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1. Investigating One Health risks for human colonisation with extended spectrum β-lactamase-producing Escherichia coli and Klebsiella pneumoniae in Malawian households: a longitudinal cohort study

Author

Cocker, Derek, Chidziwisano, Kondwani, Mphasa, Madalitso, Mwapasa, Taonga, Lewis, Joseph M, Rowlingson, Barry, Sammarro, Melodie, Bakali, Winnie, Salifu, Chifundo, Zuza, Allan, Charles, Mary, Mandula, Tamandani, Maiden, Victor, Amos, Stevie, Jacob, Shevin T, Kajumbula, Henry, Mugisha, Lawrence, Musoke, David, Byrne, Rachel, Edwards, Thomas, Lester, Rebecca, Elviss, Nicola, Roberts, Adam P, Singer, Andrew C, Jewell, Christopher, Morse, Tracy, and Feasey, Nicholas A

Published
2023
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2. Environmental surveillance for Salmonella Typhi in rivers and wastewater from an informal sewage network in Blantyre, Malawi.

Author

Uzzell, Christopher B., Gray, Elizabeth, Rigby, Jonathan, Troman, Catherine M., Diness, Yohane, Mkwanda, Charity, Tonthola, Katalina, Kanjerwa, Oscar, Salifu, Chifundo, Nyirenda, Tonney, Chilupsya, Chisomo, Msefula, Chisomo, Elviss, Nicola, Grassly, Nicholas C., and Feasey, Nicholas A.

Subjects
SALMONELLA typhi, PUBLIC health, MIXED-use developments, RIVER channels, WATERSHEDS, TYPHOID fever
Abstract

Environmental surveillance for Salmonella Typhi may provide information on the community-level dynamics of typhoid fever in resource poor regions experiencing high disease burden. Many knowledge gaps concerning the feasibility of ES remain, especially in areas lacking formal sewage systems. We implemented protocols for S. Typhi ES, including site selection and catchment population estimation, sample concentration and testing using qPCR for S. Typhi specific gene targets. Between May 2021 and May 2022, we collected grab samples and Moore swabs from 43 sites in Blantyre, Malawi. Catchment characteristics, water quality, and human faecal contamination (qPCR for Bacteroides HF183) were also recorded. Their association with S. Typhi detection was investigated using a logistic mixed-effects regression analysis. Prevalence of S. Typhi in ES samples was 2.1% (1.1–4.0%) and 3.9% (1.9–7.9%) for grab and Moore swab samples, respectively. HF183 was associated S. Typhi positivity, with a unit increase in log genome copies/microlitre increasing the odds of detection of S. Typhi by 1.56 (95% CI: 1.29–1.89) and 1.33 (1.10–1.61) in Moore swabs and grab samples, respectively. The location and timing of S. Typhi detection through ES was not associated with the incidence of typhoid fever reported in associated catchment populations. During this period of relatively low typhoid fever incidence, wastewater surveillance continued to detect S. Typhi in human sewage and wastewater suggesting that ES using natural river systems can be a sensitive indicator of transmission. Author summary: Typhoid fever is a major public health concern throughout many low- and middle-income countries, resulting in significant morbidity and mortality. In recent years, two typhoid-conjugate vaccines have been pre-qualified, with the World Health Organization recommending their targeted use in high incidence, endemic regions. However, quality assured information on the spatio-temporal distribution of typhoid fever is lacking, and scale-up of typhoid vaccination is progressing slowly. Environmental surveillance for Salmonella Typhi in sewage and wastewater may be a cost-effective and scalable approach to identify high-burden regions, thereby motivating vaccine introduction. However, many knowledge gaps regarding the use of environmental surveillance for Salmonella Typhi remain, particularly where human wastewater is unmanaged and its disposal reliant on informal drainage channels and natural river systems. Therefore, we conducted a study in Malawi, Blantyre to ascertain the feasibility of environmental surveillance throughout an urban, natural freshwater river system. We measured S. Typhi prevalence in wastewater contaminated rivers and ditches serving a mixed land use environment with diverse population densities. Whilst detection rates of S. Typhi were relatively low, and no obvious spatial pattern of distribution was observed, this study demonstrates that the presence of S. Typhi throughout the year. It suggests that wastewater testing for S. Typhi may offer a sensitive surveillance tool that complements clinical case reporting and may help identify areas to be prioritized for vaccination rollout. [ABSTRACT FROM AUTHOR]

Published
2024
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3. Salmonella carriage by geckos detected within households in Malawi

Author

Wilson, Catherine N., Musicha, Patrick, Beale, Mathew A., Diness, Yohane, Kanjerwa, Oscar, Salifu, Chifundo, Katuah, Zefaniah, Duncan, Patricia, Nyangu, John, Mungu, Andrew, Deleza, Muonaouza, Banda, Lawrence, Makhaza, Lumbani, Elviss, Nicola, Jewell, Christopher P., Pinchbeck, Gina, Thomson, Nicholas R., Feasey, Nicholas A., and Fèvre, Eric M.

