Your search keyword '"Faux, CE"' showing total 16 results

1. Community-Wide, Contemporaneous Circulation of a Broad Spectrum of Human Rhinoviruses in Healthy Australian Preschool-Aged Children During a 12-Month Period

Author

Mackay, IM, Lambert, SB, Faux, CE, Arden, KE, Nissen, MD, Sloots, TP, Nolan, TM, Mackay, IM, Lambert, SB, Faux, CE, Arden, KE, Nissen, MD, Sloots, TP, and Nolan, TM

Abstract

Human rhinovirus (HRV) replication triggers exacerbation of asthma and causes most acute respiratory illnesses (ARIs), which may manifest as influenza-like illness. The recent assignment of 60 previously unknown HRV types to a third HRV species, Human rhinovirus C, raised questions about the prevalence of these picornavirus types in the community, the extent of HRV diversity at a single site, and whether the HRVs have an equally diverse clinical impact on their hosts. We quantified HRV diversity, and there was no clinical impact attributable to HRV species and genotypes among a community population of preschool-aged children with ARI who provided respiratory samples during 2003. All HRV species were represented among 138 children with ARI, and 74 distinct HRV types were cocirculating. Fever accompanied 32.8% of HRV-positive ARI cases. HRVs were less likely than DNA viruses to be codetected with another virus, suggesting virus interference at the community level, demonstrated by the inverse correlation between influenza virus detection and HRV detection.

Published

2013

2. Usefulness of Published PCR Primers in Detecting Human Rhinovirus Infection

Author

Faux, CE, Arden, KE, Lambert, SB, Nissen, MD, Nolan, TM, Chang, AB, Sloots, TP, Mackay, IM, Faux, CE, Arden, KE, Lambert, SB, Nissen, MD, Nolan, TM, Chang, AB, Sloots, TP, and Mackay, IM

Abstract

We conducted a preliminary comparison of the relative sensitivity of a cross-section of published human rhinovirus (HRV)-specific PCR primer pairs, varying the oligonucleotides and annealing temperature. None of the pairs could detect all HRVs in 2 panels of genotyped clinical specimens; >1 PCR is required for accurate description of HRV epidemiology.

Published

2011

3. Early evidence for direct and indirect effects of the infant rotavirus vaccine program in Queensland

Author

Stephen Lambert, Faux, Ce, Hall, L., Birrell, Fa, Peterson, Kv, Selvey, Ce, Sloots, Tp, Nissen, Md, and Grimwood, K.

Subjects

General Medicine

4. Molecular biomarkers for chronological age in animal ecology.

Author

Jarman SN, Polanowski AM, Faux CE, Robbins J, De Paoli-Iseppi R, Bravington M, and Deagle BE

Subjects

Animals, Ecology methods, Humans, Telomere ultrastructure, Aging genetics, Biomarkers, Epigenesis, Genetic

Abstract

The chronological age of an individual animal predicts many of its biological characteristics, and these in turn influence population-level ecological processes. Animal age information can therefore be valuable in ecological research, but many species have no external features that allow age to be reliably determined. Molecular age biomarkers provide a potential solution to this problem. Research in this area of molecular ecology has so far focused on a limited range of age biomarkers. The most commonly tested molecular age biomarker is change in average telomere length, which predicts age well in a small number of species and tissues, but performs poorly in many other situations. Epigenetic regulation of gene expression has recently been shown to cause age-related modifications to DNA and to cause changes in abundance of several RNA types throughout animal lifespans. Age biomarkers based on these epigenetic changes, and other new DNA-based assays, have already been applied to model organisms, humans and a limited number of wild animals. There is clear potential to apply these marker types more widely in ecological studies. For many species, these new approaches will produce age estimates where this was previously impractical. They will also enable age information to be gathered in cross-sectional studies and expand the range of demographic characteristics that can be quantified with molecular methods. We describe the range of molecular age biomarkers that have been investigated to date and suggest approaches for developing the newer marker types as age assays in nonmodel animal species., (© 2015 John Wiley & Sons Ltd.)

