Your search keyword '"Gallimore, Chris"' showing total 41 results

1. The Effective Teacher in a Bilingual Context.

Author

Cheng, Liyang, Drake, Barry, Falvey, Peter, and Gallimore, Chris

Abstract

Addressing the need to develop genuine, lasting professional relationships, describes authors' experiences in bringing together teachers from Hong Kong's United World College with a mainstream Chinese school of 2000 pupils in Beijing. Workshops and seminars were designed around an "effective teacher" theme, to elucidate the skills, attributes, and personal qualities characterizing model teachers. (MLH)

Published

1998

2. Food-related norovirus outbreak among people attending two barbeques: epidemiological, virological, and environmental investigation

Author

Vivancos, Roberto, Shroufi, Amir, Sillis, Margaret, Aird, Heather, Gallimore, Chris I., Myers, Linda, Mahgoub, Hamid, and Nair, Pat

Published

2009

3. Evaluation of the Loopamp ® (loop-mediated isothermal amplification) kit for detecting Norovirus RNA in faecal samples

Author

Iturriza-Gómara, Miren, Xerry, Jaqueline, Gallimore, Chris I., Dockery, Clare, and Gray, Jim

Published

2008

4. Gastroenteritis outbreak in British troops, Iraq

Author

Bailey, Mark S., Boos, Christopher J., Vautier, Guy, Green, Andrew D., Appleton, Hazel, Gallimore, Chris I., Gray, Jim J., and Beeching, Nicholas J.

Subjects

Iraq War, 2003-2011, Military personnel -- Health aspects, Gastroenteritis -- Risk factors, Gastroenteritis -- Causes of

Abstract

Gastroenteritis affected many British military personnel during the war in Iraq. In the first month, 1,340 cases were seen; 73% of patients required hospital admission and 36% were hospital staff. [...]

Published

2005

5. Capsid Protein Diversity among Norwalk-like Viruses

Author

Green, Jonathan, Vinje, Jan, Gallimore, Chris I., Koopmans, Marion, Hale, Antony, and Brown, David W.G.

Published

2000

6. Tracking the Transmission Routes of Genogroup II Noroviruses in Suspected Food-Borne or Environmental Outbreaks of Gastroenteritis Through Sequence Analysis of the P2 Domain

Author

Xerry, Jacqueline, Gallimore, Chris I., Iturriza-Gómara, Miren, and Gray, Jim J.

Published

2009

7. Characterisation of Norovirus Strains in Rural Ghanaian Children With Acute Diarrhoea

Author

Armah, George E., Gallimore, Chris I., Binka, Fred N., Asmah, Richard H., Green, Jonathan, Ugoji, Ucheoma, Anto, Francis, Brown, David W.G., and Gray, Jim J.

Published

2006

8. Chronic excretion of a norovirus in a child with cartilage hair hypoplasia (CHH)

Author

Gallimore, Chris I, Lewis, David, Taylor, Clive, Cant, Andrew, Gennery, Andrew, and Gray, Jim J

Published

2004

9. Linking healthcare associated norovirus outbreaks: a molecular epidemiologic method for investigating transmission

Author

Andrews Nick, Vipond Ian B, Gray Jim J, Gallimore Chris, Lopman Ben A, Sarangi Joyshri, Reacher Mark H, and Brown David W

Subjects

Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Noroviruses are highly infectious pathogens that cause gastroenteritis in the community and in semi-closed institutions such as hospitals. During outbreaks, multiple units within a hospital are often affected, and a major question for control programs is: are the affected units part of the same outbreak or are they unrelated transmission events? In practice, investigators often assume a transmission link based on epidemiological observations, rather than a systematic approach to tracing transmission. Here, we present a combined molecular and statistical method for assessing: 1) whether observed clusters provide evidence of local transmission and 2) the probability that anecdotally|linked outbreaks truly shared a transmission event. Methods 76 healthcare associated outbreaks were observed in an active and prospective surveillance scheme of 15 hospitals in the county of Avon, England from April 2002 to March 2003. Viral RNA from 64 out of 76 specimens from distinct outbreaks was amplified by reverse transcription-PCR and was sequenced in the polymerase (ORF 1) and capsid (ORF 2) regions. The genetic diversity, at the nucleotide level, was analysed in relation to the epidemiological patterns. Results Two out of four genetic and epidemiological clusters of outbreaks were unlikely to have occurred by chance alone, thus suggesting local transmission. There was anecdotal epidemiological evidence of a transmission link among 5 outbreaks pairs. By combining this epidemiological observation with viral sequence data, the evidence of a link remained convincing in 3 of these pairs. These results are sensitive to prior beliefs of the strength of epidemiological evidence especially when the outbreak strains are common in the background population. Conclusion The evidence suggests that transmission between hospitals units does occur. Using the proposed criteria, certain hypothesized transmission links between outbreaks were supported while others were refuted. The combined molecular/epidemiologic approach presented here could be applied to other viral populations and potentially to other pathogens for a more thorough view of transmission.

Published

2006

10. A summertime peak of 'winter vomiting disease': Surveillance of noroviruses in England and Wales, 1995 to 2002

Author

Gray Jim J, Adak Goutam K, Gallimore Chris, Reacher Mark, Lopman Ben A, and Brown David WG

Subjects

Public aspects of medicine, RA1-1270

Abstract

Abstract Background Noroviruses are the most common cause of gastroenteritis outbreaks in industrialised countries. Gastroenteritis caused by Norovirus infection has been described as a highly seasonal syndrome, often referred to as "winter vomiting disease". Methods The Public Health Laboratory Service Communicable Disease Surveillance Centre has systematically collected reports of laboratory confirmed cases of Norovirus-gastroenteritis since 1995. We analysed these data for annual and seasonal trends and age distribution. Results A mid-summer peak in reported cases of Norovirus was observed in 2002, unlike all six previous years when there was a marked summer decline. Total reports from 2002 have also been higher than all previous years. From the first 10 months of 2002, a total of 3029 Norovirus diagnoses were reported compared the previous peak in 1996 of 2437 diagnoses for the whole 12-month period. The increase in 2002 was most marked in the 65 and older age group. Conclusion This surveillance data challenges the view that Noroviruses infections exclusively have wintertime seasonality.

