激光与抗性突变筛选技术相结合选育抗肿瘤抗生素博安霉素高产菌株

目的:获得博安霉素高产菌株,同时比较了铜蒸汽激光与妥布霉素抗性及二者复合诱变的选育效果。方法:采用铜蒸汽激光辐照30 min与妥布霉素100 r/m L抗性处理及其复合诱变选育博安霉素产生菌轮枝链霉菌(S.verticillus)B-31。结果:在复合诱变组中,获得一株高产突变株GB-160,经发酵罐应用后,发酵单位较出发菌株提高1.5倍,并且遗传性能稳定。结论:该方法能有效获得抗生素高产优质菌株。在医药生物工程中,具有较高的实用价值,为其它药物微生物选育提供借鉴。     

极端污染环境草甘膦抗性菌株的分离、鉴定及特性

[目的]筛选高抗草甘膦菌株并对其进行鉴定和特性研究.[方法]从草甘膦极端污染土壤中分离高抗草甘膦菌株,并检测其草甘膦耐受能力,最适生长pH和抗生素抗性.通过生理生化特征和分子生物学特征的测定对该菌株进行鉴定.[结果]从草甘膦极端污染土壤中分离到一株高抗草甘膦的菌株SL06500,该菌株最高耐受草甘膦浓度为500 mmol/L,并且在200～500 mmol/L之间,菌株生长迅速,最适生长pH为4.0,具有氨苄青霉素、卡那霉素、四环素和氯霉素抗性.用16S rDNA的通用引物,经PCR扩增、测序得到SL06500的16S rDNA序列,该序列在GenBank的登录号为EU006066.将此序列经NCBI Blast进行核苷酸比对发现SL06500与无色杆菌属(Achromobacter)和产碱杆菌属(Alcaligenes)的Identity值均为99%.按照1994年版伯杰氏鉴定细菌学手册的命名规则,结合生理生化指标测定的结果,将菌株命名为木糖氧化产碱杆菌木糖氧化亚种SL06500 (Alcaligenes xylosoxidans subsp.xylosoxidans SL06500).[结论]该菌株的较高草甘膦抗性和嗜药性的特点值得我们进行进一步的研究.更重要的是,这是首次关于木糖氧化产碱杆菌木糖氧化亚种草甘膦抗性的报道.     

六价铬还原细菌Bacillus cereus S5.4的筛选鉴定及还原特性研究

六价铬生物毒性极大,是造成环境污染的主要重金属之一,其生物治理策略已引起了广泛关注。已经发现许多微生物具有六价铬抗性和还原性,但能工业应用的还十分有限。从宝钢电镀污泥中分离得到一系列高六价铬抗性菌株,其中一株S5.4显示出高六价铬还原性,经形态和生理生化特征及16s rDNA序列比对,鉴定为Bacillus cereus。该菌株好氧生长,在固体LB培养基上培养48h能耐受40mmol/L Cr6 ,并对Mn2 、Ba2 和Mo6 也显出高抗性;在液体LB培养基中培养72h完全还原2mmol/L Cr6 ,并能在补充培养基和六价铬的条件下连续还原。该菌株还原六价铬时,最适浓度为2mmol/L Cr6 ,最适温度范围30~37℃,最适pH 7~9。     

新疆罗布泊周边地区极端环境嗜盐菌的研究

为了研究分析新疆罗布泊周边地区pH值5-6的盐湖嗜盐古菌资源。从湖中分离筛选出一批嗜盐古菌,对其进行了生理生化特性研究,发现其中6株菌的生理特性和产酶特性比较特殊,并采用PCR方法扩增出其16SrRNA基因（16S rDNA）,并测定了基因的核苷酸序列。基于16S rDNA序列的同源性比较以及16S rDNA序列的系统发育学研究表明,菌株B20-RDX是盐盒菌属Haloarchaeon属中新种成员,GenBank登录号为FJ561285,该菌株为革兰氏阴性菌,最适盐浓度25%,最适pH 8.0,能产过氧化氢酶、淀粉酶,对四环素有抗性,能利用精氨酸和丁二酸盐。迄今为止,国内极少有关罗布泊周边地区极端环境微生物研究的报道,该研究可为今后研究同类极端环境中新的物种资源开发应用以及微生物多样性研究提供素材和参考。     

