铜绿假单胞菌PA16株粘附性、菌毛与质粒关系的研究

为探讨PA的质粒与粘附性及质粒与菌毛的关系,围绕PA16株的耐药性与质粒的关系、质粒与菌毛及粘附性的关系作了一系列的研究,结果表明PA16对所测的7种抗生素全部耐药,其MIC＞400 mg/L;PA16仅含有一种27.3 kb(18 Mu)的质粒.转化后此质粒也使JM109获得了对四环素的耐药性.消除此质粒后,PA16对四环素的耐药性消失.粘附试验证明PA16质粒消除株对尿道上皮细胞的粘附能力较野生株显著性减小(P＜0.05),同时,透射电镜照片显示PA16野生株表面有致密、纤细刚直的菌毛,而PA16质粒消除株表面几乎无菌毛可见.     

细菌遗传学(续完)

质粒 质粒编码的特性 如前所述,质粒是环状的染色体外遗传因子,它可编码多种遗传信息,包括通过接合而自我转移(self-transfer)至其他细胞的信息.并非所有的质粒都能转移它们自己:非接合(non-conjugative)类质粒既不能编码供体的菌毛也不能进行转移.不过,它们可被存在于同一供体细胞内的其他接合性质粒所移动(mobilized).除了这种任选性的转移能力之外,所有的细菌质粒都含有其为在细胞分裂时自我复制及分离进入子细胞所必需的基本遗传信息.     

大肠杆菌K99菌毛fan操纵子的克隆、表达及活性

[目的]在体外克隆和表达猪产肠毒素大肠杆菌(ETEC) K99菌毛操纵子fan结构基因,并检测重组菌毛的相关生物学活性.[方法]以猪源分离的表达K99菌毛ETEC C83907株制取模板,成功PCR扩增出编码K99菌毛的fan操纵子,约5.7 kb.将fan操纵子克隆人表达质粒载体pBR322,筛选出含正确阳性质粒的重组菌.进一步将上述的重组质粒DNA转化至不含任何菌毛的大肠杆菌SE5000株,同时将空载体pBR322质粒转化入SE5000构建阴性对照菌株.[结果]该重组菌能与鼠抗K99菌毛单克隆抗体发生明显的凝集反应,与新生仔猪小肠上皮细胞刷状缘BBV分子有强烈凝集反应.电镜观察到上述重组菌表面大量表达K99菌毛,用热抽提法提纯其表达的K99菌毛,并经SDS-PAGE电泳和考马斯亮蓝染色,可以得到分子量约为18.5kDa的主要蛋白条带.纯化菌毛免疫小鼠后制备出高效价的鼠抗血清,能与携带K99菌毛的C83907、C83914、C83260野生株发生强烈的凝集反应,而与携带其他菌毛的ETEC不反应.玻板凝集试验和Western blot结果表明:体外表达的K99菌毛具有和野生K99菌毛相同的抗原性.用表达K99菌毛的重组菌进行HeLa细胞体外黏附试验和黏附抑制实验,结果表明:重组菌和野生菌株一样具有较强的粘附性,而且用重组菌毛制备的鼠抗血清能有效地抑制上述重组菌或野生菌株对细胞系的黏附结合.[讨论]本研究为进一步研究K99菌毛生物学作用建立了良好的实验平台.     

细菌遗传学

质　　粒质粒编码的特性如前所述 ,质粒是环状的染色体外遗传因子 ,它可编码多种遗传信息 ,包括通过接合而自我转移 (ｓｅｌｆ-ｔｒａｎｓｆｅｒ)至其他细胞的信息。并非所有的质粒都能转移它们自己 :非接合(ｎｏｎ -ｃｏｎｊｕｇａｔｉｖｅ)类质粒既不能编码供体的菌毛也不能进行转移。不过 ,它们可被存在于同一供体细胞内的其他接合性质粒所移动 (ｍｏｂｉｌｉｚｅｄ)。除了这种任选性的转移能力之外 ,所有的细菌质粒都含有其为在细胞分裂时自我复制及分离进入子细胞所必需的基本遗传信息。质粒似乎普遍存在于细菌之中 ;许多质粒编码以下…     

致肾盂肾炎大肠杆菌粘附基因群的克隆及其抗血清的制备

以柯斯质粒pHC79为载体构建致肾盂肾炎大肠杆菌代表株E.coli J96染色体基因文库,获得两个能够表达粘附特性的重组柯斯质粒.进一步用鸟枪法亚克隆到载体pACYC184,得到三个阳性重组体.其中pCT10/E.coli K-12 p678-54能够稳定表达P菌毛和MRHA,分子量为14.6kb.用该克隆子免疫新西兰白兔,抗血清用带有载体质粒的受体菌(pACYC184/E.coli K-12 P678-54)吸收后,经菌毛粗提物的SDS-聚丙烯酰胺凝胶电泳及Western blotting和血凝抑制试验检测,其特异性仅针对致肾盂肾炎大肠杆菌的粘附基因群,可用于临床菌株的鉴定.     

