生防解淀粉芽胞杆菌的研究进展

解淀粉芽胞杆菌(Bacillus amyloliquefaciens)因能抑制植物病害和促进植物生长而被广泛研究。随着测序技术的不断发展,解淀粉芽胞杆菌菌株的全基因组序列陆续被测定,综述了其拮抗作用相关的功能基因、生防机制及植物-病原物-生防菌的相互作用,并对后续研究趋势进行了展望,为解淀粉芽胞杆菌的深入研究及其更好的应用提供理论参考     

解淀粉芽胞杆菌胞外抑菌活性物质研究现状

解淀粉芽胞杆菌是芽胞杆菌属的一个种,在生长过程中可以向胞外分泌多种抑菌活性物质。按照胞外抑菌活性物质合成方式的不同分为两大类,一类是通过核糖体途径合成的核糖体类细菌素、几丁质酶和β-1,3-葡聚糖酶等抑菌物质;另一类是通过非核糖体途径合成的细菌素、表面活性素、芬荠素、伊枯草菌素等脂肽类物质。这些代谢产物种类丰富、广谱抑菌、抗逆性强,可应用于农业、食品工业和环境保护等。本文对解淀粉芽胞杆菌抑菌活性物质的研究及应用现状进行综述,为深入研究和全面开发解淀粉芽胞杆菌抑菌活性物质提供充足的理论依据。     

解淀粉芽胞杆菌产酶多样性及应用研究进展

解淀粉芽胞杆菌(Bacillus amyloliquefaciens)能产生多种有研究价值的酶类,其酶具有明显的多样性,在众多领域,如轻工业、农业、种植业、养殖业、食品加工业、果蔬的采后保鲜、饲料业等行业具有重要价值。对解淀粉芽胞杆菌产生的不同类型的蛋白酶、降解多糖的重要酶类、脂类代谢相关的酶类以及其他几种重要的酶类进行了归类,并对其在各领域的应用及前景进行综述。     

解淀粉芽胞杆菌抗真菌活性研究进展

解淀粉芽胞杆菌(Bacillus amyloliquefaciens)具有很强的抑制植物病原真菌的能力。其菌体细胞能产生多种酶类、脂肽类抗生素、生物表面活性素、聚酮类化合物和抑菌蛋白,同时具有诱导植物产生系统抗性(ISR)的能力,因此在工农业、种植业、养殖业、食品加工业、果蔬的采后保鲜和饲料业等行业具有重要价值。本文对解淀粉芽胞杆菌抗真菌作用、抗真菌能力提高策略、抗菌化合物合成调节、抑制真菌机制及其引发的ISR等问题进行了深入探讨和综述。     

芽胞形成相关基因缺失对解淀粉芽胞杆菌生物量及胞外酶表达的影响

解淀粉芽胞杆菌作为公认的安全生产宿主菌(GRAS),在高效表达异源蛋白方面具有巨大的发展潜力和应用前景.本研究以解淀粉芽胞杆菌TCCC111018为出发菌株,通过敲除芽胞形成相关基因(spo0A,sigF和sigE),构建了一系列突变菌株(BA△spo0A,BA△sigF,BA△sigE),并对突变株生物量和胞外酶表达...     

解淀粉芽胞杆菌TF28产抗菌脂肽培养基优化

采用响应面方法对解淀粉芽胞杆菌TF28产抗菌脂肽培养基进行优化,以提高其产量。利用Plackett-Burman试验设计筛选出影响抗菌脂肽产量的3个主要因素:葡萄糖、硫酸镁和磷酸氢二钠。通过最陡爬坡试验逼近最大响应值区域,利用响应面分析方法确定显著组份的最佳水平。结果表明,优化后的培养基组份为葡萄糖42.37 g/L,酵母膏2 g/L,牛肉膏2 g/L,硫酸铵2 g/L,硫酸镁2.11 g/L,氯化钙0.1 g/L,硫酸锰0.1 g/L,磷酸二氢钾1.5 g/L,磷酸氢二钠3 g/L,经3次平行试验验证,抗菌脂肽产量为1.75 g/L,比优化前提高了5.25倍。该研究优化了解淀粉芽胞杆菌TF28提高抗菌脂肽产量的培养基,为抗菌脂肽的生产奠定基础。     

