Comparison between Enterotoxigenic Escherichia coli Strains Expressing “F42,” F41 and K99 Colonization Factors

Two enterotoxigenic Escherichia coli (ETEC) strains (coded 567/7 and 103) isolated from piglets with neonatal diarrhea were described as producers of a new adhesin (F42). With the use of molecular biology and immunology techniques such as DNA hybridization with probes for F41 and K99 genes and Western-blotting of the superficial proteins of these strains and standard E. coli strains carrying genes for F41 and K99 adhesins, it was demonstrated that this new adhesin either shares extensive genetic and immunological determinants with F41 adhesin or they are the same fimbriae.     

Molecular basis of cholera blood-group dependence and implications for a world characterized by climate change

Climate change has the potential to increase the threat of water-borne diseases, through rises in temperature and sea-level, and precipitation variability. Cholera poses a particular threat, and the need to develop better intervention tools is imminent. Cholera infections are particularly severe for blood group O individuals, who are less protected by the current vaccines. Here we derive a hypothesis as to the molecular origins of blood-group dependence of this disease, based on relevant epidemiological, clinical and molecular data, and give suggestions on how to plan prevention strategies, and develop novel and improved pharmaceuticals.     

Removal of antibiotic resistance of live vaccine strain Escherichia coli MM-3 and evaluation of the immunogenicity of the new strain

MM-3 was a live vaccine strain candidate for protecting neonatal piglets from diarrhea.Designed in the 1980s,a high degree of protection from colibacillosis was afforded to piglets in a challengestudy and field trials.However MM-3 had a drawback of carrying the antibiotic resistance gene (chloramphenicolacetyltransferase gene,cat).The introduction of a host-plasmid balanced lethal system into the vaccine wasa good idea to solve the problem.The λ-Red recombination system was adopted in this study to realize thereplacement of cat by aspartate-semialdehyde dehydrogenase gene (asd) in the plasmid pMM085.The newplasmid named pMMASD was introduced into an Escherichia coli strain χ6097 and Salmonella typhimuriumχ4072 where the asd gene had been knocked out in their chromosomes.Cultured in an Erlenmeyer flask,expression levels of two antigens K88ac fimbriae and heat-labile enterotoxin B subunit (LTB) in cell lysatewere similar among MM-3,χ4072(pMMASD) and χ6097(pMMASD).However,χ4072(pMMASD) possessedthe more effective secretion mechanism to transport LTB enterotoxin into culture liquid.The relatively higherstability of pMMASD in Salmonella typhimurium χ4072 than that of pMM085 in MM-3 was determined bothin vitro in the absence of selective pressure,and in vivo following oral inoculation.Oral immunization ofBALB/c mice with χ4072(pMMASD) or χ6097(pMMASD) was sufficient to elicit IgA responses in mucosaltissues as well as systemic IgG antibody responses to the K88 fimbriae,while MM-3 failed to elicit specificantibody responses to K88 fimbriae in mucosal tissues.Among three live strains,only χ4072(pMMASD)could develop strong humoral responses against LTB enterotoxin.The results suggest that χ4072(pMMASD)is expected to be a promising live vaccine strain.     

Long-term systemic and mucosal antibody responses measured in BALB/c mice following intranasal challenge with viable enterotoxigenic Escherichia coli

The immunogenicity induced in BALB/c mice following intranasal challenge with a viable nonlethal dose (1.2 x 10(8) CFU) of enterotoxigenic Escherichia coli (ETEC) strain E23477A (O139:H28:CS1:CS3:LT+:ST+) was studied over a 140-day period. Serum IgG and IgM antibodies against coli surface antigen 3 (CS3), O139 lipopolysaccharide and heat-labile enterotoxin were measured by day 14 and remained at elevated levels out to day 140. The serum IgG response to the somatic antigens (CS3 and O139 lipopolysaccharide) was significantly greater (P < 0.05) than the IgG response to heat-labile enterotoxin, and the serum IgG response to CS3 was significantly greater (P < 0.05) than the IgG response to O139 lipopolysaccharide. The predominant serum IgG subclasses to CS3 were IgG1 and IgG2a, and they were significantly greater (P < 0.05) than IgG2b and IgG3. The predominant serum IgG subclass response to O139 lipopolysaccharide was initially IgG3 until day 56, after which IgG1 was predominant. The serum subclass response to CS3 indicated a mixed T helper 1/2 (Th1/Th2) profile, whereas the response to O139 lipopolysaccharide was primarily that of a Th2-type, at least over time. Fecal IgG and IgA responses to CS3 and O139 lipopolysaccharide were detected by day 14 and were measured out to day 140, with the CS3 fecal antibody responses being significantly greater (P < 0.05) than the O139 lipopolysaccharide and heat-labile enterotoxin fecal antibody responses. The aim of this study is the development of the intranasal mouse model that can aid in better understanding the immunopathology of ETEC infection and in screening of vaccine candidates prior to volunteer trials.     

