益生菌B. animalis V9冻干粉安全性毒理学研究

目的对益生菌B.animalis V9冻干菌粉进行安全性毒理学评价,确保该菌株在发酵乳制品及保健类食品中的应用安全。方法连续14d对小鼠灌胃不同剂量的(0.5、5和15g/kg体重)B.animalis V9菌粉,然后执行以下指标的测量,包括每天测体重,观察不同时间点(3、7和14d)小鼠生长状况,血液细胞成分、肝脏功能、脏器指数变化及脂类代谢情况等。在显微镜下进行肝、肾形态学观察。结果 B.animalis V9对小鼠的半数致死量(LD50)为15g/kg体重,灌胃14d小鼠未出现中毒症状,更无死亡现象,且对小鼠的生长发育无不良影响。小鼠体重变化与对照组比较差异无统计学意义(P0.05);血常规,肝功能、脏器指数、血清脂类等各项指标测定结果与对照组比较差异无统计学意义(P0.05);通过对小鼠肝脏、肾脏的染色镜检可知,肝脏、肾脏均无异常改变。结论急性毒性试验及相关指标检测结果显示B.animalis V9菌粉无毒副作用。     

蒙古族儿童源益生特性双歧杆菌的筛选及鉴定

【目的】双歧杆菌在人和动物胃肠道中发挥着重要的生理作用,然而双歧杆菌能否耐受胃酸、肠液及胆汁酸是影响活菌制剂益生效果的关键因素,本研究旨在从蒙古族儿童粪便中分离筛选出具有良好益生特性的双岐杆菌。【方法】本文采用双岐杆菌选择性培养基对样品进行分离纯化,并对菌株进行生理生化鉴定,以耐受人工胃肠液、耐受牛胆盐为手段对各菌株的益生特性进行评价,并且对B. animalisV9进行了16S rDNA分子生物学鉴定。【结果】本文从12位健康蒙古族儿童粪便中分离得到11株双歧杆菌,经传统生理生化试验鉴定为5株B. adolescentis：A1、H3、G4、A8、V10;3株B. longum：C6、C7、D11;1株B. pseudocatenlatum：B2;1株B. bifidum：G5;1株B. animalis：V9。B. animalis V9具有较强的耐酸性,在pH2.0的人工胃液中厌氧培养3h后存活率为92.4%,而其它10株双歧杆菌在此条件下的存活率均小于31.25%;B. animalis V9在pH2.0的人工胃液中厌氧培养3h后接入pH8.0的人工肠液中消化8h,存活率为99.7%,并且可以耐受0.3%的牛胆盐。进一步对V9菌株进行16S rDNA分子生物学鉴定,发现与Bifidobacterium animalis subsp. lactic BB12的同源性为99%。【结论】本研究结果显示B. animalis V9来源安全,并且具有良好耐酸、耐胆盐益生特性,有望在乳制品及保健类产品中得到广泛的应用。     

分型检测致泻性大肠埃希氏菌PCR技术研究进展

致泻性大肠埃希氏菌是一类能够引起人类和动物腹泻的食源性致病菌,迅速确定致泻性大肠埃希氏菌的污染来源可有效缩小疫情影响范围,建立简便高效的致泻性大肠埃希氏菌检测与分型技术是保障食品安全和控制疫情的关键。为适应对时间敏感度较高要求的现场或在线检测,基于PCR技术的检测分型方法不断地被标准化和规范化。对近年来国内外的致泻性大肠埃希氏菌分子检测与分型的PCR技术研究进展进行了综述,并详细地介绍了多重聚合酶链反应、荧光实时定量聚合酶链反应和核酸等温扩增技术的原理及其优缺点。为致病菌溯源方法的选择提供参考,对防御并控制致病菌引起流行病传播具有重要的意义。     

