中链脂肪酸及其酯对致病菌的抑菌作用

中链脂肪酸甘油酯已经成为抗生素替代物研究的新热点。文章旨在探究月桂酸、单辛酸甘油酯、单月桂酸甘油酯、辛葵酸甘油酯对大肠埃希菌、金黄色葡萄球菌、肠炎沙门氏菌和鸡白痢沙门氏菌的抑菌效果。结果显示:月桂酸、单月桂酸甘油酯、单辛酸甘油酯对大肠埃希菌有显著(P<0.05)抑制作用;月桂酸、单月桂酸甘油酯、单辛酸甘油酯、辛葵酸甘油酯对金黄色葡萄球菌有显著(P<0.05)抑制作用;月桂酸、单月桂酸甘油酯、单辛酸甘油酯、辛葵酸甘油酯对肠炎沙门氏菌有显著(P<0.05)抑制作用;月桂酸、单月桂酸甘油酯、单辛酸甘油酯对鸡白痢沙门氏菌有显著(P<0.05)抑制作用。其中,月桂酸、单月桂酸甘油酯、单辛酸甘油酯对4种致病菌的作用效果随时间延长而增强。     

禁抗后仔猪细菌性腹泻的临床诊断与防治

为了促进食品安全和养猪业的健康发展，禁止在饲料中使用促生长抗生素势在必行。随着我国的饲料禁抗相关法规的推行，饲料企业被严格禁止在饲料生产过程中加入抗生素，这也导致了猪场疾病尤其是肠道疾病的高发，而仔猪肠道发育未完全，免疫系统未发育成熟，更容易发生严重的腹泻甚至死亡。文章对几种常见的仔猪细菌性腹泻疾病进行了回顾，病原包括大肠杆菌、沙门氏菌、魏氏梭菌，讨论了它们的临床症状与防控措施，为猪场在防控这些细菌性腹泻提供参考。     

大肠杆菌多重耐药株与敏感株蛋白质组差异分析

【目的】研究临床分离的大肠杆菌多重耐药株(R)与大肠杆菌标准株ATCC 25922(S)蛋白质差异表达情况,为进一步研究大肠杆菌耐药机理奠定基础。【方法】采用串联质谱标签(tandem mass tag,TMT)法结合平行反应监测(parallel reaction monitoring,PRM)技术,对大肠杆菌R和S株的全菌体蛋白进行定量蛋白质组学研究,筛选大肠杆菌多重耐药株(S)与敏感株(R)之间的差异表达蛋白,并对其生物信息学进行分析。【结果】共筛选出300个差异表达蛋白(Fold change≥1.3,P0.05),其中上调167个,下调133个,涉及的耐药相关通路主要包括细菌趋药性、ABC转运蛋白、β-内酰胺抗性等;PRM成功定量到13个差异蛋白,且PRM验证结果与TMT定量结果一致。【结论】筛选出多个与大肠杆菌耐药性相关的差异表达蛋白和通路。     

超临界CO_2对哈密瓜汁中大肠杆菌的杀灭效果研究

以哈密瓜汁中的大肠杆菌为研究对象,采用超临界CO_2技术(压力10、20、35 MPa,温度35、45、55℃),以温度、压力、保压时间为自变量,以大肠杆菌存活对数为因变量,对哈密瓜汁中大肠杆菌进行超临界CO_2(SCCO_2)杀菌效果的研究。采用一级反应动力学模型分析超临界CO_2对大肠杆菌的杀菌动力学;采用透射电镜观察超临界CO_2对大肠杆菌超微结构的影响。试验结果表明,在35～55℃、10～35 MPa的条件下对哈密瓜汁中大肠杆菌进行超临界二氧化碳处理,灭菌速率分为先快后慢两个阶段;随温度和压力的提高,大肠杆菌的灭菌速率均逐步上升;经超临界二氧化碳处理后,大肠杆菌细胞出现明显的缺陷,部分细胞壁消失。     

Seaweed polysaccharide mitigates intestinal barrier dysfunction induced by enterotoxigenic Escherichia coli through NF-κB pathway suppression in porcine intestinal epithelial cells

This study aimed to investigate the protective effects and underlying mechanism of seaweed polysaccharide (SWP) on intestinal epithelial barrier dysfunction induced by E. coli in an IPEC-J2 model. A preliminary study was done to screen optimum SWP concentrations by cell viability, cytotoxicity, apoptosis and proliferation evaluation. The regular study was conducted to evaluate the protective effects of SWP against E. coli challenge via the analysis of transepithelial electrical resistance (TEER), tight junction proteins, NF-κB signalling pathway, proinflammatory cytokines and the E. coli adhesion and invasion. Our results show that 4 h E. coli challenge down-regulated tight junction proteins expression, decreased TEER, activated NF-κB signalling pathway and increased proinflammatory response, which indicates that the E. coli infection model was well-established. Pre-treatment with 240 μg/ml SWP for 24 h alleviated the 4 h E. coli -induced intestinal epithelial barrier dysfunction, as evidenced by the up-regulated expression of Occludin, Claudin-1 and ZO-1 at both mRNA and protein level and the increased TEER of IPEC-J2 cells. Pre-incubation with 240 μg/ml SWP for 24 h inhibited the activation of the NF-κB signalling pathway by 4 h E. coli challenge, including the decreased mRNA expression of TLR-4, MyD88, IκBα, p-65, as well as the reduced ratio of protein expression of p-p65/p65. Also, pre-treatment with 240 μg/ml SWP for 24 h decreased proinflammatory response (IL-6 and TNF-α) induced by 4 h E. coli challenge and decreased the E. coli adhesion and invasion. In conclusion, SWP mitigated intestinal barrier dysfunction caused by E. coli through NF-κB pathway in IPEC-J2 cells and 240 μg/ml SWP exhibited better effect. Our results also provide a fundamental basis for SWP in reducing post-weaning diarrhoea of weaned piglets, especially under E. coli -infected or in-feed antibiotic-free conditions.     

