缺失氨肽酶N的变铅青链霉菌的构建和鉴定*

用PCR方法扩增变铅青链霉菌 (Streptomyceslividans)TK2 4氨肽酶N基因 ,体外插入卡那霉素抗性基因进行失活 ,然后利用不含链霉菌复制起点的重组质粒 pPEPN KAN进行同源重组 ,获得了氨肽酶N缺失的菌株PEPN- 。突变株的胞外氨肽酶N活性与原株基本相同 ,而胞内氨肽酶N的活性明显低于原株 ,为原株的 42.5± 5.7%。     

产生变活霉素的变株的分离与初步鉴别

对天然无抗菌活性的链霉菌1254菌株进行诱变．获导了二株有抗菌活性的变株。变株113产生的抗生素为一组新蒽环类化合物．有抗病毒活性,定名为变活霉素。变株2—6产生碱性永溶性物质。初步实验结果表明,原株1254及变株2-6均是胞壁类型1,为链霉菌属。变株113为胞壁类型Ⅳ,不含有枝菌酸。原株1254与变株113的阻断变株共合成的产物与变活霉素相局,以放线紫红素聚酮合成酶基因act1为探针与原株1254的总DNA进行Southern杂交为阳性。根据这二个实验的结果推断,在1254菌株中可能存在一条变活霉素的合成途径,但有的基因处于未表达状态,诱发突变使其被活化。     

牲畜链霉菌异青霉素N合成酶基因的克隆与序列分析

产生含硫卜-内酰胺类抗生素的不同微生物种属间(包括原核和真核)的异青霉素N合成酶(IPNS)基因存在着明显的同源性。利用S. lipmanii IPNS基因探针验证了牲畜链霉菌(S. cattleya)染色体DNA中确实含有与之同源的区带,通过与牲畜链霉菌无活性阻断突变株互补克隆的方法,获得了同时含有硫霉素环化酶及IPNS基因的重组质粒。经基因序列分析表明牲畜链霉菌中IPNS基因,由963bp组成,起始密码子为ATG,终止密码子为TGA,共编码321个氨基酸,所克隆的牲畜链霉菌IPNS基因编码蛋白与已知的S. clavuligerus的IPNS相似性为56％,与S. lipmanii的IPNS相似性为64％。     

糖基转移酶基因双敲除对依博素生物合成的影响

以往研究已确定链霉菌胞外多糖依博素的生物合成基因簇(ste), ste15 和ste22 分别编码葡萄糖糖基转移酶和鼠李糖糖基转移酶。现通过基因同源重组双交换,在ste15基因缺失突变株Streptomyces sp. 139 (ste15-) 基础上,再进行ste22 基因阻断,经Southern 杂交验证,得到了ste15 和ste22 双基因缺失突变株Streptomyces sp. 139 (ste15-ste22-),并对该菌株进行了基因互补研究。双基因缺失株产生的胞外多糖与依博素相比,葡萄糖与鼠李糖含量明显降低,分子量下降,生物活性明显变弱。基因互补株产生的胞外多糖中葡萄糖与鼠李糖含量基本恢复至依博素水平,生物活性也显著提高。因此,进一步阐明了ste15和ste22基因参与了依博素生物合成中葡萄糖和鼠李糖重复单元序列的形成过程,在依博素的生物合成中起重要作用,变株产生的依博素新衍生物体内外生物学活性正在深入研究中。     