海州香薷（Elsholtzia splendens）根际铜抗性细菌的筛选及生物多样性

摘要：【目的】重金属耐性植物海州香薷根际铜抗性细菌的筛选及生物多样性研究将有助于了解微生物－超富集植物相互关系和植物修复机理、开发微生物－香薷重金属修复新技术。【方法】采用稀释平板涂布法从海州香薷根际筛选铜抗性菌株,测定菌株溶磷和产生吲哚乙酸、铁载体、1-氨基环丙烷-1-羧酸（ACC）脱氨酶的特性,采用16S rDNA限制性酶切多态性分析（amplified rDNA restriction analysis, ARDRA）研究铜抗性细菌的遗传多样性,根据16S rDNA相似性对产ACC脱氨酶的菌株进行了     

一株抗重金属铜镉细菌的分离、鉴定及其16S rDNA的序列分析

从湖北省大冶市矿区土壤中分离到一株高抗铜和镉的菌株,命名为NTG-01。该菌株可以单抗4.5mmol/L的铜和2mmol/L的镉,因此它是研究抗铜或镉机制的重要菌株。对分离到的NTG-01进行了形态学观察和生理生化鉴定以及16S rDNA序列分析。结果显示菌株NTG-01为细菌,革兰氏染色阴性,短杆状,鞭毛周生,菌体大小约为0.8μm×2.0μm,V-P实验阳性,甲基红实验阴性,利用葡萄糖产酸产气;通过对菌株NTG-01的16S rDNA序列进行测定和同源性比对,发现它与产气肠杆菌的16S rDNA有高达99%的同源性,结合形态和生理生化指标,将其鉴定为产气肠杆菌(Enterobacter aerogenes)。通过测定NTG-01对9种重金属的M IC值,可知它对多种重金属具有普遍较高的抗性。     

溶剂稳定性蛋白酶产生菌的筛选和鉴定

自油污土样等样品中分离获得一株具有产胞外溶剂稳定性蛋白酶的耐有机溶剂极端微生物,经BIOLOG系统鉴定及16S rDNA序列(GenBank,EF105377)分析,该菌株为Bacillus licheniformis YP1。该菌株能耐受中浓度盐、强碱性环境(pH12)及多种不同浓度的有机溶剂,但对多种抗生素敏感。在YP1产蛋白酶发酵过程中添加各种有机溶剂结果表明,丙酮虽抑制了菌体生物量的生长却促进了单位菌体的蛋白酶分泌,而长链烷醇如辛醇、十二醇等能强烈抑制该蛋白酶的分泌。该菌株所产蛋白酶经11种50%(V/V)有机溶剂处理后均能保留高活力。该溶剂稳定性蛋白酶在有机相生物催化等领域具有良好的应用前景。     

胡杨根际细菌提高木本植物对重金属胁迫的耐受性

胡杨是我国西北荒漠地区特有的、对多种非生物逆境具有高抗逆性的树种,但其相关微生物的生态和生理功能研究还比较缺乏.本文从新疆沙雅地区原始胡杨林根际土壤中分离出重金属抗性细菌共72株.其中具有单一重金属(Cu²⁺、Ni²⁺、Pb²⁺或Zn²⁺)抗性的细菌菌株50株,有三重以上重金属抗性的菌株9株.将其中5株多重重金属抗性细菌接种至生根的竹柳插条,进行重金属胁迫下的盆栽培养.结果表明: 在铜或锌胁迫下,5株多重重金属抗性细菌对竹柳的生长抑制有不同程度的缓解,其中假单胞菌Z30和贪铜菌N8菌对铜和锌两种胁迫下竹柳生物量的增长与不接菌对照相比均达到显著差异水平.说明在非重金属污染区生长的胡杨根际存在多样性的重金属抗性细菌,其中一些多重重金属抗性菌对改善重金属胁迫下植物的生长有显著作用,具有应用于木本植物-微生物联合修复环境重金属污染的价值.     