Published

2015

5. High-throughput real-time PCR and melt curve analysis for sexing Southern Ocean seabirds using fecal samples.

Author

Faux CE, McInnes JC, and Jarman SN

Subjects

Animals, Avian Proteins genetics, Base Sequence, DNA Primers chemistry, DNA-Binding Proteins genetics, Feces chemistry, Molecular Sequence Data, Oceans and Seas, Polymerase Chain Reaction methods, Sex Characteristics, Sex Determination Analysis methods, Avian Proteins chemistry, Birds physiology, DNA-Binding Proteins chemistry, Polymerase Chain Reaction veterinary, Sex Determination Analysis veterinary

Abstract

Sex identification of birds is of great interest in ecological studies, however this can be very difficult in many species because their external features are almost monomorphic between the sexes. Molecular methodology has simplified this process but limitations still occur with widely accepted methods using polymerase chain reaction and gel electrophoresis, especially when applied to degraded DNA. Real-time polymerase chain reaction assays are emerging as a more efficient, sensitive, and higher throughput means of identification, but there are very few techniques validated using fecal samples and small target sizes. We present a real-time melt curve analysis assay targeting a small region of the CHD-1 gene allowing for high-throughput, sensitive, specific, and easy-to-interpret sexing results for a variety of Southern Ocean seabirds using fecal and tissue samples., (Copyright © 2014 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2014

6. Community-wide, contemporaneous circulation of a broad spectrum of human rhinoviruses in healthy Australian preschool-aged children during a 12-month period.

Author

Mackay IM, Lambert SB, Faux CE, Arden KE, Nissen MD, Sloots TP, and Nolan TM

Subjects

Australia epidemiology, Carrier State virology, Child, Preschool, Cohort Studies, Female, Genetic Variation, Genotype, Humans, Infant, Male, Picornaviridae Infections virology, Prevalence, Respiratory Tract Infections virology, Rhinovirus classification, Rhinovirus genetics, Carrier State epidemiology, Picornaviridae Infections epidemiology, Respiratory Tract Infections epidemiology, Rhinovirus isolation & purification

Abstract

Human rhinovirus (HRV) replication triggers exacerbation of asthma and causes most acute respiratory illnesses (ARIs), which may manifest as influenza-like illness. The recent assignment of 60 previously unknown HRV types to a third HRV species, Human rhinovirus C, raised questions about the prevalence of these picornavirus types in the community, the extent of HRV diversity at a single site, and whether the HRVs have an equally diverse clinical impact on their hosts. We quantified HRV diversity, and there was no clinical impact attributable to HRV species and genotypes among a community population of preschool-aged children with ARI who provided respiratory samples during 2003. All HRV species were represented among 138 children with ARI, and 74 distinct HRV types were cocirculating. Fever accompanied 32.8% of HRV-positive ARI cases. HRVs were less likely than DNA viruses to be codetected with another virus, suggesting virus interference at the community level, demonstrated by the inverse correlation between influenza virus detection and HRV detection.

Published

2013

7. Human rhinovirus C in adult haematopoietic stem cell transplant recipients with respiratory illness.

Author

Ferguson PE, Gilroy NM, Faux CE, Mackay IM, Sloots TP, Nissen MD, Dwyer DE, and Sorrell TC

Subjects

5' Untranslated Regions, Adolescent, Adult, Aged, Australia epidemiology, Cohort Studies, Female, Genotype, Humans, Immunocompromised Host, Male, Middle Aged, Nose virology, Pharynx virology, Prospective Studies, Rhinovirus classification, Rhinovirus genetics, Sequence Analysis, DNA, Young Adult, Common Cold epidemiology, Common Cold virology, Hematopoietic Stem Cell Transplantation adverse effects, Rhinovirus isolation & purification, Transplantation

Abstract

Background: A previously unidentified species of human rhinovirus, HRV-C, was described in 2006 in association with lower respiratory tract infection (LRTI). Features of infection in immunosuppressed adults are poorly characterised., Objectives: This study aims to determine the epidemiology of HRV-C in haematopoietic stem cell transplant (HSCT) recipients in a single centre., Study Design: A prospective cohort study of all HSCT recipients admitted to Westmead Hospital, Westmead, Australia from 1 July 2005 to 30 September 2007 was undertaken. Nose/throat samples were collected from all patients at the time of admission and patients developing pre-defined symptoms and/or signs of respiratory infection during the admission. Samples were processed and tested for rhinoviruses and 14 other respiratory viruses using nucleic acid-based methods, immunofluorescence and culture. HRV genotyping was performed by sequencing a region of the rhinovirus 5' untranslated region (UTR). Clinical data on each episode were collected prospectively., Results: HRVs were identified in 24 episodes: 8% of 299 episodes of clinically- defined respiratory infections and 39% of 61 episodes in which respiratory viruses were detected. HRV-C was most frequent (HRV-C: nine, HRV-A: eight and HRV-B: two). Seven episodes of HRV-C, five with pneumonia, occurred within 100 days of HSCT. Co-pathogens were frequent., Conclusions: The newly described HRV-C was the most common rhinovirus group detected in HSCT recipients with respiratory infection, with co-pathogens being frequent. Further research is required to understand the activity and pathogenicity of this virus in HSCT recipients., (Crown Copyright © 2012. Published by Elsevier B.V. All rights reserved.)

