Your search keyword '"Monroe SS"' showing total 144 results

1. Limited variation in SARS coronavirus S and N protein genes observed by direct sequencing from patient's original clinical specimens

Author

Tong, S, Lingappa, JR, Chen, Q, Shu, B, Lamonte, AC, Cook, BT, Birge, C, Chern, SWW, Liu, X, Galloway, R, Mai, LQ, Ng, WF, Yang, JY, Butany, J, Comer, JA, Monroe, SS, Beard, RS, Ksiazek, TG, Erdman, D, Rota, PA, Pallansch, MA, and Anderson, LJ

Subjects

ddc: 610

Published

2004

2. Outbreak of norovirus illness associated with a swimming pool.

Author

Podewils LJ, Zanardi Blevins L, Hagenbuch M, Itani D, Burns A, Otto C, Blanton L, Adams S, Monroe SS, Beach MJ, and Widdowson M

Abstract

On 3 February 2004, the Vermont Department of Health received reports of acute gastroenteritis in persons who had recently visited a swimming facility. A retrospective cohort study was conducted among persons attending the facility between 30 January and 2 February. Fifty-three of 189 (28%) persons interviewed developed vomiting or diarrhoea within 72 h after visiting the facility. Five specimens tested positive for norovirus and three specimen sequences were identical. Entering the smaller of the two pools at the facility was significantly associated with illness (RR 5.67, 95% CI 1.5-22.0, P=0.012). The investigation identified several maintenance system failures: chlorine equipment failure, poorly trained operators, inadequate maintenance checks, failure to alert management, and insufficient record keeping. This study demonstrates the vulnerability of recreational water to norovirus contamination, even in the absence of any obvious vomiting or faecal accident. Our findings also suggest that norovirus is not as resistant to chlorine as previously reported in experimental studies. Appropriate regulations and enforcement, with adequate staff training, are necessary to ensure recreational water safety. [ABSTRACT FROM AUTHOR]

Published

2007

3. Outbreaks of acute gastroenteritis on cruise ships and on land: identification of a predominant circulating strain of norovirus -- United States, 2002.

Author

Widdowson M, Cramer EH, Hadley L, Bresee JS, Beard RS, Bulens SN, Charles M, Chege W, Isakbaeva E, Wright JG, Mintz E, Forney D, Massey J, Glass RI, and Monroe SS

Abstract

In 2002, a sharp increase in outbreaks of norovirus-associated illness, both on cruise ships and on land, encouraged us to examine the molecular epidemiology of detected noroviruses, to identify a common strain or source. Of 14 laboratory-confirmed outbreaks on cruise ships, 12 (86%) were attributed to caliciviruses; among these 12, outbreak characteristics included continuation on successive cruises in 6 (50%), multiple modes of transmission in 7 (58%), and high (>10%) attack rates in 7 (58%). Eleven of the 12 calicivirus outbreaks were attributed to noroviruses, 7 (64%) of which were attributed to a previously unreported lineage, provisionally named 'the Farmington Hills strain.' From May 2002 to December 2002, 10 (45%) of 22 land-based outbreaks also were attributed to this strain. Nucleotide-sequence analysis provided insights into norovirus transmission, by documenting links among outbreaks, the introduction of strains onto ships, and viral persistence on board (despite cleaning). Control measures for outbreaks should address all routes of transmission. Better outbreak surveillance and collection of data on sequences will help to monitor norovirus strains and to identify common sources. Copyright © 2004 Infectious Diseases Society of America [ABSTRACT FROM AUTHOR]

Published

2004

4. A waterborne outbreak of Norwalk-like virus among snowmobilers -- Wyoming, 2001.

Author

Anderson AD, Heryford AG, Sarisky JP, Higgins C, Monroe SS, Beard RS, Newport CM, Cashdollar JL, Fout GS, Robbins DE, Seys SA, Musgrave KJ, Medus C, Vinjé J, Bresee JS, Mainzer HM, and Glass RI

Abstract

In February 2001, episodes of acute gastroenteritis were reported to the Wyoming Department of Health from persons who had recently vacationed at a snowmobile lodge in Wyoming. A retrospective cohort study found a significant association between water consumption and illness, and testing identified Norwalk-like virus (NLV) in 8 of 13 stool samples and 1 well. Nucleotide sequences from the positive well-water specimen and 6 of the positive stool samples were identical. This multistrain NLV outbreak investigation illustrates the importance of NLV as a cause of waterborne illness and should encourage monitoring for NLVs in drinking water. [ABSTRACT FROM AUTHOR]

Published

2003

5. Epidemiologic and molecular trends of 'Norwalk-like viruses' associated with outbreaks of gastroenteritis in the United States.

Author

Fankhauser RL, Monroe SS, Noel JS, Humphrey CD, Bresee JS, Parashar UD, Ando T, and Glass RI

Abstract

Between July 1997 and June 2000, fecal specimens from 284 outbreaks of nonbacterial gastroenteritis were submitted to the Centers for Disease Control and Prevention for testing for 'Norwalk-like viruses' (NLVs). Specimens were examined by reverse-transcription polymerase chain reaction and direct electron microscopy for the presence of NLVs. Adequate descriptive data were available from 233 of the outbreaks, and, of these, 217 (93%) were positive for NLVs. Restaurants and events with catered food were the most common settings, and contaminated food was the most common mode of transmission. Genogroup II (GII) strains were the predominant type (73%), with genogroup I strains causing 26% of all NLV-positive outbreaks. Certain GII clusters (GII/1,4,j) were more commonly associated with outbreaks in nursing home settings than with outbreaks in other settings. Strain diversity was great: one potential new sequence cluster was implicated in multiple outbreaks, and strains belonging to a tentative new genogroup were identified. Copyright © 2002 Infectious Diseases Society of America [ABSTRACT FROM AUTHOR]

Published

2002

6. 'Norwalk-like viruses': public health consequences and outbreak management.

Author

Parashar UD, Quiroz ES, Mounts AW, Monroe SS, Fankhauser RL, Ando T, Noel JS, Bulens SN, Beard RS, Li J, Bresee JS, Glass RI, and US Department of Health and Human Services. Centers for Disease Control and Prevention

Abstract

'Norwalk-like viruses' (NLVs) cause outbreaks of gastroenteritis and are spread frequently through contaminated food or water. Molecular diagnostics now enables detecting viruses in clinical and environmental specimens, linking of NLV strains causing outbreaks in multiple geographic locations, and tracing them to their sources in contaminated food or water. This report reviews recent advances in NLV detection and provides guidelines and recommendations for investigating NLV-related outbreaks, including specimen collection and disease prevention and control. This report also updates information provided in CDC's previously published, Viral Agents of Gastroenteritis: Public Health Importance and Outbreak Management (MMWR 1990;39 [No. RR-5]:1-24). These CDC recommendations are intended for public health professionals who investigate outbreaks of acute gastroenteritis but could be useful in academic and research settings as well. [ABSTRACT FROM AUTHOR]

Published

2001

7. A foodborne outbreak of gastroenteritis associated with Norwalk-like viruses: first molecular traceback to deli sandwiches contaminated during preparation.

Author

Daniels NA, Bergmire-Sweat DA, Schwab KJ, Hendricks KA, Reddy S, Rowe SM, Fankhauser RL, Monroe SS, Atmar RL, Glass RI, and Mead P

Abstract

In March 1998, an outbreak of acute gastroenteritis occurred among students at a Texas university. Overall, 125 ill students sought medical care. Case-control studies revealed that illness was significantly associated with eating foods from the university's main cafeteria deli bar on 9 and 10 March. Stool specimens from 9 (50%) of 18 ill students and samples of deli ham showed evidence of Norwalk-like viruses (NLVs) by reverse-transcriptase (RT) polymerase chain reaction (PCR) assay. A food handler who prepared sandwiches for lunch on 9 March reported that her infant had been sick with watery diarrhea since just before the outbreak. A stool sample from the infant was positive for NLV by RT-PCR, and the sequence of the amplified product was identical to that of amplified product from deli ham and students' stool specimens. This is the first time RT-PCR and sequence analysis have successfully confirmed viral contamination of a food item likely to have been contaminated by a food handler. Copyright © 2000 The University of Chicago [ABSTRACT FROM AUTHOR]

Published

2000

8. Concise communications. Molecular epidemiology of childhood astrovirus infection in child care centers.

Author

Mitchell DK, Matson DO, Jiang X, Berke T, Monroe SS, Carter MJ, Willcocks MM, and Pickering LK

Abstract

This study assessed the role of human astrovirus (HAstV) in outbreaks and sporadic cases of diarrhea among children attending child care centers (CCCs) and determined the infecting astrovirus antigenic types by reverse transcriptase-polymerase chain reaction (RT-PCR) and sequence analysis. Eight astrovirus outbreaks occurred in 6 CCCs. Of 179 children with diarrhea, 36 (20%) had astrovirus-associated diarrhea. Diarrhea stools obtained during diarrhea outbreaks were more likely to contain astrovirus (40/476) than were samples not associated with a diarrhea outbreak (14/452) (P<.001). Type-specific RT-PCR and DNA sequencing identified 5 outbreaks associated with HAstV-1 and 3 outbreaks with HAstV-2. Sequential outbreaks in 2 CCCs occurred with a different type in the same year. Phylogenetic analysis identified 6 clades of HAstV-1 and 2 clades of HAstV-2 during this 1-year surveillance. Astrovirus was a significant cause of diarrhea outbreaks, and 2 antigenic types were present in the community during 1 diarrhea season. Copyright © 1999 The University of Chicago [ABSTRACT FROM AUTHOR]

Published

1999

9. Virologic features of an astrovirus diarrhea outbreak in a day care center revealed by reverse transcriptase-polymerase chain reaction.

