基于非数据依赖的鞘脂菌蛋白质组学分析方法的建立

【背景】鞘脂菌是一类可高效降解以菲为代表的多环芳烃有机污染物的菌株,其在环境污染治理及生物技术领域具有广阔的应用前景。【目的】为了优化测试方法,获得更完整的鞘脂菌Sphingobium yanoikuyae SJTF-8在菲胁迫下表达差异的蛋白。【方法】利用数据依赖型及数据非依赖型两种蛋白质组学数据采集方法,比较了鞘脂菌SJTF-8在菲胁迫下蛋白质水平的表达变化。【结果】两种技术方法下共得到580个表达差异蛋白,这些蛋白在细胞代谢、转运和调控等方面发挥一定功能。【结论】数据非依赖性采集(data-independent acquisition,DIA)技术在重复性以及低丰度蛋白的检测上明显好于数据依赖型采集(datadependentacquisition,DDA)技术,因此,DIA在实际可用的表达差异蛋白检出方面具备明显优势,为发现菲胁迫下细胞诱导表达的低丰度调控蛋白提供帮助。     

受低毒病毒调控的板栗疫病菌总蛋白质组学

【目的】为解析低毒病毒调控板栗疫病菌生理性状和致病性的机制,在总蛋白质组水平上寻找受病毒侵染调控的宿主蛋白及其编码基因。【方法】使用双向电泳方法对野生型菌株EP155和受低毒病毒感染的菌株EP713进行差异蛋白质组分析,同时,对差异表达蛋白质编码基因的mRNA水平进行定量分析。【结果】共找到71个因病毒侵染而发生差异表达的蛋白质点,分别属于58种不同蛋白质。以EP155为对照,表现为上调的19个,下调的52个,主要涉及能量代谢,蛋白质、核酸和碳水化合物代谢,信号传导以及压力应激和氧化还原反应。对10个受病毒调控的蛋白的编码基因进行了mRNA水平定量,其中7个基因受病毒感染后的mRNA水平变化与蛋白水平变化趋势一致,3个基因的mRNA水平变化与蛋白水平变化趋势不相符,表明低毒病毒对板栗疫病菌不同基因的调控可以发生在不同的调控层面上。【结论】低毒病毒的侵染弱化了宿主TCA循环的能量流动,调控了宿主体内的甲基化过程及真菌致病因子的表达。     

西瓜食酸菌RND蛋白家族外排转运体cusB基因抗铜功能研究

【目的】研究RND外排泵中cus B基因突变对西瓜食酸菌抗铜性的影响。【方法】采用Tn5转座子随机插入基因组制备筛选得到突变体,通过双亲杂交的方法构建功能互补菌株,并从西瓜食酸菌抗铜性、胞外纤维素酶和胞外蛋白酶分泌、胞外多糖产生、生物膜形成、致病性及过敏性反应等方面阐明RND外排泵中MFP蛋白亚基对西瓜食酸菌的影响。【结果】突变体Δcus B在含有1.25 mmol/L或2.5 mmol/L Cu SO4的KMB平板上不能生长,cus B基因的突变导致西瓜食酸菌的胞外多糖分泌和生物膜形成与野生型有差异,但不影响胞外纤维素酶、胞外蛋白酶、致病性及过敏性反应。【结论】RND外排泵相关基因cus B的突变会影响西瓜食酸菌的某些生物学特性,并导致病菌对铜十分敏感。研究以RND外排泵转运重金属为导向初步解析了西瓜食酸菌的抗铜机制。     

鸡白痢沙门菌ipaJ基因的克隆与鉴定

摘要：【目的】从鸡白痢沙门菌C79-13中克隆ipaJ基因,体外表达该蛋白后进行免疫原性分析。【方法】鸡白痢沙门菌C79-13与肠炎沙门菌50041进行抑制差减杂交后获得的片段PEA2、PE31和PE44与猪霍乱沙门菌C500疫苗株pSFD10质粒上ipaJ基因高度同源,拼接后获得了鸡白痢沙门菌完整的ipaJ基因序列。从鸡白痢沙门菌中克隆出ipaJ基因并将其构建到原核表达载体pET-30a(+)上,Western-blot检测体外表达蛋白的免疫原性,同时检测了该基因在鸡白痢沙门菌分离株中的分布。【结果】从鸡白痢沙门菌中克隆了大小为840 bp的ipaJ基因序列,并获得了体外原核表达的大小为37 kDa融合蛋白。该蛋白可与鸡白痢沙门菌阳性血清反应。PCR结果显示该基因广泛存在于鸡白痢沙门菌菌株中。 【结论】本文首次报道和克隆了鸡白痢沙门菌ipaJ基因,并证明了IpaJ蛋白具有免疫原性。     