Published

2003

11. Predominance of enterovirus B and echovirus 30 as cause of viral meningitis in a UK population

Author

Holmes, Christopher W, Koo, Sharon SF, Osman, Husam, Wilson, Steven, Xerry, Jacqueline, Gallimore, Chris I, Allen, David J, and Tang, Julian W

Subjects

viruses, virus diseases

Abstract

BACKGROUND/OBJECTIVES: Enteroviruses are the most common cause of aseptic or lymphocytic meningitis, particularly in children. With reports of unusually severe neurological disease in some patients infected with enterovirus D68 in North America, and a recent increase in the number of paediatric enterovirus meningitis cases presenting in this UK Midlands population, a retrospective regional surveillance study was performed. STUDY DESIGN: Cerebrospinal fluid (CSF) samples received were tested using the polymerase chain reaction (PCR) for HSV-1/2, VZV, enteroviruses and parechoviruses. Enterovirus PCR positive CSF samples were sent for further serotyping. A phylogenetic tree was constructed of the echovirus 30 VP1 sequences, where sufficient sample remained for sequencing. RESULTS: The number of enterovirus positive CSFs from each year were: 21 (2008), 7 (2011), 53 (2012), 58 (2013) and 31 (2014). Overall, 163 of the 170 serotyped enteroviruses belonged to the species B (echovirus 5, 6, 7, 9, 11, 13, 16, 17, 18, 21, 25, 30; coxsackie B1, B2, B3, B4, B5, A9), with only 7 belonging to species A (coxsackie A2, A6, A16 and enterovirus 71). Echovirus 30 was the predominant serotype overall, identified in 43 (25.3%) of samples, with a significantly higher proportion in the adult age group (37.3%) compared to the infant age group (12.3%). Phylogenetic analysis showed that these UK Midlands echovirus 30 VP1 sequences clustered most closely with those from Europe and China. CONCLUSION: This study showed a continued predominance of echovirus 30 as a cause of viral meningitis, particularly in adults, though more surveillance is needed.

Published

2016

12. Increase in viral gastroenteritis outbreaks in Europe and epidemic spread of new norovirus variant

Author

Lopman, Ben, Vennema, Harry, Kohli, Evelyne, Pothier, Pierre, Sanchez, Alicia, Negredo, Anabel, Buesa, Javier, Schreier, Eckart, Reacher, Mark, Myller, Rolf, Gray, Jim, Iturriza, Miren, Gallimore, Chris, Bottiger, Blenda, Hedlund, Kjell-Olof, Torven, Maria, von Bonsdorff, Carl-Henrik, Maunula, Leena, Poljsak-Prijatelj, Mateja, Zimsek, Janet, Reuter, Gabor, Szucs, Gyorgy, Melegh, Bela, Svennson, Lennart, van Duijnhoven, Yvonne, and Koopmans, Marion

Subjects

Gastrointestinal diseases -- Reports, Gastrointestinal diseases -- Development and progression, Gastroenteritis -- Reports, Gastroenteritis -- Development and progression

Published

2004

13. A summertime peak of 'winter vomiting disease': surveillance of noroviruses in England and Wales, 1995 to 2002

Author

Lopman, Ben A, Reacher, Mark, Gallimore, Chris, Adak, Goutam K, Gray, Jim J, and Brown, David WG

Abstract

BACKGROUND: Noroviruses are the most common cause of gastroenteritis outbreaks in industrialised countries. Gastroenteritis caused by Norovirus infection has been described as a highly seasonal syndrome, often referred to as "winter vomiting disease". METHODS: The Public Health Laboratory Service Communicable Disease Surveillance Centre has systematically collected reports of laboratory confirmed cases of Norovirus-gastroenteritis since 1995. We analysed these data for annual and seasonal trends and age distribution. RESULTS: A mid-summer peak in reported cases of Norovirus was observed in 2002, unlike all six previous years when there was a marked summer decline. Total reports from 2002 have also been higher than all previous years. From the first 10 months of 2002, a total of 3029 Norovirus diagnoses were reported compared the previous peak in 1996 of 2437 diagnoses for the whole 12-month period. The increase in 2002 was most marked in the 65 and older age group. CONCLUSION: This surveillance data challenges the view that Noroviruses infections exclusively have wintertime seasonality.

Published

2003

14. Gastroenteric Viruses.

Author

St. Georgiev, Vassil, Simjee, Shabbir, Iturriza-Gómara, Miren, Gallimore, Chris I., and Gray, Jim

Abstract

In recent years, viruses have been recognized increasingly as an important cause of foodborne infections. More than 160 enteric viruses are excreted in the feces of infected individuals, and some may also be present in the vomitus. Food and water are directly contaminated with fecal material, through the use of sewage sludge in agriculture, sewage pollution of shellfish culture beds, or may be contaminated by infected food-handlers. [ABSTRACT FROM AUTHOR]

Published

2007

15. A Preliminary Biomechanical Study of Cyclic Preconditioning Effects on Canine Cadaveric Whole Femurs.

Author

Zdero, Rad, Gallimore, Chris H., McConnell, Alison J., Patel, Harshita, Nisenbaum, Rosane, Morshed, Golam, Koo, Henry, McKee, Michael D., Schemitsch, Emil H., and Bougherara, Habiba

Subjects

*FEMUR, *BIOMECHANICS, *BIOLOGICAL specimens, *BONES, *STIFFNESS (Mechanics)

Abstract

Biomechanical preconditioning of biological specimens by cyclic loading is routinely done presumably to stabilize properties prior to the main phase of a study. However, no prior studies have actually measured these effects for whole bone of any kind. The aim of this study, therefore, was to quantify these effects for whole bones. Fourteen matched pairs of fresh-frozen intact cadaveric canine femurs were sinusoidally loaded in 4-point bending from 50 N to 300 N at 1 Hz for 25 cycles. All femurs were tested in both anteroposterior (AP) and mediolateral (ML) bending planes. Bending stiffness (i.e., slope of the force-vs-displacement curve) and linearity R2 (i.e., coefficient of determination) of each loading cycle were measured and compared statistically to determine the effect of limb side, cycle number, and bending plane. Stiffnesses rose from 809.7 to 867.7N/mm (AP, left), 847.3 to 915.6 N/mm (AP, right), 829.2 to 892.5Nlmm (AP, combined), 538.7 to 580.4 N/mm (ML, left), 568.9 to 613.8 N/mm (ML, right), and 553.8 to 597.1 N/mm (ML, combined). Linearity R2 rose from 0.96 to 0.99 (AP, left), 0.97 to 0.99 (AP, right), 0.96 to 0.99 (AP, combined), 0.95 to 0.98 (ML, left), 0.94 to 0.98 (ML, right), and 0.95 to 0.98 (ML, combined). Stiffness and linearity R versus cycle number were well-described by exponential curves whose values leveled off, respectively, starting at 12 and 5 cycles. For stiffness, there were no statistical differences for left versus right femurs (p = 0.166), but there were effects due to cycle number (p < 0.0001) and AP versus ML bending plane (p < 0.0001). Similarly, for linearity, no statistical differences were noted due to limb side (p = 0.533), but there were effects due to cycle number (p < 0.0001) and AP versus ML bending plane (p - 0.006). A minimum of 12 preconditioning cycles was needed to fully stabilize both the stiffness and linearity of the canine femurs. This is the first study to measure the effects of mechanical preconditioning on whole bones, having some practical implications on research practices. [ABSTRACT FROM AUTHOR]

Published

2012

16. Chronic norovirus infection in an HIV-positive patient with persistent diarrhoea: A novel cause

Author

Wingfield, Tom, Gallimore, Chris I., Xerry, Jacqueline, Gray, Jim J., Klapper, Paul, Guiver, Malcolm, and Blanchard, Tom J.

