3.Research Progress in Norovirus Bioaccumulation in Shellfish.
Deqing ZHOU ; Laijin SU ; Feng ZHAO ; Liping MA
Chinese Journal of Virology 2015;31(3):313-317
Noroviruses (NoVs) are one of the most important foodborne viral pathogens worldwide. Shellfish are the most common carriers of NoVs as they can concentrate and accumulate large amounts of the virus through filter feeding from seawater. Shellfish may selectively accumulate NoVs with different genotypes, and this bioaccumulation may depend on the season and location. Our previous studies found various histo-blood group antigens (HBGAs) in shellfish tissues. While HBGAs might be the main reason that NoVs are accumulated in shellfish, the detailed mechanism behind NoV concentration and bioaccumulation in shellfish is not clear. Here we review current research into NoV bioaccumulation, tissue distribution, seasonal variation, and binding mechanism in shellfish. This paper may provide insight into controlling NoV transmission and decreasing the risks associated with shellfish consumption.
Animals
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Caliciviridae Infections
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transmission
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virology
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Food Contamination
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analysis
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Foodborne Diseases
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virology
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Humans
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Norovirus
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classification
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genetics
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isolation & purification
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physiology
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Shellfish
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virology
4.Colorimetric detection of norovirus genotype GII by reverse transcription loop-mediated isothermal amplification.
Jian-Ming LUO ; Xi-Yang WU ; Zi-Qian XU ; Le LUO ; Kai NIE ; Meng-Jie YANG ; Ya-Lan ZENG ; Zhao-Jun DUAN ; Xue-Jun MA
Chinese Journal of Virology 2012;28(2):165-171
A simple, rapid and sensitive colorimetric reverse transcription loop-mediated isothermal amplification (RT-LAMP) method was established to detect norovirus genotype GII. The method employed a set of six specially designed primers that recognized eight distinct sequences of RNA-dependant RNA polymerase and capsid protein gene for amplification of nucleic acid under isothermal conditions at 65 degrees C for 60 minutes. The amplification process of RT-LAMP was monitored by the addition of HNB (Hydroxy naphthol blue) dye prior to amplification. A positive reaction was indicated by a color change from violet to sky blue and confirmed by agarose electrophoresis. The specificity of the RT-LAMP was validated by detecting several different diarrhea viruses including norovirus genotype GII. The sensitivity was determined by serial dilutions of RNA molecules from in vitro transcription of norovirus genotype GII in parallel with conventional RT-PCR detection. The assay was further evaluated with 93 clinical specimens of diarrhea patients. The results showed that the sensitivity of RT-LAMP was 1 000 copies/microL with a high specificity and the relative sensitivity was at the same level as that of conventional RT-PCR. Positive rate of RT-LAMP in analysis of clinical specimens was approximately the same as that of conventional RT-PCR as well. This colorimetric RT-LAMP assay was potential for rapid detection of norovirus genotype GII on spot due to the observation of visual result with high specificity and sensitivity, time-saving and cost benefit.
Caliciviridae Infections
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diagnosis
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virology
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Colorimetry
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methods
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Feces
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virology
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Genotype
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Humans
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Norovirus
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genetics
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isolation & purification
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Nucleic Acid Amplification Techniques
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methods
5.Molecular epidemiology of noroviruses in Shenzhen in 2006.
Ya-qing HE ; Bin FENG ; Hai-long ZHANG
Chinese Journal of Epidemiology 2009;30(11):1214-1215
6.The molecular epidemiology characteristics of norovirus in environment and clinical samples in Guangzhou from 2009 to 2011.
Lan LUO ; Xin-wei WU ; Yu-fei LIU ; Qiao-yan LI ; Hua-ping XIE ; Ye-jian WU ; Lei LI ; Li-yun JIANG ; Xia YANG
Chinese Journal of Preventive Medicine 2013;47(1):40-43
OBJECTIVETo investigate the molecular epidemiological characteristics of norovirus in Guangzhou from 2009 to 2011.
METHODSA total of 183 water samples, 1162 seafood samples and 1066 diarrhea stool specimens were collected from January 2010 to May 2011, June 2009 to June 2011 and July 2009 to December 2010 respectively in Guangzhou. Norovirus was detected by real time reverse transcript-PCR (qRT-PCR). The partial polymerase gene was amplified from norovirus positive samples, then sequenced and compared with the sequences of norovirus in GenBank. The phylogenetic tree was created.
RESULTSThe positive rate was 19.67% (36/183), 8.26% (96/1162) and 37.05% (395/1066) in water samples, seafood and diarrhea patients respectively. Noroviruses from positive samples could be divided into 10 representative strains, in which 7 representative strains of genotype of 208 samples was type G2-4. The sequences from water, seafood and stool specimens were highly homologous with the similarity of 94% - 100%.
CONCLUSIONIn Guangzhou, the predominant Norovirus genotype was G2-4 and the positive rate of samples was high.