Published

2013

8. Usefulness of published PCR primers in detecting human rhinovirus infection.

Author

Faux CE, Arden KE, Lambert SB, Nissen MD, Nolan TM, Chang AB, Sloots TP, and Mackay IM

Subjects

Humans, Picornaviridae Infections epidemiology, Picornaviridae Infections virology, RNA, Viral genetics, Rhinovirus classification, Rhinovirus genetics, Sensitivity and Specificity, Species Specificity, DNA Primers genetics, Picornaviridae Infections diagnosis, Polymerase Chain Reaction methods, Rhinovirus isolation & purification

Abstract

We conducted a preliminary comparison of the relative sensitivity of a cross-section of published human rhinovirus (HRV)-specific PCR primer pairs, varying the oligonucleotides and annealing temperature. None of the pairs could detect all HRVs in 2 panels of genotyped clinical specimens; >1 PCR is required for accurate description of HRV epidemiology.

Published

2011

9. Influenza surveillance in Australia: we need to do more than count.

Author

Lambert SB, Faux CE, Grant KA, Williams SH, Bletchly C, Catton MG, Smith DW, and Kelly HA

Subjects

Australia epidemiology, Disease Notification standards, Humans, Disease Notification statistics & numerical data, Influenza, Human epidemiology, Population Surveillance

Abstract

Laboratory-confirmed influenza is a nationally notifiable disease in Australia. According to notification data, Queensland has experienced more severe influenza seasons than other states and territories. However, this method ignores available denominator data: the number of laboratory tests performed. We propose that negative results of laboratory tests for influenza should be made notifiable, alongside laboratory-confirmed disease, and used to calculate the proportion of positive test results in real-time. Using data from the public health pathology services of three Australian states - Queensland Health laboratories, the Victorian Infectious Diseases Reference Laboratory and Western Australia's PathWest - for 2004 to 2008, we show that incorporating laboratory-negative test data into national surveillance data would add to and improve our understanding of influenza epidemiology.

Published

2010

10. A simple approach for preparing real-time PCR positive reaction controls for rare or emerging viruses.

Author

Whiley DM, Faux CE, Bialasiewicz S, Gould AR, Lambert SB, Nissen MD, and Sloots TP

Subjects

Humans, Influenza A Virus, H1N1 Subtype genetics, Metapneumovirus genetics, Parainfluenza Virus 2, Human genetics, Reference Standards, Varicellovirus genetics, Viruses genetics, Communicable Diseases, Emerging diagnosis, Polymerase Chain Reaction methods, Polymerase Chain Reaction standards, Virology methods, Virus Diseases diagnosis, Viruses isolation & purification

Abstract

Background: Laboratories often have difficulties obtaining positive control material for polymerase chain reaction (PCR) diagnosis of rare or emerging viruses. This is particularly problematic during outbreaks caused by emerging infectious diseases, when delays can impede the public health response., Objectives: The aim of this study was to develop a simple approach for preparing real-time PCR positive reaction controls for rare or emerging viruses., Study Design: We describe a universal method for preparing PCR positive reaction controls (Uni-Control), which uses two synthetic control oligonucleotides and irrelevant viral nucleic acid as an initiator template. In this study, we prepared Uni-Controls for novel influenza A(H1N1) and human metapneumovirus (HMPV) RT-PCR assays. Parainfluenza type 2 virus RNA and equine herpes virus DNA were used as initiator templates., Results: Using the Uni-Controls, characteristic sigmoidal real-time PCR amplification curves were observed in the influenza A(H1N1) and HMPV RT-PCR assays. Comparable cycle threshold values were observed in both assays when using the same concentration of the initiator template., Conclusions: The Uni-Control method for preparing real-time PCR positive reaction controls provides an interim measure by which real-time PCR assays can be rapidly introduced for rare or emerging viruses in the absence of wild-type control material. The system is versatile and we propose can readily be adapted to almost any viral template., (Copyright (c) 2010 Elsevier B.V. All rights reserved.)

Published

2010

11. Molecular characterization and distinguishing features of a novel human rhinovirus (HRV) C, HRVC-QCE, detected in children with fever, cough and wheeze during 2003.