Published

2010

17. Analysis of Amino Acid Variation in the P2 Domain of the GII-4 Norovirus VP1 Protein Reveals Putative Variant-Specific Epitopes.

Author

Allen, David J., Gray, Jim J., Gallimore, Chris I., Xerry, Jacqueline, and Iturriza-Gómara, Miren

Abstract

Background. Human noroviruses are a highly diverse group of viruses classified into three of the five currently recognised Norovirus genogroups, and contain numerous genotypes or genetic clusters. Noroviruses are the major aetiological agent of endemic gastroenteritis in all age groups, as well as the cause of periodic epidemic gastroenteritis. The noroviruses most commonly associated with outbreaks of gastroenteritis are genogroup II genotype 4 (GII-4) strains. The relationship between genotypes of noroviruses with their phenotypes and antigenic profile remains poorly understood through an inability to culture these viruses and the lack of a suitable animal model. Methodology/Principal Findings. Here we describe a study of the diversity of amino acid sequences of the highly variable P2 region in the major capsid protein, VP1, of the GII-4 human noroviruses strains using sequence analysis and homology modelling techniques. Conclusions/Significance. Our data identifies two sites in this region, which show significant amino acid substitutions associated with the appearance of variant strains responsible for epidemics with major public health impact. Homology modelling studies revealed the exposed nature of these sites on the capsid surface, providing supportive structural data that these two sites are likely to be associated with putative variant-specific epitopes. Furthermore, the patterns in the evolution of these viruses at these sites suggests that noroviruses follow a neutral network pattern of evolution. [ABSTRACT FROM AUTHOR]

Published

2008

18. Characterisation of small double stranded RNA molecule in Cryptosporidium hominis, Cryptosporidium felis and Cryptosporidium meleagridis

Author

Leoni, Francesca, Gallimore, Chris I., Green, Jonathan, and McLauchlin, Jim

Subjects

*RNA, *COCCIDIA, *AMINO acid sequence, *ORGANIC acids

Abstract

Abstract: Coding regions of double stranded RNA molecules from 3 human faecal samples containing Cryptosporidium hominis, C. felis and C. meleagridis were characterised by sequencing and compared with that previously obtained for C. parvum. Sequences outside the coding regions were also obtained. Overall similarities of between 86% and 92% and between 86% and 93% were observed in the nucleotide and amino acid sequences respectively between these species. These larger sequences will allow further molecular tools for detection, identification and characterisation of Cryptosporidium spp. [Copyright &y& Elsevier]

Published

2006

19. Linking healthcare associated norovirus outbreaks: a molecular epidemiologic method for investigating transmission.

Author

Lopman, Ben A., Gallimore, Chris, Gray, Jim J., Vipond, Ian B., Andrews, Nick, Sarangi, Joyshri, Reacher, Mark H., and Brown, David W.

Subjects

*DISEASE outbreaks, *NOROVIRUSES, *INFECTIOUS disease transmission, *MOLECULAR epidemiology, *RNA viruses

Abstract

Background: Noroviruses are highly infectious pathogens that cause gastroenteritis in the community and in semi-closed institutions such as hospitals. During outbreaks, multiple units within a hospital are often affected, and a major question for control programs is: are the affected units part of the same outbreak or are they unrelated transmission events? In practice, investigators often assume a transmission link based on epidemiological observations, rather than a systematic approach to tracing transmission. Here, we present a combined molecular and statistical method for assessing: 1) whether observed clusters provide evidence of local transmission and 2) the probability that anecdotally∣linked outbreaks truly shared a transmission event. Methods: 76 healthcare associated outbreaks were observed in an active and prospective surveillance scheme of 15 hospitals in the county of Avon, England from April 2002 to March 2003. Viral RNA from 64 out of 76 specimens from distinct outbreaks was amplified by reverse transcription-PCR and was sequenced in the polymerase (ORF 1) and capsid (ORF 2) regions. The genetic diversity, at the nucleotide level, was analysed in relation to the epidemiological patterns. Results: Two out of four genetic and epidemiological clusters of outbreaks were unlikely to have occurred by chance alone, thus suggesting local transmission. There was anecdotal epidemiological evidence of a transmission link among 5 outbreaks pairs. By combining this epidemiological observation with viral sequence data, the evidence of a link remained convincing in 3 of these pairs. These results are sensitive to prior beliefs of the strength of epidemiological evidence especially when the outbreak strains are common in the background population. Conclusion: The evidence suggests that transmission between hospitals units does occur. Using the proposed criteria, certain hypothesized transmission links between outbreaks were supported while others were refuted. The combined molecular/epidemiologic approach presented here could be applied to other viral populations and potentially to other pathogens for a more thorough view of transmission. [ABSTRACT FROM AUTHOR]

Published

2006

20. Multiple norovirus genotypes characterised from an oyster-associated outbreak of gastroenteritis

Author

Gallimore, Chris I., Cheesbrough, John S., Lamden, Kenneth, Bingham, Chris, and Gray, Jim J.

Subjects

*GENETIC polymorphisms, *GENETIC research, *AGRICULTURAL equipment, *GASTROINTESTINAL diseases

Abstract

Abstract: The diversity of norovirus (NV) genotypes was investigated in persons who were ill with acute gastroenteritis associated with the consumption of oysters. Initial results from a commercial enzyme immunoassay (EIA) indicated a mixed NV genogroup I (GI) and II (GII) outbreak. A reverse-transcriptase (RT)-PCR for NVs was applied to nucleic acid extracted from faecal specimens collected from symptomatic cases. Using primers that amplified contiguous sequences in the ORF1/2 region of the NV genome and a hemi-nested PCR derived from this assay, three different GII and two GI NV genotypes were detected and the strains were characterised by DNA sequencing. Using this approach a recombinant NV genotype, rGII-3a (recombinant Harrow/Mexico) the predominant strain identified in several symptomatic cases from the outbreak, was detected and characterised. No other gastroenteric viruses, including rotavirus, astrovirus, sapovirus and adenovirus 40/41 were detected by RT-PCR and PCR. [Copyright &y& Elsevier]

Published

2005

21. Application of the heteroduplex mobility assay (HMA) for the investigation of the genomic diversity among noroviruses in environmental samples

Author

Green, Jonathan, Gallimore, Chris I, Shore, Jane, Sellwood, Jane, and Brown, David W.G.