Author

Mitchell DK, Monroe SS, Jiang X, Matson DO, Glass RI, Pickering LK, Mitchell, D K, Monroe, S S, Jiang, X, Matson, D O, Glass, R I, and Pickering, L K

Abstract

Astroviruses cause outbreaks of diarrhea in children attending day care centers (DCCs). Reverse transcriptase-polymerase chain reaction (RT-PCR) was compared with EIA detection of astrovirus in stool specimens to characterize further the molecular epidemiology of an outbreak of astrovirus-associated gastroenteritis. Three hundred sixty-eight stool specimens collected prospectively from 36 children enrolled in a DCC during an 11-week outbreak of diarrhea were evaluated by EIA and RT-PCR. Astrovirus was detected in 32% of specimens by RT-PCR versus 10% by EIA (P < .001) and in 89% of children by RT-PCR versus 50% by EIA. The median duration of astrovirus excretion episodes detected by EIA was 1.5 days versus 4 days by RT-PCR (P = .06). Astrovirus was excreted for prolonged periods by immunocompetent children during this outbreak. RT-PCR was more sensitive than EIA for detection of astrovirus in stool specimens and redefined the epidemiology of astrovirus infection in this setting. [ABSTRACT FROM AUTHOR]

Published

1995

10. Control and prevention of viral gastroenteritis.

Author

Monroe SS and Monroe, Stephan S

Abstract

Diarrheal illness remains 1 of the top 5 causes of death in low-income and middle-income countries, especially for children <5 years of age. Introduction of universal childhood vaccination against rotaviruses has greatly reduced the incidence and severity of illness in upper-income and lower-income settings. For adults, norovirus is the leading cause of sporadic cases and outbreaks of diarrheal illness and is responsible for nearly 21 million episodes annually in the United States, of which 5.5 million are foodborne. Public health efforts to control and prevent norovirus illness have focused on rapid outbreak detection and source identification and control of transmission in institutional settings. [ABSTRACT FROM AUTHOR]

Published

2011

11. Detection of Norwalk-like virus in shellfish implicated in illness.

Author

Shieh YC, Monroe SS, Fankhauser RL, Langlois GW, Burkhardt W III, and Baric RS

Abstract

In the 1990s, Norwalk-like viruses (NLVs) were identified in patient specimens as the primary pathogen associated with shellfish-borne gastroenteritis in the United States. Identification of these viruses from implicated shellfish has been difficult due to inefficient recovery of viruses, natural polymerase chain reaction (PCR) inhibitors in shellfish, and low virus contamination. Recent improvements to the method of detecting NLVs in shellfish include enhanced processing of virus and shellfish samples, application of nested PCR and nucleotide sequencing, and increased knowledge of NLV genetic diversity. Using a newly developed and sensitive method, an NLV G2 strain was identified in 2 oyster samples implicated in a 1998 California outbreak involving 171 cases. NLV capsid primers demonstrated a greater specificity of PCR detection than did polymerase primers. The 175-base viral capsid nucleotide sequences derived from oysters were 100% identical to those derived from a patient stool sample. This finding supports the epidemiologic associations indicating that contaminated Copyright © 2000 The University of Chicago [ABSTRACT FROM AUTHOR]

Published

2000

12. International Workshop on Human Caliciviruses, Atlanta, Georgia, 29-31 March 1999.

Author

Monroe SS, Ando T, and Glass RI

Published

2000

13. The epidemiology of enteric caliciviruses from humans: a reassessment using new diagnostics.

Author

Glass RI, Noel J, Ando T, Fankhauser R, Belliot G, Mounts A, Parashar UD, Bresee JS, and Monroe SS

Abstract

In the United States, acute gastroenteritis is one of the most commonly noted illnesses on hospital discharge records and death certificates, yet few of these cases have an etiologic diagnosis. The application of new molecular diagnostic methods has shown caliciviruses (previously referred to as the Norwalk family of viruses or small round structured viruses) to be the most common cause of acute gastroenteritis (AGE) outbreaks in the United States, and they may emerge as a common cause of sporadic cases of AGE among both children and adults. Novel molecular methods have permitted outbreak strains to be traced back to their common source and have led to the first identification of virus in implicated vehicles of infection-water, shellfish, and foods contaminated both at their source and by food handlers. The broad application of these methods to routine diagnosis in hospitals and public health laboratories is advancing our appreciation of the full burden of calicivirus-associated diarrhea, and it is opening new avenues for its prevention and control. Copyright © 2000 The University of Chicago [ABSTRACT FROM AUTHOR]

Published

2000

14. Complete Genome Sequences of Human Astrovirus Prototype Strains (Types 1 to 8).

Author

Castro CJ, Reynolds E, Monroe SS, Marine RL, and Vinjé J

Abstract

We report the complete genome sequences of the eight human astrovirus Oxford prototype strains. These sequences share 94.9% to 99.9% nucleotide identity with open reading frame 2 (ORF2) genes of astrovirus genomes previously deposited in GenBank and include the first complete genome of human astrovirus type 7.

Published

2019

15. Reduced evolutionary rate in reemerged Ebola virus transmission chains.

Author

Blackley DJ, Wiley MR, Ladner JT, Fallah M, Lo T, Gilbert ML, Gregory C, D'ambrozio J, Coulter S, Mate S, Balogun Z, Kugelman J, Nwachukwu W, Prieto K, Yeiah A, Amegashie F, Kearney B, Wisniewski M, Saindon J, Schroth G, Fakoli L, Diclaro JW 2nd, Kuhn JH, Hensley LE, Jahrling PB, Ströher U, Nichol ST, Massaquoi M, Kateh F, Clement P, Gasasira A, Bolay F, Monroe SS, Rambaut A, Sanchez-Lockhart M, Scott Laney A, Nyenswah T, Christie A, and Palacios G

Subjects

Disease Outbreaks, Ebolavirus genetics, Genome, Viral genetics, Hemorrhagic Fever, Ebola genetics, Hemorrhagic Fever, Ebola virology, Humans, Liberia, Ebolavirus pathogenicity, Hemorrhagic Fever, Ebola epidemiology, Hemorrhagic Fever, Ebola transmission

Abstract

On 29 June 2015, Liberia's respite from Ebola virus disease (EVD) was interrupted for the second time by a renewed outbreak ("flare-up") of seven confirmed cases. We demonstrate that, similar to the March 2015 flare-up associated with sexual transmission, this new flare-up was a reemergence of a Liberian transmission chain originating from a persistently infected source rather than a reintroduction from a reservoir or a neighboring country with active transmission. Although distinct, Ebola virus (EBOV) genomes from both flare-ups exhibit significantly low genetic divergence, indicating a reduced rate of EBOV evolution during persistent infection. Using this rate of change as a signature, we identified two additional EVD clusters that possibly arose from persistently infected sources. These findings highlight the risk of EVD flare-ups even after an outbreak is declared over.

Published

2016

16. Low-incidence, high-consequence pathogens.

Author

Belay ED and Monroe SS

Subjects

Centers for Disease Control and Prevention, U.S. organization & administration, Hemorrhagic Fevers, Viral epidemiology, Humans, Incidence, Rabies epidemiology, Smallpox epidemiology, United States epidemiology, Hemorrhagic Fevers, Viral prevention & control, Rabies prevention & control, Smallpox prevention & control

Published

2014

17. The etiology of severe acute gastroenteritis among adults visiting emergency departments in the United States.

Author

Bresee JS, Marcus R, Venezia RA, Keene WE, Morse D, Thanassi M, Brunett P, Bulens S, Beard RS, Dauphin LA, Slutsker L, Bopp C, Eberhard M, Hall A, Vinje J, Monroe SS, and Glass RI

Subjects

Acute Disease, Adolescent, Adult, Aged, Aged, 80 and over, Caliciviridae isolation & purification, Caliciviridae pathogenicity, Caliciviridae Infections complications, Diarrhea epidemiology, Diarrhea microbiology, Diarrhea virology, Feces microbiology, Feces virology, Female, Gastroenteritis microbiology, Gastroenteritis parasitology, Gastroenteritis virology, Hospitalization, Humans, Interviews as Topic, Male, Middle Aged, Prevalence, Prospective Studies, Salmonella isolation & purification, Salmonella pathogenicity, Salmonella Infections complications, Specimen Handling methods, Surveys and Questionnaires, United States epidemiology, Young Adult, Emergency Service, Hospital, Gastroenteritis etiology

Abstract

Background: Acute gastroenteritis (AGE) remains a common cause of clinic visits and hospitalizations in the United States, but the etiology is rarely determined., Methods: We performed a prospective, multicenter emergency department-based study of adults with AGE. Subjects were interviewed on presentation and 3-4 weeks later. Serum samples, rectal swab specimens, and/or whole stool specimens were collected at presentation, and serum was collected 3-4 weeks later. Fecal specimens were tested for a comprehensive panel of viral, bacterial, and parasitic pathogens; serum was tested for calicivirus antibodies., Results: Pathogens were detected in 25% of 364 subjects, including 49% who provided a whole stool specimen. The most commonly detected pathogens were norovirus (26%), rotavirus (18%), and Salmonella species (5.3%). Pathogens were detected significantly more often from whole stool samples versus a rectal swab specimen alone. Nine percent of subjects who provided whole stool samples had >1 pathogen identified., Conclusions: Viruses, especially noroviruses, play a major role as agents of severe diarrhea in adults. Further studies to confirm the unexpectedly high prevalence of rotaviruses and to explore the causes of illness among patients from whom a pathogen cannot be determined are needed. Studies of enteric pathogens should require the collection of whole stool samples.