源于解淀粉芽胞杆菌酚酸脱羧酶的克隆与表达

【背景】酚酸脱羧酶催化分解酚酸产生的4-乙烯基酚类物质可用于食品添加剂及香精香料行业,而酚酸脱羧酶的表达水平相对较低,因此,高水平的酚酸脱羧酶是工业规模生产4-乙烯基酚类物质的先决条件。【目的】克隆解淀粉芽胞杆菌的酚酸脱羧酶基因,实现在大肠杆菌中的高效异源表达,分析酚酸脱羧酶的底物特异性,并对其表达条件进行优化。【方法】通过PCR技术获得酚酸脱羧酶的基因,构建重组基因工程菌,将测序结果与其他酚酸脱羧酶序列进行比对,利用IPTG诱导方法高效表达蛋白。将重组酚酸脱羧酶与4种不同的底物进行反应,设计响应面试验对诱导条件进行优化。【结果】酚酸脱羧酶对对香豆酸、阿魏酸、咖啡酸、芥子酸的比酶活比率为:100:23.33:15.39:10.51。结合与其他酚酸脱羧酶比对结果发现酚酸脱羧酶家族的C末端区域氨基酸序列的变异率最高,这与酚酸脱羧酶的底物特异性和催化机制有关。通过单因素和响应面试验得到酚酸脱羧酶诱导表达的最佳条件为:2×YT培养基,诱导温度30°C,接种量1.78%,诱导时机3.8 h,IPTG1.25mmol/L,诱导时间18h,此时预测酶活和实际酶活分别为47.61IU/mL和47.55...     

解淀粉芽胞杆菌启动基因的克隆及其对地衣杆菌α-淀粉酶基因的调控

用大肠杆菌启动基因探针质粒pHE5克隆了解淀粉芽胞杆菌的启动基因。供体菌DNA的HindⅢ片段与pHE5重组后转化大肠杆菌,获得一批带启动基因的抗四环素转化子,其中四株的抗性达到200μg/mL,从这四株高抗性转化子中提取质粒,并对其中的一个重组质粒pAE23的插入片段进行限制性图谱分析和缺失研究,获得了一个缺失了部份片段,四环素抗性仍达到200μg/mL的衍生质粒pAED23,经酶切分析证明其上的启动基因位于0.8kb的EcoR Ⅰ—HindⅢ片段上。点杂交分析证实该片段来自解淀粉芽胞杆菌的DNA。将地衣杆菌的α-淀粉酶基因亚克隆至pAED23启动基因下游的HindⅢ位点上能增强该基因在大肠杆菌中的表达。     

解淀粉芽胞杆菌BaX030的分离鉴定及抗菌功能

摘要:【目的】芽胞杆菌是微生物活性物的重要来源,从全国各地采集的72份土壤样品中分离出339株芽胞杆菌,研究各菌株抑菌活性,分离纯化抑菌活性物,为丰富芽胞杆菌菌种资源和微生物次级代谢物的挖掘奠定实际应用基础。【方法】采用水浴加热和稀释平板涂布等方法从河南花生地采集的土壤中筛选得到一株具有很强抑菌活性的芽胞杆菌,结合形态观察、生理生化特征和16S rRNA基因序列同源性比对分析,对该菌株进行鉴定。丙酮沉淀、葡聚糖凝胶柱层析、C18反相柱层析得到Bacillus amyloliquefaciens X030抑菌活性物,LC-MS/MS鉴定其分子量。利用滤纸片扩散法和平板对峙培养法测定抑菌谱及拮抗性质。【结果】筛选分离得到一株解淀粉芽胞杆菌,归类并命名为解淀粉芽胞杆菌Bacillus amyloliquefaciens X030。BaX030对金黄色葡萄球菌(Staphylococcus aureus)、白色念珠菌(Candida albicans)、酵母菌( Saccharomycetes)有较强抑制效果,对水稻稻瘟病菌(Pyriculariaoryzae)、辣椒尖胞炭疽病菌(Chili pointed cell anthrax)、枇杷炭疽病菌(Gloeosporium eriobotryae speg)、烟草黑胫病菌(Phytophthora parasitica)有良好拮抗活性。初步确定BaX030产生的抑菌活性物为多肽类化合物。【结论】分离得到的B． amyloliquefaciens X030产生了一个对病原细菌具有较强抑制作用的多肽,同时该菌株在拮抗植物病原真菌方面也有明显的效果。     