双歧杆菌四联活菌片体外生物拮抗作用的研究

目的 实验通过双歧杆菌四联活菌片（思连康）对肠道致病菌体外生物拮抗作用的研究,揭示此药治疗腹泻等疾病的作用机制,为临床应用提供科学依据。方法 对组成药物的4株益生菌发酵培养,定时取样,检测活菌数与pH值。先分别单独培养大肠埃希菌、沙门氏菌、志贺氏菌、思连康活菌片,调整菌液浓度,然后将思连康与每一个致病菌的菌液共同接种于GAM肉汤,并将每种菌液单独接种作为对照组,厌氧培养,定时检测致病菌与双歧杆菌的活菌数并分析。结果 思连康4株菌株发酵终点活菌数均在109 CFU/mL以上,发酵过程中3株原籍菌的pH值逐渐下降,蜡样芽孢杆菌pH值先下降后升高。思连康与致病菌共培养6 h,思连康显著影响大肠埃希菌生长（P0.05）;共培养12 h,思连康对3株致病菌均产生明显抑菌作用（P<0.05）;共培养24 h,未检测到致病菌的存在（P<0.01）。结论 双歧杆菌四联活菌片对致病菌抑制作用强。     

枯草芽孢杆菌活菌体外拮抗6种肠道致病菌的研究

对枯草芽孢杆菌BS 3株在体外对 6种常见肠道致病菌 (肠产毒性大肠杆菌、肠侵袭性大肠杆菌、肠致病性大肠杆菌、鼠伤寒沙门菌、福氏志贺菌和宋内志贺菌 )的拮抗作用进行了研究。结果表明 ,枯草芽孢杆菌BS 3株对宋内志贺菌、肠致病性大肠杆菌及肠产毒性大肠杆菌拮抗作用较为明显。     

210株肠道致病菌的分类及耐药性分析

目的：探讨本地区肠道致病菌的分类及主要致病菌的耐药性,给临床治疗腹泻疾病提供指导。方法：药敏试验采用K-B法,用WHONET4软件进行数据分析。结果：210株肠道致病菌中,志贺菌属占70％,沙门菌属占3％,致病性大肠埃希菌占4．8％,副溶血弧菌占3．8％,阴沟肠杆菌占3．3％,鼠伤寒沙门菌占2．4％,霍乱弧菌占1．9％,其他占10．8％等;在志贺菌属中,福氏占87％,宋内占13％。福氏和宋内志贺菌对三代头孢和IMP较敏感,对复方新诺明耐药率较高。结论：福氏志贺菌是肠道的主要致病菌;临床怀疑菌痢时,应首选三代头孢、IMP。     

2009~2012年黑龙江省细菌性腹泻症候群病原菌检测结果分析

为了解黑龙江省细菌性腹泻病原谱构成,探讨主要病原体的变异和流行变迁规律,提高监测实验室腹泻病原实验室诊断、监测预警、突发细菌性腹泻疫情的处置能力,并为进一步防治工作提供科学依据。收集哨点医院肠道门诊的细菌感染性腹泻患者粪便,采用分离培养、生化鉴定和血清分型的方法,检测沙门氏菌、志贺氏菌、致泻大肠杆菌等肠道致病菌。检测细菌性腹泻症候群患者标本537份,检出率为36.69%,其中,主要致病菌为致泻性大肠杆菌、志贺氏菌、副溶血弧菌、沙门氏菌、类志贺邻单胞菌、嗜水气单胞菌、小肠结肠炎耶尔森菌、霍乱弧菌、空肠弯曲菌、大肠埃希氏菌、检出率分别为9.31%、6.89%、1.30%、3.35%、0.56%、0.19%、0.37%、0.74%、5.40%、16.95%;性别差异不显著,各年龄组病原菌检出率和各月病原菌检出率差异显著,病原菌检出率存在季节性差异,其中6、7、8、9月份病原菌检出率高,检出率之和占总检出率的93.40%,0～10岁年龄组患病人数和检出率均高于其他年龄组。 分析发现:黑龙江省夏秋两季是细菌感染性腹泻高发季节,主要致病菌为大肠杆菌埃希氏菌、志贺氏菌、沙门氏菌、空肠弯曲菌。     

双歧杆菌体外对STM拮抗作用的实验研究

研究休外双歧杆菌对鼠伤寒沙门菌的拮抗作用,方法将两歧双歧杆菌ＳＴＭ混合培养。观察ＳＴＭ生长情况。结果ＳＴＭ和Ｂ．ｂｉｆｉｄｕｍ混合培养与ＳＴＭ单独培养对照相比较,菌量明显降低。结论Ｂ．ｂｉｆｉｄｕｍ在体外对ＳＴＭ有拮抗作用。     