Subjects

*VIRUSES, *WATER pollution, *SEWAGE, *RNA polymerases

Abstract

Recent studies have demonstrated the widespread contamination of river and seawater with noroviruses (NV), often with more than one strain. The heteroduplex mobility assay (HMA) in which amplicons from study samples are hybridised (by denaturing and reannealing) to amplicons from reference strains and resolved by electrophoresis, has the potential to provide a simple and rapid means to identify samples containing multiple NV strains and to establish the diversity of strains within that sample. PCR amplicons from environmental samples that were tested directly in the HMA assay were shown to contain more than one strain. In order to evaluate HMA for investigations of NV diversity in environmental samples, amplicons from three representative samples were cloned and, for each, 20 amplicons derived from individual clones were analysed by HMA. Between two and six different HMA profiles were demonstrated among clones from a single sample indicating the extent of NV diversity in the sample. Sequence analysis confirmed the relationship of HMA profile and NV ‘genotype’. Far greater diversity was seen among Genogroup (G) II (Ni/E3) amplicons than Genogroup (G) I (Ando/E3) amplicons (generated from the RNA dependent RNA polymerase region of the ORF1 of noroviruses), which often contained only a single strain, which is reflective of the greater prevalence of GII NVs over GI NVs. Overall, four GII and four GI strains were identified in these environmental water/sewage samples. [Copyright &y& Elsevier]

Published

2004

22. A rapid method for identifying diversity within PCR amplicons using a heteroduplex mobility assay and synthetic polynucleotides: application to characterisation of dsRNA elements associated with Cryptosporidium

Author

Leoni, Francesca, Gallimore, Chris I., Green, Jonathan, and McLauchlin, Jim

Subjects

*CRYPTOSPORIDIUM, *RNA

Abstract

A 173-bp fragment of the small extra-chromosomal double-stranded RNA (dsRNA) element of Cryptosporidium parvum was generated by reverse transcriptase PCR from nucleic acid extracted from whole faeces of 18 epidemiologically unrelated cases of cryptosporidiosis. Eleven different sequences were detected and two selected as reference DNA in a heteroduplex mobility assay (HMA). Although sequence diversity was detected, this was difficult to characterise because of the similarity in electrophoretic mobility of the homo- and heteroduplex bands. A PCR method was devised to generate synthetic polynucleotides of greater sequence diversity for use in the HMA. The presence of the synthetic 173-bp fragments was enriched by using, as template for the PCR, material excised from the area of the heteroduplex bands in stained electrophoresis gels. Nine novel sequences were generated and evaluated as reference sequences in the HMA. One of these with 20 bp different from the original sequence was selected for use in the HMA for improved resolution of heteroduplex and homoduplex bands and number of patterns easily resolved (nine different patterns corresponding to different DNA sequences). This method may be useful for analysis of DNA where there is limited natural variation or little sequence variation is described. [Copyright &y& Elsevier]

Published

2003

23. Evaluation of the Loopamp® (loop-mediated isothermal amplification) kit for detecting Norovirus RNA in faecal samples

Author

Iturriza-Gómara, Miren, Xerry, Jaqueline, Gallimore, Chris I., Dockery, Clare, and Gray, Jim

Subjects

*NOROVIRUSES, *EPIDEMICS, *GASTROENTERITIS, *CLINICAL pathology, *VIRAL genetics

Abstract

Abstract: Background: Noroviruses (NoVs) are associated with outbreaks of diarrhoeal illness in hospitals, nursing and residential homes and other institutional settings. NoV strains exhibit wide genetic diversity, and different virus genogroups and genotypes co-circulate in any geographical region at the same time, although most outbreaks of gastroenteritis are predominantly associated with genogroup II. The reverse transcription-polymerase chain reaction (RT-PCR) is the gold standard for detecting NoVs in clinical samples. Objectives: This study evaluates commercialised Loopamp® kits for detecting NoV GI and NoV GII in faecal samples collected from patients with gastroenteritis and compares the results with those obtained using real-time RT-PCR with NoV genogroup sequence-specific detection. Study design: Five hundred and ten faecal samples collected from patients with gastroenteritis were evaluated for the presence of NoV using the gold-standard real-time RT-PCRs and the Loopamp® assays. Results: The Loopamp® Norovirus GI and GII detection kits performed well compared to genogroup-specific real-time RT-PCR. Although the sensitivity of detection of GI strains (83.3%) was less than that for GII strains (97.4%), this will have little impact on the laboratory diagnosis of NoV, since GII strains are associated with the majority of outbreaks examined. Conclusions: The Loopamp® GII detection kit is a sensitive method for detecting all the commonly circulating GII-4 strains included in the evaluation panel. [Copyright &y& Elsevier]

Published

2008

24. Predominance of enterovirus B and echovirus 30 as cause of viral meningitis in a UK population.

Author

Holmes CW, Koo SS, Osman H, Wilson S, Xerry J, Gallimore CI, Allen DJ, and Tang JW

Subjects

Adolescent, Adult, Child, Child, Preschool, Echovirus Infections epidemiology, Echovirus Infections virology, Humans, Infant, Infant, Newborn, Phylogeny, Polymerase Chain Reaction, RNA, Viral cerebrospinal fluid, United Kingdom epidemiology, Young Adult, Enterovirus B, Human classification, Enterovirus B, Human genetics, Enterovirus Infections epidemiology, Enterovirus Infections virology, Meningitis, Viral epidemiology, Meningitis, Viral virology

Abstract

Background/objectives: Enteroviruses are the most common cause of aseptic or lymphocytic meningitis, particularly in children. With reports of unusually severe neurological disease in some patients infected with enterovirus D68 in North America, and a recent increase in the number of paediatric enterovirus meningitis cases presenting in this UK Midlands population, a retrospective regional surveillance study was performed., Study Design: Cerebrospinal fluid (CSF) samples received were tested using the polymerase chain reaction (PCR) for HSV-1/2, VZV, enteroviruses and parechoviruses. Enterovirus PCR positive CSF samples were sent for further serotyping. A phylogenetic tree was constructed of the echovirus 30 VP1 sequences, where sufficient sample remained for sequencing., Results: The number of enterovirus positive CSFs from each year were: 21 (2008), 7 (2011), 53 (2012), 58 (2013) and 31 (2014). Overall, 163 of the 170 serotyped enteroviruses belonged to the species B (echovirus 5, 6, 7, 9, 11, 13, 16, 17, 18, 21, 25, 30; coxsackie B1, B2, B3, B4, B5, A9), with only 7 belonging to species A (coxsackie A2, A6, A16 and enterovirus 71). Echovirus 30 was the predominant serotype overall, identified in 43 (25.3%) of samples, with a significantly higher proportion in the adult age group (37.3%) compared to the infant age group (12.3%). Phylogenetic analysis showed that these UK Midlands echovirus 30 VP1 sequences clustered most closely with those from Europe and China., Conclusion: This study showed a continued predominance of echovirus 30 as a cause of viral meningitis, particularly in adults, though more surveillance is needed., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

25. Genetic characterization of genogroup I norovirus in outbreaks of gastroenteritis.

Author

Xerry J, Gallimore CI, Iturriza-Gómara M, and Gray JJ

Subjects

Capsid Proteins genetics, Cluster Analysis, Feces virology, Genotype, Humans, Molecular Sequence Data, Norovirus classification, Phylogeny, Polymerase Chain Reaction, RNA, Viral chemistry, Sequence Analysis, DNA, Caliciviridae Infections epidemiology, Caliciviridae Infections virology, Disease Outbreaks, Gastroenteritis epidemiology, Gastroenteritis virology, Norovirus genetics

Abstract

In this study, we demonstrate that differences within the P2 domain of norovirus genogroup I (GI) strains can be used to segregate outbreaks which are unrelated, whereas complete conservation within this region allows tracking of strains that are part of a single outbreak and likely to have a common source.

