2009年嘉兴市食源性病原菌监测分析

目的监测2009年嘉兴市食品中致病菌污染状况。方法共采集275份生熟食品样品,分离沙门菌、单核细胞增生李斯特菌、大肠杆菌O157:H7、金黄色葡萄球菌和副溶血性弧菌。结果 75份生肉、水产品食源性病原菌总污染率45.3%,其中检出沙门菌6株,单核细胞增生李斯特菌12株,金黄色葡萄球菌4株,副溶血性弧菌18株。未检出大肠杆菌O157:H7。200份即食食品总污染率3.0%,以金黄色葡萄球菌污染为主。结论 2009年嘉兴市主要污染食品品种是冷藏冷冻生肉,污染的食源性致病菌以单核细胞增生李斯特菌和副溶血性弧菌为主。     

食品中单核细胞增生李斯特氏菌调查及毒力研究

为了解和掌握各类食品中单核细胞增生李斯特氏菌（Lm)污染状况及菌株的毒力情况,采集5类265件食品,菌株鉴定应用API细胞鉴定系统;毒力测定采用溶血实验、多聚酶链反应（PCR）以及小鼠致病力实验的方法进行,结果显示Lm检出率为4.90%;其中从生肉、熟肉、灌汤和速冻食品中的检出率分别为15.00%、2.48%、9.52%;从熟肉和速冻食品中还检出其它李斯特氏菌,检出率分别为4.96%、5.92%;乳制品和水产品中未检出Lm。13株Lm毒力测定显示,溶血实验与小鼠的致病力和PCR测定的溶血素基因无必然联系,而溶血素基因与内化素基因阳性结果相同,Lm对多种抗生素敏感,其中对氨氨苄青霉素、头孢唑啉和环丙沙星敏感率为100%。     

食品中单核增生性李斯特菌(Listeria monocytogenes) 污染状况研究

目的:了解食品中单核增生性李斯特菌(Listeria monocytogenes)的污染状况,为单增李斯特茵病的监控、检测以及追踪污染源提供依据.方法:对采自保定市各大超市及农贸市场的生内、熟肉制品、海产品、速冻食品、水果、蔬菜、奶及奶制品、豆制品、腌制品等9大类食品426份样品进行单增李斯特茵的分离与鏊定.结果:检出了单增李斯特茵79株,英诺克李斯特茵7株,格氏李斯特茵32株,西尔李斯特茵2株,威尔斯李斯特茵1株,绵羊李斯特茼1株.默氏李斯特茵2株.李斯特茵的总检出率为29.1%,其中单增李斯特茵的检出率为18.5%.结论:保定市9大类食品中存在不同程度的单增李斯特茵污染,尤其在生内中该茵的污染率高达32.4%.海产品中的污染率31.0%.应引起高度重视.     

食品中单核细胞增生性李斯特氏菌PCR快速检测方法

为建立食品中单核细胞增生性李斯特氏菌 (单增李斯特氏菌 )的快速、敏感、特异的PCR检测方法 ,选取hlyA基因作为靶序列设计一对引物 ,用该引物对 6 3株从国内食品中分离的李斯特氏菌 (进行传统方法验证 )和 2 0株非李斯特氏菌进行PCR扩增 ,并用此方法对人工污染食品进行检测 ,扩增片段表现出极好的单增李斯特氏菌种特异性 ,人工污染的生肉、冷冻虾仁、卷心菜的检出限为 39cfu g ,为食品中单增李斯特氏菌的快速、敏感并且特异的检测方法。     

实时荧光PCR定量检测食品中单增李斯特菌

目的建立快速、敏感、特异的食品中单增李斯特菌检测方法。方法针对单增李斯特菌溶素A基因（hlyA）设计一对引物和一条探针，并用该引物和探针运用实时荧光PCR技术对单增李斯特菌的DNA、细胞、质粒和样品进行实时荧光PCR定量检测。结果利用实时荧光PCR技术，建立了DNA校正曲线、细胞校正曲线和质粒校正曲线。DNA校正曲线在1～32CFU/ml、细胞校正曲线在32—320CFU／ml、质粒校正曲线在1—37Copies／ml，线形关系良好，且三种校正曲线检测样品得出的结果基本吻合。结论本试验建立起来的实时荧光PCR定量检测单增李斯特菌的方法灵敏度高、特异性好、准确，可应用于食品中单增李斯特菌的检测。     