致肾盂肾炎大肠杆菌粘附基因群的克隆及其抗血清的制备

以柯斯质粒pHC79为载体构建致肾盂肾炎大肠杆菌代表株E.coli J96染色体基因文库,获得两个能够表达粘附特性的重组柯斯质粒.进一步用鸟枪法亚克隆到载体pACYC184,得到三个阳性重组体.其中pCT10/E.coli K-12 p678-54能够稳定表达P菌毛和MRHA,分子量为14.6kb.用该克隆子免疫新西兰白兔,抗血清用带有载体质粒的受体菌(pACYC184/E.coli K-12 P678-54)吸收后,经菌毛粗提物的SDS-聚丙烯酰胺凝胶电泳及Western blotting和血凝抑制试验检测,其特异性仅针对致肾盂肾炎大肠杆菌的粘附基因群,可用于临床菌株的鉴定.     

与肾盂肾炎有关的菌毛末端蛋白:新菌苗开发中的首选者

<正> 致病性大肠菌感染一般由与上皮细胞的特殊细胞表面受体的结合开始。大肠菌的粘附素(adhesins)介导这种接合,并和固定在菌细胞壁毛状蛋白附属物纤毛或菌毛有关。一根菌毛约有1000个相同的亚单位构成。粘附素蛋白与形成菌毛亚单位主要结构性质不同,在1型,P和S菌毛中粘附素是次要的菌毛成分,它分别和甘露糖、半乳糖α(1-4)半乳糖和含神经氨酸乙酰α(2-3)半乳糖的葡萄糖结合物结合。自肾盂肾炎分离的大肠菌的P粘附素,位于P菌毛的末端,是一个35000道尔顿的多肽,带有一个与主要菌毛亚单位PapA十分不同的基本结构。S粘附素主要位于S菌毛的末端,是一个12000道尔顿的较小的蛋白质,其结构至今尚不清楚。     

肺炎克雷伯菌菌毛粘附素克隆表达及其对体外培养细胞的粘附活性

摘要：【目的】肺炎克雷伯菌(K.pn)与宿主细胞的粘附是致病的首要条件,粘附过程主要通过菌毛粘附素MrkD蛋白介导。为了进一步分析MrkD蛋白与宿主细胞间的粘附机制,进一步确定MrkD蛋白的粘附阻断作用。【方法】构建肺炎克雷伯菌菌毛粘附素融合蛋白原核表达质粒pGEX-4T-mrkD,转入大肠杆菌BL21,优化诱导表达条件,表达产物经亲和层析纯化、凝血酶切除融合蛋白GST标签后,进行SDS-PAGE和Western blot鉴定。激光共聚焦显微镜定位MrkD蛋白在宿主细胞上的结合部位;通过粘附活性试验与粘附动力学实验研究了MrkD蛋白的生物活性。【结果】实验得到了分子量为35 kDa的MrkD蛋白,定位了MrkD蛋白在宿主细胞上的结合部位,并证明了MrkD蛋白可以显著影响肺炎克雷伯菌对宿主细胞的粘附力。【结论】本试验首次证实了MrkD蛋白的粘附阻断作用并观察到了其与宿主细胞的作用位点,为研究肺炎克雷伯菌的致病机制,寻找粘附素功能表位奠定了基础。     

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.     

毒素源性大肠杆菌K88ac抗原基因的次级克隆和重组质粒的限制图

从我国引起仔猪腹泻的野生株E. coli 79-1454克隆了K88ac抗原基因,获得了重组体E. coli RR1(pNZ8801),分子量为10 Md。为了得到分子量更小的重组体,用E．coRI消化重组质粒,除去中间约3.2 Md的片段,得到次级克隆株E. coli RR1(pNZ8802),质粒分子量为6.8 Md。测定其K 88ac抗原为阳性,而且其产生的K88at抗原量略高于初级克隆株。电镜照片表明重组体表面长有菌毛。萤光抗体染色和猪刷状缘细胞粘附试验亦表明有良好的粘附生物活性。此重组体可以与本人克隆的K99抗原基因构建成复合重组体。本文还作了重组体的限制性酶切图。     

