北京市人源性单核细胞增生李斯特菌耐药特征及分子分型研究

目的研究北京市人源性单核细胞增生李斯特菌的血清学分型、耐药及分子特征。方法对2013—2015年北京市李斯特菌病专项监测中分离的32株单核细胞增生李斯特菌进行PCR法血清学分型和PFGE分型,并采用CLSI和EUCAST推荐的微量肉汤稀释法检测菌株对12种抗生素的敏感性。结果 32株单核细胞增生李斯特菌共分为4种血清型,其中位居前2位的血清型是1/2b和1/2a,分别为17株和12株,4b血清型2株,1/2c血清型1株。32株菌经Asc I酶切共分为23种PFGE带型,分为4个簇,相同血清型李斯特菌的PFGE带型聚集成簇,两种分型方法一致性为93.75%(30/32)。32株单核细胞增生李斯特菌均对青霉素、氨苄西林、复方新诺明及红霉素敏感,大部分菌株对其他8种抗生素的MIC值较小,但有少数菌株对苯唑西林和四环素的MIC值较大,高达32、64μg/ml。结论北京市人源性单核细胞增生李斯特菌血清型以1/2b和1/2a为主,PFGE图谱与血清学分型存在一定相关性,耐药率普遍较低,但需加强耐药趋势监测。     

北京市食源性非伤寒沙门菌的分子分型和耐药性研究

目的了解北京市食源性非伤寒沙门菌的分子特征及耐药情况。方法对2004—2010年北京市食源性致病菌监测网收集的100株沙门菌进行脉冲场凝胶电泳(PFGE)分型和抗生素敏感性检测。结果 100株非伤寒沙门菌通过PFGE分型分为62个不同的带型,每个带型包含1~11株菌。抗生素敏感性结果显示,100株菌中有55株菌表现为对至少1种抗生素耐药,其中多重耐药菌株15株。菌株对各抗生素的耐药率为萘啶酸40%、四环素30%、氯霉素15%、庆大霉素10%、甲氧苄啶/磺胺甲恶唑10%、环丙沙星9%、头孢西丁1%、头孢噻肟0%。结论沙门菌PFGE带型和耐药谱均与血清型存在很高的一致性。提示北京市食源性非伤寒沙门菌的耐药情况比较严重,开展对该菌分子分型与耐药特征分析的联合监测意义重大。     

2000—2018年福建省单核细胞增生李斯特菌分离株血清型及脉冲场凝胶电泳分型

目的 分析福建省食品、临床病例和环境中单核细胞增生李斯特菌分离株的血清型和脉冲场凝胶电泳(PFGE)分型,为食源性疾病的暴发识别和溯源提供参考依据。方法 采用多重聚合酶链式反应(PCR)血清学分型、免疫血清凝集和PFGE方法对2000—2018年分离的单核细胞增生李斯特菌进行分型。结果 117株单核细胞增生李斯特菌分为4组血清型,包括1/2a(3a)、1/2b(3b)、1/2c(3c)和4b(4d,4e),占比分别为67.5%(79/117)、23.1%(27/117)、5.1%(6/117)和4.3%(5/117)。9株病例分离株血清型为1/2a(6株)、4b(2株)和1/2b(1株)。采用Asc I限制性内切酶将117株单核细胞增生李斯特菌分为83种不同PFGE型别,其中10株具有独特单一的型别。9株病例分离株分为8种不同PFGE型别。结论 福建省食品和病例中分离的单核细胞增生李斯特菌,1/2a血清型占主导地位,4b血清型应引起关注。     

