Prospective Identification of Enteroviruses Involved in Meningitis in 2006 through Direct Genotyping in Cerebrospinal Fluid

Mirand, Audrey; Henquell, Cécile; Archimbaud, Christine; Chambon, M.; Charbonné, F; Peigue-Lafeuille, H.; Bailly, Jean‐Luc

doi:10.1128/jcm.01020-07

Cited by 81 publications

(79 citation statements)

References 59 publications

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“…EV infections have been known to increase in summer and early autumn in countries in temperate climates ( 1 , 2 , 13 ). As expected in a temperate climate, our surveillance data revealed a seasonal pattern of distribution, with transmission peaking in the summer and decreasing in the period from autumn to spring.…”

Section: Discussionmentioning

confidence: 99%

“…Laboratory diagnosis of EV infection is based on detection of the virus in clinical specimens such as fecal or rectal swab samples, cerebrospinal fluid (CSF), nasopharyngeal secretions collected by throat swab, and blood ( 11 , 13 ). Detection of EV is usually performed by isolation of the virus in cell culture, reverse transcription PCR (RT-PCR), or real-time RT-PCR ( 11 , 14 – 16 ).…”

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confidence: 99%

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Accuracy of Diagnostic Methods and Surveillance Sensitivity for Human Enterovirus, South Korea, 1999–2011

Hyeon¹,

Hwang²,

Kim³

et al. 2013

Emerg. Infect. Dis.

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The epidemiology of enteroviral infection in South Korea during 1999–2011 chronicles nationwide outbreaks and changing detection and subtyping methods used over the 13-year period. Of 14,657 patients whose samples were tested, 4,762 (32.5%) samples were positive for human enterovirus (human EV); as diagnostic methods improved, the rate of positive results increased. A seasonal trend of outbreaks was documented. Genotypes enterovirus 71, echovirus 30, coxsackievirus B5, enterovirus 6, and coxsackievirus B2 were the most common genotypes identified. Accurate test results correlated clinical syndromes to enterovirus genotypes: aseptic meningitis to echovirus 30, enterovirus 6, and coxsackievirus B5; hand, foot and mouth disease to coxsackievirus A16; and hand, foot and mouth disease with neurologic complications to enterovirus 71. There are currently no treatments specific to human EV infections; surveillance of enterovirus infections such as this study provides may assist with evaluating the need to research and develop treatments for infections caused by virulent human EV genotypes.

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Section: Discussionmentioning

confidence: 99%

mentioning

confidence: 99%

Accuracy of Diagnostic Methods and Surveillance Sensitivity for Human Enterovirus, South Korea, 1999–2011

Hyeon¹,

Hwang²,

Kim³

et al. 2013

Emerg. Infect. Dis.

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“…Viruses were isolated from original clinical specimens by using two cell lines, either MRC5 (human lung embryonic fibroblasts; bioMérieux) or RD (rhabdomyosarcoma; European Collection of Cell Cultures) cell lines. The virus isolates were either typed by seroneutralization test or identified with a genotyping method (Mirand et al, 2008;Nix et al, 2006). A number of virus strains included in the study were subjected to partial sequencing earlier (Diedrich et al, 2009;Huemer et al, 2008).…”

Section: Methodsmentioning

confidence: 99%

“…A specific protocol was used in one laboratory (Lyon, France) and RNA was purified from 200 ml and eluted in 70 ml. Synthesis of the cDNA was performed using SuperScript III reverse transcriptase (Invitrogen) according to a previously described method (Mirand et al, 2008). …”

Section: Methodsmentioning

confidence: 99%

Phylogenetic evidence for a recent spread of two populations of human enterovirus 71 in European countries