拉达克轮丝菌TGase在大肠杆菌中的分子改造

【背景】谷氨酰胺转氨酶是一种能够催化酰基转移反应的酶,催化各种蛋白质分子之间或之内发生交联反应,在食品、化妆品、医药等领域具有重要的潜在价值。【目的】克隆来自拉达克轮丝菌(Streptoverticillium ladakanum) B1的谷氨酰胺转氨酶(TGase)基因并对其进行分子改造,使其在大肠杆菌中获得高效异源表达。【方法】分别克隆来自拉达克轮丝菌谷氨酰胺转氨酶的自身前导肽(pro)和除前导肽以外的成熟谷氨酰胺转氨酶(TGase)基因,以pET-22b为表达载体构建pro、TGase共表达和融合表达两种表达模式,在这两种表达模式的基础上进一步用定点突变的方法对成熟TGaseN端前4个氨基酸进行改造,检测不同表达模式以及突变对酶活的影响。【结果】当采用前导肽与TGase共表达时,可以直接得到活性形式的TGase,比酶活达到37.71 U/mg。在融合表达的基础上,将TGaseN端前3个氨基酸DSD突变为AAA,比酶活达到14.04U/mg,相较于原始表达模式提高了14.05%。【结论】前导肽与TGase共表达可以直接产生活性TGase,对于融合表达模式,合适位点的突变有利于提高TGase酶活。     

产碱假单胞菌脂肪酶的克隆表达及酶学性质研究

【目的】克隆产碱假单胞菌的脂肪酶基因,实现其在大肠杆菌中异源表达并进行酶学性质研究。【方法】通过基因文库构建和PCR,获得脂肪酶基因,并以pET30a(+)为表达载体、E.coli BL21(DE3)为宿主菌,在大肠杆菌中进行异源表达,表达产物经HisTrapTM亲和层析柱纯化后进行酶学性质研究。【结果】从产碱假单胞菌中克隆得到一个脂肪酶基因,大小为1 575 bp(GenBank登录号为JN674069)。该酶分子量为55 kD,最适底物为p-NPO,最适反应温度和pH分别为35°C、pH 9.0。重组酶经1 mmol/L的Cu2+处理30 min可使酶活提高至156%。在最适反应条件下重组酶的比活力为275 U/mg,Km和Vmax分别为80μmol/L和290 mmol/(min.g protein)。【结论】产碱假单胞菌脂肪酶基因的克隆与表达不仅积累了脂肪酶基因的资源,并为其在手性拆分中的应用奠定基础。     

蓝状菌(Talaromyces leycettanus JCM12802)高温果胶甲酯酶PmeT在毕赤酵母中的高效表达及酶学性质

【目的】在毕赤酵母中高水平表达蓝状菌(Talaromyces leycettanus JCM12802)来源的高温果胶甲酯酶,并对其进行酶学性质研究,具有高催化效率的高温果胶甲酯酶有望能广泛应用于低甲氧基果胶的生产,优化生产工艺,提高转化率,降低生产成本。【方法】利用RT-PCR的方法,以蓝状菌(T.leycettanus JCM12802)总RNA为模板,克隆得到果胶甲酯酶基因(Pme T)的cDNA。将其插入表达载体p PIC9K,并转化毕赤酵母(Pichia pastoris)菌株GS115,高活性的阳性转化子进行高密度发酵研究。【结果】重组酵母的果胶甲酯酶表达水平达到428 U/m L,并进一步鉴定了重组果胶甲酯酶的酶学性质。该酶的最适反应温度为75°C,且在85°C以下具有较好的热稳定性。最适反应p H为4.0,在p H 2.0-7.0之间有较好的稳定性。【结论】用重组毕赤酵母可高效表达蓝状菌来源的高温果胶甲酯酶,为其今后在工业上的应用奠定了基础。     