Morphological and serological relationships of conjugative pili

It is now known that conjugative pili are determined by representative plasmids for all incompatibility groups in Escherichia coli K-12. They fall into three basic morphological groups, which are described: thin flexible, thick flexible, and rigid filaments or rods. The main thrust of this study, however, has been the use of immune electron microscopy to survey pili of all established incompatibility groups for serological cross-reactions. Morphologically identical thin flexible pili were determined by plasmids of the I complex, as well as IncB and IncK. Immune electron microscopy revealed two unrelated serotypes typified by Ia and I2 pili; K and B pili belonged to the first serotype. Thick flexible pili were determined by plasmids of Inc groups C, D, the F complex, H1, H2, J, T, V, X, com9, the single plasmid F0 lac, and the unclassified plasmid R687. Serological tests showed that C pili were related to J pili, H1 pili to H2 pili, com9 pili to F0 lac pili, and R687 pili to D pili, the remainder being unrelated. Rigid pili were determined by plasmids of Inc groups M, N, P, W, and by the unclassified plasmids R775, RA3, and pAr-32. The only relationship detected was between RA3 and pAr-32 pili. No cross reactions were found between pili of the three different morphological groups.     

Characterization of pili determined by drug resistance plasmids R711b and R778b.

The bacterial drug resistance plasmids R711b and R778b, at present classified in the X incompatibility group, determine pili (designated 711) that resemble F pili morphologically. Like F pili, 711 pili adsorb F-specific filamentous bacteriophages to their tips, though more often in pairs, than singly. However, F-specific RNA-containing bacteriophages are not adsorbed to their sides, and strains carrying the plasmids are resistant to these phages. Pili determined by the only IncFV plasmid Folac are similar to 711 pili in their phage adsorption properties, but they are serologically different, as are F pili. It is concluded that F, Folac and 711 pili have basic differences in spite of a morphological resemblance.     

Characteristics and function of thick and thin conjugative pili determined by transfer-derepressed plasmids of incompatibility groups I1, I2, I5, B, K and Z

Eleven transfer-derepressed plasmids from incompatibility groups I1, I5, B, K and Z were constructed using the dnaG3 mutant Escherichia coli strain BW86. All were found to determine thin flexible and thick rigid pili constitutively. Immune electron microscopy was used to relate thick and thin pilus serotypes with incompatibility grouping. Mutant plasmids that determined only thick pili constitutively transferred efficiently on an agar surface but not in a liquid, whereas plasmids with both kinds of pili transferred equally well in both environments. A mutant of the IncI2 plasmid R721 determined thin pili constitutively, and thick pili at a repressed level, as indicated by electron microscopy. Experiments with this indicated that thin pili were apparently not involved directly in conjugation but were only used to stabilize mating aggregates.     

Adsorption of bacteriophages specific for Pseudomonas aeruginosa R factors RP1 and R1822

Short, thick pili were found by electron microscopy on bacteria carrying the P group drug resistance plasmids RP1 and R1822. The R1822-specific phage PRR1 was seen to adsorb to the bases of the pili. Three RP1-specific phages, one filamentous (Pf3), and two with very thick capsids (PR3, PR4), were seen to attach all around the surface of $\text{P. aeruginosa}$ cells, and were thought to be somatic, since pilus phages appear to be strictly polar on this species. PR3 and PR4 also lysed a strain of $\text{E. coli}$ containing an N group plasmid, suggesting a relationship between the N and P group plasmids.     

Specification of surface mating systems among conjugative drug resistance plasmids in Escherichia coli K-12

Representative plasmids for most incompatibility groups in Escherichia coli K-12 were transferred to a "bald" strain to compare transfer frequencies for liquid and solid media. Standard broth matings were used for a liquid environment, but for solid surface mating, conjugation was allowed to take place on nutrient plates before washing off the cells for transconjugant selection on plates containing appropriate drugs. Plasmids that determine rigid pili transferred at least 2,000x better on plates than in broth. Some plasmids that determine thick flexible pili transferred 45 to 470x better, whereas others transferred equally well in both environments, as did plasmids of the I complex, which determine thin flexible pili. These results clearly distinguished a number of surface mating systems where most plasmids were derepressed for transfer and determined conjugative pili constitutively. The temperature-independent IncH2 plasmid R831b transferred best on plates, but other IncH plasmids transferred equally well in broth. This inconsistency led to the reclassification of R831b as IncM.     

pHH502, a plasmid with IncP and IncI alpha characters, loses the latter by a specific recA-independent deletion event