云南淡水鱼中单增李斯特氏菌污染状况及耐药性分析

目的了解云南淡水鱼中单增李斯特氏菌污染状况及耐药情况。方法从云南省昆明市、曲靖市、大理州、红河州4个淡水鱼主产区采集淡水鱼样品110件,参照GB 4789.30—2016《食品安全国家标准食品微生物学检验单核细胞增生李斯特氏菌检验》分离鉴定单增李斯特氏菌,并进一步开展16S rRNA序列鉴定和同源性分析,对鉴定菌株采用微量肉汤稀释法分析抗生素敏感性。结果110件样品检出2株单增李斯特氏菌(DZ-054、DZ-101),检出率为1.82%。2株单增李斯特氏菌之间相似度达到99.64%。DZ-101菌株对氨苄西林、青霉素敏感(S),DZ-054菌株对抗生素不敏感。结论云南省淡水鱼中单增李斯特菌的污染率较低,但仍有一定的安全隐患,相关部门应加强监管。     

食品中单增李斯特氏菌检测PCR-免疫胶体金试纸条方法的建立

目的建立食品中单核增生李斯特氏菌快速检测PCR-免疫胶体金试纸条法。方法通过设计特异性引物建立单增李斯特氏菌检测PCR方法并使用免疫胶体金技术建立PCR产物快速检测试纸条;用试验菌株检测PCR-免疫胶体金试纸条方法的检测特异度与敏感度。使用新建方法对市售肉制品和乳制品中单核增生李斯特氏菌进行检测,验证该方法在食品检测中的可行性。结果 PCR-免疫胶体金法具有良好的特异度,敏感度比标准琼脂糖凝胶电泳法高100倍。采集乳品样品131份,阳性样品1份,检出率1.53%;肉制品224份,阳性样品4份,检测率1.79%。结论建立的单增李斯特氏菌检测PCR-免疫胶体金试纸条法特异度好,敏感度高,适用于食品中单增李斯特氏菌的检测。     

食品中单核增生性李斯特菌的PCR快速检测研究

为提高食品中单增李斯特菌的检测水平,针对单增李斯特菌中多个稳定的特异性基因hlyA、plcB、prfA、iap,设计并筛选出7对引物组成多重-巢式PCR联合检测体系,并结合高灵敏性的聚丙烯酰胺凝胶电泳,对单增李斯特菌进行快速检测,多重PCR的灵敏度达到1×102CFU ml,巢式PCR的灵敏度达到1×10CFU ml。结果表明该检测体系具有快速可靠、灵敏准确及特异性好的特点,而且有效缩短了检验周期,从传统的7～14d缩短到1～2d。     

食品中单增李斯特氏菌检测PCR-免疫胶体金 试纸条方法的建立

目的 建立食品中单核增生李斯特氏菌快速检测PCR-免疫胶体金试纸条法。方法 通过设计特异性引物建立单增李斯特氏菌检测PCR方法并使用免疫胶体金技术建立PCR产物快速检测试纸条; 用试验菌株检测PCR-免疫胶体金试纸条方法的检测特异度与敏感度。使用新建方法对市售肉制品和乳制品中单核增生李斯特氏菌进行检测, 验证该方法在食品检测中的可行性。结果 PCR-免疫胶体金法具有良好的特异度, 敏感度比标准琼脂糖凝胶电泳法高100倍。采集乳品样品131份, 阳性样品1份, 检出率1.53%; 肉制品224份, 阳性样品4份, 检测率1.79%。结论 建立的单增李斯特氏菌检测PCR-免疫胶体金试纸条法特异度好, 敏感度高, 适用于食品中单增李斯特氏菌的检测。     

上海市市售带壳牡蛎微生物污染状况调查

目的了解上海市市售带壳牡蛎的微生物污染状况。方法2005年4月至2006年3月在上海市水产品批发市场每月2次采集牡蛎样品,共抽取了24份。按照GB/T4789—2003《食品卫生微生物学检验》中检验规程进行微生物检测。结果所有抽检样品均不合格,污染最严重的是大肠菌群,所检样品均超标,最高污染量达1·4×106MPN/g;其次是菌落总数,超标率达41·7%,最高污染量达2·6×107CFU/g;副溶血性弧菌污染也比较严重,检出率达29·2%,污染量在3·0×102~7·4×102MPN/100g;单核细胞增生李斯特菌未检出。结论上海市市售带壳牡蛎的微生物污染状况不容乐观,已对消费者健康构成了潜在威胁。     