Published

2010

26. Tracking environmental norovirus contamination in a pediatric primary immunodeficiency unit.

Author

Xerry J, Gallimore CI, Cubitt D, and Gray JJ

Subjects

Cluster Analysis, Feces virology, Humans, Immunocompromised Host, Infant, Intensive Care Units, Pediatric, Male, Norovirus genetics, Caliciviridae Infections microbiology, Caliciviridae Infections transmission, Environmental Microbiology, Norovirus isolation & purification

Abstract

Norovirus strains were detected in two patients and in environmental swabs from a pediatric primary immunodeficiency unit in London, United Kingdom, during an infection control incident in November and December 2007. Detailed analyses of the gene encoding the P2 domain demonstrated that the majority of the strains were not related to the patients and that the environmental contamination was most likely due to secondary transfer by the hands of staff or visitors.

Published

2010

27. The effect of cement mixing time on the biomechanics of cement augmented plated fractures in canine femora.

Author

Gallimore CH, McConnell AJ, Zdero R, Koo H, McKee MD, and Schemitsch EH

Subjects

Animals, Compressive Strength, Dogs, Elastic Modulus, Hardness, In Vitro Techniques, Stress, Mechanical, Tensile Strength, Time Factors, Bone Plates, Cementation methods, Femoral Fractures physiopathology, Femoral Fractures surgery, Fracture Fixation, Internal instrumentation

Abstract

Objective: The goal of this study was to determine the effect of cement mixing time and, hence, cement viscosity on the biomechanical behavior of femoral fracture fixation., Design: Cadaveric plated canine femoral fracture model, comparing treatments in matched pairs., Setting: Orthopaedic biomechanics laboratory., Intervention: Cement was inserted both as a liquid and as a paste in standard and oversized screw holes to augment fixation with plates and screws., Main Outcome Measurements: Standard 4-point bending tests were performed to obtain stiffness and failure load values., Results: Liquid cement had a 1.38 times increase in stiffness and a failure load 1.84 times greater compared with paste cement, regardless of hole size with a gap at the fracture site (P < 0.05). Liquid cement had a force to failure of 1.77 and 1.91 times in the standard-sized and oversized holes, respectively, when compared with paste cement (P < 0.05)., Conclusions: When the cement was inserted in a liquid state in a plated femoral diaphyseal fracture with a gap, screw purchase augmentation achieved greater bending stiffness and resisted a greater failure load.

Published

2008

28. Contamination of the hospital environment with gastroenteric viruses: comparison of two pediatric wards over a winter season.

Author

Gallimore CI, Taylor C, Gennery AR, Cant AJ, Galloway A, Xerry J, Adigwe J, and Gray JJ

Subjects

Child, Preschool, Decontamination, Humans, Molecular Sequence Data, Seasons, Astroviridae Infections prevention & control, Cross Infection prevention & control, Gastroenteritis prevention & control, Hospital Departments standards, Mamastrovirus, Norovirus, Pediatrics standards, Rotavirus, Rotavirus Infections prevention & control

Abstract

The aims of this study were to examine the extent of gastroenteric virus contamination in a pediatric primary immunodeficiency (PPI) ward and a general pediatric ward over a winter season and to determine whether changes to hospital infection control interventions would have an impact on environmental contamination levels within pediatric units. Environmental swabs were collected weekly from 11 sites in both wards from 15 December 2005 to 3 March 2006 and examined for the presence of norovirus (NoV), astrovirus, and rotavirus (RV) by reverse transcriptase PCR. Viruses were detected in 17% and 19% of swabs from both wards. Virus contamination for NoV and RV decreased from 20% to 6% and 15% to 10% of swabs, respectively, in the PPI ward from the 2004 study by Gallimore et al. (C. I. Gallimore, C. Taylor, A. R. Gennery, A. J. Cant, A. Galloway, M. Iturriza-Gomara, and J. J. Gray, J. Clin. Microbiol. 44:395-399, 2006). Overall, changes to cleaning protocols were deemed to have reduced the level of environmental contamination with gastroenteric viruses, but contamination still occurred due to a breakdown in infection control procedures indicated by contamination in areas frequented by parents but used only occasionally by staff.

Published

2008

29. Transmission events within outbreaks of gastroenteritis determined through analysis of nucleotide sequences of the P2 domain of genogroup II noroviruses.

Author

Xerry J, Gallimore CI, Iturriza-Gómara M, Allen DJ, and Gray JJ

Subjects

Base Sequence, Feces virology, Genotype, Hospitals, Humans, Norwalk virus chemistry, Norwalk virus isolation & purification, Phylogeny, Polymerase Chain Reaction, RNA, Viral analysis, RNA, Viral isolation & purification, Ships, Species Specificity, United Kingdom epidemiology, Caliciviridae Infections epidemiology, Caliciviridae Infections transmission, Caliciviridae Infections virology, Capsid Proteins genetics, Disease Outbreaks, Gastroenteritis epidemiology, Gastroenteritis virology, Norwalk virus classification, Norwalk virus genetics, Sequence Analysis, DNA

Abstract

Tracking the spread of noroviruses during outbreaks of gastroenteritis is hampered by the lack of sequence diversity in those regions of the genome chosen for virus detection and characterization. Sequence analysis of regions of the genes encoding the RNA-dependent RNA polymerase and the S domain of the capsid does not provide sufficient discrimination between genotypically related strains of different outbreaks. However, analysis of sequences derived from the region encoding the P2 domain showed 100% similarity among strains from the same outbreak and <100% similarity among strains of different outbreaks. The prolonged nature of some hospital outbreaks, links between hospitals, and the introduction of multiple strains of a single genotype associated with an outbreak aboard a cruise ship were determined using this method. This provides a powerful tool for tracking outbreak strains and the subsequent analysis and validation of interventions in a background of multiple introductions of virus strains of the same genotype or genetic cluster.