Author

Arden KE, Faux CE, O'Neill NT, McErlean P, Nitsche A, Lambert SB, Nissen MD, Sloots TP, and Mackay IM

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Amino Acid Sequence, Child, Child, Preschool, Cluster Analysis, Cough etiology, Female, Fever etiology, Genotype, Hospitalization, Humans, Infant, Infant, Newborn, Male, Middle Aged, Molecular Epidemiology, Molecular Sequence Data, Picornaviridae Infections epidemiology, Picornaviridae Infections pathology, Prevalence, Respiratory Sounds etiology, Respiratory Tract Infections epidemiology, Respiratory Tract Infections pathology, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, DNA, Sequence Homology, Young Adult, Picornaviridae Infections virology, RNA, Viral genetics, Respiratory Tract Infections virology, Rhinovirus classification, Rhinovirus isolation & purification

Abstract

Background: Human rhinoviruses (HRVs) are associated with more acute respiratory tract infections than any other viral group yet we know little about viral diversity, epidemiology or clinical outcome resulting from infection by strains, in particular the recently identified HRVs., Objectives: To determine whether HRVC-QCE was a distinct HRV-C strain, by determining its genome and prevalence, by cataloguing genomic features for strain discrimination and by observing clinical features in positive patients., Study Design: Novel real-time RT-PCRs and retrospective chart reviews were used to investigate a well-defined population of 1247 specimen extracts to observe the prevalence and the clinical features of each HRV-QCE positive case from an in- and out-patient pediatric, hospital-based population during 2003. An objective illness severity score was determined for each HRVC-QCE positive patient., Results: Differences in overall polyprotein and VP1 binding pocket residues and the predicted presence of a cis-acting replication element in 1B defined HRVC-QCE as a novel HRV-C strain. Twelve additional HRVC-QCE detections (1.0% prevalence) occurred among infants and toddlers (1-24 months) suffering mild to moderate illness, including fever and cough, who were often hospitalized. HRVC-QCE was frequently detected in the absence of another virus and was the only virus detected in three (23% of HRVC-QCE positives) children with asthma exacerbation and in two (15%) toddlers with febrile convulsion., Conclusions: HRVC-QCE is a newly identified, genetically distinct HRV strain detected in hospitalized children with a range of clinical features. HRV strains should be independently considered to ensure we do not overestimate the HRVs in asymptomatic illness.

Published

2010

12. A Novel Duplex Real-Time Reverse-Transcription PCR Assay for the Detection of Influenza A and the Novel Influenza A(H1N1) Strain.

Author

Rockett RJ, Bialasiewicz S, Whiley DM, Bletchly C, Faux CE, Lambert SB, Nimmo GR, Nissen MD, and Sloots TP

Abstract

Timely implementation of antiviral treatment and other public health based responses are dependent on accurate and rapid diagnosis of the novel pandemic influenza A(H1N1) strain. In this study we developed a duplex real-time PCR (RT-PCR) (dFLU-TM) assay for the simultaneous detection of a broad range of influenza A subtypes and specific detection of the novel H1N1 2009 pandemic strain. The assay was compared to the combined results of two previously described monoplex RT-PCR assays using 183 clinical samples and 10 seasonal influenza A isolates. Overall, the results showed that the dFLU-TM RT-PCR method is suitable for detection of influenza A, including the novel H1N1 pandemic strain, in clinical samples.

Published

2009

13. Early evidence for direct and indirect effects of the infant rotavirus vaccine program in Queensland.

Author

Lambert SB, Faux CE, Hall L, Birrell FA, Peterson KV, Selvey CE, Sloots TP, Nissen MD, and Grimwood K

Subjects

Child, Preschool, Female, Gastroenteritis epidemiology, Gastroenteritis prevention & control, Humans, Infant, Male, Queensland epidemiology, Rotavirus Infections epidemiology, Gastroenteritis virology, Immunization Programs, Rotavirus Infections prevention & control, Rotavirus Vaccines

Abstract

Objective: To assess the impact of introducing a publicly funded infant rotavirus vaccination program on disease notifications and on laboratory testing and results., Design and Setting: Retrospective analysis of routinely collected data (rotavirus notifications [2006-2008] and laboratory rotavirus testing data from Queensland Health laboratories [2000-2008]) to monitor rotavirus trends before and after the introduction of a publicly funded infant rotavirus vaccination program in Queensland in July 2007., Main Outcome Measures: Age group-specific rotavirus notification trends; number of rotavirus tests performed and the proportion positive., Results: In the less than 2 years age group, rotavirus notifications declined by 53% (2007) and 65% (2008); the number of laboratory tests performed declined by 3% (2007) and 15% (2008); and the proportion of tests positive declined by 45% (2007) and 43% (2008) compared with data collected before introduction of the vaccination program. An indirect effect of infant vaccination was seen: notifications and the proportion of tests positive for rotavirus declined in older age groups as well., Conclusions: The publicly funded rotavirus vaccination program in Queensland is having an early impact, direct and indirect, on rotavirus disease as assessed using routinely collected data. Further observational studies are required to assess vaccine effectiveness. Parents and immunisation providers should ensure that all Australian children receive the recommended rotavirus vaccine doses in the required timeframe.