Published

2012

18. Multidrug-resistant typhoid fever with neurologic findings on the Malawi-Mozambique border.

Author

Lutterloh E, Likaka A, Sejvar J, Manda R, Naiene J, Monroe SS, Khaila T, Chilima B, Mallewa M, Kampondeni SD, Lowther SA, Capewell L, Date K, Townes D, Redwood Y, Schier JG, Nygren B, Tippett Barr B, Demby A, Phiri A, Lungu R, Kaphiyo J, Humphrys M, Talkington D, Joyce K, Stockman LJ, Armstrong GL, and Mintz E

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Antibodies, Bacterial blood, Child, Child, Preschool, Electrophoresis, Gel, Pulsed-Field, Female, Fever diagnosis, Fever etiology, Humans, Immunoglobulin M blood, Infant, Malawi epidemiology, Male, Microbial Sensitivity Tests, Middle Aged, Molecular Typing, Mozambique epidemiology, Nervous System Diseases etiology, Salmonella typhi classification, Salmonella typhi genetics, Salmonella typhi isolation & purification, Typhoid Fever microbiology, Young Adult, Disease Outbreaks, Drug Resistance, Multiple, Bacterial, Nervous System Diseases epidemiology, Salmonella typhi drug effects, Typhoid Fever complications, Typhoid Fever diagnosis, Typhoid Fever epidemiology

Abstract

Background: Salmonella enterica serovar Typhi causes an estimated 22 million cases of typhoid fever and 216 000 deaths annually worldwide. We investigated an outbreak of unexplained febrile illnesses with neurologic findings, determined to be typhoid fever, along the Malawi-Mozambique border., Methods: The investigation included active surveillance, interviews, examinations of ill and convalescent persons, medical chart reviews, and laboratory testing. Classification as a suspected case required fever and ≥1 other finding (eg, headache or abdominal pain); a probable case required fever and a positive rapid immunoglobulin M antibody test for typhoid (TUBEX TF); a confirmed case required isolation of Salmonella Typhi from blood or stool. Isolates underwent antimicrobial susceptibility testing and subtyping by pulsed-field gel electrophoresis (PFGE)., Results: We identified 303 cases from 18 villages with onset during March-November 2009; 214 were suspected, 43 were probable, and 46 were confirmed cases. Forty patients presented with focal neurologic abnormalities, including a constellation of upper motor neuron signs (n = 19), ataxia (n = 22), and parkinsonism (n = 8). Eleven patients died. All 42 isolates tested were resistant to ampicillin, chloramphenicol, and trimethoprim-sulfamethoxazole; 4 were also resistant to nalidixic acid. Thirty-five of 42 isolates were indistinguishable by PFGE., Conclusions: The unusual neurologic manifestations posed a diagnostic challenge that was resolved through rapid typhoid antibody testing in the field and subsequent blood culture confirmation in the Malawi national reference laboratory. Extending laboratory diagnostic capacity, including blood culture, to populations at risk for typhoid fever in Africa will improve outbreak detection, response, and clinical treatment.

Published

2012

19. Enhanced surveillance of norovirus outbreaks of gastroenteritis in Georgia.

Author

Widdowson MA, Bulens SN, Beard RS, Lane KM, Monroe SS, Lance S, Bresee JS, and Glass RI

Subjects

Caliciviridae Infections transmission, Feces microbiology, Gastroenteritis microbiology, Georgia epidemiology, Humans, Prospective Studies, Caliciviridae Infections epidemiology, Feces virology, Gastroenteritis epidemiology, Gastroenteritis virology, Norovirus, Sentinel Surveillance

Abstract

Objectives: The role of noroviruses in both foodborne and person-to-person outbreaks of acute gastroenteritis (AGE) has been difficult to determine in the U.S. because of lack of routine norovirus testing and of national reporting of person-to-person outbreaks. We conducted a prospective study in one state in which enhanced testing for noroviruses was performed to better understand the relative contribution of all gastroenteric pathogens., Methods: During the two-year period, 2000-2001, we took all fecal specimens from AGE outbreaks reported in Georgia that were negative for bacteria and tested these for norovirus., Results: We investigated 78 AGE outbreaks, from which suitable fecal samples were collected from 57 of them. Norovirus was identified in 25 (44%) outbreaks, bacteria in 20 (35%) outbreaks, and parasites in one (2%) outbreak. Forty-three (75%) of the outbreaks tested were foodborne, of which 17 (40%) were attributable to norovirus and 18 (42%) were attributable to bacteria. Adjusting for incomplete testing, we estimated that 53% of all AGE outbreaks were attributable to norovirus. A total of 2,674 people were reported ill in the 57 outbreaks, and norovirus infections accounted for 1,735 (65%) of these cases. Norovirus outbreaks tended to be larger than bacterial outbreaks, with a median number of 30 vs. 16 cases per outbreak, respectively (p = 0.057)., Conclusions: This study provides further evidence that noroviruses are, overall, the most common cause of AGE outbreaks in the U.S. Improved specimen collection, reporting person-to-person outbreaks, and access to molecular assays are needed to further understand the role of these viruses and methods for their prevention.

Published

2011

20. Chronic norovirus and adenovirus infection in a solid organ transplant recipient.

Author

Lee BE, Pang XL, Robinson JL, Bigam D, Monroe SS, and Preiksaitis JK

Subjects

Diarrhea virology, Feces virology, Humans, Infant, Male, Adenoviridae isolation & purification, Adenoviridae Infections virology, Caliciviridae Infections virology, Liver Failure complications, Norovirus isolation & purification, Transplants adverse effects

Abstract

A 10-month-old boy developed chronic diarrhea 2 months after a combined liver, pancreas, and small bowel transplant. Norovirus and adenovirus were detected in multiple stool specimens during a 114-day period. Enteric viral infectious should be considered in solid organ transplant recipients with chronic diarrhea.

Published

2008

21. Norovirus detection and genotyping for children with gastroenteritis, Brazil.

Author

Soares CC, Santos N, Beard RS, Albuquerque MC, Maranhão AG, Rocha LN, Ramírez ML, Monroe SS, Glass RI, and Gentsch J

Subjects

Brazil epidemiology, Caliciviridae Infections epidemiology, Child, Child, Preschool, Female, Gastroenteritis epidemiology, Gastroenteritis genetics, Genotype, Humans, Infant, Male, Reverse Transcriptase Polymerase Chain Reaction methods, Caliciviridae Infections virology, Gastroenteritis virology, Norovirus genetics

Abstract

During 1998-2005, we analyzed stool samples from 289 children in Rio de Janeiro to detect and genotype no-rovirus strains. Previous tests showed all samples to be negative for rotavirus and adenovirus. Of 42 (14.5%) no-rovirus-positive specimens, 20 (47.6%) were identified as genogroup GI and 22 (52.3%) as GII.

Published

2007

22. Comparing serologic response against enteric pathogens with reported diarrhea to assess the impact of improved household drinking water quality.

Author

Crump JA, Mendoza CE, Priest JW, Glass RI, Monroe SS, Dauphin LA, Bibb WF, Lopez MB, Alvarez M, Mintz ED, and Luby SP

Subjects

Animals, Cryptosporidium parvum isolation & purification, Diarrhea blood, Diarrhea epidemiology, Diarrhea parasitology, Diarrhea pathology, Environmental Monitoring methods, Epidemiological Monitoring, Escherichia coli isolation & purification, Female, Giardia lamblia isolation & purification, Guatemala epidemiology, Humans, Infant, Male, Norovirus isolation & purification, Population Surveillance methods, Predictive Value of Tests, Prevalence, Diarrhea microbiology, Housing, Water Microbiology, Water Supply

Abstract

We evaluated enteric infection serology as an alternative outcome measure to diarrhea prevalence in a randomized controlled trial of household-based drinking water treatment; 492 households were randomly assigned to 5 household-based water treatment interventions or control. Individuals were followed weekly over 52 weeks to measure diarrhea prevalence. Study subjects of age

Published

2007

23. A large outbreak of Brainerd diarrhea associated with a restaurant in the Red River Valley, Texas.

Author

Kimura AC, Mead P, Walsh B, Alfano E, Gray SK, Durso L, Humphrey C, Monroe SS, Visvesvera G, Puhr N, Shieh WJ, Eberhard M, Hoekstra RM, and Mintz ED

Subjects

Case-Control Studies, Chronic Disease, Environmental Monitoring, Epidemiological Monitoring, Food Microbiology, Humans, Restaurants, Texas epidemiology, Water Microbiology, Diarrhea epidemiology, Diarrhea etiology, Disease Outbreaks

Abstract

Background: In June 1996, an outbreak of chronic diarrhea was reported to the Texas Department of Health (Austin)., Methods: We initiated active case finding, performed 2 case-control studies, and conducted an extensive laboratory and environmental investigation., Results: We identified 114 persons with diarrhea that lasted > or = 4 weeks. Symptoms among 102 patients who were studied included urgency (87%), fatigue (86%), fecal incontinence (74%), and weight loss (73%); the median maximum 24-h stool frequency was 15 stools. Diarrhea persisted for > 6 months in 87% and for > 1 year in 70% of patients who were observed. Fifty-one (89%) of 57 ill persons had eaten at a particular restaurant within 4 weeks before onset, compared with 8 (14%) of 59 matched control subjects (matched odds ratio [OR], undefined; 95% confidence interval [CI], 11.2-infinity). At the restaurant, patients were more likely than their unaffected dining companions to have drunk tap water (OR, 2.8; 95% CI, 1.0-9.9) and to have eaten several specific food items, and they were less likely to have drunk iced tea made from boiled water and store-bought ice (OR, 0.3; 95% CI, 0.05-1.0). A multivariable model that included consumption of tap water and salad bar tomatoes best fit the data. The restaurant had multiple sanitary and plumbing deficiencies. Extensive laboratory and environmental testing for bacterial, parasitic, mycotic, and viral agents did not identify an etiologic agent., Conclusions: The clinical, laboratory, and epidemiologic findings are consistent with those of previous outbreaks of Brainerd diarrhea. To our knowledge, this is the largest reported outbreak of Brainerd diarrhea associated with a restaurant.