Occurrence and distribution of listeria species in facilities producing ready-to-eat foods in British Columbia, Canada

In British Columbia (BC), Canada, food processing facilities licensed under provincial authority are not required to sample for Listeria monocytogenes in food products or processing environments. In 2009, we conducted a survey of dairy, fish, and meat facilities under BC authority to estimate the prevalence of Listeria spp. and L. monocytogenes in ready-to-eat (RTE) foods and production environments. From August to October, 250 RTE food samples and 258 swabs from the food processing environments of 43 facilities were collected. Standard culture methods were applied to both food samples and swabs. Of swabs collected from all 258 environmental surfaces, 15% were positive for Listeria spp. Significantly (P, 0.001) more fish facilities than dairy and meat facilities had food contact surfaces contaminated with Listeria spp. L. monocytogenes was found in RTE foods from fish facilities alone (5 of 12); in all five of the fish facilities with contaminated product, one or more environmental swabs were also positive for L. monocytogenes. The results suggest that while control of L. monocytogenes in BC-inspected dairy and meat facilities is effective in limiting food contamination, there is a need for provincial inspectors to initiate improved monitoring and management of contamination by L. monocytogenes in RTE fish processing facilities.     

Incidence and characterization of Listeria spp. from foods available in Korea

A total of 410 domestic Korean food samples were analyzed for the presence of Listeria spp. by the conventional U.S. Department of Agriculture protocol, and presumptive strains were identified by morphological, cultural and biochemical tests according to Bergey's manual and confirmed by API-Listeria kit. Among the total 410 food samples, 46 samples (11.2%) were found to be contaminated with Listeria species. Among the 46 strains of Listeria spp. isolates, 8 strains (17.42%) for Listeria monocytogenes, 3 strains (6.5%) for Listeria seeligeri, 33 strains (71.7%) for Listeria innocua, and 2 strains (4.4%) for Listeria welshimeri were identified, respectively. Also, only beef, chicken, pork, frozen foods, and sausage were contaminated with L. monocytogenes, and the other products were free of L. monocytogenes. Of 46 Listeria spp. isolates, L. innocua (71.7%) was the most predominantly isolated in a variety of foods compared to other Listeria spp. An in vitro virulence assay for Listeria spp. using myeloma and hybridoma cells from murine and human sources was performed. The result showed that only L. monocytogenes killed approximately 95 to 100% hybridoma cells after 6 h and the other Listeria species, such as L. innocua, L. seeligeri, and L. welshimeri strains had about 0 to 10% lethal effect on hybridoma cells. Also, an antibiotic susceptibility test showed that Listeria spp. isolates were very susceptible to the antibiotics tested, except for nalidixic acid. Also, serotyping results showed 75% of L. monocytogenes isolates from beef, chicken, and frozen pizza belonged to serotype 1 and 25% from sausage were type 4.     

新疆食源性单增李斯特菌监测及血清型分析

目的 了解新疆食品中单增李斯特菌的污染状况,为食源性疾病的监测提供科学依据。方法 按照GB 4789.30和^,监测分析了2013-2019年的3329份样品。结果 共检出59份单增李斯特菌阳性样品,检出率为1.78%;共分离得到63株单增李斯特菌,分为4个血清型(1/2a、1/2b、1/2c和4b),优势血清型为1/2a,占57.14%(36株)。食品中存在不同血清型混合污染,尤其在即食食品中监测到4b型。结论 ^{新疆食品中存在单增李斯特菌的污染,卫生监督部门尤其要加强肉制品和即食食品的监管力度。}      