Published
2024
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4. Development and application of Helicobacter pylori surveillance to improve antimicrobial treatment

Author

Elviss, Nicola Clare

Subjects
616.33014, QD Chemistry
Abstract

The determination of H. pylori in vitro antibiotic susceptibility to the four key antibiotics and the underlying mechanisms of resistance were investigated. Levels of antibiotic resistance in two independent populations in England and Wales were determined. In the urban London-based population, metronidazole resistance was present in 59% and clarithromycin resistance was in 11% of the 101 H. pylori isolates. Of 363 isolates from rural Bangor, North Wales, 23% were metronidazole resistant and 7% were clarithromycin resistant. Combined clarithromycin and metronidazole resistance occurred in 9% of London and in 4% from Bangor isolates. Analysis of patient questionnaires completed at the London centres identified a significant association between metronidazole resistance and birth outside the UK. Analysis of the method used to determine metronidazole susceptibility status indicated that anaerobic pre-incubation gave results falsely indicating susceptibility. This study would recommend the use of Etest strips on 10% Mueller-Hinton blood agar, incubated microaerophilically at 37°C for 48 h. Comparison of detection methods for 23Sr rDNA mutations associated with H. pylori clarithromycin resistance showed a novel 3’-mismatched reverse primer PCR to be the most sensitive approach. Sequence analysis of 16S rDNA in tetracycline resistant isolates identified the A926g mutation for the first time from a UK H. pylori isolate and a novel A926C mutation. The mechanism of unstable amoxicillin resistance was investigated. Novel PCR-RFLP assays, exploiting sequence variability in the outer membrane protein genes hopB and hopC, indicated no association with antibiotic resistance, but have potential for use as a novel genotyping tool for H. pylori. This study highlights the need for H. pylori antibiotic resistance surveillance at the regional level to help guide treatment regimens.

Published
2005

5. Drivers of Resistance in Uganda and Malawi (DRUM): a protocol for the evaluation of One-Health drivers of Extended Spectrum Beta Lactamase (ESBL) resistance in Low-Middle Income Countries (LMICs)

Author

Cocker, Derek, primary, Sammarro, Melodie, additional, Chidziwisano, Kondwani, additional, Elviss, Nicola, additional, Jacob, Shevin T., additional, Kajumbula, Henry, additional, Mugisha, Lawrence, additional, Musoke, David, additional, Musicha, Patrick, additional, Roberts, Adam P., additional, Rowlingson, Barry, additional, Singer, Andrew C., additional, Byrne, Rachel L., additional, Edwards, Thomas, additional, Lester, Rebecca, additional, Wilson, Catherine N., additional, Hollihead, Beth, additional, Thomson, Nicholas, additional, Jewell, Christopher P., additional, Morse, Tracy, additional, and Feasey, Nicholas A., additional

Published
2023
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6. Drivers of resistance in Uganda and Malawi (DRUM): a protocol for the evaluation of One-Health drivers of extended spectrum beta lactamase (ESBL) resistance in low-middle income countries (LMICs)

Author

Cocker, Derek, Sammarro, Melodie, Chidziwisano, Kondwani, Elviss, Nicola, Jacob, Shevin T., Kajumbula, Henry, Mugisha, Lawrence, Musoke, David, Musicha, Patrick, Roberts, Adam P., Rowlingson, Barry, Singer, Andrew C., Byrne, Rachel L., Edwards, Thomas, Lester, Rebecca, Wilson, Catherine N., Hollihead, Beth, Thomson, Nicholas R., Jewell, Christopher P., Morse, Tracy, Feasey, Nicholas A., Cocker, Derek, Sammarro, Melodie, Chidziwisano, Kondwani, Elviss, Nicola, Jacob, Shevin T., Kajumbula, Henry, Mugisha, Lawrence, Musoke, David, Musicha, Patrick, Roberts, Adam P., Rowlingson, Barry, Singer, Andrew C., Byrne, Rachel L., Edwards, Thomas, Lester, Rebecca, Wilson, Catherine N., Hollihead, Beth, Thomson, Nicholas R., Jewell, Christopher P., Morse, Tracy, and Feasey, Nicholas A.