土霉素菌渣源酵母菌的筛选及其培养条件的优化

【背景】随着制药行业的蓬勃发展,中国每年产生大量的抗生素菌渣,已造成了不可忽视的环境污染和资源浪费等问题。由于抗生素菌渣中含有丰富的蛋白质等有机物质,利用其蛋白质等进行二次生产或将成为解决抗生素菌渣处理问题的一种有效方法。【目的】从土霉素菌渣中筛选出天然酵母菌菌株,并利用土霉素菌渣作为酵母菌生长的主要培养基成分,通过其培养条件的优化,实现土霉素菌渣的资源化利用。【方法】以土霉素菌渣为样品,运用稀释涂布法进行酵母菌的筛选,通过其形态学观察和18S rRNA基因序列分析等方法对菌株进行鉴定。通过单因素试验与Box-Behnken Design试验结合,对培养条件进行优化,确定筛选菌株在以土霉素菌渣为主要成分培养基中的最佳生长条件。【结果】筛选的土霉素菌渣源酵母菌为一株希腊接合囊酵母菌(Zygoascus hellenicus)Y1,其最佳培养条件为:土霉素菌渣添加量为5%,葡萄糖添加量为0.5%,接菌量为2%,在pH 5.0、32℃、160r/min条件下培养24h。【结论】筛选到一株希腊接合囊酵母菌Y1,该菌能够很好地利用土霉素菌渣进行生长,实现了土霉素菌渣的资源化利用,大大减少了菌渣的...     

低频电磁场对酿酒酵母蛋白质表达及酶活性的影响

【背景】低频电磁场(Lowfrequencyelectromagneticfield,LF-EMF)可导致一系列健康效应的事实已被普遍接受。【目的】进一步探究LF-EMF辐射对细胞蛋白质表达及相关酶活性的影响。【方法】以酿酒酵母为研究对象,采用50HzLF-EMF对其进行持续暴露辐射,随后对其胞内蛋白质表达、相关酶活性进行分析。【结果】LF-EMF辐射对酿酒酵母超氧化物歧化酶(Superoxide dismutase,SOD)、过氧化氢酶(Catalase,CAT)和苹果酸脱氢酶(Malate dehydrogenase,MDH)活性的影响存在先促进后抑制的趋势。辐射处理使SOD活性在72 h提高了43.18%,CAT活性在16 h提高了12.22%,MDH活性在20h提高了12.90%(P0.05);而LF-EMF辐射作用对乙醇脱氢酶(Alcohol dehydrogenase,ADH)和乳酸脱氢酶(Lactatedehydrogenase,LDH)的活性并未观察到显著的影响(P0.05)。此外,蛋白质电泳和蛋白质组学分析的结果表明,LF-EMF可改变酿酒酵母部分胞内蛋白质的表达水平,其中3种蛋白质的表达发生显著上调,9种蛋白质的表达发生显著下调(P0.05)。【结论】LF-EMF辐射可影响酿酒酵母的部分酶活性,改变其胞内部分蛋白质的表达水平。     

进口竹荚鱼中单核细胞增生李斯特菌的鉴定及其鞭毛蛋白的原核表达

【目的】对进口竹荚鱼中分离的一株病原菌S1-2进行鉴定,并在大肠杆菌中表达其鞭毛蛋白。【方法】采用全自动微生物鉴定仪和革兰氏阳性菌鉴定卡进行生理生化反应测试,利用iap基因实时荧光PCR特异性扩增检测病原菌。通过PCR技术扩增病原菌S1-2的鞭毛蛋白flaA基因,克隆筛选和测序鉴定后,构建该基因的原核表达质粒pET22b-flaA,镍柱法纯化表达产物,通过免疫印迹鉴定其免疫原性。【结果】分离病原菌为革兰氏阳性菌,生理生化特征与单核细胞增生李斯特菌(Listeria monocytogenes)的相似性为99%,协同溶血实验在靠近金黄色葡萄球菌的接种端溶血增强。SDS-PAGE结果表明融合表达产物分子量约为32 kD,Western blot结果表明重组表达的鞭毛蛋白具有免疫原性。【结论】flaA基因的原核表达为制备单核细胞增生李斯特菌的单克隆抗体及其检测方法的建立奠定了基础。     

