大肠杆菌F18菌毛操纵子全基因克隆、表达及生物学活性

利用PCR技术以猪产肠毒素大肠杆菌F18标准菌株107/86和2134P基因组DNA为模板成功地扩增出编码F18ab和F18ac完整菌毛操纵子fed基因。将它们分别克隆入表达质粒载体pET-22b( ),结合酶切和核苷酸序列分析证明了PCR预期扩增产物的正确性。然后将克隆的重组载体DNA转化至大肠杆菌BL21(DE3),构建和筛选出分别含F18ab和F18ac完整fed基因的重组菌,经过IPTG诱导表达,在电镜下观察到上述两种重组菌能分别大量表达F18ab和F18ac菌毛。用热抽提法提纯其诱导表达的F18ab和F18ac菌毛,经SDS-PAGE电泳和考马斯亮蓝染色发现提纯后菌毛获单一分子量约为15kDa蛋白条带,免疫家兔后制备出高效价的兔抗血清,玻板凝集试验和Western blot结果表明:体外诱导表达的F18ab和F18ac菌毛具有和野生F18菌毛相同的抗原性。用表达F18ab和F18ac菌毛的上述2株重组菌分别进行小肠上皮细胞体外吸附试验和吸附抑制试验,结果表明:2株重组菌和野生菌株一样具有较强的粘附易感仔猪小肠上皮细胞的能力,而用表达F18ab和F18ac重组菌提纯的菌毛制备出兔抗血清都能有效地抑制上述重组菌或野生菌株对易感仔猪小肠上皮细胞的吸附结合。     

大肠杆菌K88ac菌毛操纵子fae全基因的克隆、表达及生物学活性初步研究

目的：在体外克隆和表达猪肠产毒性大肠杆菌（ETEC）K88ae菌毛操纵子,触结构基因,并检测重组菌毛的相关生物学活性。方法：利用长PCR技术以猪ETECK88ae株C83902基因组DNA为模板扩增编码K88菌毛操纵子触基因,克隆入表达质粒载体pBR322,构建和筛选重组质粒pBR322-fae,转化至不含任何菌毛的大肠杆菌EP株;电镜观察重组菌表面菌毛表达情况;用热抽提法提纯表达的重组菌毛;用纯化菌毛免疫小鼠制备高效价抗血清;用SDS-PAGE和Western blot检测重组菌毛的抗原性,用细胞黏附和黏附抑制试验检测其生物学活性。结果和结论：在电镜下观察到重组菌表面大量表达K88ae菌毛,该重组菌与兔抗K88ae菌毛单因子阳性血清、鼠抗K88ac菌毛单克隆抗体均产生凝集反应;纯化菌毛经SDS-PAGE,结构单位菌毛呈单一的相对分子质量约26×10^3的蛋白条带;纯化菌毛免疫小鼠后可制备出高效价的鼠抗血清,玻板凝集试验和Western blot结果表明体外表达的K88ae菌毛具有与K88ae野生菌毛相同的抗原性;猪小肠上皮细胞系黏附和黏附抑制实验结果表明重组EP菌和野生菌株一样具有较强的黏附猪小肠上皮细胞系的能力,而且提纯重组菌毛制备出的鼠抗血清能有效抑制上述重组菌或野生菌株对猪小肠上皮细胞系的黏附结合。     

大肠杆菌K99噬菌体的分离鉴定及在小鼠上的防治效果

【背景】产肠毒素大肠杆菌K99是引起仔猪腹泻的主要致病菌之一,目前对该病的治疗主要依赖于抗生素,但大量抗生素的长期使用造成了病原菌耐药性的增强,亟待寻求一种新的产品来解决这一问题。【目的】以一株产肠毒素大肠杆菌K99为宿主菌,从畜禽粪水中分离噬菌体并对其基本生物学特性进行研究,同时在小鼠上检验噬菌体对小鼠大肠杆菌感染的防治效果。【方法】双层平板法分离筛选烈性噬菌体并观察噬菌斑形态;纯化后进行电镜观察、核酸类型鉴定;测定噬菌体热稳定性、p H稳定性、最佳感染复数及一步生长曲线;通过小鼠体内实验检测噬菌体对小鼠大肠杆菌感染的防治效果。【结果】从畜禽粪水中分离出1株产肠毒素大肠杆菌K99强裂解性噬菌体,命名为ФK99-1,经电镜观察及核酸类型鉴定,应属于肌尾噬菌体科(Myoviridae)。噬菌体能耐受50°C左右的高温,在p H 3.0-10.0范围内效价稳定。最佳感染复数为0.000 01,暴发量为108 333 PFU/cell;运用噬菌体ФK99-1预防和治疗小鼠产肠毒素大肠杆菌K99感染,结果显示小鼠发病症状较阳性对照组明显减轻,小鼠血液内大肠杆菌K99含量也显著低于阳性对照组,通过病理切片观察显示脏器发病情况也较阳性对照组减轻。【结论】ФK99-1是一株在不同温度、不同酸碱性环境中有较强适应能力,且在小鼠大肠杆菌感染上表现出良好防治效果的裂解性肌尾科大肠杆菌噬菌体。     