Published

2006

24. Use of TaqMan real-time reverse transcription-PCR for rapid detection, quantification, and typing of norovirus.

Author

Trujillo AA, McCaustland KA, Zheng DP, Hadley LA, Vaughn G, Adams SM, Ando T, Glass RI, and Monroe SS

Subjects

Caliciviridae Infections virology, Disease Outbreaks, Feces virology, Gastroenteritis virology, Norovirus genetics, Phylogeny, Reverse Transcriptase Polymerase Chain Reaction, Sensitivity and Specificity, Caliciviridae Infections diagnosis, Norovirus isolation & purification, Taq Polymerase metabolism

Abstract

Noroviruses (NoVs) are the most commonly identified cause of outbreaks and sporadic cases of acute gastroenteritis. We evaluated and optimized NoV-specific TaqMan real-time reverse transcription (RT)-PCR assays for the rapid detection and typing of NoV strains belonging to genogroups GI and GII and adapted them to the LightCycler platform. We expanded the detection ability of the assays by developing an assay that detects the GIV NoV strain. The assays were validated with 92 clinical samples and 33 water samples from confirmed NoV outbreaks and suspected NoV contamination cases. The assays detected NoV RNA in all of the clinical specimens previously confirmed positive by conventional RT-PCR and sequencing. Additionally, the TaqMan assays successfully detected NoV RNA in water samples containing low viral concentrations and inhibitors of RT and/or PCR, whereas the conventional method with region B primers required dilution of the inhibitors. By means of serially diluted NoV T7 RNA transcripts, a potential detection limit of <10 transcript copies per reaction mixture was observed with the GII assay and a potential detection limit of <100 transcript copies per reaction mixture was observed with the GI assay. These results and the ability to detect virus in water that was negative by RT-PCR demonstrate the higher sensitivity of the TaqMan assay compared with that of a conventional RT-PCR assay. The TaqMan methods dramatically decrease the turnaround time by eliminating post-PCR processing. These assays have proven useful in assisting scientists in public health and diagnostic laboratories report findings quickly to outbreak management teams.

Published

2006

25. Norovirus classification and proposed strain nomenclature.

Author

Zheng DP, Ando T, Fankhauser RL, Beard RS, Glass RI, and Monroe SS

Subjects

Animals, Capsid Proteins chemistry, Humans, Norovirus genetics, Open Reading Frames, Phylogeny, Protein Structure, Tertiary, Sequence Alignment, Sequence Homology, Amino Acid, Capsid Proteins genetics, Norovirus classification, Terminology as Topic

Abstract

Without a virus culture system, genetic analysis becomes the principal method to classify norovirus (NoV) strains. Currently, classification of NoV strains beneath the species level has been based on sequences from different regions of the viral genome. As a result, the phylogenetic insights of some virus were not appropriately interpreted, and no consensus has been reached to establish a uniform classification scheme. To provide a consistent and reliable scientific basis for classifying NoVs, we analyzed the amino acid sequences for the major capsid protein of 164 NoV strains by first using an alignment based on the predicted 3D structures. A Bayesian tree was generated, and the maximum likelihood pairwise distances of the aligned sequences were used to evaluate the results from the uncorrected pairwise distance method. Analyses of the pairwise distances demonstrated three clearly resolved peaks, suggesting that NoV strains beneath the species level can be classified at three levels: strain (S), cluster (C), and genogroup (G). The uncorrected pairwise distance ranges for S, C, and G were 0-14.1%, 14.3-43.8%, and 44.9-61.4%, respectively. A scheme with 29 genetic clusters [8 in genogroup 1 (G1), 17 in G2, 2 in G3, and 1 each in G4 and G5] was defined on the basis of the tree topology with the standards provided and was supported by the distance analysis. Of these, five clusters in G2 and one in G1 are newly described. This analysis can serve as the basis for a standardized nomenclature to genetically describe NoV strains.

Published

2006

26. Molecular and epidemiologic trends of caliciviruses associated with outbreaks of acute gastroenteritis in the United States, 2000-2004.

Author

Blanton LH, Adams SM, Beard RS, Wei G, Bulens SN, Widdowson MA, Glass RI, and Monroe SS

Subjects

Acute Disease, Caliciviridae classification, Caliciviridae isolation & purification, Caliciviridae Infections virology, Gastroenteritis virology, Humans, Norwalk virus classification, Norwalk virus genetics, Norwalk virus isolation & purification, Phylogeny, Reverse Transcriptase Polymerase Chain Reaction, Seasons, Sequence Analysis, DNA, United States epidemiology, Caliciviridae genetics, Caliciviridae Infections epidemiology, Disease Outbreaks, Gastroenteritis epidemiology, Molecular Epidemiology

Abstract

Between July 2000 and June 2004, fecal specimens from 270 outbreaks of acute gastroenteritis were sent to the Centers for Disease Control and Prevention by local or state health departments for calicivirus testing. Of the 226 outbreaks that met the criteria for inclusion in the present study, caliciviruses were detected in 184 (81%) by reverse-transcription polymerase chain reaction and nucleotide sequencing. Nursing homes, retirement centers, and hospitals were the most frequently reported settings, and person-to-person contact was the most common mode of transmission, followed by foodborne spread. Overall, genogroup II norovirus (NoV) strains were the most abundant (79%), followed by genogroup I NoV strains (19%) and sapovirus (2%). Nucleotide-sequence analysis indicated a great diversity of NoV strains and implicated the emergence of one particular sequence variant in outbreaks occurring between July 2002 and June 2003. The public health impact of caliciviruses will not be fully appreciated, nor will interventions be completely evaluated, until methods to detect these viruses are more routinely used.

Published

2006

27. Molecular analysis of noroviruses involved in acute gastroenteritis outbreaks in military units in Israel, 1999-2004.

Author

Halperin T, Yavzori M, Amitai A, Klement E, Kayouf R, Grotto I, Huerta M, Hadley LA, Monroe SS, Cohen D, and Orr N

Subjects

Acute Disease, Adolescent, Adult, Caliciviridae Infections virology, Female, Gastroenteritis virology, Humans, Israel epidemiology, Male, Norovirus classification, Norovirus isolation & purification, Phylogeny, RNA-Dependent RNA Polymerase genetics, Sequence Analysis, DNA, Caliciviridae Infections epidemiology, Disease Outbreaks, Gastroenteritis epidemiology, Military Personnel, Norovirus genetics

Abstract

The study presented here was conducted to determine the genetic properties of noroviruses (NoVs) identified between 1999 and 2004 in army recruits with acute gastroenteritis. Partial sequence analysis of the RNA-dependent RNA polymerase gene revealed the presence of two major sub-genogroups, all of which were related to genogroup II of NoV. Serological analysis using recombinant antigens confirmed this observation. Local strains associated with a 1999 outbreak were closely related to GII-6 strains, while those identified later were very closely related to GII-4 strains. GII-4 strains were also associated with an outbreak in civilian nursing homes in Israel in 2002 and samples from this outbreak were included in this study for comparison. This is the first report describing the molecular properties of NoV strains associated with diarrhea-related morbidity in Israel.

Published

2005

28. Norovirus and child care: challenges in outbreak control.

Author

Isakbaeva ET, Bulens SN, Beard RS, Adams S, Monroe SS, Chaves SS, Widdowson MA, and Glass RI

Subjects

Adult, Caliciviridae Infections prevention & control, Caliciviridae Infections transmission, Caliciviridae Infections virology, Feces virology, Female, Gastroenteritis prevention & control, Humans, Infant, Caliciviridae Infections epidemiology, Child Day Care Centers, Disease Outbreaks, Gastroenteritis epidemiology, Gastroenteritis virology, Norovirus isolation & purification

Abstract

An infant with diarrhea attended a community playgroup. In the subsequent 48 hours, 6 of the 7 mothers and children reported gastroenteritis; fecal specimens from 5 persons tested positive for norovirus, with identical sequences. No breach of hygiene or contact with fecal matter was identified. Excluding the child with gastroenteritis from the playgroup could have prevented this outbreak.