一株抗水稻纹枯病菌的解淀粉芽胞杆菌分离与鉴定

【目的】筛选对水稻纹枯病菌(Rhizoctonia solani)具有强拮抗作用的细菌菌株。【方法】用指示菌法筛选拮抗菌株;通过形态观察、生理生化实验、Biolog及16S rDNA序列分析鉴定目标菌株;利用平板双向培养法和滤纸片扩散法测定抑菌谱及拮抗性质。【结果】分离到一株高活力的水稻纹枯病菌拮抗菌株YB-3,该菌株属于解淀粉芽胞杆菌(Bacillus amyloliquefaciens);菌株YB-3对常见的14株病原真菌和7株细菌具有较强的拮抗作用,并发现其对亲缘关系较近的芽孢菌属有较强的拮抗作用;该菌株的抑制活性具有温度稳定、耐酸、但对蛋白酶敏感的特点。【结论】通过指示菌法筛选到一株对水稻纹枯病菌有强拮抗作用的解淀粉芽胞杆菌(B.amyloliquefaciens)YB-3,它具有广谱、高效的植物病原菌拮抗活性。     

SARS病毒NS-1株稳定性及培养条件的研究

用SARS病毒NS-1株接种Vero细胞,37℃培养,于培养1、2、3、4d收获病毒液,分别置-70℃冻融和4℃释放,于不同时期取样进行病毒滴定。结果显示,SARS病毒NS-1株各代次培养特性和形态学变化完全相同,有较好的抗原特异性,病毒滴度稳定,4℃保存125d,滴度下降2．25lgCCID50／ml,-70℃保存6个月,滴度未见明显下降。SARS病毒NS-1株未经冻融或释放,1d收获的病毒滴度比2、3、4d收获的病毒滴度低,经冻融或释放,1、2、3、4d收获的病毒滴度无明显区别,病毒收获时的病毒滴度与形态学变化成正相关。不同接种条件收获的病毒液,病毒滴度无明显区别。SARS NS-1株有较好的遗传稳定性和保存稳定性,培养2d,4℃释放收获病毒液,细胞悬液与病毒混合接种更简单,易操作,更适合疫苗规模生产。     

蜡状芽孢杆菌S1发酵条件的研究

对一种新近分离的蜡状芽孢杆菌（Bacillus Cereus)菌株S1发酵产新型抗真菌多肽APS的发酵培养基组成（碳,氮源）和工艺条件（发酵温度,初始,PH,通气方式和通气量）进行了摸索,通过单因互实验和正交优化实验,确定了S1发酵培养基的组成。麸皮5％,玉米粉5％,尿素0．2％,或NH4NO31．5％,酵母浸亮1．5％,葡萄糖6％,NaCl0．1％;最适发酵培养温度为28度;最适发酵培养初始Ph为7．4或6．8,。在优化条件下,效价最高为8－10mg/ml,S1生长的最适温度和初始PH为30度和7．0,通气对S1发酵具有显著的影响。     

离子及表面活性剂对蜡状芽孢杆菌S1发酵的影响

APS是一种由新近分离的蜡状芽孢杆菌（Bacillus cereus）菌株S1分泌产生的新型抗真菌环状多肽。研究了不同的离子对菌株S1发酵生产APS的影响，结果表明，阳离子如K^ ,Na^ ,Al^3 对S1产素APS的产生有促进作用，而Ca^2 ,Fe^2 ,Mg^2 表现出抑制作用，有离子中H2PO4^-,HPO^2-4，对产素的产生具有较强的抑制作用，其它阴离子表现出中性作用，在S1发酵的过程，加入浓度为0．2％－0．8％Tween20和10－100u/mL的青霉素G能够增加APS的效价。     

Replication and segregational stability of Bacillus plasmid pBAA1.