Degeneration of hrpZ gene in Pseudomonas syringae pv. tabaci to evade tobacco defence: an arms race between tobacco and its bacterial pathogen

The HrpZ harpin of Pseudomonas syringae is known to induce a hypersensitive response (HR) in some plants. In P. syringae pv. tabaci (Pta), the harpin gene hrpZ has been spontaneously disrupted by an internal deletion in its open reading frame and a frame shift. The loss of the ability of the recombinant harpin polypeptide of Pta to induce HR despite the high sensitivity of tobacco plants to harpin led us to investigate the meaning of the disrupted hrpZ gene in the virulence of Pta 6605. The hrpZ gene from P. syringae pv. pisi was introduced into wild-type (WT) Pta. The hrpZ-complemented Pta secreted harpin into the culture medium, but failed to cause disease symptoms by both infiltration and spray inoculation. Inoculation with the hrpZ-complemented Pta induced defence responses in tobacco plants, whereas the defence responses of tobacco plants were not prominent on inoculation with WT Pta. These results indicate that an ancestor of Pta might have disrupted hrpZ by an internal deletion to evade plant defences and confer the ability to cause disease in tobacco plants.     

Post-translational modification of flagellin determines the specificity of HR induction

Flagellin, a constituent of the flagellar filament, is a potent elicitor of hypersensitive cell death in plant cells. Flagellins of Pseudomonas syringae pvs. glycinea and tomato induce hypersensitive cell death in their non-host tobacco plants, whereas those of P. syringae pv. tabaci do not remarkably induce it in its host tobacco plants. However, the deduced amino acid sequences of flagellins from pvs. tabaci and glycinea are identical, indicating that post-translational modification of flagellins plays an important role in determining hypersensitive reaction (HR)-inducibility. To investigate genetically the role of modification of flagellin in HR-induction, biological and phytopathological phenotypes of a flagella-defective Delta fliC mutant and Delta fliC mutants complemented by the introduction of the flagellin gene (fliC) from different pathovars of P. syringae were investigated. The Delta fliC mutant of pv. tabaci lost flagella, motility, the ability to induce HR cell death in non-host tomato cells and virulence toward host tobacco plants, whereas all pv. tabaci complemented by the introduction of the fliC gene of pvs. tabaci, glycinea or tomato recovered all the abilities that the Delta fliC mutant had lost. These results indicate that post-translational modification of flagellins is strongly correlated with the ability to cause HR cell death.     

A gene from Pseudomonas syringae pv. glycinea with homology to avirulence gene D from P. s. pv. tomato but devoid of the avirulence phenotype

A gene was cloned from Pseudomonas syringae pv. glycinea that hybridized to avirulence gene D (avrD), previously cloned from P. s. pv. tomato. Unlike avrD, the hypersensitive response (HR) was not elicited when the P. s. pv. glycinea gene was reintroduced into P. s. pv. glycinea race 4 on a broad host range plasmid and the bacteria were inoculated into soybean leaves. DNA sequence data disclosed that the P. s. pv. glycinea homologue of avrD encoded a protein containing 86% identical amino acids to avrD, with substitutions distributed throughout the protein. Two ORFs immediately downstream from the avrD homologue were more similar in P. s. pv. tomato and P. s. pv. glycinea, with 98 and 99% identical amino acids. Expression of the wildtype P. s. pv. glycinea gene and recombinant genes constructed between the P. s. pv. tomato avrD gene and its P. s. pv. glycinea homologue in both Escherichia coli and P. s. pv. glycinea indicated that the P. s. pv. glycinea gene product was formed less efficiently or was less stable than was the P. s. pv. tomato protein encoded by avrD. The data indicated that the P. s. pv. glycinea homologue represents a recessive allele of the P. s. pv. tomato avrD gene which has been modified by mutation such that it does not lead to an avirulence phenotype on the normal host plant, soybean.     