粤蓝链霉菌榴菌素生物合成基因orf20的功能

【目的】在大肠杆菌中,转录因子SoxR作为胞内氧化还原感应器,参与抗氧化胁迫的全局性调控。粤蓝链霉菌榴菌素生物合成基因簇内存在一个类soxR基因orf20,但其生理功能仍不清楚。【方法】将orf20基因在大肠杆菌中进行表达,分析携带重组质粒的大肠杆菌对百草枯抗性的变化。同时通过修改后的PCR-targeting方法构建粤蓝链霉菌orf20删除的突变株,分析突变株的表型变化和对百草枯抗性水平的变化。【结果】重组ORF20在羧基端含有组氨酸标签,并在大肠杆菌中获得可溶性表达,携带重组质粒pET28b-orf20的大肠杆菌对百草枯的抗性水平显著提高。粤蓝链霉菌orf20删除突变株仍具有产孢能力,生长特性没有改变,对百草枯的抗性水平也没有变化,但榴菌素的产量大幅提高,是野生株的3.3倍。【结论】在大肠杆菌中,orf20基因的编码产物能够被百草枯激活,替代SoxR参与抗氧化胁迫的调控。在粤蓝链霉菌中,orf20基因不参与抗氧化胁迫,而对榴菌素的产生有负调控效应。     

不吸水链霉菌梧州新亚种胆固醇氧化酶基因的克隆与序列分析

克隆不吸水链霉菌梧州新亚种胆固醇氧化酶基因.以不吸水链霉菌梧州新亚种基因组DNA作为模板,根据已知的胆固醇氧化酶基因的保守序列设计简并引物进行PCR扩增,PCR产物与载体连接、转化,构建重组质粒.获得了不吸水链霉菌梧州新亚种胆固醇氧化酶基因重组质粒,序列测定并分析.     

生米卡链霉菌变株丙酰化酶基因的克隆和表达

麦迪霉素产生菌生米卡链霉菌(streptomyces mycarofaciens)变株具有丙酰化酶活性,可以将螺旋霉素转化为丙酰螺旋霉素。为了进行丙酰化酶基因克隆,本实验以质粒pIJ702为载体通过鸟枪克隆法将变株DNA片段克隆至变铅青链霉菌TK54(Streptomyces livdansTK54),经薄层层析和高压液相色谱分析结果表明,在转化子中,N0．9菌株可以将螺旋霉素转化为丙酰螺旋霉素,这证明丙酰化酶基因已在变铅青链霉菌TK54中克隆并得到初步表达,№．9重组质粒插入DNA片段为4．16kb,经southern杂交表明确实来源于变株。此外还构建了N0．9重组质粒的限制酶酶切图谱。     

棒状链霉菌lat基因的中断对棒酸产量的影响

从棒状链霉菌中克隆1.8kb的lat基因片段,构建了基因置换质粒pXAL1和pXAL2。运用接合转移方法把中断载体导入棒状链霉菌中进行lat的中断,得到1株接合转移子AmrThios,命名为XAL863。通过Southern杂交分析及赖氨酸转氨酶活性测定,证明此菌株的lat基因被中断。通过发酵培养,HPLC方法检测棒酸含量,发现棒酸产量明显提高,约为原产量的1.8倍。     

ste3与ste4基因双敲除对依博素生物合成的影响

目的:以往研究已确定链霉菌胞外多糖依博素的生物合成基因簇(ste),生物信息学分析基因簇中ste3和ste4编码糖转运相关膜蛋白,现研究分析ste3和ste4与依博素生物合成的相关性。方法:通过基因同源重组双交换获得ste3和ste4双基因缺失突变株,经Southern杂交验证后,对该菌株进行了基因互补研究。分离提取各菌株发酵液的胞外多糖,并计算产量。结果:双基因缺失株产生的胞外多糖依博素与野生株相比,产量从319mg/L降低至153mg/L,平均产量降低52%以上;基因互补后,依博素平均产量上升到299mg/L,基本恢复至野生株依博素产量水平。结论:本研究首次阐明了编码糖转运相关膜蛋白基因ste3和ste4在依博素的生物合成中起重要作用,为研究链霉菌139的初级代谢和次级代谢之间的相关性奠定了基础。     