2011~2019年吉林省市售食品中单增李斯特菌污染情况分析

目的 了解吉林省市售餐饮食品中单增李斯特菌的污染情况,为食品安全管理、食源性疾病的监测提供科学依据。方法 对2011年-2019年从吉林省9个监测地区采集到的8279件市售食品样本进行单增李斯特菌的分离鉴定。结果 2011年 -2019年从吉林省市售食品中共检测出单增李斯特菌阳性菌株352株,总检出率4.25%；各检测地区间长春市阳性检出率最高(7.63%),其次为四平市(6.03%)；12类市售食品中肉及肉质品阳性检出率最高(9.41%),其次为速冻米面食品(6.72%)；各类采样地点中超市的阳性检出率最高(6.89%),其次为农贸市场(5.64%)和快餐店(5.08%)；散装食品的阳性检出率明显高于预包装食品。结论 2019年吉林省的单增李斯特菌阳性检出率较临近三年呈回升态势；长春市与四平市单增李斯特菌污染情况较其他地区严重；肉与肉制品单增李斯特菌的污染情况最为严重,其次为速冻米面食品；流通环节中单增李斯特菌阳性检出率较高；散装食品的单增李斯特菌污染情况较预包装食品严重。有关部门应针对地区现状、食品类型和包装类型的不同加强管理力度。     

食品中单核细胞增生李斯特菌株的分离及聚合酶链式反应鉴定

目的 建立单核细胞增生李斯特菌的聚合酶链式反应(PCR)检测方法,了解市售食品中单核细胞增生李斯特菌的污染情况.方法 采集成都市市售生畜肉、生禽肉、熟肉制品、水产品、生食蔬菜以及其他熟食等食品样品共135份,采用李氏增菌肉汤(LB1,LB2)进行初增菌,应用选择性分离培养基PALCAM和在TSA-YE平板上进行分离,利用单增李斯特显色平板进行鉴定;根据李斯特菌的特异性基因iap基因设计引物,采用PCR方法检测所有分离的李斯特菌株;根据单增李斯特菌的特异性基因hly基因和prfA基因设计引物检测单核细胞增生李斯特菌株.结果 135份样品中共检出李斯特菌17株,检出率为12.6％;其中单核细胞增生李斯特菌4株,检出率为3.0％.结论 本研究建立的PCR方法具有特异性,本市市售食品不同程度受到李斯特菌的污染.     

An 8-year surveillance of the diversity and persistence of Listeria monocytogenes in a chilled food processing plant analyzed by amplified fragment length polymorphism

Contamination routes of Listeria monocytogenes were examined in a chilled food processing plant that produced ready-to-eat and ready-to-reheat meals during an 8-year period by amplified fragment length polymorphism (AFLP) analysis. A total of 319 L. monocytogenes isolates were recovered from raw materials (n = 18), the environment (n = 77), equipment (n = 193), and products (n = 31), and 18 different AFLP types were identified, five of which were repeatedly found to be persistent types. The three compartments (I to III) of the plant showed markedly different contamination statuses. Compartment I, which produced cooked meals, was heavily contaminated with three persistent AFLP types. AFLP type A1 dominated, and it comprised 93% of the isolates of the compartment. Compartment II, which produced uncooked chilled food, was contaminated with four persistent and five nonpersistent AFLP types. The equipment of compartment III, which produced cooked ready-to-reheat meals, was free of contamination. In compartments that produced cooked meals, the cleaning routines, product types, and lack of compartmentalization seemed to predispose production lines to persistent contamination. The most contaminated lines harbored L. monocytogenes in coolers, conveyors, and packing machines. Good compartmentalization limited the flow of L. monocytogenes into the postheat-treatment area and prevented the undesired movement of equipment and personnel, thus protecting the production lines from contamination. In compartment II, grated cheese was shown to cause product contamination. Therefore, special attention should be paid to continuous quality control of raw ingredients when uncooked ready-to-eat foods are produced. In compartment II, reconstruction of the production line resulted in reduced prevalence rates of L. monocytogenes and elimination of two persistent AFLP types.     

Distribution of Listeria monocytogenes molecular subtypes among human and food isolates from New York State shows persistence of human disease--associated Listeria monocytogenes strains in retail environments

While there is considerable information available regarding Listeria monocytogenes contamination patterns in food processing plants, our understanding of L. monocytogenes contamination and transmission in retail operations is limited. We characterized 125 food, 40 environmental, and 342 human clinical L. monocytogenes isolates collected in New York State from 1997 to 2002 using automated ribotyping and hly allelic variation. All environmental isolates were obtained from retail establishments and the majority of food isolates (98 isolates) were obtained from foods that were prepared or handled at retail. Overall, food and/or environmental isolates from 50 different retail establishments were characterized. The 125 food and 40 environmental isolates were differentiated into 29 and 10 ribotypes, respectively. For 16 retail establishments, we found evidence for persistence of one or more specific L. monocytogenes strains as indicated by isolation of the same EcoRI ribotype from food or environmental samples collected in a given establishment on different days. The human isolates were differentiated into 48 ribotypes. Statistical analyses showed that two ribotypes were significantly (P < 0.0001) more common among food isolates as compared with human isolates. However, a total of 17 ribotypes found among the human clinical isolates were also found among the food and environmental isolates. We conclude that L. monocytogenes, including subtypes that have been linked to human disease, can persist in retail environments. Implementation of Listeria control procedures in retail operations, which process and handle products that permit the growth of L. monocytogenes, are thus a critical component of a farm-to-table L. monocytogenes control program.     