Abstract

In sub-Saharan Africa (sSA), there is high morbidity and mortality from severe bacterial infection and this is compounded by antimicrobial resistance, in particular, resistance to 3rd-generation cephalosporins. This resistance is typically mediated by extended-spectrum beta lactamases (ESBLs). To interrupt ESBL transmission it will be important to investigate how human behaviour, water, sanitation, and hygiene (WASH) practices, environmental contamination, and antibiotic usage in both urban and rural settings interact to contribute to transmission of ESBL E. coli and ESBL K. pneumoniae between humans, animals, and the environment. Here we present the protocol for the Drivers of Resistance in Uganda and Malawi (DRUM) Consortium, in which we will collect demographic, geospatial, clinical, animal husbandry and WASH data from a total of 400 households in Uganda and Malawi. Longitudinal human, animal and environmental sampling at each household will be used to isolate ESBL E. coli and ESBL K. pneumoniae. This will be complimented by a Risks, Attitudes, Norms, Abilities and Self-Regulation (RANAS) survey and structured observations to understand the contextual and psychosocial drivers of regional WASH practices. Bacterial isolates and plate sweeps will be further characterised using a mixture of short-,long-read and metagenomic whole-genome sequencing. These datasets will be integrated into agent-based models to describe the transmission of EBSL resistance in Uganda and Malawi and allow us to inform the design of interventions for interrupting transmission of ESBL-bacteria.

Published
2023

7. Environmental surveillance for Salmonella Typhi as a tool to estimate the incidence of typhoid fever in low-income populations.

Author

Uzzell, Christopher B., primary, Troman, Catherine M., additional, Rigby, Jonathan, additional, Raghava Mohan, Venkata, additional, John, Jacob, additional, Abraham, Dilip, additional, Srinivasan, Rajan, additional, Nair, Satheesh, additional, Meschke, John Scott, additional, Elviss, Nicola, additional, Kang, Gagandeep, additional, Feasey, Nicholas A., additional, and Grassly, Nicholas C., additional

Published
2023
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8. Norovirus attribution study: Detection of norovirus from the commercial food preparation environment in outbreak and non-outbreak premises

Author

Elviss, Nicola C, Allen, David J, Kelly, Daniel, Akello, Joyce Odeke, Hau, Sarah, Fox, Andrew J, Hopkins, Mark, Derrick, Jade, O'Brien, Sarah, Iturriza-Gomara, Miren, and Conducted as part of NoVAS

Abstract

AIMS: Norovirus remains the most significant virological risk that is transmitted via food and the environment to cause acute gastroenteritis. This study aimed to investigate the hypothesis that the contamination of the commercial food production environment with norovirus will be higher in premises that have recently reported a foodborne norovirus outbreak than those that have not. METHODS: Sampling of commercial food production environments was carried out across a 16-month period between January 2015 and April 2016 in the South East and the North West of England by local authority environmental health departments as part of routine surveillance visits to premises. A total of 2982 samples, 2038 virological and 944 bacteriological, were collected from 256 premises. Sixteen of these premises, six from South East and ten from North West England, were sampled as part of a public health outbreak investigation. RESULTS & CONCLUSIONS: Overall, 2038 swabs were submitted for norovirus testing, with an average of eight swabs per premises (range 4 to 23) and a median of seven. Of the premises sampled, 11.7% (30/256) yielded at least one norovirus-positive sample (environmental, and/or food handler hand swab), and 2.5% of the swabs were positive for norovirus. A peak in the positivity rate was seen in the South East in April 2016. No associations were found between norovirus positivity and bacteriology indicators, or between bacteriology indicators and hygiene ratings. SIGNIFICANCE AND IMPACT OF STUDY: This study demonstrates that food premises and food handlers remain a potential source of norovirus transmission and outbreaks.

Published
2022

9. Drivers of resistance in Uganda and Malawi (DRUM): a protocol for the evaluation of One-Health drivers of extended spectrum beta lactamase (ESBL) resistance in low-middle income countries (LMICs)

Author

Cocker, Derek, Sammarro, Melodie, Chidziwisano, Kondwani, Elviss, Nicola, Jacob, Shevin T., Kajumbula, Henry, Mugisha, Lawrence, Musoke, David, Musicha, Patrick, Roberts, Adam P., Rowlingson, Barry, Singer, Andrew C., Byrne, Rachel L., Edwards, Thomas, Lester, Rebecca, Wilson, Catherine N., Hollihead, Beth, Thomson, Nicholas, Jewell, Christopher P., Morse, Tracy, Feasey, Nicholas, Cocker, Derek, Sammarro, Melodie, Chidziwisano, Kondwani, Elviss, Nicola, Jacob, Shevin T., Kajumbula, Henry, Mugisha, Lawrence, Musoke, David, Musicha, Patrick, Roberts, Adam P., Rowlingson, Barry, Singer, Andrew C., Byrne, Rachel L., Edwards, Thomas, Lester, Rebecca, Wilson, Catherine N., Hollihead, Beth, Thomson, Nicholas, Jewell, Christopher P., Morse, Tracy, and Feasey, Nicholas