黑暗链霉菌DNA同源重组系统的构建

以黑暗链霉菌Tt-49基因组为模板,利用PCR方法,扩增安普霉素生物合成关键基因aprF-G的上、下游序列,作为同源交换臂,并将红霉素抗性基因筛选标记及其启动子插入两交换臂之间,以温敏型质粒pKC1139为基础,构建用于阻断黑暗链霉菌Tt-49安普霉素生物合成的重组质粒pFD8.该质粒通过E.coil ET12567/pUZ8002去甲基化修饰后,经接舍转移进入黑暗链霉菌Tt-49,利用红霉素抗性筛选得到3株阳性转化子,分别命名为Tt-49 AG1、Tt-49 AG2和Tt-49 AG3.通过PCR鉴定,证明pFD8已插入黑暗链霉菌Tt-49基因组的目标位点.以亲株作对照,对3株工程菌进行红霉素抗性能力考察,发现3株工程菌的抗红霉素能力均高迭1 000 μg/mL以上.     

Mutation that affects pepN translation initiation in Escherichia coli

Mutants altered in their expression of the hybrid pepN-lacZ gene have been selected for resistance to p-nitrophenyl-beta-D-thiogalactopyranoside (a bacteriostatic compound that enters the cells via lac permease). A unique mutation decreasing the level of pepN expression to 9% of that of the wild type has been studied in detail. This mutation controls in cis the expression of the pepN gene. The pepN region from a pepN-lacZ gene fusion has been cloned and sequenced. Comparison of the mutant and wild type sequences indicates that the mutation lies between the Shine-Dalgarno sequence (AGGT) and the initiation codon (AUG). This mutation is a T----C transition which might allow the formation of a stable secondary structure in the region of translation initiation thus decreasing the level of pepN expression.     

Cloning of Streptomyces griseus and Streptomyces lividans genes for glycerol dissimilation

Streptomyces lividans gyl DNA (for glycerol utilisation) was cloned by complementation of a Streptomyces coelicolor gyl mutant. Restriction mapping showed that the cloned DNA was highly homologous (perhaps 99%) to S. coelicolor gyl DNA. Using phage-mediated mutational cloning, an internal fragment of the S. coelicolor gyl operon was used to generate a gyl mutant of S. lividans, which subsequently served as recipient in the cloning of gyl DNA from S. griseus. A 7.5-kb SstI-generated fragment of S. griseus DNA was obtained which, as judged by analysis of restriction sites, was only perhaps 87% homologous with the S. coelicolor gyl operon. The cloned S. griseus DNA appears to contain intact gylA and gylB genes and probably also an upstream gene related to the putative gyl regulatory '0.9-kb' gene of S. coelicolor. Cloning of the fragment on a high-copy-number vector in S. lividans did not lead to high levels of the enzymes encoded by gylA and gylB. The S. griseus gylA and gylB genes were not detectably expressed in Escherichia coli glp mutants.     

变铅青链霉菌与放线菌噬菌体φHAU3相互关系的研究

变铅青链霉菌ＺＸ１,是由变铅青链霉菌ＪＴ４６经ＮＴＧ诱变后产生的一株修饰基因突变株,与其亲本ＪＴ４６相比,ＺＸ１除了与ＤＮＡ降解有关的基因发生了突变（Ｄｎｄ－,即该突变株的ＤＮＡ在含有Ｆｅ２＋的缓冲液中电泳不受到降解,而野生型变铅青链霉菌在同样条件下则遭到降解）以外,对噬菌体　ＨＡＵ３的抗性也随之消失,这项特征主要表现在噬菌斑大小和成斑单位（效价）上的显著变化。研究结果表明,噬菌体　ＨＡＵ３以同等的频率吸附野生型变铅青链霉菌及其突变菌株ＺＸ１,从　ＨＡＵ３基因组中没有克隆到被变铅青链霉菌识别的特异性靶位点;噬菌体ＨＡＵ３的ＤＮＡ也可以转染野生型变铅青链霉菌原生质,但其释放的噬菌体粒子只能感染突变菌株ＺＸ１,而不能感染野生型变铅青链霉菌。噬菌体ＨＡＵ３在突变株ＺＸ１中的繁殖遵循一步生长曲线,单菌释放量大约为１００,而　ＨＡＵ３感染野生型变铅青链霉菌后,则检测不到噬菌体的释放。     