Published

2009

14. Detection of novel influenza A(H1N1) virus by real-time RT-PCR.

Author

Whiley DM, Bialasiewicz S, Bletchly C, Faux CE, Harrower B, Gould AR, Lambert SB, Nimmo GR, Nissen MD, and Sloots TP

Subjects

Animals, Australia, Humans, Influenza A Virus, H1N1 Subtype genetics, Reassortant Viruses genetics, Sensitivity and Specificity, Swine, Influenza A Virus, H1N1 Subtype isolation & purification, Influenza, Human diagnosis, Influenza, Human virology, Reassortant Viruses isolation & purification, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

Accurate and rapid diagnosis of novel influenza A(H1N1) infection is critical for minimising further spread through timely implementation of antiviral treatment and other public health based measures. In this study we developed two TaqMan-based reverse transcription PCR (RT-PCR) methods for the detection of novel influenza A(H1N1) virus targeting the haemagglutinin and neuraminidase genes. The assays were validated using 152 clinical respiratory samples, including 61 Influenza A positive samples, collected in Queenland, Australia during the years 2008 to 2009 and a further 12 seasonal H1N1 and H3N2 influenza A isolates collected from years 2000 to 2002. A wildtype swine H1N1 isolate was also tested. RNA from an influenza A(H1N1) virus isolate (Auckland, 2009) was used as a positive control. Overall, the results showed that the RT-PCR methods were suitable for sensitive and specific detection of novel influenza A(H1N1) RNA in human samples.

Published

2009

15. Do rhinoviruses reduce the probability of viral co-detection during acute respiratory tract infections?

Author

Greer RM, McErlean P, Arden KE, Faux CE, Nitsche A, Lambert SB, Nissen MD, Sloots TP, and Mackay IM

Subjects

Acute Disease epidemiology, Adolescent, Adult, Analysis of Variance, Child, Child, Preschool, Data Interpretation, Statistical, Female, Humans, Infant, Male, Nasopharynx virology, Picornaviridae Infections epidemiology, Polymerase Chain Reaction, Regression Analysis, Respiratory Tract Infections epidemiology, Retrospective Studies, Virus Diseases epidemiology, Viruses isolation & purification, Picornaviridae Infections virology, Respiratory Tract Infections virology, Rhinovirus isolation & purification, Virus Diseases virology

Abstract

Background: Human rhinoviruses (HRVs) are often concurrently detected with other viruses found in the respiratory tract because of the high total number of HRV infections occurring throughout the year. This feature has previously relegated HRVs to being considered passengers in acute respiratory infections. HRVs remain poorly characterized and are seldom included as a target in diagnostic panels despite their pathogenic potential, infection-associated healthcare expenditure and relatively unmoderated elicitation of an antiviral state., Objectives: To test the hypothesis that respiratory viruses are proportionately more or less likely to co-occur, particularly the HRVs., Study Design: Retrospective PCR-based analyses of 1247 specimens for 17 viruses, including HRV strains, identified 131 specimens containing two or more targets. We investigated the proportions of co-detections and compared the proportion of upper vs. lower respiratory tract presentations in the HRV positive group. Both univariate contingency table and multivariate logistic regression analyses were conducted to identify trends of association among the viruses present in co-detections., Results: Many of the co-detections occurred in patterns. In particular, HRV detection was associated with a reduced probability of detecting human adenoviruses, coronaviruses, bocavirus, metapneumovirus, respiratory syncytial virus, parainfluenza virus, influenza A virus, and the polyomaviruses KIPyV and WUPyV (p < or = 0.05). No single HRV species nor cluster of particular strains predominated., Conclusions: HRVs were proportionately under-represented among viral co-detections. For some period, HRVs may render the host less likely to be infected by other viruses.

Published

2009

16. Prior evidence of putative novel rhinovirus species, Australia.

Author

Mackay IM, Lambert SB, McErlean PK, Faux CE, Arden KE, Nissen MD, and Sloots TP

Subjects

Australia epidemiology, Communicable Diseases, Emerging epidemiology, Disease Outbreaks, Humans, New York epidemiology, Picornaviridae Infections epidemiology, Rhinovirus isolation & purification, Communicable Diseases, Emerging virology, Picornaviridae Infections virology, Rhinovirus classification

Published

2008