青海甜醅中乳酸菌种群构成及病原菌拮抗性菌株的分离鉴定

应用高通量测序方法对采集自青海地区的甜醅样品中的乳酸菌种群进行分析,以探索青海传统发酵食品甜醅中的乳酸菌构成并进行功能乳酸菌分离,同时以大肠杆菌、沙门氏菌、蜡样芽孢杆菌和金黄色葡萄球菌4种病原菌为指示菌,对其中病原菌拮抗性菌株进行了筛选与鉴定。结果表明:青海甜醅优势乳酸菌为Pediococcus acidilactici、Lactobacillus plantarum、Lactobacillus crustorum、Leuconostoc pseudomesenteroides,以及4种未能分类的乳酸杆菌(Lactobacillus sp.)。抑菌试验结果显示:1株乳酸菌分离株B29对4种指示菌均具有高效抑制效应,胞外产物抑菌作用受蛋白酶影响最大。通过革兰氏染色镜检、扫描电镜进行细胞形态观察、生理生化特征鉴定及16S rDNA测序鉴定,结果表明分离株B29为植物乳杆菌。

虾酱中益生芽孢杆菌的筛选及其潜在益生效果的研究

为了获得具有潜在促生长及拮抗病原菌能力的水产动物益生菌,本研究在分离和筛选的基础上,从虾酱中获得6株菌,经测序和分子鉴定后,进一步评估了其耐人工胃肠液性能、自凝集率、表面疏水活性和抗生素敏感性.结果表明:这6株菌均产酸和不溶血,其中A20、B3、B47和B89的产酸能力较好,可使发酵液pH降低1.5;A20、A27、A35、B47的蛋白酶和淀粉酶活性显著高于其他菌株,水解圈大小在4 mm以上;A20和B3对5种鱼类致病菌均具有较强的拮抗能力,抗菌圈直径H(mm)和菌落直径C(mm)的比值H/C超过1.5;16S rRNA测序鉴定表明,A20、A27、B3和B89为巨大芽孢杆菌(Bacillus megaterium),A35和B47则分别为枯草芽孢杆菌(B.subtilis)和弯曲芽孢杆菌(B.flexus).进一步的实验表明:A20、A27、B47和B89具有较强的耐人工胃液能力,菌株存活率在60%左右,A27在肠液处理后的存活率高达90%;A20和A27于各个时间段的自凝集率都高于其他菌株,24 h时达到了98%;A35和B89在三种溶剂中都表现出较高的疏水活性;A20对21种抗生素敏感,敏感率最高为80.7%.综合以上结果,巨大芽孢杆菌A20具有优良的益生潜能,可将其用于后续益生菌制剂的开发和利用.

Antagonistical Mode of Pichia membranefaciens to Rhizopus stolonifer in Wounds of Peach Fruit

膜醭毕赤酵母 (PichiamembranefaciensHansen)是本实验室从果实上分离获得的一种能有效防治桃果实采后软腐病的拮抗菌。本文将P .membranefaciens与葡枝根霉 (Rhizopusstolonifer)在桃果实伤口部位共培养 2 4h后 ,用扫描电子显微镜观测了它们的拮抗作用。结果表明 ,在有病原菌的地方聚集了大量的酵母拮抗菌 ,而且拮抗菌紧密地吸附在病原菌的菌丝体上。结合以前的研究结果可以推断 ,P .membranefaciens主要通过与病原菌进行营养和空间的竞争 ,紧密地吸附在病原菌菌丝体上分泌能降解病原菌细胞壁的水解酶 (如几丁质酶和 β_1,3_葡聚糖酶 ) ,并可能诱导寄主产生抗性 ,从而抑制桃软腐病的发生。

猪源发酵乳杆菌的筛选及其潜在益生性能

【目的】对从健康仔猪粪便中筛选分离出一株发酵乳杆菌的益生性能进行测试,为其在畜禽动物养殖中的应用提供参考。【方法】采用Rogosa SL完全选择性培养基分离出106株乳酸菌,通过革兰氏染色、酸和胆盐耐受初步筛选出1株潜在的饲用乳酸菌,经16S rDNA序列鉴定为发酵乳杆菌LF1,并对其益生性能潜力进行评估,包括抑菌活性(针对大肠杆菌K88、金黄色葡萄球菌、猪链球菌、沙门氏菌以及弧菌等12种病原菌)、对模拟胃液中酸性环境的耐受性、对胆盐的耐受性以及对小肠上皮细胞的粘附性。【结果】发酵乳杆菌LF1耐酸和耐胆盐的能力较强,显示出较强的益生菌潜力,但LF1菌株对猪肠道上皮细胞的粘附能力不强。在生物拮抗作用方面,发酵乳杆菌LF1的培养上清可以显著抑制多种常见动物病原菌生长。【结论】发酵乳杆菌LF1具有较好的益生性能,通过进一步的动物实验评估后,可以作为应用于畜禽养殖业的益生菌候选菌株。