Plasmid pHH502, of molecular weight 70 X 10(6), determined resistance to tetracycline, chloramphenicol, trimethoprim, sulphonamides and mercuric chloride and was incompatible with members of IncP and IncI alpha. It resembled other plasmids of IncI alpha in the following properties: it determined pili that were morphologically and serologically I alpha pili, whose production was repressed in established plasmid-carrying (R+) cultures; its transfer was equally efficient in liquid or on solid medium; it exerted surface exclusion against other IncI alpha plasmids; it was non-transferable to Proteus. In a reproducible, recA-independent event, pHH502 gave rise to pHH502-1, a plasmid of molecular weight 40 X 10(6), lacking determinants for resistance to tetracycline and chloramphenicol and all detectable IncI alpha characteristics. pHH502-1 was incompatible only with IncP plasmids and resembled other IncP plasmids in determining constitutive production of rigid pili, in its surface exclusion, in transferring at greater frequency on solid than in liquid medium and in being transmissible to Proteus mirabilis. It differed from other IncP plasmids in the morphology and serological type of its pili and in failing to transfer to Pseudomonas aeruginosa or Acinetobacter calcoaceticus. Small numbers of pHH502-1 rigid pili were present on bacteria carrying pHH502. Possible mechanisms for the generation of pHH502 and pHH502-1 are discussed.     

Drug resistance and conjugative R plasmids in fecal Escherichia coli strains isolated from healthy younger animals (chickens, piglets, calves) and children

A total of 11,777 Escherichia coli strains were isolated from 90 chickens, 103 piglets, 96 calves, and 104 children in 1979 in Gunma Prefecture and tested for drug resistance and the presence of conjugative R plasmids. The percentages of individuals that excreted drug-resistant strains were: chickens, 100%; piglets, 99%; calves, 100%; and children, 64%. The frequency of isolation of drug-resistant strains among the total isolates was: chickens, 98%; piglets, 93%; calves, 94%; and children, 41%. Frequency of isolation of R plasmids among the strains tested was: chickens, 48%; piglets, 33%; calves, 38%; and children, 10%. Resistance patterns of the strains isolated most frequently among the four groups were tetracycline (TC), sulfonamides (SA) in single resistance, TC.SA in double resistance, TC.streptomycin (SM).SA in triple resistance and TC.SM.SA. kanamycin (KM) in quadruple resistance. R plasmids were isolated frequently from animals (over 33%) but infrequently from children (about 10%). The high frequency of isolation of drug-resistant strains and R plasmids from animals was caused by the heavy use of chemicals in the period of growth of younger animals.     

Serological characteristics of pili determined by the plasmids R711b and F0lac.

The plasmids R711b (at present IncX) and F0lac (IncFV) both determine pili morphologically like those of F (IncFI), and confer sensitivity to the F-specific filamentous bacteriophages, but not to the F-specific isometric RNA phages. Detailed serological studies show that the two pilus types are unrelated, and that neither is related to any of the previously defined F pilus serotypes. Adsorption of the isometric RNA phage MS2 to R711b pili occurs in the presence but not in the absence of formalin, which presumably prevents elution of reversibly adsorbed virions. No adsorption occurs with F0lac pili. MS2 multiplication, as measured by titre increase tests in liquid medium, is found with neither plasmid. The two plasmids are not incompatible. These observations indicate that R744b and F0lac are different both from one another and from the plasmids belonging to the incompatibility groups IncFI--IV.     

Horizontal transfer of CS1 pilin genes of enterotoxigenic Escherichia coli

CS1 is one of a limited number of serologically distinct pili found in enterotoxigenic Escherichia coli (ETEC) strains associated with disease in people. The genes for the CS1 pilus are on a large plasmid, pCoo. We show that pCoo is not self-transmissible, although our sequence determination for part of pCoo shows regions almost identical to those in the conjugative drug resistance plasmid R64. When we introduced R64 into a strain containing pCoo, we found that pCoo was transferred to a recipient strain in mating. Most of the transconjugant pCoo plasmids result from recombination with R64, leading to acquisition of functional copies of all of the R64 transfer genes. Temporary coresidence of the drug resistance plasmid R64 with pCoo leads to a permanent change in pCoo so that it is now self-transmissible. We conclude that when R64-like plasmids are transmitted to an ETEC strain containing pCoo, their recombination may allow for spread of the pCoo plasmid to other enteric bacteria.     

A physical map of pPH1JI and pJB4JI

The antibiotic resistance plasmid pPH1JI was derived from two IncP plasmids, R751 and R1033. The suicide vector for Tn5, pJB4JI, contains pPH1JI, bacteriophage Mu, and Tn5. Restriction enzyme cleavage maps for pPH1JI and pJB4JI, and the antibiotic resistance levels determined by pPH1JI and its parent plasmids are presented. The relationships between pPH1JI and its parent plasmids, and pJB4JI, are discussed.