Mirand

Schuffenecker

Henquell

et al. 2010

Journal of General Virology

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Human enterovirus 71 (EV-71) is a cause of seasonal epidemics of hand, foot and mouth disease, and of less common but severe neurological manifestations. Uncertainty persists regarding the circulation of virus populations in several geographical areas and the timescale of their dissemination. We determined EV-71 sequences at loci 1D (VP1 capsid protein) and 3CD (nonstructural proteins) in 86 strains recovered in Austria, France and Germany and performed an evolutionary genetic study of extant virus populations. Phylogenetic analyses positioned 78 of the 86 sequences within two clades among subgenogroups C1 and C2. A minor sequence cluster was assigned to subgenogroup C4. Analyses incorporating the available sequences estimated the substitution rate in genogroup C at 3.66¾10 "3 and 4.46¾10 "3 substitutions per site year "1 for loci 1D and 3CD, respectively, assuming a relaxed molecular-clock model for sequence evolution. Most of the 'European' strains belonged to clades C1b and C2b, which originated in 1994 [95 % confidence interval (CI), 1992.7"1995.8] and 2002 (95 % CI, 2001.6"2003, respectively. Estimates of divergence times for locus 3CD were consistent with those measured for locus 1D. Intertwining between clades representing EV-71 subgenogroups and clades corresponding to other enterovirus types (notably early coxsackievirus A prototype strains) in the 3CD phylogeny is highly indicative of ancestral recombination events. Incongruent phylogenetic patterns estimated for loci 1D and 3CD show that a single tree cannot model the epidemic history of circulating EV-71 populations. The evolutionary timescale of genogroup C estimated for both loci was measured only in decades, indicating recent dissemination.

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“…Isolated EV were prospectively genotyped and CSF specimens underwent retrospective genotyping as described elsewhere [Mirand et al, 2006;Mirand et al, 2008].…”

Section: Cultures For Virus Isolation and Genotypingmentioning

confidence: 99%

Impact of rapid enterovirus molecular diagnosis on the management of infants, children, and adults with aseptic meningitis

Archimbaud

Chambon

Bailly

et al. 2008

Journal of Medical Virology

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Enteroviruses (EV) are the main etiological agents of aseptic meningitis. Diagnosis is made by detecting the genome using RT-PCR. The aim of the study was to evaluate the impact of a positive diagnosis on the management of infants, children, and adults. During 2005, 442 patients were admitted to hospital with suspected meningitis. Clinical and laboratory data and initial treatment were recorded for all patients with enteroviral meningitis. The turnaround time of tests and the length of hospital stay were analyzed. The results showed that EV-PCR detected EV in 69 patients (16%), 23% (16/69) were adults. About 18% of CSF samples had no pleocytosis. After positive PCR results, 63% of children were discharged immediately (mean 2 hr 30 min) and 95% within 24 hr. Infants and adults were discharged later (after 1.8 and 2 days, respectively). The use of antibiotics was significantly lower in children than in infants and adults. The PCR results allowed discontinuation of antibiotics in 50-60% of all patients treated. Patients received acyclovir in 16% of cases (7% children vs. 50% adults) and 23% (11% vs. 69%) underwent a CT scan. Clinical data were compared between patients whose positive EV-PCR results were available within 24 hr (n ¼ 32) and those whose results were available > 24 hr after collection of CSF (n ¼ 14). Duration of antibiotic treatment (difference: 2.3 days; P ¼ 0.05) was reduced between the two groups. No statistical difference in the length of stay was observed. The EV-PCR assay should be performed daily in hospital laboratory practice and considered as part of the initial management of meningitis.

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Prospective Identification of Enteroviruses Involved in Meningitis in 2006 through Direct Genotyping in Cerebrospinal Fluid

Cited by 81 publications

References 59 publications

Accuracy of Diagnostic Methods and Surveillance Sensitivity for Human Enterovirus, South Korea, 1999–2011

Accuracy of Diagnostic Methods and Surveillance Sensitivity for Human Enterovirus, South Korea, 1999–2011

Phylogenetic evidence for a recent spread of two populations of human enterovirus 71 in European countries

Impact of rapid enterovirus molecular diagnosis on the management of infants, children, and adults with aseptic meningitis

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