辽宁省2012年食源性致病菌监测结果分析

目的监测了解辽宁省食品中致病菌污染状况,对食源性致病菌监测结果分析,为有效防治疾病提供科学依据。方法2012年采集辽宁省及8个市疾病预防控制中心的7大类食品共l824件食品样品,按照“食源性致病菌监测工作手册”标准操作程序,对常见食源性致病菌、卫生指标菌和寄生虫进行检测。结果各类指标菌样品1824份,阳性检出率为11．24％。其中副溶血性弧菌检出率最高,为19．78％;其次为蜡样芽孢杆菌,检出率为10．04％。结论辽宁主要食品均受到食源性致病菌不同程度的污染,要注意加强即食性食品的致病菌污染监测,防止食物中毒的爆发流行。     

酪酸菌对动物肠道致病菌体外拮抗作用的研究

探讨了酪酸菌对三种畜禽肠道致病菌的体外拮抗作用。将酪酸菌分别和猪大肠杆菌、鸡大肠杆菌、鸡白痢沙门氏菌三种畜禽肠道致病菌按不同的比例混合接种于CL液体培养基中进行厌氧培养,培养过程中三种致病菌的活菌数急剧下降,30h后的菌落数都逐渐降为零。说明酪酸菌在体外实验中对上述三种畜禽肠道致病菌都有较强的拮抗作用,其中酪酸菌对猪大肠杆菌、鸡大肠杆菌和鸡白痢沙门氏菌的最佳接种比例分别为：10：1～100：1、10：1～100：1和5：1～10：1。     

B-animalisV9质粒检测及抗生素敏感性试验

本实验对动物双歧杆菌Vg（B．animalisvg）菌株进行质粒检测及抗生素敏感性测试。结果表明,Baninalis V9菌株无质粒检出。该菌株对针对G＋菌的抗生素,如青霉素类（青霉素G、氨苄青霉素）和大环内酯类（氯霉素、红霉素）表现出高度敏感;对抑制细菌蛋白质合成的广谱（G＋、G-）抗生素（四环素、利福平、痢特灵）表现出中度敏感;对G-菌的抗生素,如氨基糖苷类（庆大霉素、链霉素）、喹诺酮类（诺氟沙星）及内酰胺类（卡那霉素、丁胺卡那霉素）表现出耐药性;而对广谱抗生素磺胺甲基异嗯唑也表现为耐药。     

中草药复方对拟态弧菌的体内外抗菌和拮抗外毒素的作用

目的探明拟态弧菌外毒素的致病性,筛选出对拟态弧菌具有良好抗菌和拮抗外毒素作用的中草药复方。方法培养拟态弧菌安徽分离株,采用蛋白分离技术提取其外毒素,测定其对实验草鱼的致病性。以黄连、大黄、金银花、夏枯草、丹皮、地锦草、连翘、茯苓、车前子、黄芪和甘草组成3个复方,采用改良微量稀释法测定不同中草药复方对拟态弧菌的体外抑菌作用。同时使用动物模型测定不同中草药复方拮抗外毒素作用和对拟态弧菌感染草鱼的保护作用。结果4株拟态弧菌产生的外毒素对实验鱼均具有较强的致死性。复方3的体外抑菌作用最强,对4株拟态弧菌的MIC值均为1.96g/L;其次为复方1,其MIC值介于3.92～7.84g/L;复方2的抑菌作用最差,其MIC值介于62.72～125g/L。复方3拮抗外毒素作用最强,其次为复方2,复方1不具有抗毒素作用。复方3对拟态弧菌感染草鱼具有最好的保护作用,保护率为100%;其次为复方2,保护率为23.81%;复方1的保护率最低,仅为19.05%。结论拟态弧菌外毒素在腹水病发生过程中起着重要致病作用。复方3具有良好的抗菌和拮抗外毒素作用,为筛选出的最佳复方,可进一步研制成为治疗腹水病的中草药复方制剂。     

Comparison of in vitro models to study bacterial adhesion to the intestinal epithelium