耐盐碱菌株的分离筛选及生物学特性和盐碱去除效率的研究

将采集于黑龙江省大庆市盐碱地的土壤样品经适当稀释后,涂布于高盐碱的培养基中,分离纯化获得41株菌。经过不断分别或同时提高培养基的盐、碱浓度进行耐盐碱菌株的筛选,获得1株耐盐碱菌株7,其在pH值13且盐(NaCl)浓度达到200g.L-1的培养基中仍可生长,该菌株既属于极端嗜盐微生物又属于极端嗜碱微生物。分别于不同碳源、氮源、碳氮比、初始pH值和培养温度条件下,对菌株7的生物学特性和盐、碱去除能力进行研究。结果表明,该菌株生长和去除盐碱的最佳碳源为牛肉膏;最佳氮源为蛋白胨;碳氮比为4:1时,最有利于菌株的生长和对盐、碱的去除;菌株生长的最适初始pH值为9.5,最适温度为20℃,而盐、碱去除的最佳温度则为30～35℃。     

粪臭素高效降解菌YKSW-6的分离、鉴定及降解特性

【背景】粪臭素是畜牧堆肥中有机污染物的主要成分,造成养殖场及周边环境恶化,粪臭素污染问题亟待解决,利用微生物降解粪臭素是一种环保节能的有效方法。【目的】分离鉴定粪臭素高效降解菌株,研究其降解特性,为粪臭素降解提供高效的菌种资源,为该菌株应用于臭味污染环境的净化提供基础。【方法】以粪臭素为唯一碳源的无机盐培养基作为培养基质,从猪粪堆肥样品中分离筛选粪臭素高效降解菌株,通过形态特征和16S rRNA基因序列分析进行分离菌株的初步鉴定,分析其生长规律及粪臭素降解特性,并利用气相色谱质谱联用(GC-MS)对菌株代谢粪臭素的产物进行分析。【结果】从样品中分离获得一株能以粪臭素为唯一碳源的细菌YKSW-6菌株,形态学和16S rRNA基因序列分析初步鉴定该菌株为戈登氏红球菌(Rhodococcus gordoniae)。接种量为10%时,该菌培养14 h对100 mg/L的粪臭素降解率达到100%。其能够利用D-山梨醇、溴-丁二酸等18种碳源,对亚碲酸钾、溴酸钾等13种化学敏感物具有抗性。菌株YKSW-6在5%接种量、温度30-42℃和pH值为6.0-9.0时对100 mg/L的粪臭素降解效率均能达到100%,菌株生长和降解粪臭素的最佳条件为：pH 7.2,温度37℃,转速180 r/min。GC-MS结果表明,粪臭素在菌株的作用下C2先被氧化,转变为3-甲基羟基吲哚,随后进一步被氧化为N-(2-乙酰基苯基)甲酰胺。同时中间产物还有苯乙醛和苯乙酸。【结论】红球菌YKSW-6为目前已报道的降解粪臭素能力较强的菌株,丰富了粪臭素降解菌种的资源库,为实际环境微生物修复应用提供了理论参考。     

一株分离于工业污水池的耐碱酵母

目的:从新疆温泉县一个碱性工业污水处理池中分离并鉴定耐碱酵母菌。方法:用稀释平板法分离菌种,通过形态学观察、生理生化特征及26S rDNA D1/D2区基因序列分析鉴定菌种。结果:从水样中分离得到一株耐碱酵母菌,它们能在pH3.5~11.0,12%NaCl,4~45℃生长,经形态观察及生理生化特征鉴定为酵母属,对其26S rDNA 5’端D1/D2区基因序列进行了PCR扩增并测序,GenBank注册号为DQ132884,同源序列分析结果表明该序列与酿酒酵母(Saccharomyces cerevisiae)Sb4有99.8%的同源性,因此将其命名为酿酒酵母(Saccharomyces cerevisiae)XJU-2,该菌种已保藏于中国微生物菌种保藏委员会普通微生物中心(CGM-CC),保藏号为CGMCC No.2.3095。结论:XJU-2的最高耐碱值可达pH 11.0,而且酸碱耐受范围很大,性能明显优于国内外已报道的酿酒酵母菌种。     

斑马鱼肠道中一株酵母菌菌株的鉴定与系统发育分析

从斑马鱼肠道中分离到一株酵母菌,编号为ZF-5,进行了形态学观察、生理特征测定和26S rDNA D1/D2序列分析,并构建系统发育树。结果表明ZF-5菌株细胞呈卵圆形或杆状,为芽殖,有假菌丝;除乳糖外,能够发酵葡萄糖、蔗糖、麦芽糖等多种碳源;26S rDNA D1/D2区序列分析表明与季也蒙毕赤酵母Pichia guilliermondii的序列相似性最高,构建的系统发育进化树显示菌株ZF-5与Pichia guilliermondii模式菌株CBS 2030（= NRRL Y-2075）亲缘关系最近,     