Abstract

In sub-Saharan Africa (sSA), there is high morbidity and mortality from severe bacterial infection and this is compounded by antimicrobial resistance, in particular, resistance to 3rd-generation cephalosporins. This resistance is typically mediated by extended-spectrum beta lactamases (ESBLs). To interrupt ESBL transmission it will be important to investigate how human behaviour, water, sanitation, and hygiene (WASH) practices, environmental contamination, and antibiotic usage in both urban and rural settings interact to contribute to transmission of ESBL E. coli and ESBL K. pneumoniae between humans, animals, and the environment. Here we present the protocol for the Drivers of Resistance in Uganda and Malawi (DRUM) Consortium, in which we will collect demographic, geospatial, clinical, animal husbandry and WASH data from a total of 400 households in Uganda and Malawi. Longitudinal human, animal and environmental sampling at each household will be used to isolate ESBL E. coli and ESBL K. pneumoniae. This will be complimented by a Risks, Attitudes, Norms, Abilities and Self-Regulation (RANAS) survey and structured observations to understand the contextual and psychosocial drivers of regional WASH practices. Bacterial isolates and plate sweeps will be further characterised using a mixture of short-,long-read and metagenomic whole-genome sequencing. These datasets will be integrated into agent-based models to describe the transmission of EBSL resistance in Uganda and Malawi and allow us to inform the design of interventions for interrupting transmission of ESBL-bacteria.

Published
2022

10. Drivers of Resistance in Uganda and Malawi (DRUM):a protocol for the evaluation of One-Health drivers of Extended Spectrum Beta Lactamase (ESBL) resistance in Low-Middle Income Countries (LMICs)

Author

Cocker, Derek, Sammarro, Melodie, Chidziwisano, Kondwani, Elviss, Nicola, Jacob, Shevin T., Kajumbula, Henry, Mugisha, Lawrence, Musoke, David, Musicha, Patrick, Roberts, Adam P., Rowlingson, Barry, Singer, Andrew C., Byrne, Rachel L., Edwards, Thomas, Lester, Rebecca, Wilson, Catherine, Hollihead, Beth, Thomson, Nicholas, Jewell, Christopher P., Morse, Tracy, Feasey, Nicholas, Cocker, Derek, Sammarro, Melodie, Chidziwisano, Kondwani, Elviss, Nicola, Jacob, Shevin T., Kajumbula, Henry, Mugisha, Lawrence, Musoke, David, Musicha, Patrick, Roberts, Adam P., Rowlingson, Barry, Singer, Andrew C., Byrne, Rachel L., Edwards, Thomas, Lester, Rebecca, Wilson, Catherine, Hollihead, Beth, Thomson, Nicholas, Jewell, Christopher P., Morse, Tracy, and Feasey, Nicholas

Abstract

In sub-Saharan Africa (sSA), there is high morbidity and mortality from severe bacterial infection and this is compounded by antimicrobial resistance, in particular, resistance to 3rd-generation cephalosporins. This resistance is typically mediated by extended-spectrum beta lactamases (ESBLs). To interrupt ESBL transmission it will be important to investigate how human behaviour, water, sanitation, and hygiene (WASH) practices, environmental contamination, and antibiotic usage in both urban and rural settings interact to contribute to transmission of ESBL E. coli and ESBL K. pneumoniae between humans, animals, and the environment. Here we present the protocol for the Drivers of Resistance in Uganda and Malawi (DRUM) Consortium, in which we will collect demographic, geospatial, clinical, animal husbandry and WASH data from a total of 400 households in Uganda and Malawi. Longitudinal human, animal and environmental sampling at each household will be used to isolate ESBL E. coli and ESBL K. pneumoniae. This will be complimented by a Risks, Attitudes, Norms, Abilities and Self-Regulation (RANAS) survey and structured observations to understand the contextual and psychosocial drivers of regional WASH practices. Bacterial isolates and plate sweeps will be further characterised using a mixture of short-,long-read and metagenomic whole-genome sequencing. These datasets will be integrated into agent-based models to describe the transmission of EBSL resistance in Uganda and Malawi and allow us to inform the design of interventions for interrupting transmission of ESBL-bacteria.

Published
2022

11. Optimised methods for detecting Salmonella Typhi in the environment using validated field sampling, culture, and confirmatory molecular approaches

Author

Rigby, Jonathan, Diness, Yohane, Mkwanda, Charity, Tonthola, Katalina, Galloway, Heather, Miles, Rory, Henrion, Marc, Edwards, Thomas, Gauld, Jillian, Msefula, Chisomo, Johnston, Rob, Nair, Satheesh, Feasey, Nicholas, and Elviss, Nicola

