Development and Evaluation of Serotype- and Group-Specific Fluorogenic Reverse Transcriptase PCR (TaqMan) Assays for Dengue Virus

Callahan, Johnny D.; Wu, Shuenn-Jue; Dion-Schultz, Amanda; Mangold, Beverly E.; Peruski, Leonard F.; Watts, Douglas M.; Porter, Kevin R.; Murphy, Gerald R.; Wuryadi, Suharyono; King, Chwan-Chuen; Hayes, Curtis G.; Temenak, Joseph J.

doi:10.1128/jcm.39.11.4119-4124.2001

Cited by 181 publications

(153 citation statements)

References 19 publications

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“…The amount of viral RNA present in samples was determined using the Superscript III One-Step Quantitative RT-PCR System (qRT-PCR; Invitrogen, Carlsbad, CA) with a Light Cycler 480 system (Roche, Mannheim, Germany) using methods described elsewhere. 47 A standard curve method was used to relate the amount of DENV RNA present in samples to 10-fold serial dilutions of virus stock with known concentrations expressed in pfu per milliliter. 48,49 Mosquitoes were categorized based on status of infection: disseminated infections, positively infected bodies and legs; non-disseminated infections, infected bodies but the absence of virus in legs; and uninfected, absence of virus in the body.…”

Section: Methodsmentioning

confidence: 99%

Temperature and Dengue Virus Infection in Mosquitoes: Independent Effects on the Immature and Adult Stages

Alto

Bettinardi²

2013

The American Journal of Tropical Medicine and Hygiene

153

137

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Abstract. Temperature is one of the most important environmental factors affecting biological processes of mosquitoes, including their interactions with viruses. In these studies, we show independent effects of rearing temperature on the immature aquatic stages and holding temperature on the adult terrestrial stage in terms of alterations in adult survival and progression of dengue-1 virus infection in the Asian tiger mosquito Aedes (Stegomyia) albopictus. Our studies show that adult survival was determined by adult-holding temperature, regardless of rearing conditions of the immature stages. In contrast, spread of virus throughout the body of the mosquito, a pre-requisite for transmission, was reduced when the immature stages were reared in cool conditions. These results show that immature-rearing temperature selectively modified mosquito traits that influence competency for viruses, and they further our understanding of the nature of temperature effects on interactions between mosquitoes and virus pathogens and risk of disease transmission.

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Section: Methodsmentioning

confidence: 99%

Temperature and Dengue Virus Infection in Mosquitoes: Independent Effects on the Immature and Adult Stages

Alto

Bettinardi²

2013

The American Journal of Tropical Medicine and Hygiene

153

137

View full text Add to dashboard Cite

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“…The same fluorescence combination format has been applied for detection of DENV-1 to -4 in serum specimens from patients with dengue fever (4,14). The combination of universal primer pairs with four virus-specific probes simplifies the optimization step (4; this study); in contrast, other multiplex designs require four unique primer pairs and four different probes (2,14). Another significant improvement is the development of an in vitro-transcribed RNase-resistant RNA template for use as the copy number control.…”

Section: Vol 45 2007mentioning

confidence: 99%

Development of Multiplex Real-Time Reverse Transcriptase PCR Assays for Detecting Eight Medically Important Flaviviruses in Mosquitoes

2007

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. This assay had a specificity of 100% and various sensitivities of at least 3.5 PFU/ml for YFV, 2.0 PFU/ml for JEV, 10.0 PFU/ml for WNV, and 10.0 PFU/ml for SLEV. Additionally, we have developed an in vitro transcription system to generate RNase-resistant RNA templates for each of these eight viruses. These templates can be incorporated into the assay as RNA copy number controls and/or as external controls for RNA-spiked mosquito pools for quality assurance purposes. Although further study with mosquitoes collected in the field is needed, the incorporation of this assay into mosquito surveillance could be used as an early-warning system for the detection of medically important flaviviruses, particularly when the cocirculation of multiple viruses in the same region is suspected.Flaviviruses are significant causes of disease worldwide and can be classified serologically into several antigenic complexes (12,20). Medically important members of the Japanese encephalitis virus (JEV) serocomplex include JEV, St. Louis encephalitis virus (SLEV), and West Nile virus (WNV). Each of these viruses causes similar disease syndromes in humans, ranging from an asymptomatic or a mild flu-like illness to clinical encephalitis (18). Until 1999, SLEV was the only mosquito-borne flavivirus causing significant human morbidity and mortality in the United States (22). WNV, traditionally found in Europe, Africa, the Middle East, and Asia, emerged in New York City in the late summer of 1999 (1). By 2005 the distribution of WNV had expanded into areas of known recent SLEV activity, such as the states of Florida, Mississippi, Louisiana, Texas, Arizona, Colorado, and California (3). Mosquito surveillance for detection of virus activity during the transmission season is an essential tool for implementation of an effective mosquito control strategy. As WNV and SLEV occupy similar ecological niches in North America, it is critical to develop a cost-effective assay capable of detecting the presence of either one or both viruses simultaneously in the mosquito pools. In addition, dengue virus (DENV) serotypes 1 to 4 (DENV-1 to DENV-4, respectively), SLEV, and yellow fever virus (YFV) are endemic in Latin America (5). The situation is further complicated by the detection of WNV activity in Mexico and Central America (3). Therefore, the development of a real-time, multiplex reverse transcriptase (RT) PCR platform for the simultaneous detection of viral RNA genomes in the Americas is crucial for supporting mosquito surveillance efforts and clinical diagnosis.The RNA-dependent RNA polymerase (RdRp) domain, located at the carboxy terminus of nonstructural protein 5 (NS5), is the most conserved coding region in the Flavivirus genomes (15,16,23). The consensus sequence primers (primers FU1 and CFD2; YFV genomic positions, nucleotide [nt] 8997 and nt 9233, respectively) have been used in our previous study for genetic characterization of this domain for all registered flaviviruses (16). The nucleotide sequences flanked by these two primers were variable...