市售活鸡和腹泻患者中非伤寒沙门菌分子特征和耐药性研究

分析市售活鸡及腹泻患者中非伤寒沙门菌的分子特征的相似性及耐药性,预防沙门菌的感染流行。方法 收集2012年1月—2013年10月从1 054份腹泻患者粪便样品及440份农贸市场的活鸡肛拭子中分离出的非伤寒沙门菌株93株,进行血清分型,对常见的非伤寒沙门菌采用脉冲场凝胶电泳(PFGE)进行分子分型、Bionumerisc v4.0进行聚类分析、纸片扩散法(K-B法)进行药物敏感性试验。结果 1 054份腹泻样品中共检出非伤寒沙门菌88株,分离率为8.35%,分为25种血清型,肠炎沙门菌居多。其中0～2岁的婴幼儿检出率较高,占52.27%(46/88)。PFGE结果:16株肠炎沙门菌分成14个PFGE型、12株斯坦利沙门菌分成11个PFGE型、14株鼠伤寒沙门菌分成14个PFGE型、6株德尔卑沙门菌分成5个PFGE型;对菌株间的相似性进行比较发现两个100%同源的肠炎沙门菌PFGE型,其他菌株的分子特征的相似性不大,鸡源菌株与人源菌株的分子特征相似性不大;对12种抗菌药物的耐药率在50%以下,不同的血清型耐药率各不相同,耐药较严重的为德尔卑沙门菌。440份活体鸡肛拭子分离出的非伤寒沙门菌5株,分离率为1.14%,共分得4种血清型,其中姆班达卡沙门菌病人中未检出。结论 该地区由非伤寒沙门菌引起腹泻的感染率高,尤以婴幼儿多见,患者与鸡未发现有同一克隆株,对常用抗生素有很好的敏感性。     

中国食源性鼠伤寒沙门菌株耐药谱及PFGE分型研究

目的了解掌握中国食品中鼠伤寒沙门菌的耐药状况，并对2002—2005年国家食源性疾病监测网分离的23株鼠伤寒沙门菌进行耐药性监测及PFGE分型研究。方法利用血清学方法对2002—2005年食源性疾病监测网分离的沙门菌进行分型，并运用CLSI（Clinical and Laboratory Standards Institute）推荐的纸片法对鼠伤寒沙门菌株进行耐药性检测。采用脉冲场凝胶电泳法（PFGE）进行PFGE分型。结果发现15株多重耐药鼠伤寒沙门菌，其中耐4～5种抗生素的6株（40％），耐6～9种抗生素的5株（33．3％），耐10种抗生素的4株（26．7％）；可分为16个PFGE型。其中5个PFGE型的菌株数超过1株。结论我国食源性鼠伤寒沙门菌分离株的多重耐药性严重，PFGE分型方法对鼠伤寒沙门菌的分型能力较好，同一PFGE型菌株的耐药谱非常接近。     

宁波地区食品中致病菌监测与流行株分析

目的了解宁波地区食品中致病菌检出情况和菌株的耐药性,发现其流行优势菌。方法致病菌检测采用直接分离与增菌分离相结合的方法;细菌鉴定采用生化筛检和API等方法;细菌分型采用诊断血清和PFGE基因分型;药敏试验采用K-B法,耐药基因检测采用PCR法。结果 6 812份食品样品中检出目标菌7类12种,共2 331份,检出率为34.22%,致病性弧菌检出数最高,其次为沙门菌和致病性气单胞菌。副溶血性弧菌与其他致病菌差异有统计学意义(P0.01),分离出10个血清群和29个PFGE型,其中O6、O5血清群和PFGE 1型是副溶血性弧菌的主要优势流行型。检出的致病菌对大多数抗生素敏感,其中3株气单胞菌为带aacc耐药基因的多重耐药菌。结论宁波地区食品中致病菌种类较多,易引起食源性疾病;各类致病菌均有流行优势株,副溶血性弧菌是最主要的流行优势株;血清分型和PFGE型能发现优势菌,但均有一定的局限性。     

2011~2018年红河州食品中沙门氏菌血清分型及脉冲场凝胶电泳分型研究

目的 了解红河州2011~2018年食品中沙门氏菌血清型分布及分子分型特征, 初步建立沙门氏菌脉冲场凝胶电泳(pulsed field gel electrophoresis, PFGE)分型的数据库。方法 使用全自动微生物鉴定系统对收集的49株沙门氏菌进行鉴定, 依据沙门氏菌White-Kauffmann-LeMinor抗原表用沙门氏菌属诊断血清确定血清型, 参照国家食源性疾病分子溯源网络(TraNet)的沙门氏菌PFGE分子分型法进行基因分型, 用Bionumerics(7.6)软件聚类分析。结果 49株沙门氏菌属于B、C、D、E和G群5个群25个血清型; 伦敦沙门氏菌是主要血清型, 占24.5%(12/49); 49株沙门氏菌分成了42个PFGE带型(P001-P042), 其中P038型包含8株菌, 其余各型分别只包含1株菌。结论 红河州食品中沙门氏菌具有不同血清型及PFGE型别, 相同血清型菌株PFGE型别聚集成簇。     