Identification of oligopeptide permease (opp) gene cluster in Vibrio fluvialis and characterization of biofilm production by oppA knockout mutation

Oligopeptides play important roles in bacterial nutrition and signaling. The oligopeptide permease (opp) gene cluster was cloned from Vibrio fluvialis. The V. fluvialis opp operon encodes five proteins: OppA, B, C, D and F. The deduced amino acid sequence of these proteins showed high similarity with those from other Gram-negative bacteria. To investigate whether OppA is involved in biofilm production, an oppA knockout mutant was constructed by homologous recombination. The oppA mutant produced more abundant biofilm than the wild type in BHI medium. When both strains were grown in minimal medium, we could not detect biofilm formation. However, it was found that the biofilm productivity of the oppA mutant was two folds greater than that of the wild type in minimal medium containing peptone or tryptone. This variation in biofilm production was demonstrated by scanning electron microscopy (SEM). In minimal medium containing C-sources, both strains produced some biofilm without significant difference in the biofilm productivity. Complementation of oppA gene with the plasmid pOAC2, which contains oppA ORF plus promoter regions, was sufficient to restore growth rate and biofilm to the wild type. These results suggest that the OppA protein is involved in uptake of peptides and affects biofilm productivity.     

Characterization of the Streptomyces clavuligerus argC gene encoding N-acetylglutamyl-phosphate reductase: expression in Streptomyces lividans and effect on clavulanic acid production.

The argC gene of Streptomyces clavuligerus encoding N-acetylglutamyl-phosphate reductase (AGPR) has been cloned by complementation of argC mutants Streptomyces lividans 1674 and Escherichia coli XC33. The gene is contained in an open reading frame of 1,023 nucleotides which encodes a protein of 340 amino acids with a deduced molecular mass of 35,224 Da. The argC gene is linked to argE, as shown by complementation of argE mutants of E. coli. Expression of argC from cloned DNA fragments carrying the gene leads to high levels of AGPR in wild-type S. lividans and in the argC mutant S. lividans 1674. Formation of AGPR is repressed by addition of arginine to the culture medium. The protein encoded by the argC gene is very similar to the AGPRs of Streptomyces coelicolor, Bacillus subtilis, and E. coli and, to a lesser degree, to the homologous enzymes of Saccharomyces cerevisiae and Anabaena spp. A conserved PGCYPT domain present in all the AGPR sequences suggests that this may be the active center of the protein. Transformation of S. clavuligerus 328, an argC auxotroph deficient in clavulanic acid biosynthesis, with plasmid pULML30, carrying the cloned argC gene, restored both prototrophy and antibiotic production.     

头状轮生链霉菌中丝裂霉素C抗性基因的克隆及功能研究

头状轮生链霉菌(\%Streptoverticillium caespitosus\%)ATCC27422是抗肿瘤药物丝裂霉素的主要产生菌,实验通过诱变筛选获得不产生丝裂霉素同时对丝裂霉素C敏感的阻断变种S6,并以它为受体宿主,以质粒pIJ699为载体,建立野生型头状轮生链霉菌菌株ATCC27422的基因库。采用鸟枪法克隆技术,从库中筛选获得含有丝裂霉素C抗性基因的62kb外源片段的克隆子。将含此外源片段的质粒pLX5导入变铅青链霉菌(\%Streptomyces lividans\%)获得表达。并且首次成功地运用电穿孔法将pLX5导入野生型菌株中,使其对丝裂霉素C的抗性大幅度提高：最低抑制浓度(MIC)由原来的200μg/mL上升至1000μg/mL以上。摇瓶发酵实验表明：单位菌量的ATCC27422(pLX5)的丝裂霉素产量高于野生菌株ATCC27422,因此丝裂霉素C抗性与产量之间存在一定的相关性。     