肠产毒性大肠埃希菌F4ac菌毛蛋白FaeG亚单位的原核表达及免疫学鉴定

目的克隆并表达肠产毒性大肠埃希菌（ETEC）F4ac菌毛蛋白亚单位FaeG,为制备预防幼畜ETEC感染的疫苗奠定基础。方法以ETEC（C83902）基因组DNA为模板,PCR扩增faeG基因,插入原核表达质粒pGEX-6P-1,构建重组质粒pGEX-faeG。将pGEX-faeG转化大肠埃希菌BL-21I,PTG诱导表达。SDS-PAGE分析表达蛋白的相对分子质量和表达形式,Western blot鉴定其抗原性。将表达菌超声破碎后离心提取包涵体制备抗原,经口灌喂免疫小鼠,检测小鼠血清中抗FaeG的IgGI、gA,鉴定其免疫原性。结果扩增的faeG基因全长786 bp,与基因文库中的faeG基因同源性达96%。重组质粒pGEX-faeG经PCR及双酶切鉴定确有插入片段,且序列完整。表达产物FaeG相对分子质量约53 kD,主要存在于碎菌后的沉淀中,以包涵体形式表达。Western blot显示该蛋白可与ETEC F4ac阳性血清特异性结合,免疫后小鼠血清抗FaeG IgGI、gA明显高于PBS和GST对照组。结论成功构建了ETEC F4ac菌毛蛋白亚单位FaeG的重组质粒pGEX-faeC,表达了重组蛋白FaeG,该蛋白具有良好的抗原表达了重组蛋白FaeG,该蛋白具有良好的抗原性和免疫原性,可用于研制预防幼畜ETEC感染的疫苗。     

肠产毒性大肠杆菌分子生物学及基因工程疫苗的研究进展

综述了肠产毒性大肠杆菌(ETEC)的分子生物学和基因工程疫苗的最新进展。ETEC的肠毒素基因和菌毛蛋白基因对于ETEC的致病性起主要作用,肠毒素基因工程疫苗为预防ETEC引起的腹泻开辟了新的途径。     

Determination of antimicrobial resistance and virulence gene signatures in surface water isolates of Escherichia coli

Aims: To determine the occurrence of Escherichia coli harbouring virulence markers of shiga‐ or entero‐toxins and resistance to antimicrobials in surface waters. Methods and Results: Surface water samples were collected at six locations of the river Gomti. E. coli isolates (n = 90) were characterized for their pathogenic potential using polymerase chain reaction to detect virulence genes as well as their sensitivity to antimicrobial agents using disc diffusion methods. In this study, 57·8% of E. coli isolates exhibited resistance to three or more antimicrobial agents. Sensitivity to cephotaxime, gentamicin and norfloxacin was observed in 7·8%, 48·9% and 77·8% of isolates, respectively. Both stx1 and stx2 genes were present in 15·6% of isolates while remaining isolates had either stx1 (17·8%) or stx2 (6·7%). The stx1 gene (33·3%) was more prevalent than stx2 (22·2%). The results indicate that the LT1 and ST1 genes were positive in 21·2% of isolates. Conclusions: The presence of multi‐drug resistance and virulence genes in E. coli isolated from surface water being used for domestic and recreational purposes may result in waterborne outbreaks. Significance and Impact of the Study: The data will be useful in monitoring surface waters for forecasting and management of waterborne outbreaks.