Aims:  To evaluate the adhesion ability of intestinal bacteria to different in vitro models of intestinal epithelia, and to estimate the suitability of these models and the type of interactions involved.
Methods and results:  The adhesion of probiotic ( Lactobacillus rhamnosus GG and Bifidobacterium animalis subsp . lactis Bb12), commensal ( B. animalis IATA-A2 and B. bifidum IATA-ES2) and potentially pathogenic bacteria ( E. coli and L. monocytogenes ) was determined. The adhesion models used were polycarbonate-well plates, with or without mucin, and different configurations of Caco-2 and/or HT29-MTX cell cultures. All bacteria adhered to wells without mucin (2·6–27·3%), the values being highly variable depending on the bacterial strain. Adhesion percentages of potentially probiotic bacteria to Caco-2 cultures were remarkably lower ( P  <   0·05) than those to mucin, and more similar to those of pathogenic strains. The lowest adhesion of different bacterial strains was detected on HT29-MTX (0·5–2·3%) cultures and Caco-2/HT29-MTX (0·6–3·2%) cocultures, while these values were increased in Caco-2 cultures plus mucin.
Conclusions:  The results suggested that bacterial strains exhibit different capacities to adhere to cellular components and several types of mucin present in different models, showing preferences for intestinal MUC2.
Significance and impact of the study:  The use of Caco-2 cells monolayer plus mucin (type II) better approaches the physiological characteristics of in vivo situation, providing a reliable and suitable in vitro model to evaluate bacterial adhesion.     

多噬伯克霍尔德氏菌WS-FJ9对林木病原菌物的拮抗作用及代谢产物的稳定性

【背景】伯克霍尔德氏菌(Burkholderia)是一类重要的植物根际促生细菌,许多菌株具有抑制植物病原菌生长和促进植物生长等功能。【目的】探究高效解磷促生细菌多噬伯克霍尔德氏菌(B. multivorans) WS-FJ9对不同林木病原菌物的抑菌作用。【方法】采用平板对峙法检测菌株WS-FJ9对5株林木病原真菌和卵菌的抑制效果;基于比色法检测经菌株WS-FJ9处理后病原菌菌丝细胞内含物的变化;使用antiSMASH 5.0在线预测网站对其次生代谢物质进行预测;通过菌丝生长抑制速率法对其无菌发酵滤液的抑菌活性和稳定性进行研究。【结果】菌株WS-FJ9对5种林木病原菌均具有不同程度的抑制作用,其中菌悬液对樟疫霉(Phytophthora cinnamomi)的抑制作用最好,抑菌带宽度为14.82±0.20mm,无菌发酵滤液对真菌拟茎点霉(Phomopsismacrospore)和松杉球壳孢(Sphaeropsis sapinea)的抑制效果显著,抑菌率分别为62.22%和62.78%;经无菌发酵滤液处理后的病原菌菌丝内的丙二醛含量增高,还原糖和可溶性蛋白含量显著降低。WS-FJ9菌株的基因组中含27个不同的次级代谢产物编码基因簇,其中包含编码嗜铁素、细菌素和抗生素等抑菌基因簇;该菌株发酵液在高温、紫外照射和强酸强碱环境条件下及经蛋白酶处理后,其抑菌活性均未受到影响。【结论】多噬伯克霍尔德氏菌WS-FJ9对林木病原菌物具有很好的生防潜力。     

两株生防芽孢细菌筛选、鉴定及拮抗研究

【目的】筛选出广谱、高效的生防芽孢细菌,并对其拮抗作用进行研究。【方法】以8种植物病原真菌为靶标菌,通过皿内拮抗和发酵液拮抗能力的测定筛选出2株广谱性和高效性的芽孢细菌B06和B07。【结果】B06对8种植物病原真菌的R2/R1为0.4-1.8,无菌滤液对8种植物病原真菌的抑制率为66.7%-87.5%。B07对8种植物病原真菌的R2/R1为0.23-1.21,无菌滤液对8种植物病原真菌的抑制率为55.56%-81.25%。经16S rRNA序列鉴定,菌株B06和B07都被鉴定为解淀粉芽孢杆菌。【结论】芽孢细菌能够抑制多种植物病原真菌,具有较好的抑病作用。广谱和高效芽孢细菌的筛选在农业生物防治方面具有很大的开发和应用价值。     

Successful strategy for the selection of new strawberry-associated rhizobacteria antagonistic to Verticillium wilt