一株分离自酸梅酱的酵母菌的分离鉴定

目的:分离及鉴定来自于新疆塔城民间自制酸梅酱中的酵母菌。方法:用NL1/NL4引物对扩增酵母菌株的26S rDNAD1/D2区,测序结果进行序列分析,用Neighbour-joining(N-J)方法构建系统发育进化树,同时结合酵母的传统形态学鉴定对菌株进行鉴定。结果:26S rDNA D1/D2区序列分析表明菌株KKS与Metschnikowia aff.fructicola D3895相近,相似率为99.2%。在N-J法构建的系统发育进化树中,菌株KKS与Metschnikowia aff.fructicola聚类在同一分枝上。结论:从新疆塔城民间自制酸梅酱中分离得到一株酵母菌并将该菌株鉴定为Metschnikowia aff.fructicola。     

Trichosporon mycotoxinivorans sp. nov., a new yeast species useful in biological detoxification of various mycotoxins

A yeast strain isolated from the hindgut of the lower termite Mastotermes darwiniensis (Mastotermitidae) was found to represent a new member of the genus Trichosporon. Trichosporon mycotoxinivorans is closely related to T. loubieri on the basis of the phylogenetic trees based on the D1/D2 region of 26S rDNA, an approx. 600 bp fragment of the 18S rDNA and both ITS regions. However, the two species differ at nine positions in the D1/D2 region of 26S rDNA. The IGS1 region of T. mycotoxinivorans is 401 bp long. T. mycotoxinivorans is distinguished from T. loubieri by its ability to assimilate inulin and galactitol, and its inability to grow at 40 °C. The name of this newly isolated strain refers to an important characteristics of T. mycotoxinivorans to detoxify mycotoxins such as ochratoxin A and zearalenone. Therefore this strain can be used for the deactivation of the respective mycotoxins in animal feeds.     

Identification of a newly isolated erythritol-producing yeast and cloning of its erythritol reductase genes

A new erythritol-producing yeast (strain BH010) was isolated in this study. Analysis of the D1/D2 domain of the 26S rDNA sequence, the ITS/5.8S rDNA sequence, and the 18S rDNA sequence allowed the taxonomic position of strain BH010 to be discussed and it was identified and named Moniliella sp. BH010. Physiological characteristics were described. Scanning electron micrography clearly indicated that the cells were cylindrical to elliptical with an average size of 5?×?10?μm when growing in liquid medium, and that pseudohyphae and blastoconidia were observed when cultivated in agar plates. The erythritol reductase genes were cloned, sequenced, and analyzed. BLAST analysis and multiple sequence alignment demonstrated that erythritol reductase genes of Moniliella sp. BH010 shared very high homology with that of Trichosporonoides megachiliensis SNG-42 except for the presence of introns. The deduced amino acid sequences showed high homology to the aldo–keto reductase superfamily.     

Rhodotorula lamellibrachii sp. nov., a new yeast species from a tubeworm collected at the deep-sea floor in Sagami Bay and its phylogenetic analysis

A new species of the genus Rhodotorula was isolated from a tubeworm (Lamellibrachia sp.) collected at a depth of 1156 m in Sagami Bay, Japan. Strain SY-89 had physiological properties quite similar to R. aurantiaca. Two phylogenetic trees, one based on internal transcribed spacer (ITS) regions and 5.8S rDNA sequences and the other based on the D1/D2 region of the large subunit (26S) rDNA sequences, united strain SY-89 to the type strain of Sakaguchia dacryoides through a considerable evolutionary distance. Strain SY-89 was differentiated from S. dacryoides by the G+C content of the nuclear DNA and differences in the ability to utilize specific carbon and nitrogen compounds. The low complementarity of strain SY-89 DNA to that of the type strain of S. dacryoides confirmed that this strain was genetically unrelated to previously known species. The tubeworm isolates are described as R. lamellibrachii sp. nov. The type strain of R. lamellibrachii is strain SY-89 (= JCM 10907). R. lamellibrachii formed a cluster with Erythrobasidium hasegawianum, R. lactosa, S. dacryoides and Sporobolomyces elongatus on the ITS and 5.8S rDNA phylogenetic tree. These five species shared a signature sequence in 26S rDNA, although this relationship was not supported by phylogeny based on the D1/D2 region of 26S rDNA.     

