.3-97.1]) positive samples, had significantly higher sensitivity than the other 3 kits; in a complementary evaluation of 111 consecutive patients' samples, its performance and genotyping agreed with the hemi-nested gold-standard assay.

CONCLUSIONS

The SimplexaTM Dengue RT-PCR's good performance to detect and genotype DENV1-4 requires further evaluation in multicenter and prospective studies, particularly in settings of clinical diagnosis during dengue outbreaks.

摘要

背景

登革热是全球最常见的节肢动物传播的病毒性疾病。由于登革热的表现与许多其他发热综合征相似,因此登革热特异性实验室检测有助于鉴别诊断。及时、准确地诊断登革病毒(DENV)感染对于并发症的适当管理、病理生理学研究、流行病学调查以及病媒控制措施的优化至关重要。已经开发了几种“内部”逆转录聚合酶链反应(RT-PCR)方法来检测、分型和/或定量DENV。最近推出了带有内部对照的标准化登革热RT-PCR试剂盒,但需要进行临床评估。我们评估了4种商用DENV实时RT-PCR试剂盒的性能。

研究结果

使用一组162份样本对这4种试剂盒进行评估,这些样本通过现有的用于急性发热性疾病患者常规DENV感染诊断的半巢式RT-PCR检测呈阳性。该样本组包括46份DENV-1、37份DENV-2、33份DENV-3和46份DENV-4。此外,还使用了70份阴性血清标本确定特异性。Geno-Sen公司的登革热1-4实时RT-PCR试剂盒是唯一一种使用标准品进行定量的检测方法,但对DENV-4检测缺乏敏感性。SimplexaTM登革热RT-PCR检测法检测出151份(93.2%[95%置信区间,89.3-97.1])阳性样本,其敏感性显著高于其他3种试剂盒;在对111例连续患者样本的补充评估中,其性能和基因分型与半巢式金标准检测法一致。

结论

SimplexaTM登革热RT-PCR检测法在检测和分型DENV1-4方面的良好性能需要在多中心前瞻性研究中进一步评估,尤其是在登革热暴发期间的临床诊断环境中。