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“…The real-time PCR assay has many advantages over conventional RT-PCR methods, including lower contamination rate, higher sensitivity and specificity, and they are rapid, providing results in minutes instead of hours. Several investigators have reported the use of real-time PCR assays for detecting some viral causes of hemorrhagic fevers (Drosten et al, 2002a), including Ebola (Gibb et al, 2001;Towner et al, 2004;Weidmann et al, 2004), Rift Valley fever (Garcia et al, 2001), and dengue (Laue et al, 1999;Callahan et al, 2001;Houng et al, 2000) viruses. Drosten et al (2002a) developed a one-step real-time RT-PCR assay for detecting CCHFV using primers to the nucleoprotein gene; however, they used the DNA-intercalating dye, SybrGreen I, for detecting the PCR product because no conserved binding site for a 5 -nuclease probe could be found.…”

Section: Molecular Diagnostic Assaysmentioning

confidence: 99%

Crimean–Congo hemorrhagic fever

2004

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Crimean-Congo hemorrhagic fever (CCHF) is a tick-borne disease caused by the arbovirus Crimean-Congo hemorrhagic fever virus (CCHFV), which is a member of the Nairovirus genus (family Bunyaviridae). CCHF was first recognized during a large outbreak among agricultural workers in the mid-1940s in the Crimean peninsula. The disease now occurs sporadically throughout much of Africa, Asia, and Europe and results in an approximately 30% fatality rate. After a short incubation period, CCHF is characterized by a sudden onset of high fever, chills, severe headache, dizziness, back, and abdominal pains. Additional symptoms can include nausea, vomiting, diarrhea, neuropsychiatric, and cardiovascular changes. In severe cases, hemorrhagic manifestations, ranging from petechiae to large areas of ecchymosis, develop. Numerous genera of ixodid ticks serve both as vector and reservoir for CCHFV; however, ticks in the genus Hyalomma are particularly important to the ecology of this virus. In fact, occurrence of CCHF closely approximates the known world distribution of Hyalomma spp. ticks. Therefore, exposure to these ticks represents a major risk factor for contracting disease; however, other important risk factors are known and are discussed in this review. In recent years, major advances in the molecular detection of CCHFV, particularly the use of real-time reverse transcription-polymerase chain reaction (RT-PCR), in clinical and tick samples have allowed for both rapid diagnosis of disease and molecular epidemiology studies. Treatment options for CCHF are limited. Immunotherapy and ribavirin have been tried with varying degrees of success during sporadic outbreaks of disease, but no case-controlled trials have been conducted. Consequently, there is currently no antiviral treatment for CCHF approved by the U.S. Food and Drug Administration (FDA). However, renewed interested in CCHFV, as well as increased knowledge of its basic biology, may lead to improved therapies in the future. This article reviews the history, epidemiology, ecology, clinical features, pathogenesis, diagnosis, and treatment of CCHF. In addition, recent advances in the molecular biology of CCHFV are presented, and issues related to its possible use as a bioterrorism agent are discussed.

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Development and Evaluation of Serotype- and Group-Specific Fluorogenic Reverse Transcriptase PCR (TaqMan) Assays for Dengue Virus

Cited by 181 publications

References 19 publications

Temperature and Dengue Virus Infection in Mosquitoes: Independent Effects on the Immature and Adult Stages

Temperature and Dengue Virus Infection in Mosquitoes: Independent Effects on the Immature and Adult Stages

Development of Multiplex Real-Time Reverse Transcriptase PCR Assays for Detecting Eight Medically Important Flaviviruses in Mosquitoes

Crimean–Congo hemorrhagic fever

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