双价工程菌K99和F41菌毛抗原的提纯、特征分析及免疫效果观察

本文利用加热搅拌及Sephadex G-100凝胶过滤方法,从双价重组工程菌RRI(pMG611)中分离了重组K99和F41菌毛抗原。SDS-PAGE测定其分子量,重组K99和F41抗原亚单位分子量分别是17200和29800,与各自野生菌毛亚单位分子量相同。甘露糖抗性血凝试验(MRHA)性质与野生K99和F41抗原相似。双向扩散试验和Western blot分析证实其免疫学性质亦与野生菌毛抗原相似。重组K99和F41抗原的免疫原性较强,能够刺激家兔产生高效价的抗体出现。     

大肠杆菌耐热性肠毒素STI三重串联突变体与黏附素K99融合基因的表达研究

产肠毒素大肠杆菌（ETEC）是一种导致仔畜和婴儿腹泻的主要病原之一,它的毒力因子主要有两类：黏附素（CFAs）和耐热性肠毒素（ST）或不耐热性肠毒素（LT）。通过PCR技术及双酶切连接技术,成功构建了含有3个STI突变体和1个黏附素K99基因的重组表达质粒pE3S(S)LK和pE3S(G)LK。重组菌株BL21(DE3) (pE3S(S)LK)和BL21(DE3)(pE3S(G)LK)的表达产物经SDS-PAGE和免疫印迹分析,表明以上两种重组菌株均能高效表达3STI(S)-K99和3STI(G)-K99融合蛋白,且融合蛋白能够被产肠毒素性大肠杆菌强毒株C83922 抗血清特异性识别。其次,利用乳鼠灌胃实验检测重组蛋白的生物学毒性,结果均为阴性(G/C值≤0.083),这表明该菌株已无STI生物学毒性。这些为研发预防大肠杆菌性腹泻的新型高效多价基因工程疫苗提供了基本素材和理论指导。     

共表达ETEC K99、GFP重组大肠杆菌的构建及表达北大核心

[目的]构建K99、GFP基因重组质粒并在大肠杆菌BL21(DE3)感受细胞中表达。[方法]利用PCR扩增技术扩增K99基因和GFP基因,经连接和转化将目的片段克隆到pLA载体上,利用双酶切技术及PCR技术对重组质粒进行鉴定并测序分析,利用Western Blot技术分析蛋白质表达情况。[结果]测序分析结果表明,基因具有正确的阅读框;双酶切和PCR鉴定得到498 bp和720 bp的特异性条带;荧光检测表明重组菌表达了蛋白;Western Blot结果表明重组菌表达为融合蛋白。[结论]成功构建了大肠重组菌,并表达外源融合蛋白。     

动物源产肠毒素大肠杆菌(ETEC)黏附素研究进展

动物源产肠毒素大肠杆菌(enterotoxigenic Escherichia coli,ETEC)是引起动物(尤其是幼龄动物)腹泻的主要病原菌。已知黏附素和肠毒素是ETEC中两种重要的毒力因子,在致病性中两者缺一不可。其中黏附素结合到宿主易感肠上皮细胞是ETEC感染的第一步,也是最重要的关键步骤。动物源ETEC的菌毛黏附素主要包括K88、K99、987P、F18、F17和F41等。人们从20世纪60年代就开始了ETEC菌毛黏附素的相关研究,包括菌毛的基因、结构组成、生物合成、菌毛表达的调控机制以及黏附素和宿主受体相互作用等,这些研究基础有助于我们深入了解ETEC病原菌的感染机理;并且在疾病诊断和新疫苗的开发中具有重大意义。     

产肠毒素性大肠杆菌K88菌毛装配

K88菌毛介导产肠毒索性大肠杆菌在小肠上皮细胞的粘附,是引起新生仔猪腹泻的主要致病因子之一.菌毛的合成与装配是由fae操纵子调控的,fae操纵子包含10个基,faeA-fae J,其中有些基因表达菌毛装配所需的各种结构蛋白、分子伴侣和调控因子.菌毛的装配过程是由fae操纵子调控,通过分子伴侣,锚定蛋白的相互协同作用完成,组装成结构蛋白的多聚体.继阐明K88菌毛装配调控机理之后,K88菌毛在非毒素源性大肠杆菌及其它原核生物中装配也取得成功,同时菌毛结构蛋白在真核生物中组装也取得了很大进展.     

大肠杆菌苏氨酸操纵子的体内克隆和诱变

报道了产1.2%大肠杆菌菌株的选育、野生型苏氨酸操纵子的体内克隆、体外再克隆、再克隆的体外诱变以及苏氨酸克隆pTHR12-9-1的获得.还研究了产酸克隆对产酸受体产苏氨酸的影响.发现pTHR12-9-1对低产菌有增产效应,对高产菌则相反;并对此现象作了讨论.     

