Highly Sensitive Assay for Detection of Enterovirus in Clinical Specimens by Reverse Transcription-PCR with an Armored RNA Internal Control

Beld, Marcel; Minnaar, R. P.; Weel, Jan; Sol, C. J. A.; Damen, Marjolein; Avoort, Harry van der; Dillen, Pauline Wertheim-van; Breda, Alex van; Boom, R.

doi:10.1128/jcm.42.7.3059-3064.2004

Cited by 103 publications

(99 citation statements)

References 31 publications

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“…Reverse transcription using SuperScript III reverse transcriptase (Invitrogen, UK) was performed according to the manufacturer's instruction. EVs were screened by a real-time PCR protocol (Beld et al, 2004). Typing of EVs from 177 positive samples, including 10 from diarrhoeic pigs, representing ranges of geography, C t values and ages of infected pigs, was performed by amplification and sequencing of the VP1 region as described previously (Van Dung et al, 2014).…”

Section: Methodsmentioning

confidence: 99%

Large-scale screening and characterization of enteroviruses and kobuviruses infecting pigs in Vietnam

Dũng

Anh

Cương

et al. 2016

Journal of General Virology

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A recent survey of pigs in Dong Thap province, Vietnam identified a high frequency of enterovirus species G (EV-G) infection (144/198; 72.7 %). Amongst these was a plethora of EV-G types (EV-G1, EV-G6 and four new types EV-G8-EV-G11). To better characterize the genetic diversity of EV-G and investigate the possible existence of further circulating types, we performed a larger-scale study on 484 pig and 45 farm-bred boar faecal samples collected in 2012 and 2014, respectively. All samples from the previous and current studies were also screened for kobuviruses. The overall EV infection frequency remained extremely high (395/484; 81.6 %), but with comparable detection rates and viral loads between healthy and diarrhoeic pigs; this contrasted with less frequent detection of EV-G in boars (4/45; 8.9 %). EV was most frequently detected in pigs j14 weeks old (,95 %) and declined in older pigs. Infections with EV-G1 and EV-G6 were most frequent, whilst less commonly detected types included EV-G3, EV-G4 and EV-G8-EV-G11, and five new types (EV-G12-EV-G16). In contrast, kobuvirus infection frequency was significantly higher in diarrhoeic pigs (40.9 versus 27.6 %; P50.01). Kobuviruses also showed contrasting epizootiologies and age associations; a higher prevalence was found in boars (42 %) compared with domestic pigs (29 %), with the highest infection frequency amongst pigs .52 weeks old. Although genetically diverse, all kobuviruses identified belonged to the species Aichivirus C. In summary, this study confirms infection with EV-G was endemic in Vietnamese domestic pigs and exhibits high genetic diversity and extensive inter-type recombination.

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Section: Methodsmentioning

confidence: 99%

Large-scale screening and characterization of enteroviruses and kobuviruses infecting pigs in Vietnam

Dũng

Anh

Cương

et al. 2016

Journal of General Virology

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“…Both oligonucleotides overlap over a sequence stretch of 24 nucleotides. The mutagenesis cassette was constructed according to Beld et al (2004) by hybridization and elongation of 1 ng of sense and antisense oligonucleotide in a 50 µL reaction containing 6 mM MgSO 4 , 0.2 mM dNTPs (Roche Diagnostics), 3.0 U of proofreading Platinum Pfx DNA Polymerase (Invitrogen), 1× PCR reaction buffer, and 1 µg non-acetylated BSA (Sigma). The reaction was incubated for 10 min at 95°C, 5 min at 55°C, and 20 min at 68°C.…”

Section: Rueckert and Carymentioning

confidence: 99%

Use of an armored RNA standard to measure microcystin synthetase E gene expression in toxic Microcystis sp. by reverse‐transcription QPCR

Rueckert

Cary

2009

Limnology & Ocean Methods

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Microcystin is a secondary metabolic peptide toxin known to cause hepatotoxicosis and carcinogenicity in vertebrates. It is produced by various bloom-forming cyanobacterial species constituting a serious threat to the quality of freshwater reservoirs worldwide. There is an intense interest to understand the biological function of microcystin and the regulatory mechanism behind its biosynthesis in order to develop strategies for freshwater management. To date, changes in toxin production in response to various environmental parameters have been studied using direct toxin analysis. Despite extensive research over the past two decades, the function of microcystin remains poorly understood. In this study, we developed an alternative method to study the regulation of microcystin production in toxic Microcystis sp. (and alternatively in Anabaena sp.) at the level of gene expression targeting microcystin synthetase E (mcyE) transcripts. We developed a durable and ribonuclease-resistant armored RNA standard to monitor for the integrity of all nucleic acid processing steps including extraction, reverse transcription, amplification, and detection. The armored RNA was designed to consist of the mcyE target matrix with a unique internal probe-binding sequence. To validate the efficacy of the method, we conducted a comprehensive survey of mcyE expression profiling in batch cultures of Microcystis sp. during exponential, linear, and stationary growth phase. Our transcriptional analysis indicates a growth-phase-dependent expression of mcyE, with the maximal level of expression observed during mid-log growth. With progressing age of the cultures, mcyE was gradually down-regulated, with expression levels having declined by more than three orders of magnitude during the stationary growth phase.

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“…Therefore, PCR is the preferred method for detection of viruses in this material (Espy et al, 2006;Read et al, 1997;Romero 1999;Rotbart HA & Romero JR, 1995;van Doornum et al, 2007). But while with cell culture, both EVs and HPeVs can be diagnosed, PCR specific for EVs will fail to detect HPeVs because the targeted 5'UTR is too diverse between HPeVs and EVs (Beld et al, 2004;Benschop et al, 2006a;Hyypia, 1989;Hyypia et al, 1989;Oberste et al, 1999). Therefore a separate RT-PCR specifically targeting the 5'UTR of HPeVs is required.…”

Section: Laboratory Findings and Diagnosis Of Hpev Infectionmentioning

confidence: 99%

Human Parechoviruses, New Players in the Pathogenesis of Viral Meningitis

Benschop

Wildenbeest²,

Wolthers³

2012

Meningitis

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Highly Sensitive Assay for Detection of Enterovirus in Clinical Specimens by Reverse Transcription-PCR with an Armored RNA Internal Control

Cited by 103 publications

References 31 publications

Large-scale screening and characterization of enteroviruses and kobuviruses infecting pigs in Vietnam

Large-scale screening and characterization of enteroviruses and kobuviruses infecting pigs in Vietnam

Use of an armored RNA standard to measure microcystin synthetase E gene expression in toxic Microcystis sp. by reverse‐transcription QPCR

Human Parechoviruses, New Players in the Pathogenesis of Viral Meningitis

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