Detection and sequence analysis of an altered pectate lyase gene in Pseudomonas syringae pv. glycinea and related bacteria

Pectate lyase (PL) is a potent cell wall-degrading enzyme known to play a role in the microbial infection of plants. We re-examined the pectolytic property of seven representative pathovars of Pseudomonas syringae. None of the 10 P. syringae pv. glycinea strains examined exhibited pectolytic activity. However, the PL gene (pel) was detected by Southern hybridization in four out of four P. syringae pv. glycinea strains examined. A P. syringae pv. glycinea pel gene was cloned, sequenced, and predicted to encode a protein sharing 70%-90% identity in amino acid sequence with PLs produced by pectolytic pseudomonads and xanthomonads. A series of amino acid and nucleotide sequence analyses reveal that (i) the predicted P. syringae pv. glycinea PL contains two regions in the amino acid sequence that may affect the formation of a beta-helix structure important for the enzyme activity, and (ii) the P. syringae pv. glycinea pel gene contains a single-base insertion, a double-base insertion, and an 18-bp deletion, which can lead to the synthesis of an inactive PL protein. The function of P. syringae pv. glycinea PL could be restored by removing the unwanted base insertions and by filling in the 18-bp deletions by site-directed mutagenesis. The altered pel sequence was also detected by polymerase chain reaction and nucleotide sequencing in the genomes of other pathovars of P. syringae, including phaseolicola and tagetis.     

Analysis of the role of the Pseudomonas syringae pv. syringae HrpZ harpin in elicitation of the hypersensitive response in tobacco using functionally non-polar hrpZ deletion mutations, truncated HrpZ fragments, and hrmA mutations

Pseudomonas syringae pv. syringae , like many plant pathogenic bacteria, secretes a 'harpin' protein that can elicit the hypersensitive response (HR), a defensive cellular suicide, in non-host plants. The harpin-encoding hrpZ gene is located in an operon that also encodes Hrp secretion pathway components and is part of the functional cluster of hrp genes carried on cosmid pHIR11 that enables saprophytic bacteria like Escherichia coli and Pseudomonas fluorescens to elicit the HR in tobacco leaves. We have constructed functionally non-polar hrpZ deletion mutations, revealing that HrpZ is necessary for saprophytic bacteria carrying pHIR11 to elicit a typical HR, whereas it only enhances the elicitation activity of P. s. syringae . Partial deletion mutations revealed that the N-terminal 153 amino acids of HrpZ can enable E. coli MC4100-(pHIR11) to elicit a strong HR. hrpZ subclone products comprising the N-terminal 109 amino acids and C-terminal 216 amino acids, respectively, of the 341 amino acid protein were isolated and found to elicit the HR. P. fluorescens (pHIR11 hrmA  ::Tn phoA ) mutants do not elicit the HR, but cell fractionation and immunoblot analysis revealed that they produce and secrete wild-type levels of HrpZ. Therefore, elicitor activity resides in multiple regions of HrpZ, P. syringae produces elicitor(s) in addition to HrpZ, and HrpZ is essential but not sufficient for HR elicitation by saprophytic bacteria carrying pHIR11.     

大豆斑疹病菌harpin编码基因的克隆与特性研究

根据黄单胞菌harpin编码基因的同源性,设计简并引物,采用PCR方法从大豆斑疹病菌（Xanthomonas axonopodis pv.glycines, Xag）中克隆了402 bp的[STBX]hpa1[STBZ]同源基因,构建于表达载体pET30(a)上经转化大肠杆菌BL21菌株,获得基因工程菌BHR_3。基因工程菌诱导表达后经收集菌体和破碎细胞,得到表达产物为151kD的蛋白质。该蛋白质富含甘氨酸,不含半胱氨酸,对热稳定,对蛋白酶K敏感,可在非寄主烟草上激发过敏反应。激发的过敏反应需要植物体内水杨酸的积累,还可被真核生物代谢抑制剂抑制。序列比较显示,该基因与Xag中hpaG基因相同,与其它黄单胞菌中的hpa1基因有51.4%～93.8%的同源性,与其它革兰氏阴性植物病原细菌的harpin编码基因无同源性。据此把该基因产物鉴定为harpinXag。黄单胞菌harpin蛋白质序列比较发现,GG_GGG基序的多少并不是harpin蛋白的唯一特性。这为利用harpin蛋白开展植物病害控制的基因药物学设计提供了科学线索。     

Molecular characterization of avirulence gene D from Pseudomonas syringae pv. tomato

Avirulence gene D, cloned from Pseudomonas syringae pv. tomato, caused P. s. pv. glycinea to elicit a hypersensitive defense response on certain cultivars of soybean. Nucleotide sequence data for a 5.6-kb HindIII fragment containing avrD disclosed five long open-reading frames (ORFs) occurring in tandem. The phenotype conferred by avrD was expressed in P. s. pv. glycinea solely by the first of these ORFs (933 bases) that encoded a protein of 34,115 daltons. Neither a signal peptide sequence nor significant regions of hydrophobicity were present that would indicate secretion of the protein or its membrane association. Hybridization analyses revealed that some but not all P. syringae pathovars contained DNA homologous to avrD. This included weak hybridization to all tested races of P. s. pv. glycinea, although none of them express the phenotype conferred by avrD. The avrD gene occurred on an indigenous 75-kb plasmid in several P. s. pv. tomato isolates.     