Published

2005

29. Are noroviruses emerging?

Author

Widdowson MA, Monroe SS, and Glass RI

Subjects

Caliciviridae Infections virology, Communicable Diseases, Emerging, Disease Outbreaks, Food Microbiology, Humans, Water Microbiology, Caliciviridae Infections epidemiology, Gastroenteritis virology, Norovirus isolation & purification

Published

2005

30. Norovirus transmission on cruise ship.

Author

Isakbaeva ET, Widdowson MA, Beard RS, Bulens SN, Mullins J, Monroe SS, Bresee J, Sassano P, Cramer EH, and Glass RI

Subjects

Caliciviridae Infections epidemiology, Caliciviridae Infections virology, Gastroenteritis virology, Humans, Norovirus classification, Norovirus genetics, Caliciviridae Infections transmission, Disease Outbreaks, Gastroenteritis epidemiology, Norovirus isolation & purification, Ships, Travel

Abstract

An outbreak of norovirus gastroenteritis affected passengers on two consecutive cruises of ship X and continued on 4 subsequent cruises despite a 1-week sanitization. We documented transmission by food and person-to-person contact; persistence of virus despite sanitization onboard, including introductions of new strains; and seeding of an outbreak on land.

Published

2005

31. Norovirus and foodborne disease, United States, 1991-2000.

Author

Widdowson MA, Sulka A, Bulens SN, Beard RS, Chaves SS, Hammond R, Salehi ED, Swanson E, Totaro J, Woron R, Mead PS, Bresee JS, Monroe SS, and Glass RI

Subjects

Animals, Caliciviridae Infections epidemiology, Caliciviridae Infections virology, Centers for Disease Control and Prevention, U.S. statistics & numerical data, Food Contamination, Foodborne Diseases virology, Gastroenteritis virology, Humans, United States epidemiology, Disease Outbreaks, Foodborne Diseases epidemiology, Gastroenteritis epidemiology, Norovirus isolation & purification

Abstract

Efforts to prevent foodborne illness target bacterial pathogens, yet noroviruses (NoV) are suspected to be the most common cause of gastroenteritis. New molecular assays allow for better estimation of the role of NoV in foodborne illness. We analyzed 8,271 foodborne outbreaks reported to the Centers for Disease Control and Prevention from 1991 to 2000 and additional data from 6 states. The proportion of NoV-confirmed outbreaks increased from 1% in 1991 to 12% in 2000. However, from 1998 to 2000, 76% of NoV outbreaks were reported by only 11 states. In 2000, an estimated 50% of foodborne outbreaks in 6 states were attributable to NoV. NoV outbreaks were larger than bacterial outbreaks (median persons affected: 25 versus 15), and 10% of affected persons sought medical care; 1% were hospitalized. More widespread use of molecular assays will permit better estimates of the role of NoV illness and help direct efforts to control foodborne illness.

Published

2005

32. Genogroup I and II noroviruses detected in stool samples by real-time reverse transcription-PCR using highly degenerate universal primers.

Author

Richards GP, Watson MA, Fankhauser RL, and Monroe SS

Subjects

Caliciviridae Infections diagnosis, Caliciviridae Infections virology, Gastroenteritis diagnosis, Gastroenteritis virology, Genotype, Humans, Norovirus genetics, RNA, Viral analysis, Transition Temperature, DNA Primers, Feces virology, Norovirus classification, Norovirus isolation & purification, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

Genogroup I noroviruses from five genetic clusters and genogroup II noroviruses from eight genetic clusters were detected in stool extracts using degenerate primers and single-tube, real-time reverse transcription-PCR (RT-PCR) with SYBR Green detection. Two degenerate primer sets, designated MON 431-433 and MON 432-434, were designed from consensus sequences from the major clusters of norovirus based on the RNA-dependent RNA polymerase region of the norovirus genome. Viruses were extracted from stool samples within 20 min using a viral RNA extraction kit. Real-time RT-PCR for noroviruses generated semiquantitative results by means of the cycle threshold data and dilution endpoint standard curves. Presumptive product verification was achieved by evaluation of first-derivative melt graphs. Multiple clusters of noroviruses were identified simultaneously in a multiplex fashion by virtue of slight differences in melting temperature. The detection of 13 different genetic clusters suggests that the MON primers may serve as universal primers for most, if not all, of the noroviruses in a multiplex assay. Our technique provides a framework for broad application of real-time RT-PCR in clinical, environmental, and food testing laboratories for a wide range of noroviruses.

Published

2004

33. Use of stool collection kits delivered to patients can improve confirmation of etiology in foodborne disease outbreaks.

Author

Jones TF, Bulens SN, Gettner S, Garman RL, Vugia DJ, Blythe D, Hawkins MA, Monroe SS, Angulo FJ, and Parashar UD

Subjects

Humans, Pilot Projects, Specimen Handling, Disease Outbreaks, Feces microbiology, Food Microbiology, Infections diagnosis, Infections microbiology, Reagent Kits, Diagnostic

Abstract

Background: In 68% of foodborne disease outbreaks, no etiologic pathogen is identified. In two-thirds of outbreaks with no identified etiology, no stool specimens are submitted for testing., Methods: From April 2001 to March 2003, we pilot-tested use of prepackaged, self-contained stool specimen collection kits in 3 states, delivered to and from patients by courier or mail, to improve rates of specimen collection in the outbreak setting. Specimens were tested for bacterial and viral pathogens at health department laboratories, and results were correlated with epidemiological investigation data., Results: Specimens were returned by > or =1 person in 52 (96%) of 54 outbreaks in which kits were deployed; in total, 263 (76%) of 347 persons who received kits returned specimens. Resolution of symptoms was the most commonly cited reason for nonsubmission of kits. An etiology was confirmed in 37 (71%) of 52 outbreaks with specimens returned; 28 (76%) were attributable to norovirus, and 9 (24%) were attributed to bacterial pathogens. Stool kits were well received and cost an average of approximately 43 dollars per specimen returned., Conclusions: In two-thirds of foodborne disease outbreaks in which delivered stool collection kits were successfully deployed, an etiologic organism was identified. Delivery of kits to and from patients to improve rates of stool collection in outbreaks in which specimens might otherwise not be submitted could substantially reduce the number of outbreaks with an unknown etiology.

Published

2004

34. Evaluation and validation of real-time reverse transcription-pcr assay using the LightCycler system for detection and quantitation of norovirus.

Author

Pang X, Lee B, Chui L, Preiksaitis JK, and Monroe SS

Subjects

Benzothiazoles, Child, Child, Preschool, Diamines, Feces virology, Hot Temperature, Humans, Norovirus classification, Norovirus genetics, Organic Chemicals metabolism, Quinolines, RNA, Viral analysis, RNA, Viral isolation & purification, Sensitivity and Specificity, Caliciviridae Infections virology, Gastroenteritis virology, Norovirus isolation & purification, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

We developed an assay for the detection and quantitation of norovirus with the LightCycler SYBR Green-based real-time reverse transcription-PCR (real-time LC RT-PCR) and previously published primers in the capsid and the polymerase gene. One hundred thirty-two stool specimens from the Provincial Laboratory for Public Health (Microbiology), Alberta, Canada, and the Centers for Disease Control and Prevention, Atlanta, Ga., were used to validate the new assay. The samples were collected from patients involved in outbreaks of acute gastroenteritis or children who presented with sporadic gastroenteritis. The real-time LC RT-PCR assay detected norovirus strains from three genogroup I (G-I) clusters (G-I/1, G-I/2, and G-I/3) and 10 genogroup II (G-II) clusters (G-II/1, G-II/2, G-II/3, G-II/4, G-II/6, G-II/7, G-II/10, G-II/12, G-II/15, and G-II/16). There was 100% concordance with the results from 58 stool specimens which tested positive by conventional RT-PCR assays. By dilution analysis, the real-time LC RT-PCR was 10,000 times more sensitive than the conventional RT-PCR. The new assay increased the number of samples in which noroviruses were detected by 19%. The real-time LC RT-PCR had a wide dynamic range, detecting from 5 to 5 x 10(6) copies of RNA per reaction, resulting in a theoretical lower limit of detection of 25,000 copies of RNA per g of stool. No cross-reactions were found with specimens containing sapovirus, rotavirus, astrovirus, and adenovirus. Because of the high sensitivity and specificity of the assay with a relatively rapid and simple procedure, the real-time LC RT-PCR will be useful as a routine assay for the clinical diagnosis of norovirus infection.

Published

2004

35. Human caliciviruses as a cause of severe gastroenteritis in Peruvian children.

Author

Parashar UD, Li JF, Cama R, DeZalia M, Monroe SS, Taylor DN, Figueroa D, Gilman RH, and Glass RI

Subjects

Antibodies, Viral blood, Caliciviridae genetics, Caliciviridae immunology, Case-Control Studies, Child, Preschool, Feces virology, Female, Humans, Immunoenzyme Techniques, Infant, Infant, Newborn, Male, Peru, RNA, Viral analysis, Reverse Transcriptase Polymerase Chain Reaction, Serum virology, Caliciviridae isolation & purification, Caliciviridae Infections virology, Gastroenteritis virology

Abstract

To define the role of human caliciviruses (HuCVs) in severe childhood gastroenteritis, fecal and paired serum samples from 233 Peruvian children hospitalized with gastroenteritis (case patients) and fecal samples from 248 control subjects were evaluated. Overall, 128 case patients (55%) demonstrated HuCV infection by either fecal (n=81 [35%]) or serological (n=96 [41%]) testing. HuCVs were more prevalent in fecal samples from case patients than those from control subjects (35% vs. 13%; P<.001). HuCV infection was more prevalent among case patients without another pathogen than in those who had a coinfecting pathogen (77% [40/52] vs. 49% [88/181]; P<.001). HuCVs appear to be an important cause of gastroenteritis in Peruvian children.