温州市食品中沙门菌污染状况及特征分析

目的了解温州市食品中沙门菌的污染状况,分析分离的沙门菌血清型分布、耐药性及脉冲场凝胶电泳(PFGE)分子分型特征。方法依据GB 4789.4—2016《食品安全国家标准食品微生物学检验沙门氏菌检验》进行菌株分离鉴定及血清学分型,采用微量肉汤稀释法进行药敏试验,PFGE法进行分子分型。结果 6类食品2 039份样品中,37份样品检出沙门菌,检出率为1.8%,其中生禽肉和生畜肉检出率较高,分别为6.9%(20/290)和3.4%(10/290)。37株沙门菌分属16种血清型,居前三位分别为鼠伤寒沙门菌、德尔卑沙门菌和肠炎沙门菌。81.1%(30/37)的菌株对17种抗生素产生不同程度的耐药,呈现24种耐药谱,多重耐药率为56.8%(21/37)。PFGE图谱分为31种PFGE带型,呈多态性。结论沙门菌在温州市食品中存在一定的污染率,耐药情况形式严峻,PFGE图谱的聚集性与沙门菌的血清型有一定的联系,与耐药谱之间的关联性并不明确。     

进出境食品中单核增生李斯特菌的血清分型与脉冲场凝胶电泳分型分析

目的研究进出境食品中的单核增生李斯特菌(LMO)的血清分型与脉冲场凝胶电泳(PFGE)分型的特性及其关系。方法采用标准方法对39株分离的LMO进行PFGE分型,分别用ApaI和Asc I酶切,电泳图谱进行聚类分析,以上菌株同时进行血清分型检测。结果 39株LMO分成6个血清型;经ApaI酶切后,分成29种带型,相似度在57.4%～100%;Asc I酶切后,分成34种带型,相似度在48.6%～100%。讨论 AscI酶切的PFGE分离效果优于ApaI酶切,与血清分型的一致性低于ApaI酶切;PFGE分型效果优于血清分型。     

进出境食品中单核增生李斯特氏菌的血清分型与脉冲场凝胶电泳分型分析研究

目的 研究进出境食品中的单核增生李斯特氏菌（LMO）的血清分型与脉冲场凝胶电泳分型的特性及其关系。方法 采用标准方法对39株分离的LMO进行PFGE分型,分别用ApaI和Asc I酶切,电泳图谱进行聚类分析,以上菌株同时进行血清分型检测。结果 39株LMO分成6个血清型;经ApaI酶切后,分成29种带型,相似度在57.4%~100%;Asc I酶切后,分成34种带型,相似度在48.6%~100%。讨论 AscI酶切的PFGE分离效果优于ApaI酶切,与血清分型的一致性低于ApaI酶切;PFGE分型效果优于血清分型。     

1例急性淋巴细胞白血病患者感染单核细胞增生李斯特菌病原学及分子分型特征分析

目的对北京市1名急性淋巴细胞白血病患者感染单核细胞增生李斯特菌病例进行病因溯源,对分离到的单核细胞增生李斯特菌进行血清学分型、耐药及分子分型研究。方法对患者不同时期外周血分离的2株单核细胞增生李斯特菌和1株环境涂抹样品单核细胞增生李斯特菌分离株进行血清学分型、耐药性分析、脉冲场凝胶电泳(PFGE)和多位点序列分析(MLST)。结果 3株单核细胞增生李斯特菌均为1/2a-3a血清型,耐药结果一致,均对青霉素、氨苄西林、复方新诺明、美罗培南及红霉素敏感,3株菌的PFGE带型一致,MLST型别均为ST155。结论本研究中患者生活环境中存在单核细胞增生李斯特菌的污染情况,高度怀疑患者感染单核细胞增生李斯特菌与其生活环境中分离到的菌株为同一来源。     

Serological and molecular ecology of Listeria monocytogenes isolates collected from 13 French pork meat salting-curing plants and their products