Published

2008

30. European multicenter evaluation of commercial enzyme immunoassays for detecting norovirus antigen in fecal samples.

Author

Gray JJ, Kohli E, Ruggeri FM, Vennema H, Sánchez-Fauquier A, Schreier E, Gallimore CI, Iturriza-Gomara M, Giraudon H, Pothier P, Di Bartolo I, Inglese N, de Bruin E, van der Veer B, Moreno S, Montero V, de Llano MC, Höhne M, and Diedrich SM

Subjects

Antigens, Viral immunology, Caliciviridae Infections diagnosis, Caliciviridae Infections immunology, Europe, Gastroenteritis diagnosis, Gastroenteritis immunology, Humans, Reagent Kits, Diagnostic, Sensitivity and Specificity, Antigens, Viral analysis, Feces virology, Immunoenzyme Techniques standards, Norovirus immunology

Abstract

A total of 2,254 fecal samples were tested in a European multicenter evaluation of commercially available norovirus antigen detection assays. Two commercial enzyme immunoassays, IDEIA Norovirus (Oxoid; Thermo Fisher Scientific, Ely, United Kingdom) and RIDASCREEN Norovirus (R-Biopharm, Darmstadt, Germany), were included in the evaluation, and their performance was compared with the results of reverse transcription-PCR (RT-PCR). Included in the evaluation were samples collected in sporadic cases of gastroenteritis, samples from outbreaks in which two or more samples were collected, well-characterized samples representing genotypes currently cocirculating within Europe, and samples collected from patients with gastroenteritis caused by a pathogen other than norovirus. The sensitivities and specificities of the IDEIA Norovirus and RIDASCREEN Norovirus assays were 58.93 and 43.81% and 93.91 and 96.37%, respectively, compared with RT-PCR. The sensitivities of both assays for outbreak investigations improved when six or more samples from an outbreak were examined. The IDEIA Norovirus assay exhibited reactivity to a broader range of norovirus genotypes than the RIDASCREEN Norovirus assay, which showed genotype-dependent sensitivities. The results indicate that, if used, these assays should serve as screening assays and the results should be confirmed by RT-PCR.

Published

2007

31. Characterization of sapoviruses collected in the United Kingdom from 1989 to 2004.

Author

Gallimore CI, Iturriza-Gomara M, Lewis D, Cubitt D, Cotterill H, and Gray JJ

Subjects

Adult, Caliciviridae Infections virology, Capsid metabolism, Child, Child, Preschool, Feces virology, Genes, Viral genetics, Humans, Infant, Iraq, Open Reading Frames genetics, RNA-Dependent RNA Polymerase genetics, RNA-Dependent RNA Polymerase metabolism, Sapovirus classification, Species Specificity, United Kingdom epidemiology, Caliciviridae Infections epidemiology, Disease Outbreaks, Gastroenteritis epidemiology, Genetic Variation, Molecular Epidemiology, Sapovirus genetics

Abstract

A fecal archive containing 115 sapovirus (SaV) strains detected in samples collected from 15 outbreaks and 98 sporadic cases of gastroenteritis between 1989 and 2004 in the UK were characterized in order to determine the genomic diversity within SaV co-circulating in the human population. Strains were characterized by partial sequencing of the genes encoding the RNA-dependent RNA polymerase (RdRp) region and/or the polymerase/capsid (Pol/Cap) junction of the open reading frame (Orf) 1. Overall, SaV of genogroup I genotype 1 (GI 1) were the predominant strains circulating in the UK in each year between 1989 and 2004. During 2004, GII 1 was the predominant strain. These two SaV types accounted for 89.5% of the sporadic cases and outbreaks in the UK. The remaining cases were caused by six other SaV genotypes. On the basis of partial sequencing of the RdRp and capsid encoding genes of strains, which did not show sufficient homology to any of the currently recognized genotypes, we propose the inclusion of a presumptive fourth genotype within genogroup I (GI 4)., (Copyright 2006 Wiley-Liss, Inc.)

Published

2006

32. Environmental monitoring for gastroenteric viruses in a pediatric primary immunodeficiency unit.

Author

Gallimore CI, Taylor C, Gennery AR, Cant AJ, Galloway A, Iturriza-Gomara M, and Gray JJ

Subjects

Child, Preschool, Environmental Microbiology, Feces virology, Humans, Infant, Male, Pediatrics, RNA Virus Infections virology, Reverse Transcriptase Polymerase Chain Reaction, Environmental Monitoring methods, Gastroenteritis virology, Hospital Units, Immunologic Deficiency Syndromes complications, Mamastrovirus isolation & purification, Norovirus isolation & purification, Rotavirus isolation & purification

Abstract

The aim of this study was to determine if gastroenteric viruses were present on surfaces and equipment in a pediatric primary immunodeficiency unit (PPIU) by environmental sampling using swabs and subsequent nucleic acid extraction and reverse transcriptase PCR assays. A PPIU was chosen, and 11 swabs were taken at the same sites every 2 weeks for 6 months. Nested/heminested PCR assays were used to screen for astroviruses (AsV), noroviruses (NoV), and rotaviruses (RV). AsV, NoV, and RV were detected at multiple swab sites during the study period. NoV was the most frequently detected virus on environmental surfaces; however, RV was detected on 79% and NoV on 50% of swabbing dates during the study period. Toilet taps were the most contaminated sites. Fecal samples from selected patients in the unit were also screened during the study period, and patients excreted AsV, NoV, and RV at times during the study. New cleaning schedules and changes in some of the PPIU sanitary furniture have been suggested as a means of reducing environmental contamination.

Published

2006

33. Use of a heminested reverse transcriptase PCR assay for detection of astrovirus in environmental swabs from an outbreak of gastroenteritis in a pediatric primary immunodeficiency unit.

Author

Gallimore CI, Taylor C, Gennery AR, Cant AJ, Galloway A, Lewis D, and Gray JJ

Subjects

Astroviridae Infections epidemiology, Environmental Microbiology, Gastroenteritis epidemiology, Humans, Infant, Astroviridae Infections virology, Disease Outbreaks, Gastroenteritis virology, Immunologic Deficiency Syndromes complications, Mamastrovirus isolation & purification, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

An outbreak of astrovirus gastroenteritis occurred in the Primary Immunodeficiency Unit at Newcastle General Hospital in March 2004. Environmental swabbing of the unit was undertaken after the outbreak, with multiple sites swabbed pre- and postcleaning. Astroviruses were detected in four environmental swabs and from two patient fecal samples using heminested reverse transcriptase PCR. An astrovirus genotype 3 strain was identified in both environmental swabs and fecal specimens and was the strain identified as being responsible for the outbreak. Environmental transmission of the virus was thought to have occurred by contamination of a syringe pump outside the laminar-flow curtain of a patient who was admitted with astrovirus gastroenteritis. This was subsequently transmitted to a cubicle next door and to a television/games console in a parents' room in the ward. Environmental monitoring of surfaces/equipment, using PCR assays for gastroenteric viruses in hospital situations where infection can give rise to serious clinical complications, may have a role in controlling and monitoring cleaning and the subsequent prevention of nosocomial transmission of gastroenteritis.