Base Sequence ; Caliciviridae Infections ; epidemiology ; virology ; China ; epidemiology ; Diarrhea ; virology ; Genotype ; Humans ; Molecular Epidemiology ; Norovirus ; classification ; genetics ; isolation & purification ; Phylogeny ; RNA, Viral ; genetics ; Seafood ; virology ; Water Microbiology
7.Epidemic and control strategy on nosocomial outbreak of norovirus gastroenteritis.
Acta Academiae Medicinae Sinicae 2008;30(5):614-617
Noroviruses are the leading cause of acute viral gastroenteritis in human beings and frequently cause the outbreaks of nosocomial infections. Based on the pathogenic characteristics of noroviruses, this article describes the epidemiological and clinical characteristics of norovirus gastroenteritis outbreak in hospital and explores the measures to prevent and control the nosocomial outbreak.
Caliciviridae Infections
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epidemiology
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prevention & control
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virology
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Cross Infection
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epidemiology
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prevention & control
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virology
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Disease Outbreaks
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Gastroenteritis
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epidemiology
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prevention & control
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virology
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Humans
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Infection Control
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Norovirus
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physiology
8.Systematic review on the characteristics of acute gastroenteritis outbreaks caused by sapovirus.
Y YU ; X H GUO ; H Q YAN ; Z Y GAO ; W H LI ; B W LIU ; Q Y WANG
Chinese Journal of Epidemiology 2019;40(1):93-98
Objective: To understand the epidemiological and etiological characteristics of outbreaks on acute gastroenteritis caused by sapovirus (SaV) worldwide. Methods: Literature about the outbreaks on acute gastroenteritis caused by SaV were retrieved from the databases including WanFang, CNKI, PubMed and Web of Science after evaluation. Time, geography, setting and population distributions of outbreaks, transmission mode, SaV genotype and clinical characteristics of the patients were analyzed. Results: A total of 34 papers about SaV were included, involving 146 outbreaks occurred between October 1976 and April 2016. In these papers, 138 outbreaks were reported on the related months. All these outbreaks occurred in northern hemisphere. SaV outbreaks occurred all year around, but mainly in cold season, the incidence was highest in December (25 outbreaks) and lowest in in August (2 outbreaks). Most outbreaks were reported by Japan, followed by Canada, the United States of America and the Netherlands. There were 141 outbreaks for which the occurring settings were reported, child-care settings were most commonly reported setting (48/141, 34.04%), followed by long-term care facility (41/141, 29.08%) and hospital (16/141, 11.35%). Clinical symptoms of 1 704 cases in 31 outbreaks were reported, with the most common symptom was diarrhea (1 331/1 704, 78.12%), followed by nausea (829/1 198, 69.20%), abdominal pain (840/1 328, 63.25%), vomiting (824/1 704, 48.36%) and fever (529/1 531, 34.53%). Genotypes of SaV were determined for 119 outbreaks. GⅠ(51/119, 42.86%) and GⅣ (45/119, 37.82%) were predominant. The outbreaks of GⅣ SaV increased suddenly in 2007, and the outbreaks of GⅠ SaV mainly occurred in 2008 and during 2011-2013. Conclusions: SaV outbreaks were reported mainly by developed countries, with most outbreaks occurred in cold season, in child-care settings and long term care facility. GⅠ and GⅣ were the most common genotypes of SaV. Prevention and control of SaV outbreak in China seemed relatively weak, and it is necessary to conduct related training and to strengthen the SaV outbreak surveillance in areas where service is in need.
Caliciviridae Infections/virology*
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Child
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China/epidemiology*
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Disease Outbreaks
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Feces/virology*
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Gastroenteritis/virology*
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Genotype
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Humans
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Phylogeny
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RNA, Viral/genetics*
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Sapovirus/isolation & purification*
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Sequence Analysis, DNA
10.Prevalence of feline herpesvirus 1, feline calicivirus and Chlamydophila felis in clinically normal cats at a Korean animal shelter.
Byeong Teck KANG ; Hee Myung PARK
Journal of Veterinary Science 2008;9(2):207-209
The prevalence of feline herpesvirus-1 (FHV-1), feline calicivirus (FCV), and Chlamydophila (C.) felis was studied in cats of an animal shelter in Korea. Total 78 cats without ocular and upper respiratory tract disease were examined. Specimens were obtained from ocular conjunctiva and oropharynx. Using multiplex polymerase chain reaction (PCR) and reverse transcription PCR, three pathogens were simultaneously detected. In examined 78 cats, 49 (63%) cats were positive for FHV-1. However, all specimens were negative for C. felis and FCV. In conclusion, many cats recovered from FHV-1 infection remain subclinical carriers in shelter environment.
Animals
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Caliciviridae/genetics
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Caliciviridae Infections/epidemiology/*veterinary
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Cat Diseases/*epidemiology/*microbiology/*virology
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Cats
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Chlamydophila/genetics
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Chlamydophila Infections/epidemiology/*veterinary
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DNA Primers/genetics
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Herpesviridae/genetics
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Herpesviridae Infections/epidemiology/*veterinary
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Housing, Animal
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Korea/epidemiology
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Prevalence
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Reverse Transcriptase Polymerase Chain Reaction