2010-2016年四川省食品动物源大肠杆菌的耐药性研究

【目的】了解2010-2016年四川省食品动物源大肠杆菌产超广谱β内酰胺酶(ESBLs)情况及其耐药基因的变迁。【方法】以2010―2016年收集的444株食品动物源大肠杆菌(鸡源225株，猪源219株)为对象，采用纸片扩散法和微量肉汤稀释法分别检测其产ESBLs情况和药物敏感性；采用PCR测序法和脉冲场凝胶电泳(PFGE)检测携带ESBLs菌株的基因型特征和部分菌株的亲缘关系。【结果】444株大肠杆菌中，产ESBLs菌株的检出率为27.7%，其中鸡源菌和猪源菌检出率分别为42.2%和12.8%。2010-2016年产ESBLs菌株从16.9%升高至40.4%，鸡源菌株ESBLs检出率随时间变化比猪源菌更明显；ESBLs阳性菌株对大多数药物的耐药率显著高于阴性菌株，且多重耐药性问题更严重；产ESBLs菌株携带的耐药基因以bla_TEM和bla_CTX-M为主，并以bla_TEM-1(63.3%)、bla_TEM-52(32.1%)、bla_CTX-M-55(42.2%)、bla_CTX-M-65(27.8%)和bla_CTX-M-14(21.1%)为主要流行亚型，且检出率及ESBLs基因亚型复杂性呈逐年上升趋势；ESBLs阳性菌株有广泛PFGE谱型，即便携带相同基因型的菌株也不存在亲缘关系。【结论】四川食品动物源大肠杆菌产ESBLs菌株检出率及其耐药基因亚型的复杂程度呈逐年上升趋势，ESBLs是造成多重耐药性的主要原因，ESBLs耐药基因以水平传播为主。     

Study on Drug Resistance of Escherichia coli Isolated from Chicken and Swine in Organic Farm

To determine the drug resistance of E.coli strains from swine and chicken in organic farm,collection of stool specimens was conducted in one organic farm in Conghua city,Guangdong province in 2014,in which 118 E.coli strains were separated,including 55 from chicken and 63 from swine.The sensitivity of the E.coli strains from swine and chicken to 18 kinds of drugs was detected through agar dilution method.Similar properties in drug resistance were observed both in E.coli strains from swine and chicken in the same organic farm.In consideration of the resistance rate,samples were relatively sensitive to ceftazidime,cefquinome,cefoxitin,amikacin,apramycin,gentamicin,neomycin,florfenicol,chloramphenicol,imipenem,ciprofloxacin and olaquindox (chicken 0 to 21.8%;swine 0 to 14.3%).These isolates showed moderate resistance to ampicillin and streptomycin (chicken 29.1% to 38.2%;swine 23.8% to 27.0%).About 56.4% chicken isolates and 47.6% swine isolates showed resistant to more than 3 kinds of drugs.However,severe resistance was observed in trimethoprim-sulphamethoxazole,tetracyclineand and doxycycline (chicken 45.5%,76.4% and 72.7%;swine 50.8%,81.0% and 68.3%).The results also indicated that under organic farming mode,the drug resistance rates of E.coli strains from swine and chicken were relatively low in general.Multi-drug resistance existed but was relatively slight.Although the drug resistance rate to several specific antimicrobials was high,it was still lower than that in conventional farms.Since most studies focused on the drug resistance of the bacteria under conventional farming model,this study filled the blank of the research of drug resistance under organic farming model.     

Construction and Identification of PRRSV ORF5 Gene Prokaryotic Expression Vector

The present study was designed to construct recombinant plasmids,which could express porcine reproductive and respiratory syndrome virus (PRRSV) ORF5 gene.RNA was extracted from spleen and lung samples of the suspected pigs which were infected with PRRSV.According to PRRSV ORF5 gene,a pair of primers was designed for RT-PCR amplification.The ORF5 target gene was cloned into pMD19-T vector and then the recombinant pMD19-ORF5 was achieved.According to the sequencing results and the characteristics of expression vectors,a pair of primers with NcoⅠand XbaⅠenzyme cleavage sites was designed.Target fragment dORF5 was amplified and then connected to pProEXHTb and pNZ8149 vectors,respectively.And recombinant HTb-dORF5/DE3 and pNZ8149-dORF5/NZ3900 was induced by IPTG and Nisin,respectively,and analyzed by SDS-PAGE and Western blotting.Recombinant HTb-dORF5/DE3 induced by 1.5 mmol/L IPTG was expressed in the highest quantity.There were specific band at about 22 ku with reactionogenicity when it was tested by SDS-PAGE and Western blotting.Recombinant pNZ8149-dORF5/NZ3900 induced by 20 ng/mL Nisin was expressed in the highest quantity.There were specific band at about 19 ku with reactionogenicity when it was tested by SDS-PAGE and Western blotting.The IFA result showed specific green fluorescence.This study successfully constructed recombinant plasmids HTb-dORF5 and pNZ8149-dORF5 and expressed,the result laid a solid foundation for further development of PRRS vaccines.     

大肠杆菌生物被膜与耐药性的关系

生物被膜的形成是大肠杆菌引起消化道反复难治性感染的重要因素。大肠杆菌形成生物被膜后使感染易于慢性化、控制困难,具有高度耐药性的同时还能逃避免疫系统的攻击和抗菌药物的杀伤作用。生物被膜的耐药机制主要包括营养限制、渗透障碍、表型结构学说等。现就大肠杆菌生物被膜的形成、耐药机制及其防治策略等研究现状做一综述。