Published

2005

34. Diversity of enteric viruses detected in patients with gastroenteritis in a tertiary referral paediatric hospital.

Author

Gallimore CI, Cubitt DW, Richards AF, and Gray JJ

Subjects

Adolescent, Astroviridae Infections epidemiology, Caliciviridae Infections epidemiology, Child, Child, Preschool, Cluster Analysis, Cross Infection epidemiology, Cross Infection virology, Feces virology, Hospitals, Pediatric, Humans, Infant, London, Mamastrovirus isolation & purification, Norovirus isolation & purification, Phylogeny, RNA, Viral genetics, RNA, Viral isolation & purification, Reverse Transcriptase Polymerase Chain Reaction, Sapovirus isolation & purification, Sequence Analysis, DNA, Sequence Homology, Astroviridae Infections virology, Caliciviridae Infections virology, Gastroenteritis virology, Mamastrovirus genetics, Norovirus genetics, Sapovirus genetics

Abstract

The genetic diversity of enteric viruses co-circulating in a cohort of patients with viral gastroenteritis in a large tertiary paediatric hospital in London, UK, was determined. Multiple strains of noroviruses (NV), sapoviruses (SV) and astroviruses (HAsV) were detected in these patients, indicating the likelihood of multiple introductions from different sources, possible sub-clinical infections and simultaneous infection with different viruses in immunocompromised and other patients. Routine screening of immunocompromised patients and infection control procedures are important to prevent nosocomial infection., (Copyright 2004 Wiley-Liss, Inc.)

Published

2004

35. Methods for the detection and characterisation of noroviruses associated with outbreaks of gastroenteritis: outbreaks occurring in the north-west of England during two norovirus seasons.

Author

Gallimore CI, Green J, Richards AF, Cotterill H, Curry A, Brown DW, and Gray JJ

Subjects

Antigens, Viral analysis, Caliciviridae Infections epidemiology, Cluster Analysis, England epidemiology, Enzyme-Linked Immunosorbent Assay, Feces virology, Gastroenteritis epidemiology, Genotype, Heteroduplex Analysis, Hospitals, Humans, Microscopy, Electron, Molecular Epidemiology, Norovirus genetics, Norovirus immunology, Norovirus ultrastructure, Nursing Homes, Phylogeny, Polymorphism, Genetic, RNA, Viral analysis, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, DNA, Caliciviridae Infections virology, Disease Outbreaks, Gastroenteritis virology, Norovirus isolation & purification

Abstract

This article describes the methods used to investigate 407 outbreaks of acute non-bacterial gastroenteritis occurring in the North-West of England between January 2000 and July 2001 and suspected to be caused by noroviruses (NV) [Mayo (2002) Arch Virol 147:1655-1663]. These included 319 outbreaks in hospitals and nursing homes and 88 other settings. Eight hundred and seventy-one faecal samples from 407 outbreaks were tested using electron microscopy (EM), an enzyme-linked immunosorbent assay (ELISA) specific for Grimsby virus (GRV) capsid antigen and/or by reverse transcriptase-polymerase chain reaction (RT-PCR) for NV, allowing the utility of each assay for routine diagnosis to be assessed. Preliminary genomic characterisation of detected strains was performed using the heteroduplex mobility assay (HMA) and DNA sequencing. The results demonstrate the continuing predominance of GII-4 GRV strain of NV as a cause of outbreaks, particularly in hospital and nursing home settings. Overall, NV were detected in 223/407 (55%) of outbreaks tested. However, a wide range of apparently diverse strains was identified, including several not previously reported. Genomic characterisation revealed clusters of linked outbreaks not recognised previously., (Copyright 2004 Wiley-Liss, Inc.)

Published

2004

36. Asymptomatic and symptomatic excretion of noroviruses during a hospital outbreak of gastroenteritis.

Author

Gallimore CI, Cubitt D, du Plessis N, and Gray JJ

Subjects

Carrier State epidemiology, Carrier State virology, DNA, Viral genetics, Genes, Viral, Humans, London epidemiology, Personnel, Hospital, Phylogeny, Polymerase Chain Reaction, Caliciviridae Infections epidemiology, Caliciviridae Infections virology, Cross Infection epidemiology, Cross Infection virology, Disease Outbreaks, Gastroenteritis epidemiology, Gastroenteritis virology, Norovirus classification, Norovirus genetics, Norovirus isolation & purification

Abstract

During an investigation of a hospital outbreak of norovirus gastroenteritis identified as being caused by a recombinant genogroup II (rGII-3a) strain, fecal specimens collected from asymptomatic staff and patients were tested by nested PCR. A GII-4 norovirus strain, the predominant strain associated with outbreaks in hospitals over the last few years, was detected in 26 and 33% of asymptomatic staff and patients, respectively. No rGII-3a (Harrow/Mexico) norovirus strains were detected in the samples of asymptomatic staff or patients.

Published

2004

37. Quantitation of group A rotavirus by real-time reverse-transcription-polymerase chain reaction: correlation with clinical severity in children in South India.

Author

Kang G, Iturriza-Gomara M, Wheeler JG, Crystal P, Monica B, Ramani S, Primrose B, Moses PD, Gallimore CI, Brown DW, and Gray J

Subjects

Base Sequence, DNA, Viral genetics, Gastroenteritis epidemiology, Gastroenteritis virology, Humans, Immunoenzyme Techniques, India epidemiology, Infant, Reverse Transcriptase Polymerase Chain Reaction, Rotavirus isolation & purification, Rotavirus pathogenicity, Rotavirus Infections epidemiology, Virulence genetics, Rotavirus classification, Rotavirus genetics, Rotavirus Infections virology

Abstract

The epidemiology and pathogenesis of rotaviruses are not completely understood, although recent developments in polymerase chain reaction (PCR) techniques now make it possible to quantify the viral load during an infective episode and investigate its relevance to clinical features of the disease. We studied rotavirus-positive stool samples collected from 10 children without symptoms of gastroenteritis and from 81 children with acute gastroenteritis and in whom the clinical severity of disease was recorded. A semi-quantitative real-time reverse-transcription (RT)-PCR was used to estimate the rotavirus load and to assess its correlation with the Vesikari score for severity of diarrhoea. There was a significant negative correlation (r = -0.80, P < 0.001) between severity and the PCR cycle at which the PCR amplicons were detectable (crossing point) on the assay, indicating that children with more severe diarrhoea excrete more virus than children with less severe disease., (Copyright 2004 Wiley-Liss, Inc.)