Subjects
wa_675, wc_270, wa_395, wc_269, qw_55
Abstract

Aims\ud This study evaluated detection methods for Salmonella Typhi (S. Typhi) in the environment, to establish a novel pathway from field sampling to isolation of viable organisms and molecular confirmation from complex environmental samples, thus enabling environmental surveillance of typhoid.\ud \ud Methods and Results\ud Multiple media were assessed using clinical isolates from the Public Health England’s (PHE) Culture collection. The culture pathway selected consisted of a primary 2% bile broth and secondary Selenite F broth, followed by modified Chromogenic Agar for Salmonella Esterase (mCASE). A qPCR assay was adapted from a validated S. Typhi PCR panel for confirmation of isolates, with comparison to biochemical and serological tests showing good specificity. Sampling locations in Blantyre, Malawi were used to compare sampling methods. Viable S. Typhi were isolated from a mixture of trap and grab river water samples on six occasions.\ud \ud Conclusions\ud Culture of viable S. Typhi from environmental samples was possible using effective capture and culture techniques.\ud Significance and impact of study\ud \ud Whilst several studies have attempted to detect S. Typhi from the environment, this is the first successful attempt to isolate the organism from river water since the 1980’s. Supplementing clinical data with environmental screening offers the potential for enhanced surveillance, which might inform interventions and assess vaccination programmes.

Published
2022

12. Drivers of Resistance in Uganda and Malawi (DRUM): a protocol for the evaluation of One-Health drivers of Extended Spectrum Beta Lactamase (ESBL) resistance in Low-Middle Income Countries (LMICs)

Author

Cocker, Derek, primary, Sammarro, Melodie, additional, Chidziwisano, Kondwani, additional, Elviss, Nicola, additional, Jacob, Shevin T., additional, Kajumbula, Henry, additional, Mugisha, Lawrence, additional, Musoke, David, additional, Musicha, Patrick, additional, Roberts, Adam P., additional, Rowlingson, Barry, additional, Singer, Andrew C., additional, Byrne, Rachel L., additional, Edwards, Thomas, additional, Lester, Rebecca, additional, Wilson, Catherine N., additional, Hollihead, Beth, additional, Thomson, Nicholas, additional, Jewell, Christopher P., additional, Morse, Tracy, additional, and Feasey, Nicholas A., additional

Published
2022
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14. Utility of Whole Genome Sequencing To Describe the Persistence and Evolution of Listeria monocytogenes Strains within Crabmeat Processing Environments Linked to Two Outbreaks of Listeriosis

Author

Elson, Richard, primary, Awofisayo-Okuyelu, Adedoyin, additional, Greener, Trevor, additional, Swift, Craig, additional, Painset, Anaïs, additional, Amar, Corinne Francoise Laurence, additional, Newton, Autilia, additional, Aird, Heather, additional, Swindlehurst, Mark, additional, Elviss, Nicola, additional, Foster, Kirsty, additional, Dallman, Timothy J., additional, Ruggles, Ruth, additional, and Grant, Kathie, additional

Published
2019
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18. Utility of Whole Genome Sequencing To Describe the Persistence and Evolution of Listeria monocytogenesStrains within Crabmeat Processing Environments Linked to Two Outbreaks of Listeriosis

Author

Elson, Richard, Awofisayo-Okuyelu, Adedoyin, Greener, Trevor, Swift, Craig, Painset, Anaïs, Amar, Corinne Francoise Laurence, Newton, Autilia, Aird, Heather, Swindlehurst, Mark, Elviss, Nicola, Foster, Kirsty, Dallman, Timothy J., Ruggles, Ruth, and Grant, Kathie

Abstract

This article describes the identification and investigation of two extended outbreaks of listeriosis in which crabmeat was identified as the vehicle of infection. Comparing contemporary and retrospective typing data of Listeria monocytogenesisolates from clinical cases and from food and food processing environments allowed the detection of cases going back several years. This information, combined with the analysis of routinely collected enhanced surveillance data, helped to direct the investigation and identify the vehicle of infection. Retrospective whole genome sequencing (WGS) analysis of isolates provided robust microbiological evidence of links between cases, foods, and the environments in which they were produced and demonstrated that for some cases and foods, identified by fluorescent amplified fragment length polymorphism, the molecular typing method in routine use at the time, were not part of the outbreak. WGS analysis also showed that the strains causing illness had persisted in two food production environments for many years and in one producer had evolved into two strains over a period of around 8 years. This article demonstrates the value of reviewing L. monocytogenestyping data from clinical cases together with that from foods as a means of identifying potential vehicles and sources of infection in outbreaks of listeriosis. It illustrates the importance of reviewing retrospective L. monocytogenestyping alongside enhanced surveillance data to characterize extended outbreaks and inform control measures. Also, this article highlights the advantages of WGS analysis for strain discrimination and clarification of evolutionary relationships that refine outbreak investigations and improve our understanding of L. monocytogenesin the food chain.