The purpose of this study was dual: 1. to evaluate the serotype distribution of 1028 Listeria monocytogenes isolates collected in 13 French salting factories and their products and 2. to identify sources of L. monocytogenes contamination in these factories and trace the routes of spread by PFGE (Pulsed-Field Gel Electrophoresis) typing. Serotypes 1/2a, 1/2b, 1/2c, 4b and 4e occurred. Pulsotype diversity was high among strains collected in plants and products. Furthermore, strains showing similar pulsotypes occurred on the same surfaces after an interval of at least two weeks and in unrelated factories. Forty five strains were genetically closely related to a 4b serotype L. monocytogenes strain isolated from a human clinical case of listeriosis. Our results highlighted the fact that L. monocytogenes is introduced into meat processing plants through raw meat. To overcome such contamination, suppliers of raw material should adhere to specific microbiological control measures. In addition, more attention should be focused on the appropriateness and compliance with procedures of cleaning and disinfection.     

Comparative characterization of Listeria monocytogenes isolated from Portuguese farmhouse ewe's cheese and from humans

In order to investigate the possible relationships between Listeria monocytogenes strains isolated from farmhouse ewe's cheese and clinical strains collected, in partially overlapping dates, from the same geographical area in Portugal, a total of 109 isolates from seven ewe's cheese manufactures (n=94) and from humans (n=15) were characterized by serotyping, RAPD, PFGE and allelic analysis of the virulent actA gene. Serotyping indicated the presence of four different serovars: 1/2a, 1/2b, 1/2c and 4b. The 15 clinical isolates were either serovar 4b (86.7%) or serovar 1/2b (13.3%). Among the 94 isolates from cheese and related environments the serovars prevalence was 1/2a (1.1%), 1/2b (17.0%), 1/2c (12.8%) and, unexpectedly, 4b (69.1%). Based on results obtained with PFGE typing of the strains, 25 genotypes were identified, 10 from farmhouses and 15 from human cases. Isolates from serovars 1/2a and 1/2c were assigned to single genotypes, respectively. Within serovars 1/2b and 4b three and 20 genotypes were established, respectively. RAPD typing of the isolates rendered 18 types indicating the lack of accuracy of the primers used in strain differentiation within serovar 4b. The actA gene typing of the strains showed a prevalence of actA gene type I (90.4%) compared with the rest of the strains that were all actA gene type II (9.6%). In spite of the fact that all the farmhouses were completely independent, the distribution of L. monocytogenes genotypes, intra and inter cheese manufactures, was relatively homogeneous, suggesting the existence of resident strains. In contrast, among human isolates there was a great genetic diversity. There was no common genotype between L. monocytogenes implicated in the cases of listeriosis and these cheese-related isolates, suggesting the absence of a causal relationship.     

腹泻患儿粪便中沙门菌的血清型、药敏分析及脉冲场凝胶电泳分子分型研究

目的 研究2019年北京市朝阳区0-10岁腹泻患儿粪便中分离出的沙门菌的血清型、PFGE分子分型研究及耐药特点。方法 对分离自腹泻患儿病例的47株沙门菌进行血清分型,采用微量肉汤稀释法进行27种抗生素的药敏实验;采用PFGE脉冲场凝胶电泳进行指纹图谱分型研究。结果 47株沙门分为9种血清型,优势血清型两种,分别为肠炎沙门菌23株占48.94%,鼠伤寒沙门菌14株占29.79%。47株沙门菌对磺胺异恶唑耐药率(57.45%)最高,其次为氨苄西林(48.94%)和链霉素(48.94%)。23株肠炎沙门菌可分成8个PFGE指纹图谱,15株鼠伤寒沙门菌可分成14个PFGE指纹图谱。结论 北京市朝阳区0-10岁儿童食源性沙门菌血清主要为肠炎沙门菌和鼠伤寒沙门菌,各血清型的耐药性有所不同,PFGE指纹图谱呈多样性。     