肺炎克雷伯菌KP1＿4563基因突变株的构建及其生物膜表型分析

KP1_4563基因是肺炎克雷伯菌NTUH-K2044中假设的蛋白编码基因,与Ⅲ型菌毛的功能有关。本实验首先采用同源重组基因敲除方法构建肺炎克雷伯菌KP1_4563基因缺失的突变株(Kp-△4563),然后PCR扩增KP1_4563基因片段,克隆到质粒p BAD33上,将重组质粒导入Kp-△4563获得回补株(Kpc-△4563)。分别测定野生株、突变株、回补株用普通LB培养基,改良Minka培养基以及含胆汁盐的LB培养基培养时生物膜形成能力,以此来探讨KP1_4563基因以及不同培养基对肺炎克雷伯菌体外生物膜形成的影响。我们成功构建KP1_4563基因缺失的突变株和回补株Kpc-△4563。与野生株相比,突变株Kp-△4563生物膜形成能力减弱,回补株介于野生株和突变株之间。使用改良Minka培养基使菌株菌毛化以及加入胆汁盐可以增加生物膜的形成能力。这些分析表明肺炎克雷伯菌KP1_4563基因能正调控细菌生物膜的形成。体外培养使细菌菌毛化以及加入胆汁盐可以促进生物膜的形成。     

Amino acid transport and metabolism in mycobacteria: cloning, interruption, and characterization of an L-Arginine/gamma-aminobutyric acid permease in Mycobacterium bovis BCG

Genes encoding L-arginine biosynthetic and transport proteins have been shown in a number of pathogenic organisms to be important for metabolism within the host. In this study we describe the cloning of a gene (Rv0522) encoding an amino acid transporter from Mycobacterium bovis BCG and the effects of its deletion on L-arginine transport and metabolism. The Rv0522 gene of BCG was cloned from a cosmid library by using primers homologous to the rocE gene of Bacillus subtilis, a putative arginine transporter. A deletion mutant strain was constructed by homologous recombination with the Rv0522 gene interrupted by a selectable marker. The mutant strain was complemented with the wild-type gene in single copy. Transport analysis of these strains was conducted using (14)C-labeled substrates. Greatly reduced uptake of L-arginine and gamma-aminobutyric acid (GABA) but not of lysine, ornithine, proline, or alanine was observed in the mutant strain compared to the wild type, grown in Middlebrook 7H9 medium. However, when the strains were starved for 24 h or incubated in a minimal salts medium containing 20 mM arginine (in which even the parent strain does not grow), L-[(14)C]arginine uptake by the mutant but not the wild-type strain increased strongly. Exogenous L-arginine but not GABA, lysine, ornithine, or alanine was shown to be toxic at concentrations of 20 mM and above to wild-type cells growing in optimal carbon and nitrogen sources such as glycerol and ammonium. L-Arginine supplied in the form of dipeptides showed no toxicity at concentrations as high as 30 mM. Finally, the permease mutant strain showed no defect in survival in unactivated cultured murine macrophages compared with wild-type BCG.     

胶孢炭疽菌CgRGS2基因的克隆及生物学功能

【目的】G蛋白信号调控因子(Regulators of G-protein signaling,RGS)是G蛋白的一类负调控因子,在植物病原菌生长发育及致病过程中发挥着重要的作用,然而目前还未有关于胶孢炭疽菌RGS蛋白生物学功能的研究。本试验的目的是克隆胶孢炭疽菌的一个RGS基因CgRGS2,并分析其生物学功能。【方法】利用PCR技术扩增CgRGS2的基因并进行生物信息学分析,利用同源重组的方法获得CgRGS2基因的敲除突变体,并在突变体的基础上获得互补株,通过表型分析确定该基因的生物学功能。【结果】通过PCR扩增获得了CgRGS2的基因,其编码一个574个氨基酸的蛋白,在N末端含有一个RGS功能域。该基因敲除突变体同野生型相比,表现为营养生长缓慢,气生菌丝浓密,分生孢子产量降低且孢子呈多端萌发,对氧化压力及SDS敏感,致病性减弱等。【结论】CgRGS2蛋白参与调控胶孢炭疽菌的营养生长,分生孢子产量及萌发,氧化应激反应及细胞壁完整性,对其致病性也具有一定的影响。