Published

2004

36. Direct sequencing of SARS-coronavirus S and N genes from clinical specimens shows limited variation.

Author

Tong S, Lingappa JR, Chen Q, Shu B, LaMonte AC, Cook BT, Birge C, Chern SW, Liu X, Galloway R, Mai le Q, Ng WF, Yang JY, Butany J, Comer JA, Monroe SS, Beard SR, Ksiazek TG, Erdman D, Rota PA, Pallansch MA, and Anderson LJ

Subjects

Amino Acid Substitution genetics, Coronavirus Nucleocapsid Proteins, Genome, Viral, Humans, Mutation, Missense, Point Mutation, Polymorphism, Genetic, RNA, Viral isolation & purification, Severe acute respiratory syndrome-related coronavirus isolation & purification, Spike Glycoprotein, Coronavirus, Membrane Glycoproteins genetics, Nucleocapsid Proteins genetics, RNA, Viral genetics, Severe acute respiratory syndrome-related coronavirus genetics, Severe Acute Respiratory Syndrome virology, Viral Envelope Proteins genetics

Abstract

Severe acute respiratory syndrome-associated coronavirus (SARS-CoV) emerged, in November 2002, as a novel agent causing severe respiratory illness. To study sequence variation in the SARS-CoV genome, we determined the nucleic acid sequence of the S and N genes directly from clinical specimens from 10 patients--1 specimen with no matched SARS-CoV isolate, from 2 patients; multiple specimens from 3 patients; and matched clinical-specimen/cell-culture-isolate pairs from 6 patients. We identified 3 nucleotide substitutions that were most likely due to natural variation and 2 substitutions that arose after cell-culture passage of the virus. These data demonstrate the overall stability of the S and N genes of SARS-CoV over 3 months during which a minimum of 4 generations for transmission events occurred. These findings are a part of the expanding investigation of the evolution of how this virus adapts to a new host.

Published

2004

37. Molecular epidemiology of outbreaks of viral gastroenteritis in New York State, 1998-1999.

Author

Chatterjee NK, Moore DW, Monroe SS, Glass RI, Cambridge MJ, Kondracki SF, and Morse DL

Subjects

Amino Acid Sequence, Caliciviridae Infections genetics, Disease Outbreaks, Enzyme-Linked Immunosorbent Assay, Gastroenteritis genetics, Gastroenteritis virology, Genetic Variation, Humans, Molecular Epidemiology, Molecular Sequence Data, New York epidemiology, RNA, Viral analysis, Reverse Transcriptase Polymerase Chain Reaction, Sequence Homology, Amino Acid, Caliciviridae Infections epidemiology, Gastroenteritis epidemiology, Norovirus classification, Norovirus genetics

Abstract

This investigation evaluated the role of Norwalk-like virus (NLV) and other viruses (rotavirus, enteric adenovirus, and enterovirus) in 11 outbreaks of acute nonbacterial gastroenteritis that occurred in multiple settings in a span of 18 months in New York State. To determine the etiology of illness, patients' stool specimens were analyzed with a combination of reverse-transcription polymerase chain reaction (RT-PCR) and nucleotide sequencing, cell culture, and ELISA diagnostic techniques. NLV was detected from all of these outbreaks, with an overall detection rate of 64% (51 of 79) for all specimens tested. Repeated attempts to isolate other viral pathogens were unsuccessful. Phylogenetic analysis of a subset of 27 specimens from these outbreaks showed the presence of both genogroup I and genogroup II NLVs. A spectrum of different nucleotide sequences were detected, demonstrating interoutbreak sequence variation and unrelated infections. NLV is a significant causative agent of diarrhea outbreaks in New York State.

Published

2004

38. Molecular characterization of noroviruses detected in diarrheic stools of Michigan and Wisconsin dairy calves: circulation of two distinct subgroups.

Author

Wise AG, Monroe SS, Hanson LE, Grooms DL, Sockett D, and Maes RK

Subjects

Amino Acid Sequence, Animals, Base Sequence, Capsid Proteins genetics, Cattle, Cattle Diseases diagnosis, Circoviridae Infections diagnosis, Conserved Sequence, DNA Primers, Dairying, Diarrhea diagnosis, Feces virology, Female, Michigan, Molecular Sequence Data, Open Reading Frames, Phylogeny, Reverse Transcriptase Polymerase Chain Reaction, Sequence Alignment, Sequence Homology, Amino Acid, Wisconsin, Cattle Diseases virology, Circoviridae Infections veterinary, Diarrhea veterinary, Norovirus classification, Norovirus genetics

Abstract

Noroviruses have emerged as the leading worldwide cause of acute non-bacterial gastroenteritis in humans. The presence of noroviruses in diarrheic stool samples from calves on Michigan and Wisconsin dairy farms was investigated by RT-PCR. Norovirus-positive samples were found on all eight farms studied in Michigan and on 2 out of 14 farms in Wisconsin. Phylogenetic analyses of partial polymerase and capsid sequences, derived for a subset of these bovine noroviruses, showed that these strains formed a group which is genetically distinct from the human noroviruses, but more closely related to genogroup I than to genogroup II human noroviruses. Examination of 2 full and 10 additional partial capsid (ORF2) sequences of these bovine strains revealed the presence of two genetic subgroups or clusters of bovine noroviruses circulating on Michigan and Wisconsin farms. One subgroup is "Jena-like", the other "Newbury agent-2-like".

Published

2004

39. Prevalence of rotavirus and norovirus antibodies in non-human primates.

Author

Jiang B, McClure HM, Fankhauser RL, Monroe SS, and Glass RI

Subjects

Animals, Capsid Proteins, Disease Models, Animal, Immunoenzyme Techniques, Primates immunology, Rotavirus immunology, Antibodies, Viral blood, Caliciviridae Infections immunology, Gastroenteritis virology, Norovirus immunology, Primates virology, Rotavirus Infections immunology

Abstract

Rotavirus and norovirus are associated with a substantial burden of diarrheal disease in humans and some animals, but their role in acute viral gastroenteritis in non-human primates has not been established. We examined sera from five species of Old and New World monkeys and chimpanzees for antibodies to rotavirus and norovirus by enzyme immunoassays using RRV and three recombinant human norovirus capsid proteins, respectively. Most (88%) of the 3 Old World monkey species (mangabey, pigtail, and rhesus) and apes were seropositive for rotavirus. Norovirus antibody was prevalent in the three monkey species, with 53% (44/83) and 58% (48/83) seropositive for GI and GII strains, respectively. Eleven (92%) of the 12 chimpanzees tested were seropositive for GI norovirus. Given the high rate of infection with both viruses, the role of these agents in causing acute gastroenteritis in non-human primates and the value of these animals as models of infection and disease need to be assessed.

Published

2004

40. SARS-associated coronavirus transmission, United States.

Author

Isakbaeva ET, Khetsuriani N, Beard RS, Peck A, Erdman D, Monroe SS, Tong S, Ksiazek TG, Lowther S, Pandya-Smith I, Anderson LJ, Lingappa J, and Widdowson MA

Subjects

Adolescent, Adult, Child, Contact Tracing, Disease Outbreaks, Family Characteristics, Feces virology, Female, Humans, Male, Middle Aged, Severe acute respiratory syndrome-related coronavirus isolation & purification, Severe Acute Respiratory Syndrome epidemiology, Severe Acute Respiratory Syndrome virology, Sputum virology, Time Factors, United States epidemiology, Severe Acute Respiratory Syndrome transmission

Abstract

To better assess the risk for transmission of the severe acute respiratory syndrome-associated coronavirus (SARS-CoV), we obtained serial specimens and clinical and exposure data from seven confirmed U.S. SARS patients and their 10 household contacts. SARS-CoV was detected in a day-14 sputum specimen from one case-patient and in five stool specimens from two case-patients. In one case-patient, SARS-CoV persisted in stool for at least 26 days after symptom onset. The highest amounts of virus were in the day-14 sputum sample and a day-14 stool sample. Residual respiratory symptoms were still present in recovered SARS case-patients 2 months after illness onset. Possible transmission of SARS-CoV occurred in one household contact, but this person had also traveled to a SARS-affected area. The data suggest that SARS-CoV is not always transmitted efficiently. Routine collection and testing of stool and sputum specimens of probable SARS case-patients may help the early detection of SARS-CoV infection.

Published

2004

41. Prevalence of infection with waterborne pathogens: a seroepidemiologic study in children 6-36 months old in San Juan Sacatepequez, Guatemala.