丁香假单胞大豆致病变种两个III型效应因子的克隆及功能分析

为了研究Ⅲ型泌出效应因子在丁香假单胞大豆致病变种中的作用,利用反向PCR技术,首次从丁香假单胞大豆致病变种全基因组中克隆得到两个效应因子HopAB1和HopAF1基因的同源物,分别命名为HopAB1s和HopAF1s。生物信息学分析表明,HopAB1s基因全长是1 572 bp,编码523个氨基酸;HopAF1s基因全长是855 bp,编码284个氨基酸。即基因的登录号分别为JF826562和JF826563。保守功能区预测显示HopAB1s在N末端包含一个E3泛素连接酶功能区。将这2个基因克隆到PVX二元表达载体并转化农杆菌,利用农杆菌介导的瞬时侵染技术在本生烟中表达,发现2个效应因子均能抑制由鼠凋亡因子激发的细胞程序性死亡;将烟草疫霉接种在表达效应基因的区域,发现效应因子能促进烟草疫霉侵染烟草,因此本研究得到的两个效应因子是免疫抑制因子,为进一步研究该菌的致病机理奠定基础。     

Characterization and expression of two avirulence genes cloned from Pseudomonas syringae pv. glycinea.

Two avirulence genes, avrB and avrC, from race 0 of Pseudomonas syringae pv. glycinea, were sequenced and found to encode single protein products of 36 and 39 kilodaltons, respectively. The proteins had neither recognizable signal peptide sequences nor significant stretches of hydrophobic amino acids that might indicate membrane association. Both avrB and avrC had relatively low position 3 and overall G+C contents, which suggests that they may have been recently introduced into P. syringae pv. glycinea. The deduced amino acid sequences of the proteins encoded by avrB and avrC shared 42% identical amino acids. However, when introduced into race 4 of P. syringae pv. glycinea, each gene directed a unique pattern of hypersensitive reactions on several differential soybean cultivars. The avrC protein was overproduced in Escherichia coli cells and deposited as insoluble inclusion bodies in the cell cytoplasm. The avrC protein could be solubilized with urea-octyl glucoside treatment, but neither the solubilized protein nor the intact inclusion bodies elicited a hypersensitive reaction in soybean leaves.     

The cloned avirulence gene avrPto induces disease resistance in tomato cultivars containing the Pto resistance gene.

Resistance of tomato plants to the bacterial pathogen Pseudomonas syringae pv. tomato race 0 is controlled by the locus Pto. A bacterial avirulence gene was cloned by constructing a cosmid library from an avirulent P. syringae pv. tomato race, conjugating the recombinants into a strain of P. syringae pv. maculicola virulent on a tomato cultivar containing Pto, and screening for those clones that converted the normally virulent phenotype to avirulence. The cloned gene, designated avrPto, reduced multiplication of P. syringae pv. tomato transconjugants specifically on Pto tomato lines, as demonstrated by bacterial growth curve analyses. Analysis of F2 populations revealed cosegregation of resistance to P. syringae pv. tomato transconjugants carrying avrPto with resistance to P. syringae pv. tomato race 0. Surprisingly, mutation of avrPto in P. syringae pv. tomato race 0 does not eliminate the avirulent phenotype of race 0, suggesting that additional, as yet uncharacterized, avirulence genes and/or resistance genes may contribute to specificity in the avrPto-Pto interaction. Genetic analysis indicates that this resistance gene(s) would be tightly linked to Pto. Interestingly, P. syringae pv. glycinea transconjugants carrying avrPto elicit a typical hypersensitive resistant response in the soybean cultivar Centennial, suggesting conservation of Pto function between two crop plants, tomato and soybean.