牛奶源金黄色葡萄球菌血清型、毒力基因及PFGE分型

目的：研究生鲜牛奶中金黄色葡萄球菌分离、荚膜多糖血清型分布、毒力基因携带及脉冲场凝胶电泳（pulsed field gel electrophoresis,PFGE）分型情况。方法：从河南省4?个地区奶牛养殖场采集生鲜牛奶样品按照国标法进行分离,扩增耐热核酸酶基因nuc鉴定金黄色葡萄球菌,利用聚合酶链式反应方法测定荚膜多糖血清型和毒力基因携带情况,采用PFGE分析菌株间的相关性和遗传关系。结果：从350?份生鲜牛奶样品中分离鉴定到80?株金黄色葡萄球菌,分离率为22.86%。荚膜多糖血清型测定发现,cap5（60%）是流行血清型。从这些阳性菌株中,发现有62?株（77.5%）携带有毒力基因,毒力基因set、hlb、hld、lukED、ebp、clfA和clfB,检出率分别为40.00%、51.25%、57.50%、60.00%、58.75%、57.50%和58.75%。此外,47?株（58.75%）菌携带不少于6?个毒力基因,流行的毒力基因谱型为set-hla-hlb-hld-lukED-cna-ebp-clfA-clfB。PFGE结果显示,获得72?株菌的PFGE图谱,按90%的相似性可分为12?个簇和46?种PFGE型。D簇（3?种PFGE型）、G簇（3?种PFGE型）和J簇（5?种PFGE型）菌株中均检出一定基因类型的毒力基因,表明河南地区生鲜牛奶中金黄色葡萄球菌毒力基因广泛存在于多种PFGE型别中。结论：生鲜牛奶均有一定程度的金黄色葡萄球菌污染,多数菌株携带毒力基因,且毒力基因的类型较为复杂,这对消费这些牛奶的人群构成潜在的健康威胁。PFGE分型菌株主要以克隆形式进行传播,且克隆型具有多样性和差异性,故临床应加强生奶及乳品血清型、毒力基因检测及分子分型研究。     

Application of Random Amplified Polymorphic DNA (RAPD) and Pulsed-Field Gel Electrophoresis (PFGE) Analysis to Listeria monocytogenes: A Review of Methodology and Results

Random amplified polymorphic DNA (RAPD) and pulsed-field gel electrophoresis (PFGE) analyses have been found to be powerful molecular methods for differentiating isolates of a given bacterial species. When applied to Listeria monocytogenes, both methods have been found highly effective in tracking isolates involved in food borne outbreaks of listeriosis and in identifying routes of contamination in food processing plants. Among the two methods, PFGE is considered somewhat superior in discriminatory power. However, the use of two or more independent random primers with RAPD is considered to result in a level of discrimination equal to that of PFGE. When results from both methods are combined, a maximum level of discrimination that exceeds that obtained with both methods independently can be achieved. Individually, both methods far exceed the discriminatory power of serotyping and phage typing of L. monocytogenes strains in that serotypes 1/2a, 1/2b, and 4b, represent over 90% of all human isolates, and phage typing at times has allowed typing of no more than about 50% of isolates. In addition, both RAPD and PFGE on occasion have been found to be superior to ribotyping, multilocus enzyme electrophoresis, and restriction enzyme analysis of L. monocytogenes isolates.     

Traceback identification of an ingredient (pork dewlap) as the possible source of Listeria monocytogenes serotype 4b contamination in raw chicken products

In surveys conducted on finished product samples from a single poultry processing plant in Spain, Listeria monocytogenes was found in 14 different uncooked products. To track contamination patterns, 77 L. monocytogenes isolates were characterized by PCR-based serotyping, pulsed-field gel electrophoresis (PFGE) restriction analysis, and PCR-based allelic analysis of the virulence gene actA. Serotyping revealed that 12 isolates (15.6%) were of the L. monocytogenes serotype 4b complex (serotype 4b or the closely related serotypes 4d and 4e). A combination of endonucleases AscI and ApaI PFGE patterns yielded 15 different pulsotypes among all 77 tested isolates. All the serotype 4b isolates belonged to one pulsotype. Sequencing of the actA gene confirmed that all serotype 4b isolates corresponded to the same allelic subtype. The subtype was recovered from five product types, but its presence was not correlated with the production line or the date of isolation, suggesting a possible association of this strain with a common ingredient. This traceback investigation established that pork dewlap, an ingredient common to all the products contaminated with this strain, was the most probable source of L. monocytogenes 4b. The same 4b strain was isolated from four samples of pork dewlap from one specific supplier. After replacement of this contaminated ingredient in the fresh products, this strain of L. monocytogenes serotype 4b was not detected. This study confirms the effectiveness of molecular subtyping to control contamination by specific strains of L. monocytogenes and the importance of testing the different ingredients added to the food products.     