Author

Steinberg EB, Mendoza CE, Glass R, Arana B, Lopez MB, Mejia M, Gold BD, Priest JW, Bibb W, Monroe SS, Bern C, Bell BP, Hoekstra RM, Klein R, Mintz ED, and Luby S

Subjects

Animals, Antibodies, Bacterial blood, Antibodies, Protozoan blood, Antibodies, Viral blood, Child, Preschool, Cryptosporidium parvum isolation & purification, Enzyme-Linked Immunosorbent Assay, Escherichia coli isolation & purification, Female, Guatemala epidemiology, Helicobacter pylori isolation & purification, Hepatitis A virus isolation & purification, Humans, Infant, Male, Norovirus isolation & purification, Prevalence, Rural Population, Seroepidemiologic Studies, Caliciviridae Infections epidemiology, Cryptosporidiosis epidemiology, Escherichia coli Infections epidemiology, Helicobacter Infections epidemiology, Hepatitis A epidemiology, Water parasitology, Water Microbiology

Abstract

Water and sanitation interventions in developing countries have historically been difficult to evaluate. We conducted a seroepidemiologic study with the following goals: 1) to determine the feasibility of using antibody markers as indicators of waterborne pathogen infection in the evaluation of water and sanitation intervention projects; 2) to characterize the epidemiology of waterborne diarrheal infections in rural Guatemala, and 3) to measure the age-specific prevalence of antibodies to waterborne pathogens. Between September and December 1999, all children 6-36 months of age in 10 study villages were invited to participate. We collected sufficient serum from 522 of 590 eligible children, and divided them into six-month age groups for analysis (6-12, 13-18, 19-24, 25-30, and 31-36 months). The prevalence of antibodies was lowest in children 6-12 months old compared with the four older age groups for the following pathogens: enterotoxigenic Escherichia coli (48%, 81%, 80%, 77%, and 83%), Norwalk virus (27%, 61%, 83%, 94%, and 94%), and Cryptosporidium parvum (27%, 53%, 70%, 67%, and 73%). The prevalence of total antibody to hepatitis A virus increased steadily in the three oldest age groups (40%, 28%, 46%, 60%, and 76%). In contrast, the prevalence of antibody to Helicobacter pylori was relatively constant in all five age groups (20%, 19%, 21%, 25%, and 25%). Serology appears to be an efficient and feasible approach for determining the prevalence of infection with selected waterborne pathogens in very young children. Such an approach may provide a suitable, sensitive, and economical alternative to the cumbersome stool collection methods that have previously been used for evaluation of water and sanitation projects.

Published

2004

42. Development of a rapid method using nucleic acid sequence-based amplification for the detection of astrovirus.

Author

Tai JH, Ewert MS, Belliot G, Glass RI, and Monroe SS

Subjects

Child, Preschool, Feces virology, Humans, Infant, Infant, Newborn, Liposomes, Luminescent Measurements, Mamastrovirus genetics, RNA, Viral analysis, Reagent Strips, Reverse Transcriptase Polymerase Chain Reaction, Time Factors, Astroviridae Infections diagnosis, Astroviridae Infections virology, Mamastrovirus isolation & purification, Self-Sustained Sequence Replication methods

Abstract

We have developed a rapid method to detect astrovirus in fecal specimens utilizing nucleic acid sequence-based amplification (NASBA) and several detection methodologies, including a sandwich hybridization assay based on DNA-tagged liposomes (liposome-strip detection assay). RNA was extracted from 65 stool specimens that were positive for astrovirus by enzyme immunoassay and was amplified by both NASBA and reverse transcriptase PCR (RT-PCR). Also extracted and amplified were 19 specimens containing rotavirus, 20 specimens containing norovirus, five specimens containing adenovirus, 15 water negative control specimens, and eight specimens containing astrovirus reference strains. NASBA products were detected by electrochemiluminescence detection (ECL) and by liposome-strip detection; RT-PCR products were detected by ethidium bromide staining following gel electrophoresis and by liquid hybridization assay (LHA). There was no significant difference in the detection rates of NASBA- and RT-PCR-based assays, with one exception in which the NASBA/ECL assay detected astrovirus in eight specimens that tested negative by the RT-PCR/LHA assay. These results suggest that these NASBA-based detection methods have detection rates that are as good as or better than those of RT-PCR-based methods. Both NASBA and liposome-strip detection may be useful for field studies and environmental testing because these methods are rapid and do not require specialized equipment.

Published

2003

43. Characterization of a novel coronavirus associated with severe acute respiratory syndrome.

Author

Rota PA, Oberste MS, Monroe SS, Nix WA, Campagnoli R, Icenogle JP, Peñaranda S, Bankamp B, Maher K, Chen MH, Tong S, Tamin A, Lowe L, Frace M, DeRisi JL, Chen Q, Wang D, Erdman DD, Peret TC, Burns C, Ksiazek TG, Rollin PE, Sanchez A, Liffick S, Holloway B, Limor J, McCaustland K, Olsen-Rasmussen M, Fouchier R, Günther S, Osterhaus AD, Drosten C, Pallansch MA, Anderson LJ, and Bellini WJ

Subjects

Amino Acid Sequence, Conserved Sequence, Coronavirus classification, Coronavirus genetics, Coronavirus M Proteins, Coronavirus Nucleocapsid Proteins, DNA, Complementary, Endopeptidases chemistry, Endopeptidases genetics, Humans, Membrane Glycoproteins chemistry, Membrane Glycoproteins genetics, Molecular Sequence Data, Nucleocapsid Proteins chemistry, Nucleocapsid Proteins genetics, Open Reading Frames, Phylogeny, Polyproteins chemistry, Polyproteins genetics, RNA, Messenger genetics, RNA, Messenger metabolism, RNA-Dependent RNA Polymerase chemistry, RNA-Dependent RNA Polymerase genetics, Regulatory Sequences, Nucleic Acid, Severe acute respiratory syndrome-related coronavirus chemistry, Severe acute respiratory syndrome-related coronavirus classification, Severe acute respiratory syndrome-related coronavirus isolation & purification, Sequence Analysis, DNA, Severe Acute Respiratory Syndrome virology, Spike Glycoprotein, Coronavirus, Transcription, Genetic, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Viral Matrix Proteins chemistry, Viral Matrix Proteins genetics, Viral Proteins chemistry, Genome, Viral, RNA, Viral genetics, Severe acute respiratory syndrome-related coronavirus genetics, Viral Proteins genetics

Abstract

In March 2003, a novel coronavirus (SARS-CoV) was discovered in association with cases of severe acute respiratory syndrome (SARS). The sequence of the complete genome of SARS-CoV was determined, and the initial characterization of the viral genome is presented in this report. The genome of SARS-CoV is 29,727 nucleotides in length and has 11 open reading frames, and its genome organization is similar to that of other coronaviruses. Phylogenetic analyses and sequence comparisons showed that SARS-CoV is not closely related to any of the previously characterized coronaviruses.

Published

2003

44. International collaborative study to compare reverse transcriptase PCR assays for detection and genotyping of noroviruses.

Author

Vinjé J, Vennema H, Maunula L, von Bonsdorff CH, Hoehne M, Schreier E, Richards A, Green J, Brown D, Beard SS, Monroe SS, de Bruin E, Svensson L, and Koopmans MP

Subjects

Caliciviridae Infections diagnosis, Caliciviridae Infections virology, DNA Primers, Europe, Feces virology, Gastroenteritis virology, Genotype, Humans, Norovirus classification, Norovirus genetics, RNA, Viral analysis, RNA, Viral isolation & purification, Sensitivity and Specificity, Sequence Analysis, DNA, Gastroenteritis diagnosis, International Cooperation, Laboratories, Norovirus isolation & purification, Reverse Transcriptase Polymerase Chain Reaction methods, Reverse Transcriptase Polymerase Chain Reaction standards

Abstract

To allow more rapid and internationally standardized assessment of the spread of noroviruses (previously called Norwalk-like viruses [NLVs]) as important food-borne pathogens, harmonization of methods for their detection is needed. Diagnosis of NLVs in clinical diagnostic laboratories is usually performed by reverse transciptase PCR (RT-PCR) assays. In the present study, the performance of five different RT-PCR assays for the detection of NLVs was evaluated in an international collaborative study by five laboratories in five countries with a coded panel of 91 fecal specimens. The assays were tested for their sensitivity, detection limit, and ease of standardization. In total, NLVs could be detected by at least one RT-PCR assay in 69 (84%) of the samples that originally tested positive. Sensitivity ranged from 52 to 73% overall and from 54 to 100% and 58 to 85% for genogroup I and II viruses, respectively. In all, 64% of the false-negative results were obtained with a set of diluted stools (n = 20) that may have lost quality upon storage. Sensitivity was improved when these samples were excluded from analysis. No one single assay stood out as the best, although the p1 assay demonstrated the most satisfactory overall performance. To promote comparability of data, this assay will be recommended for newly starting groups in future collaborative studies.

Published

2003

45. Foodborne viral gastroenteritis: challenges and opportunities.

Author

Bresee JS, Widdowson MA, Monroe SS, and Glass RI

Subjects

Caliciviridae Infections immunology, Caliciviridae Infections physiopathology, Caliciviridae Infections prevention & control, Cost of Illness, Forecasting, Gastroenteritis immunology, Gastroenteritis physiopathology, Gastroenteritis prevention & control, Humans, Caliciviridae Infections transmission, Food Contamination, Gastroenteritis virology, Norovirus

Abstract

Norwalk-like viruses (NLVs) are estimated to be the most common causes of foodborne disease in the United States, accounting for two-thirds of all food-related illnesses. The epidemiologic features and disease burden associated with NLVs have, until recently, been poorly understood because of the lack of sensitive detection assays and the underuse of available diagnostic tools. However, the application of molecular techniques to diagnose and investigate outbreaks of infection during recent years has led to a growing appreciation of the importance of these agents. NLVs are a principal cause of outbreaks of acute-onset vomiting and diarrhea in all age groups-most commonly, via contamination of uncooked foods by infected foodhandlers, but also via foods contaminated at their sources, such as oysters and raspberries. NLVs may also account for >10% of sporadic cases of gastroenteritis in children and adults. Future research will focus on the development of easy-to-use diagnostic assays based on antigen and antibody detection as well as vaccine development. Implementation of simple prevention measures, including correct food-handling practices, will continue to be a priority.