Published
2019
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19. Public Health Investigation of Two Outbreaks of Shiga Toxin-Producing Escherichia coli O157 Associated with Consumption of Watercress

Author

Jenkins, Claire, primary, Dallman, Timothy J., additional, Launders, Naomi, additional, Willis, Caroline, additional, Byrne, Lisa, additional, Jorgensen, Frieda, additional, Eppinger, Mark, additional, Adak, Goutam K., additional, Aird, Heather, additional, Elviss, Nicola, additional, Grant, Kathie A., additional, Morgan, Dilys, additional, and McLauchlin, Jim, additional

Published
2015
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22. Prevalence and Subtypes of Ciprofloxacin-Resistant Campylobacterspp. in Commercial Poultry Flocks before, during, and after Treatment with Fluoroquinolones

Author

Humphrey, Tom J., Jørgensen, Frieda, Frost, Jennifer A., Wadda, Haddy, Domingue, Gil, Elviss, Nicola C., Griggs, Deborah J., and Piddock, Laura J. V.

Abstract

ABSTRACTFive commercial broiler chicken flocks were treated with either difloxacin or enrofloxacin for a clinically relevant infection, as instructed by a veterinarian. Campylobacters were isolated from individual fecal samples and from samples associated with the broiler environment before, during, and after treatment. Ciprofloxacin-resistant Campylobacter jejuniand/or C. colistrains were detected pretreatment in four flocks, but they constituted a very small proportion of the campylobacters present. When the broilers were treated with a fluoroquinolone, a rapid increase in the proportion of ciprofloxacin-resistant campylobacters was observed. During treatment nearly 100% of campylobacters were resistant, and in some flocks a high proportion of resistant strains persisted for up to 4 weeks after treatment. Prior to treatment a variety of campylobacter subtypes were present. During and after treatment considerable changes in both species and subtype prevalence were observed, but no single fluoroquinolone-resistant clone became dominant. Instead, resistant C. colistrains or a mixture of resistant C. coliand C. jejunistrains became dominant, whereas susceptible C. jejunistrains had usually been dominant prior to treatment. The resistant subtypes which emerged and became dominant were not always the same as those detected pretreatment. The persistence of resistant strains for up to 4 weeks posttreatment has important implications for any strategy designed to avoid the introduction of such strains into the food chain.

Published
2005
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23. Differentiation of Metronidazole-Sensitive and -Resistant Clinical Isolates of Helicobacter pyloriby Immunoblotting with Antisera to the RdxA Protein

Author

Latham, Stephanie R., Owen, Robert J., Elviss, Nicola C., Labigne, Agne`s, and Jenks, Peter J.

Abstract

ABSTRACTAntimicrobial resistance in Helicobacter pyloriis a serious and increasing problem, and the development of rapid, reliable methods for detecting resistance would greatly improve the selection of antibiotics used to treat gastric infection with this organism. We assessed whether detection of the RdxA protein could provide the basis for determining the susceptibility of H. pylorito metronidazole. In order to raise polyclonal antisera to RdxA, we cloned the rdxAgene from H. pyloristrain 26695 into the commercial expression vector pMAL-c2, purified the resultant fusion protein by affinity chromatography, and used this recombinant RdxA preparation to immunize rabbits. We then used this specific anti-RdxA antibody to perform immunoblotting on whole bacterial cell lysates of 17 metronidazole-sensitive and 27 metronidazole-resistant clinical isolates of H. pylori. While a 24-kDa immunoreactive band corresponding to the RdxA protein was observed in all metronidazole-sensitive strains, this band was absent in 25 of 27 resistant isolates. Our results indicate that testing for the absence of the RdxA protein would identify the majority of clinical isolates that will respond poorly to metronidazole-containing eradication regimens and have implications for the development of assays capable of detecting metronidazole resistance in H. pylori.

Published
2001
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24. To develop and optimise methods for the detection and isolation of Salmonella typhi from the environment

Author

Rigby, Jonathan, Feasey, Nicholas, Elviss, Nicola, and Roberts, Adam

Subjects
WC 20 Research (General), WC 269 Salmonella infections, WC 270 Typhoid fever
Abstract