高寒草地优势植物根际细菌促生特性及初步鉴定

筛选获得能促进高寒草地退化植被生长的优良耐低温植物根际促生细菌(PGPR),能够丰富高寒草地优良菌株资源库。本研究以前期分离的18株细菌菌株为研究对象,采用乙炔还原法、钼锑抗比色法、Salkowski比色法和平板对峙法分别检测了18株菌株的固氮、溶磷、分泌植物生长激素(IAA)和抑制植物病原真菌的能力。结果表明:有14株菌均具有固氮、溶磷、分泌IAA特性,其中固氮酶活性为25.43~230.52nmol·(h·mL)^(-1),溶有机磷量为66.90~115.06μg·mL^(-1),溶无机磷量为9.22~380.28μg·mL^(-1),分泌IAA量为12.45~71.71μg·mL^(-1)。其中2株菌编号为LMG2、LMJ2拮抗病原菌锐顶镰孢菌(Gibberella acuminata)效果显著,对其抑制率分别为30.75%和31.00%。综合比较各菌株特性,筛选出6株优良PGPR进行16S rRNA基因序列比对分析以确定其分类地位。经鉴定:菌株LMG2和LMJ2菌株与Pseudomonas piscium P50^(T)的亲缘关系最近,菌株LMY8与Pseudomonas kairouanensis KC12^(T)的亲缘关系最近,菌株CND1与猴假单胞菌(Pseudomonas simiae Oli^(T))的亲缘关系最近,菌株LNA2、LPA7与Pseudomonas neuropathica P155^(T)的亲缘关系最近。研究筛选的6株耐低温菌株兼具多种优良特性,对高寒退化草地的植被修复具有应用潜力,可为后续制备修复高寒退化草地微生物菌剂提供优质菌株资源。

Proteomic study of three component interactions: plant, pathogens and antagonistic fungi

The molecular factors involved in the three-way interaction between plant, pathogenic fungi and antagonistic/biocontrol fungi, such as Trichoderma, are still poorly understood, even if they represent a matter of interest for improving crop management and developing new strategies for plant diseases control. The aim of this work is to investigate the components involved in this interaction and, for this purpose, a proteomic approach was used. 2-D maps of the protein extracts from the single components in various interactions between plants (potato, bean, tobacco or tomato), pathogens (Botrytis cinerea, Rhizoctonia solani or Pythium ultimum) and biocontrol fungi (Trichoderma atroviride strain P1 or Trichoderma harzianum strain T22) were obtained. The proteome of each partner was collected separately and extracted by acetone precipitation in presence of trichloroacetic acid and a reducing agent (DTT). The extracted proteins were separated by isoelectrofocusing (IEF), using IPG (Immobilized pH gradient) strips, followed by SDS-PAGE. In order to improve resolution the separations were performed both on wide than narrow pH range and on different gel lengths. Differential spots were noted in the proteome of the three-way interaction when compared to each single component. These were further characterized by mass spectrometry and in silico analysis with the aim of identifying and cloning the relative genes. During the in vitro interaction of T. harzianum strain T22 with tomato and the culture filtrate or cell walls of pathogens, the spot number was higher than in the presence of pathogen biomass. In terms of Trichoderma differential proteins displayed on 2D gels, the most important changes were obtained in the presence of P. ultimum . During the in vivo interaction with tomato, the antagonist proteome changed much more in presence of soilborne fungi R. solani and P. ultimum than with the foliar fungus B. cinerea, both in terms of total and increased or novel spots. In silico analysis of some of those spots revealed homology with intracellular enzymes (GTPases, hydrolases) and with stress-related proteins (heat shock proteins HSP70, bacteriocin cloacin). Specific proteins in the plant proteome, i.e. pathogenesis-related proteins, have been identified during the in vivo interaction of bean with R. solani and T. atroviride strain P1. This is in agreement with the demonstrated ability of these beneficial fungi to induce plant systemic disease resistance by activating expression of defence-related genes. Proteins extracted from T. atrovride strain P1 which were analysed by mass spectrometry, revealed some interesting homologies with a fungal hydrophobin of Pleurotus ostreatus and an ABC transporter of Ralstonia metallidurans. These could represent molecular factors involved in the antagonistic mechanisms of Trichoderma and play a role in the three-way interaction with the plant and other microbes.