A cryptic plasmid, pBAA1, was identified in an industrial Bacillus strain. The plasmid is 6.8 kilobases in size and is present in cells at a copy number of approximately 5 per chromosome equivalent. The plasmid has been maintained under industrial fermentation conditions without apparent selective pressure and so is assumed to be partition proficient. The minimal replicon was localized to a 1.4-kilobase fragment which also contains the functions required for copy number control. The very low level of segregational instability of the minimal replicon suggests that it also contains functions involved in plasmid maintenance. Comparison with other plasmids indicates that pBAA1 belongs to the group of small gram-positive plasmids which replicate by a rolling cycle-type mechanism. A sequence was identified which is required for the efficient conversion of the single plus strand to the double-stranded form during plasmid replication. Deletion of this sequence resulted in a low level of segregational plasmid instability.     

Characterization of Bacillus anthracis typical virulent test strain 81/1

The results of the prolonged and many-sided study of B. anthracis strain 81/1 by different authors are presented. The cultural and morphological, biochemical, antigenic, molecular-genetic characteristics of this strain give grounds for regarding it as a typical test strain to be used for the determination of the vaccines immunogenicity, the effectiveness of antibiotics and immunomodulators.     

Re-identification of the halotolerant, biosurfactant-producing Bacillus licheniformis strain JF-2 as Bacillus mojavensis strain JF-2

Bacillus strain JF-2 (ATCC 39307) is a halotolerant, biosurfactant-producing bacterium that was initially described as a member of the species Bacillus licheniformis based on a limited set of phenotypic characteristics. Here, genetic and phenotypic analyses were employed to determine the relationship of Bacillus strain JF-2 to other Bacillus strains. The restriction patterns with AluI and analysis of gyrA and 16S rRNA gene sequences grouped Bacillus strain JF-2 with B. mojavensis^T and not with B. licheniformis^T. DNA–DNA similarity showed JF-2 was 75% similar to B. mojavensis^T and only 11% similar to B. licheniformis^T. Both strain JF-2 and B. mojavensis^T required DNA for anaerobic growth, but B. licheniformis^T did not. B. mojavensis^T and strain JF-2 did not grow anaerobically in thioglycollate medium or aerobically with propionate while B. licheniformis^T grew under these conditions. DNA–DNA similarity, gene sequence data and phenotypic characteristics all support the assignment of JF-2 as a member of the species B. mojavensis.     

Bioenergetic properties of the thermoalkaliphilic Bacillus sp. strain TA2.A1

The thermoalkaliphilic Bacillus sp. strain TA2.A1 was able to grow in pH-controlled batch culture containing a nonfermentable growth substrate from pH 7.5 to 10.0 with no significant change in its specific growth rate, demonstrating that this bacterium is a facultative alkaliphile. Growth at pH 10.0 was sensitive to the protonophore carbonyl cyanide m-chlorophenylhydrazone, suggesting that a proton motive force (Deltap) generated via aerobic respiration was an obligate requirement for growth of strain TA2.A1. Strain TA2.A1 exhibited intracellular pH homeostasis as the external pH increased from 7.5 to 10.0; however, the maximum DeltapH generated over this pH range was only 1.1 units at an external pH of 9.5. The membrane potential (Deltapsi) was maintained between -114 mV and -150 mV, and little significant change was observed over the pH range for growth. In contrast, the Deltap declined from -164 mV at pH 7.5 to approximately -78 mV at pH 10.0. An inwardly directed sodium motive force (DeltapNa(+)) of -100 mV at pH 10.0 indicated that cellular processes (i.e., solute transport) dependent on a sodium gradient would not be affected by the adverse Deltap. The phosphorylation potential of strain TA2.A1 was maintained between -300 mV and -418 mV, and the calculated H(+)/ATP stoichiometry of the ATP synthase increased from 2.0 at pH 7.5 to 5.7 at pH 10.0. Based on these data, vigorous growth of strain TA2.A1 correlated well with the DeltapNa(+), phosphorylation potential, and the ATP/ADP ratio, but not with Deltap. This communication represents the first report on the bioenergetics of an extremely thermoalkaliphilic aerobic bacterium.