Published

2002

46. Norwalk-like virus-associated gastroenteritis in a large, high-density encampment--Virginia, July 2001.

Author

Cheek JE, Young P, Branch L, Dupnik KM, Kelly ST, Sharp JM, Toney DM, Bresee JS, Monroe SS, Beard RS, Bulens S, and Leman R

Subjects

Caliciviridae Infections diagnosis, Camping, Gastroenteritis epidemiology, Humans, Virginia epidemiology, Caliciviridae Infections epidemiology, Gastroenteritis virology, Norovirus isolation & purification

Published

2002

47. Detection and characterisation of human astroviruses in children with acute gastroenteritis in Blantyre, Malawi.

Author

Cunliffe NA, Dove W, Gondwe JS, Thindwa BD, Greensill J, Holmes JL, Bresee JS, Monroe SS, Glass RI, Broadhead RL, Molyneux ME, and Hart CA

Subjects

Acute Disease, Astroviridae Infections complications, Astroviridae Infections pathology, Child, Preschool, Female, Gastroenteritis complications, Gastroenteritis pathology, Genotype, HIV Infections complications, Humans, Infant, Malawi epidemiology, Male, Mamastrovirus classification, Reverse Transcriptase Polymerase Chain Reaction, Risk Factors, Astroviridae Infections epidemiology, Astroviridae Infections virology, Gastroenteritis epidemiology, Gastroenteritis virology, Mamastrovirus genetics, Mamastrovirus isolation & purification

Abstract

In a 2-year hospital-based study of paediatric gastroenteritis in Blantyre, Malawi, astroviruses were detected by enzyme immunoassay in 15 (1.9%) of 786 inpatients and in 9 (2.3%) of 400 outpatients. Greater disease severity was noted in children coinfected with human immunodeficiency virus (HIV). Six human astrovirus (HAstV) genotypes were identified, including HAstV-1 (25%), HAstV-2 (21%), HAstV-3 (25%), HAstV-4 (13%), HAstV-5 (4%), and HAstV-8 (13%). Although astroviruses are not major causes of gastroenteritis among children admitted to hospital in Blantyre, concomitant HIV infection appears to be a risk factor for increased severity of disease., (Copyright 2002 Wiley-Liss, Inc.)

Published

2002

48. Determination of a universal nucleic acid extraction procedure for PCR detection of gastroenteritis viruses in faecal specimens.

Author

Rasool NB, Monroe SS, and Glass RI

Subjects

Adenoviruses, Human genetics, Adenoviruses, Human isolation & purification, Animals, Cell Line, Chloroform, Diarrhea virology, Genome, Viral, Humans, Macaca mulatta, Mamastrovirus genetics, Mamastrovirus isolation & purification, Phenol, Polymerase Chain Reaction methods, RNA, Double-Stranded isolation & purification, Rotavirus genetics, Rotavirus isolation & purification, Tumor Cells, Cultured, Adenovirus Infections, Human virology, Astroviridae Infections virology, DNA, Viral isolation & purification, Feces virology, Gastroenteritis virology, RNA, Viral isolation & purification, Rotavirus Infections virology

Abstract

Four nucleic acid extraction protocols were examined for their suitability for extraction of the ssRNA, dsRNA and dsDNA genomes of gastroenteritis viruses, for PCR detection. Protocol (A), employed specimen lysis with guanidinium thiocyanate, extraction with phenol-chloroform-isoamyl alcohol and nucleic acid purification by size-fractionated silica particles. Protocol (B), utilised specimen lysis with guanidinium thiocyanate and nucleic acid purification by silica, followed by phenol-chloroform-isoamyl alcohol extraction. Protocol (C), employed specimen lysis with guanidinium thiocyanate and nucleic acid purification by RNAID glass powder. Protocol (D), employed specimen lysis with sodium dodecyl sulphate, proteinase K digestion and extraction with phenol-chloroform-isoamyl alcohol. Of the four protocols, (B) appeared to be a suitable candidate 'universal' nucleic acid extraction procedure for PCR detection of different viral agents of gastroenteritis in a single nucleic acid extract of a faecal specimen, irrespective of genome composition. Omission of the phenol-chloroform extraction step did not affect negatively the ability of protocol (B) to allow PCR detection of gastroenteritis viruses in faecal specimens. PCR detection of NLVs, astroviruses, rotaviruses and adenoviruses, in single nucleic acid extracts of faecal specimens obtained from the field, confirmed the universality of the modified protocol (B). We propose the modified protocol (B) as a 'universal' nucleic acid extraction procedure, for monoplex PCR detection of gastroenteritis viruses in single nucleic acid extracts of faecal specimens and for development of multiplex PCR for their simultaneous detection.

Published

2002

49. Norwalk virus gastroenteritis among Israeli soldiers: lack of evidence for flyborne transmission.

Author

Cohen D, Monroe SS, Haim M, Slepon R, Ashkenazi I, Estes MK, and Glass RI

Subjects

Adolescent, Adult, Animals, Caliciviridae Infections epidemiology, Caliciviridae Infections virology, Capsid genetics, Capsid immunology, Humans, Insect Control, Israel epidemiology, Male, Recombinant Proteins genetics, Recombinant Proteins immunology, Antibodies, Viral blood, Caliciviridae Infections transmission, Capsid Proteins, Diptera virology, Gastroenteritis virology, Military Personnel, Norwalk virus immunology

Abstract

Background: Paired sera collected from subjects before and after a fly-control intervention trial conducted in the Israel Defense Force (IDF) were tested for seroconversion to Norwalk virus (NV) to examine the role of NV as a cause of diarrhea in this population and to ascertain whether flies might also be implicated in transmission., Materials and Methods: An enzyme-linked immunosorbent assay (ELISA), using recombinant NV capsid proteins (rNV) as antigen was employed to determine the seroconversion rate in a sample of 444 subjects., Results: During 11-week field training cycles, 18% of IDF soldiers who were tested had an NV infection defined as a > or = 4-fold rise in antibody, yielding a cumulative incidence of nearly one infection (0.95) per soldier per year. The rate of seroconversion was nearly twice as high among soldiers who recalled having diarrhea as among those who did not, but the rates did not differ significantly between soldiers in the fly intervention areas and those in the control areas., Conclusion: NV is a common cause of enteric infections and diarrhea among Israeli soldiers who serve under field conditions, but unlike infections with Shigella and enterotoxigenic Escherichia coli, transmission of NV cannot be interrupted with an aggressive program of fly-control.

Published

2002

50. Characterization of capsid genes, expressed in the baculovirus system, of three new genetically distinct strains of "Norwalk-like viruses".

Author

Belliot G, Noel JS, Li JF, Seto Y, Humphrey CD, Ando T, Glass RI, and Monroe SS

Subjects

Amino Acid Sequence, Animals, Antibodies, Viral blood, Antigens, Viral genetics, Antigens, Viral immunology, Antigens, Viral metabolism, Baculoviridae genetics, Caliciviridae Infections epidemiology, Caliciviridae Infections immunology, Caliciviridae Infections virology, Capsid immunology, Capsid metabolism, Gastroenteritis immunology, Gastroenteritis virology, Humans, Molecular Sequence Data, Norovirus genetics, Norovirus immunology, Recombination, Genetic, Spodoptera, Baculoviridae metabolism, Capsid genetics, Disease Outbreaks, Gastroenteritis epidemiology, Norovirus classification, Virion metabolism

Abstract

"Norwalk-like viruses" (NLVs), members of a newly defined genus of the family Caliciviridae, are the most common agents of outbreaks of gastroenteritis in the United States. Two features of NLVs have hindered the development of simple methods for detection and determination of serotype: their genetic diversity and their inability to grow in cell culture. To assess the immune responses of patients involved in outbreaks of gastroenteritis resulting from infection with NLVs, we previously used recombinant-expressed capsid antigens representing four different genetic clusters, but this panel proved insufficient for detection of an immune response in many patients. To extend and further refine this panel, we expressed in baculovirus the capsid genes of three additional genetically distinct viruses, Burwash Landing virus (BLV), White River virus (WRV), and Florida virus. All three expressed proteins assembled into virus-like particles (VLPs) that contained a full-length 64-kDa protein, but both the BLV and WRV VLPs also contained a 58-kDa protein that resulted from deletion of 39 amino acids at the amino terminus. The purified VLPs were used to measure the immune responses in 403 patients involved in 37 outbreaks of acute gastroenteritis. A majority of patients demonstrated a fourfold rise in the titer of immunoglobulin G to the antigen homologous to the outbreak strain, but most seroconverted in response to other genetically distinct antigens as well, suggesting no clear pattern of type-specific immune response. Further study of the antigenicity of the NLVs by use of VLPs should allow us to design new detection systems with either broader reactivity or better specificity and to define the optimum panel of antigens required for routine screening of patient sera.

Published

2001