Development of a multilocus variable-number of tandem repeat typing method for Listeria monocytogenes serotype 4b strains

Listeria monocytogenes serotype 4b strains have been identified as the causative agent in many human listeriosis epidemics as well as in a considerable number of sporadic cases. Due to the genetic homogeneity of serotype 4b isolates, development of rapid subtyping methods with high discriminatory power for serotype 4b isolates is required to allow for improved outbreak detection and source tracking. In this study, multilocus variable-number tandem repeat analysis (MLVA) was developed and used to characterize 60 serotype 4b isolates from various sources. All isolates were also characterized by automated EcoRI ribotyping, single enzyme pulsed-field gel electrophoresis (PFGE) with ApaI, and a multilocus sequence typing (MLST) scheme targeting six virulence and virulence-associated genes. Discriminatory power of MLVA (as determined by Simpson Index of Discrimination) was higher than the discriminatory power of any of the other three methods. MLVA markers targeted were found to be stable and did not change when three isolates were passaged daily for 70 days. Cluster analyses of MLVA, PFGE and MLST consistently grouped the same isolates into three major clusters, each of which includes one of the three major L. monocytogenes epidemic clones (i.e., ECI, ECIa and ECII). We conclude that the MLVA method described here (i) provides for more discriminatory subtyping of L. monocytogenes serotype 4b strains than the other three methods, (ii) identifies three major groups within the serotype 4b, which are consistent with the groups identified by other subtyping methods, and (iii) is easy to interpret. Use of MLVA may thus be recommended for subtyping of serotype 4b isolates, including as a secondary more discriminatory subtyping method that could be used after initial isolate characterization by PFGE or ribotyping.     

Antimicrobial resistance and phage and molecular typing of Salmonella strains isolated from food for human consumption in Spain

The aims of this study were to ascertain the population structure and antimicrobial susceptibility of Salmonella enterica serovars isolated in 2002 from food in 16 Spanish regions. Serovars were characterized by serotyping, phage typing, antimicrobial susceptibility, and pulsed-field gel electrophoresis (PFGE) typing, and 264 nonrelated strains were selected for further analysis. The main sources were eggs and their derivatives (21.6% of strains), poultry and related products (16.6%), and seafood (16.3%). High serotype diversity was detected (51 serotypes); the most common were Enteritidis (n = 96, 36.3%) and Typhimurium (n = 53, 20.1%), followed by a miscellaneous group of 49 different serotypes (n = 115, 43.5%). A 15% increase in Salmonella Enteritidis isolation was observed. Common phage types for Salmonella Enteritidis were PT1 (41.6% of isolates), PT4 (9.4%), PT6 (9.4%), and PT6a (9.4%), and common types for Salmonella Typhimurium were DTU302 (18.8%), DT104 (15.1%), and DT104B (13.2%). Salmonella Enteritidis strains were categorized into eight PFGE types with a similarity of 81 to 96%, and 73.9% of the strains were grouped into just one cluster. Salmonella Typhimurium isolates were divided into 13 PFGE types with a similarity of 64 to 86%, and one predominant clone contained 41.5% of the strains. Resistance rates for Salmonella Enteritidis, Salmonella Typhimurium, and the miscellaneous group were, respectively, 8.3, 69.8, and 13.9% for ampicillin, 3.1, 52.8, and 59% for streptomycin, 40.6, 22.6, and 10.4% for nalidixic acid, 15.6, 71.7, and 31.1% for tetracycline, 7.3, 18.8, and 9.5% for trimethoprim-sulfamethoxazole, 0, 50.9, and 4.3% for chloramphenicol, and 6.2, 71.7, and 17.4% for multiple (at least four) antimicrobials. All the strains remained susceptible to other beta-lactams and fluoroquinolones. Surveillance of S. enterica isolated from food is strongly recommended to reduce community exposure to antimicrobial resistant strains.