Published

2004

38. Diversity of noroviruses cocirculating in the north of England from 1998 to 2001.

Author

Gallimore CI, Green J, Lewis D, Richards AF, Lopman BA, Hale AD, Eglin R, Gray JJ, and Brown DW

Subjects

Caliciviridae Infections virology, Enzyme-Linked Immunosorbent Assay, Gastroenteritis virology, Heteroduplex Analysis, Hospitals, Humans, Microscopy, Electron, Norovirus genetics, Norovirus isolation & purification, Nursing Homes, Prevalence, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, DNA, United Kingdom epidemiology, Caliciviridae Infections epidemiology, Disease Outbreaks, Gastroenteritis epidemiology, Genetic Variation, Norovirus classification

Abstract

A study was undertaken to investigate the diversity of noroviruses (NVs) in fecal samples from patients from 529 outbreaks and 141 sporadic cases of gastroenteritis in the North of England from September 1998 to August 2001. NV strains were detected by electron microscopy and characterized by a combination of the Grimsby virus antigen enzyme-linked immunosorbent assay, reverse transcriptase PCR, the heteroduplex mobility assay, and DNA sequencing. Twenty-one distinct NV strains, including several novel or variant strains not seen previously, were found circulating in the population studied. Genogroup II NVs were responsible for 83% of the outbreaks. Several strains cocirculated at any one time. The Bristol (Grimsby/Lordsdale) and Hawaii (Girlington) genotypes were the most prevalent among the NVs identified, detected in 49 and 20% of the outbreaks, respectively. A limited number of other genogroup II and I strains were cocirculating. The virus populations detected in hospitals and nursing homes were distinct from those found in community-based outbreaks. Outbreaks in hospitals and nursing homes were more likely to be caused by genogroup II strain Grimsby or Girlington (P < 0.0001) than by other genogroup II or I strains.

Published

2004

39. Evidence for genetic linkage between the gene segments encoding NSP4 and VP6 proteins in common and reassortant human rotavirus strains.

Author

Iturriza-Gòmara M, Anderton E, Kang G, Gallimore C, Phillips W, Desselberger U, and Gray J

Subjects

Animals, DNA, Viral genetics, DNA, Viral isolation & purification, Genetic Linkage, Genotype, Humans, Phylogeny, Rotavirus classification, Rotavirus isolation & purification, Toxins, Biological, Antigens, Viral, Capsid Proteins genetics, Glycoproteins genetics, Rotavirus genetics, Rotavirus Infections genetics, Viral Nonstructural Proteins genetics

Abstract

NSP4-encoding genes of 78 human rotavirus strains of common or reassortant genotypes were characterized by reverse transcription-PCR followed by sequencing and phylogenetic analysis. It was found that all the human strains characterized clustered into only two of the five known NSP4 genotypes. Linkage between NSP4 genotypes and VP6 subgroups was 100%, NSP4 genotype A being linked to VP6 of subgroup I (SGI) and NSP4 of genotype B being linked to VP6 of SGII. The diversity among the NSP4- and VP6-encoding genes was significantly less than that among the VP7 and VP4 genes in cocirculating human rotavirus strains. Whereas G and P types appear to be shared among different animal species and humans, the NSP4- and VP6-encoding genes appear to segregate according to their host of origin, suggesting that these two proteins may be host restriction determinants. The NSP4-VP6 association may be structurally determined during rotavirus replication (morphogenesis).

Published

2003

40. A summertime peak of "winter vomiting disease": surveillance of noroviruses in England and Wales, 1995 to 2002.

Author

Lopman BA, Reacher M, Gallimore C, Adak GK, Gray JJ, and Brown DW

Subjects

Adolescent, Adult, Age Distribution, Aged, Caliciviridae Infections diagnosis, Child, Child, Preschool, England epidemiology, Enzyme-Linked Immunosorbent Assay, Gastroenteritis diagnosis, Gastroenteritis virology, Humans, Infant, Infant, Newborn, Infection Control, Microscopy, Electron, Middle Aged, Norovirus pathogenicity, Population Surveillance, Reverse Transcriptase Polymerase Chain Reaction, Wales epidemiology, Caliciviridae Infections epidemiology, Disease Outbreaks, Gastroenteritis epidemiology, Norovirus isolation & purification, Seasons

Abstract

Background: Noroviruses are the most common cause of gastroenteritis outbreaks in industrialised countries. Gastroenteritis caused by Norovirus infection has been described as a highly seasonal syndrome, often referred to as "winter vomiting disease"., Methods: The Public Health Laboratory Service Communicable Disease Surveillance Centre has systematically collected reports of laboratory confirmed cases of Norovirus-gastroenteritis since 1995. We analysed these data for annual and seasonal trends and age distribution., Results: A mid-summer peak in reported cases of Norovirus was observed in 2002, unlike all six previous years when there was a marked summer decline. Total reports from 2002 have also been higher than all previous years. From the first 10 months of 2002, a total of 3029 Norovirus diagnoses were reported compared the previous peak in 1996 of 2437 diagnoses for the whole 12-month period. The increase in 2002 was most marked in the 65 and older age group., Conclusion: This surveillance data challenges the view that Noroviruses infections exclusively have wintertime seasonality.

Published

2003

41. Molecular epidemiological analysis of Cryptosporidium isolates from humans and animals by using a heteroduplex mobility assay and nucleic acid sequencing based on a small double-stranded RNA element.

Author

Leoni F, Gallimore CI, Green J, and McLauchlin J

Subjects

Animals, Base Sequence, Cryptosporidiosis veterinary, Cryptosporidium isolation & purification, Heteroduplex Analysis methods, Humans, Molecular Sequence Data, Mutation, RNA, Protozoan analysis, Sequence Homology, Nucleic Acid, Animal Diseases epidemiology, Cryptosporidiosis epidemiology, Cryptosporidium genetics, Disease Outbreaks, Molecular Epidemiology, RNA, Double-Stranded analysis

Abstract

Two extrachromosomal double-stranded RNA (dsRNA) elements occur in Cryptosporidium parvum. A heteroduplex mobility assay (HMA) was developed for the rapid characterization of sequence diversity in a 173-bp fragment of the small dsRNA element of Cryptosporidium with either a natural sequence from Cryptosporidium meleagridis or a synthetic sequence as reference DNA. The 173-bp fragment was generated from 265 samples of whole feces (242 from humans and 18 from livestock with C. parvum genotype 1 or 2, 4 from humans with Cryptosporidium felis, and 1 from a human with C. meleagridis). The HMA method identified 21 patterns in C. parvum (8 in genotype 1, 12 in genotype 2, and a type common to both genotypes), 4 patterns in C. felis, and 1 pattern in C. meleagridis. All patterns were confirmed as distinct by DNA sequencing. For genotype 1, a single HMA type was found in 89% of samples: 64 of 65 cases from three waterborne outbreaks, all 16 cases from eight intrafamilial outbreaks, and 17 of 28 sporadic cases. Among the remaining 11 sporadic cases due to genotype 1, seven other HMA types were detected. For genotype 2, a single HMA type was found in 72% of samples: 36 of 43 cases from three waterborne outbreaks, 11 of 15 cases from seven intrafamilial outbreaks, 44 of 75 sporadic cases, and all 18 samples from livestock. Within the intrafamilial outbreaks, two other HMA types were identified: the same HMA type was detected in samples from cases within the same outbreak. Among the sporadic cases due to genotype 2, 10 additional HMA types were detected.

Published

2003