Introduction: Salmonella Typhi is a globally important pathogen that causes Typhoid fever, responsible for an estimated 11.9-26.9 million cases and 129,000-216,510 typhoid-related deaths per year worldwide. Surveillance of clinical disease based on quality assured diagnostic clinical microbiology services is often not performed, making it difficult to understand the true burden of typhoid. Environmental surveillance (ES) has the potential to be a cheaper alternative to clinical surveillance of Typhoid and S. Typhi in endemic settings that does not rely on patients attending hospitals or consenting to research. Between April 2015 and January 2017, 546 culture-confirmed cases were reported at Queen Elizabeth Central Hospital in Malawi, however it is likely that case numbers are under-reported, and ES data can provide supplementary insight for spatially targeted interventions. Methods: A novel culture method for S. Typhi was developed at the UK Health Security Agency in London and optimized in Blantyre, Malawi with environmental samples collected in 2019, including water (via trap and gran methods), sediments, food, and biofilms. The method used two enrichment broths (2% bile, then selenite F broths) before plating onto modified chromogenic agar for Salmonella esterase agar. Isolates were identified by real-time PCR and confirmed by biochemistry and serology. The method was validated and used for city-wide surveillance in Blantyre, Malawi between May 2021 and April 2022, alongside a method proposed by the Bill and Melinda Gates Foundation S. Typhi ES working group. After findings between these two methods, further refinements to the culture pathway were started. Results: The six-month pilot study, from 2019 to 2020, isolated six S. Typhi cultures from three Moore swabs, two water samples, and one biofilm. PCR positivity was confirmed by biochemistry and serology. Non-typhoidal salmonellae (NTS) accounted for 377 isolates, 16 of which amplified staG. Between 2021 and 2022, 33 samples were S. Typhi positive and 80 positives for NTS by direct PCR detection only, with two S. Typhi and 255 NTS positive isolates cultured. An alternative extraction method for PCR was shown to have good performance under laboratory conditions, but the inclusion of antimicrobial-containing broths required further development. Conclusion: This work demonstrates that ES of Typhoid by culture is achievable in low- and middle-income countries. Moore swabs yielded a higher detection rate than water samples. Direct detection by PCR appeared to be more sensitive than culture, but still had a low positivity rate. This low positivity rate coincided with the lowest rates of blood culture positivity in a decade and the SARS-CoV-2 pandemic. Work to integrate a PCR screening tool before culture is ongoing but shows potential viability.

Published
2022

25. The development of viral capture, concentration and molecular detection method for norovirus in foods to establish the risk to public health

Author

Derrick, Jade, Iturriza-Gomara, Miren, Elviss, Nicola, and Allen, David

Subjects
579.2
Abstract

Norovirus has been identified as a common cause of gastroenteritis worldwide, and food as a transmission vehicle has been well documented. Standardised detection methods exist for the detection of norovirus from fresh produce and molluscan bivalves, whilst detection methods for a wider range of food matrices that may be implicated in transmission of norovirus do not currently exist. The detection of norovirus in foods suspected to be implicated in transmission is paramount for appropriate outbreak investigation. The contamination of foods other than shellfish and fresh produce often occurs via food handlers. The proportion of norovirus that is typically transferred from food handlers to food also remains unknown. Understanding this is necessary in order to estimate the risk of infection and the burden of gastroenteritis caused by norovirus that is attributable to food contaminated by food handlers. These questions were addressed by the development of a combined capture, concentration and quantitative detection protocol with the aim to enhanced norovirus recovery from a range of food types. A food surface wash and norovirus capture method that was sensitive, reduced processing time, and increased throughput capacity was applied to a range of ready to eat foods. An automated nucleic acid extraction method which further reduced processing time and increased throughput was validated. Finally the validated method demonstrated that two real time RT-PCR assays currently used for the detection of norovirus in shellfish and fresh produce or in faecal samples were comparable overall, and hence either could be used in combination with the norovirus capture, concentration and extraction protocol described in this thesis. The protocol was applied to a range of food matrices and resulted in < 1% to 55% recovery of norovirus GI and < 1% to 25% recovery of norovirus GII. The optimised protocol was then used to quantify virus transfer between food handlers hands and to food, in simulation experiments where food handlers’ gloved hands were artificially contaminated prior to preparation of a sandwich. This enabled norovirus transfer to food items and to other food handlers to be measured at each stage. Quantitative data demonstrated that 5.9 ± (SD ± 0.1) log10 cDNA copies/μl of norovirus GII inoculum, resulted in a percentage recovery of between 3.0% and 0.02% from Food Handlers and 7.8 ± (SD ± 0.1) log10 cDNA copies/μl of norovirus GI inoculum resulted in a percentage recovery between 9.6% and 0.004% from Food Handlers. The average percentage recovered from sandwich pieces over six replicates was 0.2% for norovirus GII and 1.2% for norovirus GI. The method and protocols developed could be rolled out to official control laboratories and aid foodborne outbreak investigation by allowing testing of food categories that currently are not investigated. Furthermore, this work demonstrated the extent of norovirus transfer from hands to food ingredients and the environment and could be used in risk assessment models. Further work applying these protocols to quantify the transfer from contaminated hands using a range of viral loads will be useful in determining risk more accurately, and to monitor and investigate food premises by introducing this as an additional food and hand hygiene marker.