大肠杆菌ptsHIcrr操纵子的快速敲除及敲除菌生长性能测定

敲除大肠杆菌磷酸烯醇式丙酮酸-糖磷酸转移酶系统(简称PTS系统)ptsHIcrr操纵子,考察敲除菌株生长特性并将其与ptsG敲除菌进行比较。利用I-SceⅠ特异性切割和Red同源重组方法成功构建了大肠杆菌DH5α△ptsHIcrr敲除菌。在LB培养基中,DH5α△ptsHIcrr的生长行为与DH5α和DH5α△ptsG明显不同,其最高菌密度是DH5α和DH5α△ptsG的近2倍,而DH5α△ptsG生长行为与DH5α无明显差异。但在含1%葡萄糖的LB中,DH5α△ptsHIcrr和DH5α△ptsG均表现出生长优势,最高菌密度依次是DH5α的2.8和2倍;培养液中最终乙酸含量分别是DH5α的12.2%、47%。在M9修饰培养基中,DH5α△ptsHIcrr比生长速率(1/h)和比葡萄糖消耗速率[g/(g.h)]明显低于DH5α,并略低于DH5α△ptsG。结果说明,ptsHIcrr操纵子敲除菌改变了葡萄糖的代谢速率,并呈现与ptsG基因敲除菌不同的代谢特点。     

Cloning of regulator genes controlling fimbrial production by enterotoxigenic Escherichia coli

Sequences regulating production of fimbriae were cloned from two enterotoxigenic Escherichia coli strains. One cloned region, from E. coli 0.25.H42, controlled expression of coli surface-associated (CS) antigen 4, whereas the function of the other, from E. coli 0167.H5, was unclear. Both regulators were related to the cfaD gene that controls expression of colonization factor antigen I (CFA/I) although low stringency conditions were required to show significant hybridization between cfaD and the regulatory fragment from E. coli 0167. The cloned regulatory genes promoted expression of CFA/I, CS1, CS2 and CS4 antigens but the levels of production in the presence of the 0167 regulator were lower than those promoted by the CS4 regulator or cfaD.     

Structure-function analysis of the K88ab fimbrial subunit protein from porcine enterotoxigenic Escherichia coli

Several in-frame linker insertions have been made in various positions in the faeG gene encoding the K88ab fimbrial subunit protein from porcine enterotoxigenic Escherichia coli. The effects of the linker insertions have been investigated with regard to the ability of the mutated fimbrial subunits to be exported to the surface of the bacterial cell and assembled into a fimbrial structure. The structure/function relationship of the subunit protein is discussed in the light of the phenotypes of the mutations constructed, secondary structure predictions, and hydrophilicity plots.     

The nucleotide sequence of the gene encoding the K99 subunit of enterotoxigenic Escherichia coli

Abstract The nucleotide sequence of the gene encoding the K99 fimbrial subunit of enterotoxigenic Escherichia coli was determined. It appeared that the subunit is composed of 159 amino acid residues preceded by a N-terminal signal sequence of 22 amino acid residues. The secondary structure of the mature K99 polypeptide and the location of potential antigenic determinants were predicted. A comparison was made between the amino acid sequence of the K99 subunit and the subunits of other fimbrial adhesins.     

A chromatographic method for the purification of K99 pili from enterotoxigenic Escherichia coli

Details of a relatively inexpensive method for the purification of K99 pili in their native conformation are reported. The method involved sequential precipitation of K99 pili with (NH4)2SO4, followed by precipitation in 12% (w/v) mannose or sorbitol solution. The crude pili preparation was adsorbed with Bio-Gel A-5m and subjected to sequential gel filtration on Bio-Gel A-5m equilibrated with Tris/EDTA/NaN3/NaCl buffer and KSCN/KCl solution, respectively. The K99 containing peak was subjected to sequential ion-exchange chromatography on DEAE-Bio-Gel A equilibrated with 0.02 M-Tris/HCl, pH 8.6 containing 0.05 M-NaCl and DEAE-Sephadex A-50 equilibrated with 0.05 M-phosphate buffer, pH 7.2. The purified pili yielded a single band on SDS-PAGE with an estimated molecular weight of 13000. Attempts to purify pili by other methods evaluated, viz. MgCl2 precipitation and chromatofocusing were unsuccessful. While the amino acid composition of purified K99 pili was similar to that reported previously the N-terminal amino acid was apparently blocked.     

磷脂酰丝氨酸合成酶基因pss的克隆与表达

磷脂酰丝氨酸合成酶能催化转酯反应,是定向合成特定磷脂类物质特别是磷脂酰丝氨酸的工具酶,但出发菌株产量低,很大程度上限制了酶法合成磷脂酰丝氨酸的工业化应用。利用表达载体pET-22b,实现了大肠杆菌磷脂酰丝氨酸合成酶基因在大肠杆菌BL21(DE3)中的同源高效表达。利用镍亲和柱对表达产物进行纯化,并用HPLC法对纯化后的重组酶的活力进行检测。结果表明,目的蛋白可在短时间内进行大量表达,蛋白含量是出发菌株的100倍,同时经6h的转酯反应转化率达到33%,重组磷脂酰丝氨酸合成酶活力达到69U/mg蛋白。