Isolation and phylogenetic characterization of acidophilic microorganisms indigenous to acidic drainage waters at an abandoned Norwegian copper mine

The biodiversity of culturable acidophilic microbes in three acidic (pH 2.7–3.7), metal-rich waters at an abandoned subarctic copper mine in central Norway was assessed. Acidophilic bacteria were isolated by plating on selective solid media, and dominant isolates were identified from their physiological characteristics and 16S rRNA gene sequences. The dominant iron-oxidizing acidophile in all three waters was an Acidithiobacillus ferrooxidans -like eubacterium, which shared 98% 16S rDNA identity with the type strain. A strain of Leptospirillum ferrooxidans was obtained from one of the waters after enrichment in pyrite medium, but this iron oxidizer was below detectable levels in the acidic waters themselves. In two sites, there were up to six distinct heterotrophic acidophiles, present at 10³ ml⁻¹. These included Acidiphilium -like isolates (one closely related to Acidiphilium rubrum , a second to Acidiphilium cryptum and a third apparently novel isolate), an Acidocella -like isolate (96% 16S rDNA identity to Acidocella facilis ) and a bacterium that shared 94.5% 16S rDNA identity to Acidisphaera rubrifaciens. The other numerically significant heterotrophic isolate was not apparently related to any known acidophile, with the closest match (96% 16S rDNA sequence identity) to an acetogen, Frateuria aurantia . The results indicated that the biodiversity of acidophilic bacteria, especially heterotrophs, in acidic mine waters may be much greater than previously recognized.     

Penicillium chrysogenum var. halophenolicum, a new halotolerant strain with potential in the remediation of aromatic compounds in high salt environments

A halotolerant phenylacetate-degrading fungus Penicillium CLONA2, previously isolated from a salt mine at Algarve (Portugal), was identified as a variant of P. chrysogenum using the ITS-5,8S rDNA and the D1/D2 domain of 28S rDNA sequences. The metabolic features and genetic characteristics suggest that this strain belongs to a subgroup of P. chrysogenum, named var. halophenolicum. The presence of the penicillin biosynthetic cluster was proven by Southern hybridizations using probes internal to the pcbAB and penDE genes and sequencing of the pcbAB-pcbC intergenic region. However the pcbAB-pcbC divergent promoter region contained 20 point modifications with respect to that of the wild type P. chrysogenum NRRL1951. The CLONA2 strain produced non-aromatic natural penicillins rather than benzylpenicillin in a medium containing potassium phenylacetate (the precursor of benzylpenicillin) and was able to grow well on phenylacetatic acid using it as sole carbon source. Due to the ability of P. chrysogenum CLONA2 to degrade aromatic compounds, this strain may be an interesting organism for aromatic compounds remediation in high salinity environments.     

Zygosaccharomyces kombuchaensis,a new ascosporogenous yeast from 'Kombucha tea'

A new ascosporogenous yeast, Zygosaccharomyces kombuchaensis sp. n. (type strain NRRL YB-4811, CBS 8849), is described; it was isolated from Kombucha tea, a popular fermented tea-based beverage. The four known strains of the new species have identical nucleotide sequences in domain D1/D2 of 26S rDNA. Phylogenetic analysis of D1/D2 and 18S rDNA sequences places Z. kombuchaensis near Zygosaccharomyces lentus. The two species are indistinguishable on standard physiological tests used for yeast identification, but can be recognized from differences in restriction fragment length polymorphism patterns obtained by digestion of 18S-ITS1 amplicons with the restriction enzymes DdeI and MboI.     

Bullera hoabinhensis sp. nov., a new ballistoconidiogenous yeast isolated from a plant leaf collected in Vietnam

VY-68, a ballistoconidiogenous yeast strain, isolated from a plant leaf at Cuc Phuong National Park of Ninh Binh Province, Vietnam, was assigned to the genus Bullera based on morphological and chemotaxonomical characteristics. Based on the sequence analyses of 18S rDNA, D1/D2 region of 26S rDNA, and internal transcribed spacer regions (ITS), VY-68 was phylogenetically closely related to Bullera pseudoalba and Cryptococcus cellulolyticus. DNA-DNA reassociation experiments among VY-68, B. pseudoalba and C. cellulolyticus revealed that strain VY-68 is a distinct species, and the latter two are conspecific. Bullera hoabinhensis is proposed for VY-68.