Published
2018
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26. The development of viral capture, concentration and molecular detection method for norovirus in foods to establish the risk to public health

Author

Derrick, Jade, Iturriza-Gomara, Miren, Elviss, Nicola, and Allen, David

Subjects
fluids and secretions, viruses, digestive, oral, and skin physiology, virus diseases
Abstract

Norovirus has been identified as a common cause of gastroenteritis worldwide, and food as a transmission vehicle has been well documented. Standardised detection methods exist for the detection of norovirus from fresh produce and molluscan bivalves, whilst detection methods for a wider range of food matrices that may be implicated in transmission of norovirus do not currently exist. The detection of norovirus in foods suspected to be implicated in transmission is paramount for appropriate outbreak investigation. The contamination of foods other than shellfish and fresh produce often occurs via food handlers. The proportion of norovirus that is typically transferred from food handlers to food also remains unknown. Understanding this is necessary in order to estimate the risk of infection and the burden of gastroenteritis caused by norovirus that is attributable to food contaminated by food handlers. These questions were addressed by the development of a combined capture, concentration and quantitative detection protocol with the aim to enhanced norovirus recovery from a range of food types. A food surface wash and norovirus capture method that was sensitive, reduced processing time, and increased throughput capacity was applied to a range of ready to eat foods. An automated nucleic acid extraction method which further reduced processing time and increased throughput was validated. Finally the validated method demonstrated that two real time RT-PCR assays currently used for the detection of norovirus in shellfish and fresh produce or in faecal samples were comparable overall, and hence either could be used in combination with the norovirus capture, concentration and extraction protocol described in this thesis. The protocol was applied to a range of food matrices and resulted in

27. Microbiological Quality of Cooked Chicken: Results of Monitoring in England (2013-17).

Author

McLauchlin J, Aird H, Charlett A, Elviss N, Jorgensen F, and Willis C

Abstract

Results from monitoring of the microbiological quality of 2,721 samples of ready-to-eat cooked chicken collected between 2013 to 2017 in England were reviewed: 70% of samples were from retail, catering or manufacture and 30% were imported and collected at English ports. Samples were tested for a range of bacterial pathogens and indicator organisms. Six samples (<1%) had unsatisfactory levels of pathogens which were potentially injurious to health. Neither Salmonella nor Campylobacter were recovered from any sample. Two samples from catering settings contained either an unsatisfactory level of Bacillus cereus (5 x 10 6 CFU/g) or an unsatisfactory level of coagulase positive staphylococci (1.6 x 10 4 CFU/g). Listeria monocytogenes was recovered from 36 samples (one at manufacture, 26 at catering and nine at retail) and in four instances, unsatisfactory levels (≥10 2 CFU/g) were detected (three samples collected at catering and one at retail). For L. monocytogenes there were no significant differences between the rates of contamination with between the samples collected from ports, manufacture, retail supermarkets and other retailers (p = 0.288). There were no differences between the rates of contamination for other potential pathogens detected between samples from different settings. The prevalence of hygiene indicators ( Escherichia coli , Enterobacteriaceae and Aerobic Colony Counts) at import was significantly lower than in samples collected from manufacturers, retail or catering (p < 0.01). Samples collected from catering gave poorer results than all other settings. Regardless of the stage in the food chain, samples from Thailand and from other non-EU countries were of significantly better microbiological quality with respect to indicator organisms than those from the UK or from other EU countries (p = <0.001)., (Copyright © 2020 International Association for Food Protection. Published by Elsevier Inc. All rights reserved)

Published
2020
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28. National outbreak of Pseudomonas aeruginosa associated with an aftercare solution following piercings, July to September 2016, England.

Author

Evans H, Bolt H, Heinsbroek E, Lloyd B, English P, Latif S, Elviss N, Turton J, Hoffman P, Crook P, and Puleston R

Subjects
Adolescent, Adult, Aftercare, Cohort Studies, England epidemiology, Female, Humans, Minisatellite Repeats, Pseudomonas Infections diagnosis, Pseudomonas Infections microbiology, Pseudomonas Infections therapy, Pseudomonas aeruginosa isolation & purification, Retrospective Studies, Wound Infection complications, Wound Infection therapy, Young Adult, Body Piercing adverse effects, Disease Outbreaks, Pseudomonas Infections epidemiology, Pseudomonas aeruginosa genetics, Wound Infection microbiology
Abstract

We report a national Pseudomonas aeruginosa outbreak from a common source following piercings between July and September 2016 in England. The multi-agency outbreak investigation included active case finding, microbiological testing of environmental samples and case specimens including Variable Number Tandem Repeat (VNTR) typing and a retrospective cohort study. Overall, 162 outbreak cases (29 confirmed, 14 probable and 119 possible) and 14 non-outbreak cases were identified; all confirmed cases had ear piercings (93% cartilage). Outbreak cases were predominantly female (95%) and had a median age of 18 years (interquartile range: 13-56 years). Nineteen outbreak cases required surgery under general anaesthetic The same outbreak VNTR type (11,3,5,3,3,3,6,4,7) was isolated from bottles of an aftercare solution from a single manufacturer and in specimens from confirmed cases who attended eight different piercing studios supplied with this product. In the cohort study, use of aftercare solution was associated with becoming a case (aOR: 4.60, 95% confidence interval: 1.65-12.90). Environmental, microbiological and epidemiological investigations confirmed that contamination during production of aftercare solution was the source of this national outbreak; highlighting challenges in the regulation of a cosmetic products used in the piercing industry and that guidance on piercing aftercare may need to be reviewed.

Published
2018
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