In order to isolate and characterize new strawberry-associated bacteria antagonistic to the soil-borne pathogenic fungus Verticillium dahliae Kleb., rhizobacterial populations from two different strawberry species, Greenish Strawberry (Fragaria viridis) and Garden Strawberry (F. x ananassa) obtained after plating onto King's B and glycerol-arginine agar, were screened for in vitro antagonism toward V. dahliae. The proportion of isolates with antifungal activity determined in in vitro assay against V. dahliae was higher for the Garden Strawberry than for the Greenish Strawberry. From 300 isolates, 20 isolates with strong antifungal activity were selected characterized by physiological profiling and molecular fingerprinting methods. Diversity among the isolates was characterized with molecular fingerprints using amplified ribosomal DNA restriction analysis (ARDRA) and the more discriminating BOX-PCR fingerprint method. The physiological profiles were well correlated with molecular fingerprinting pattern analysis. Significant reduction of Verticillium wilt by bacterial dipping bath treatment was shown in the greenhouse and in fields naturally infested by V. dahliae. The relative increase of yield ranged from 117% (Streptomyces albidoflavus S1) to 344% (Pseudomonas fluorescens P10) in greenhouse trials, and 113% (Streptomyces albidoflavus S1) to 247% (Pseudomonas fluorescens P6) in field trials. Evaluation resulted in the selection of three effective biocontrol agents (Pseudomonas fluorescens P6, P10, and Streptomyces diastatochromogenes S9) antagonistic to the Verticillium wilt pathogen.     

The probiotic potential against vibriosis of the indigenous microflora of rainbow trout

The antibacterial properties of the indigenous microflora of rainbow trout ( Oncorhynchus mykiss Walbaum) and the potential use of inhibitory bacteria as fish probiotics were investigated. A total of 1018 bacteria and yeasts were isolated on tryptone soy agar (TSA) from skin, gills and intestine. Forty-five of these inhibited growth of the fish pathogenic bacterium Vibrio anguillarum in a well diffusion assay. The antagonism was most prominent among Pseudomonas spp., as 28 (66%) of the antagonistic bacteria belonged to this genus, despite constituting only 15% of the total tested flora. As pseudomonads are typically siderophore producers, chrome azurol S (CAS) agar was used as a semi-selective medium for isolation of antagonistic bacteria. On this medium, 75% of the iron-chelating strains were inhibitory to V. anguillarum . Eight strains out of a subset of 11 antagonists caused a 3–6 log unit reduction in the density of V. anguillarum [measured by polymerase chain reaction (PCR) detection in a most probable number (MPN) regimen] in a broth co-culture assay. Survival of rainbow trout infected with vibriosis was improved 13–43% by six out of nine antagonistic strains tested in vivo. All disease-protecting strains were pseudomonads, isolated from CAS plates, whereas two Carnobacterium spp. that were antagonistic in in vitro well diffusion assays did not alter the accumulated mortality of rainbow trout. The addition of live bacterial cultures to fish-rearing water may thus improve survival of the fish; however, in vitro antagonism could not completely predict an in vivo effect. Further studies on the underlying mechanism of activity are required to design appropriate selection criteria for fish probiotic bacteria.     

The role of lipopolysaccharide in toxicity of Francisella genus bacteria

It was demonstrated that the lipopolysaccharides (LPS) preparations, which were isolated from all representatives of Francisella Genus bacteria, i.e. F. tularensis, F. novicida, F. novicida-like and F. philomiragia by using the method of R.P. Darveau, R.E. Hancock (1983), were not toxic for white rats and white mice. A comparative study of toxicity of live F. tularensis bacteria (both wild and LPS-defective strains) made it possible to establish a direct correlation between the toxicity of microbes and LPS chemotype. It was found that only typical strains, which synthesize the wild-type S-LPS, caused the death of white rats and white mice in 24 hours after intraperitoneal contamination (10(9), 10(10) CFU/animal). Live bacteria of F tularensis R-mutants were not able to induce a lethal infection of rats and retained only residual virulence for mice. Other representatives of Francissela genus possessed less pronounced pathogenic properties. Thus, the toxic effect was registered, in case of white rats, only for F. novicida but not for F. novicida-like or F. philomiragia. At the same time, the two last mentioned species displayed a certain degree of virulence at high challenge doses (10(9), 10(10) CFU/animal) in respect to white mice. F. philomiragia, which generated lipoolygosaccharide (LOS) with an unusual structure, was found to be least pathogenic (25-75% of dead mice). The toxicity of bacteria, killed experimentally by different means (heating, UV-light, chloroform, acetone and formalin), was studied to define the role of bacterial proteins in the realisation of F. tularensis toxic potential in vivo. No lethal effect was exerted on experimental animals by killed microbes or purified LPS preparations. Finally, the study results show a priority role of the LPS molecule in the toxic effect of F. tularensis, which is possible in vivo only if structurally valuable molecules of live bacterial cells are available.