Molecular Subtyping and Tracking of Listeria monocytogenes in Latin-Style Fresh-Cheese Processing Plants

Latin-style fresh cheeses, which have been linked to at least 2 human listeriosis outbreaks in the United States, are considered to be high-risk foods for Listeria monocytogenes contamination. We evaluated L. monocytogenes contamination patterns in 3 Latin-style fresh-cheese processing plants to gain a better understanding of L. monocytogenes contamination sources in the manufacture of these cheeses. Over a 6-mo period, 246 environmental samples were collected and analyzed for L. monocytogenes using both the Food and Drug Administration (FDA) method and the Biosynth L. monocytogenes detection system (LMDS). Finished cheese samples from the same plants (n = 111) were also analyzed by the FDA method, which was modified to include L. monocytogenes plating medium (LMPM) and the L. monocytogenes confirmatory plating medium (LMCM) used in the LMDS method. Listeria monocytogenes was detected in 6.3% of cheese and 11.0% of environmental samples. Crates, drains, and floor samples showed the highest contamination rates, with 55.6, 30.0, and 20.6% L. monocytogenes positive samples, respectively. Finished products and food contact surfaces were positive in only one plant. The FDA method showed a higher sensitivity than the LMDS method for detection of L. monocytogenes from environmental samples. The addition of LMPM and LMCM media did not further enhance the performance of the FDA method for L. monocytogenes detection from finished products. Molecular subtyping (PCR-based allelic analysis of the virulence genes actA and hly and automated ribotyping) was used to track contamination patterns. Ribotype DUP-1044A, which had previously been linked to a 1998 multistate human listeriosis outbreak in the United States, was the most commonly identified subtype (20/36 isolates) and was isolated from 2 plants. This ribotype was persistent and widespread in one factory, where it was also responsible for the contamination of finished products. We hypothesize that this ribotype may represent a clonal group with a specific ability to persist in food processing environments. While previous listeriosis outbreaks were linked to Latin-style fresh cheeses made from unpasteurized milk, the presence of this organism in pasteurized cheese products illustrates that persistent environmental contamination also represents an important source of finished product contamination.     

Prevalence of Listeria species in food products in Isfahan, Iran

A total of 617 meat and meat products, diary, vegetables and ready to eat food samples were collected. Listeria spp. isolated by using USDA method of isolation and L. monocytogenes identified by biochemical and Polymerase Chain Reaction (PCR). The incidence of Listeria spp. was 4.6% in all food samples. L. monocytogenes was found in 1.2% of food samples. It was found that Listeria spp. was present in 6.7% of meat and meat product samples, 1.3% of diary samples, 1.2% of vegetable samples and 12% ready to eat samples. The results presented in this study indicate, the potential risk of eating ready to eat food or raw and undercooked foods.     

2011~2015年吉林省食品中单增李斯特菌的 监测数据分析

摘要：目的 掌握吉林省市售食品中单增李斯特菌污染情况,为预防食源性疾病及保障食品安全工作提供科学研究数据。方法 根据国家标准GB 4789.30-2010及《2013年国家食品污染和有害因素风险监测工作手册》进行不同地区、不同类别及不同采样地点的食品中单增李斯特菌的风险监控。结果 2011-2015年在5093件11大类食品中共检出单增李斯特菌294株,总检出率为5.77%。九个监测地区中白山、长春及四平的食品污染高于其他地区。肉与肉制品、速冻米面制品和动物性水产品的阳性检出率偏高,分别为12.43%、5.88%和5.43%。相对餐饮服务环节,流通环节污染率更高。散装与预包装食品检出率无显著性差别。结论 吉林省各地区市售食品存在单增李斯特菌不同程度的污染,需要对存在高污染风险食物的生产加工、运输销售及餐饮服务多个环节加强监督监管。