应用分散和差速离心法分离嗜酸和耐酸链霉菌的试验及评价*

新的微生物资源的开发离不开菌种分离技术的改进和分离效率的提高。我们采用一种新的分离方法——分散和差速离心法(Dispersion and Differential Centrifugation,DDC),以传统的振荡法做对照,对12份酸性土壤样品进行了链霉菌的分离。结果表明DDC方法的分离效率是传统方法的2—20倍,且选择性好。用DDC方法共分离出链霉菌249株,归属于12个颜色类群,其中的45株代表菌株的形态和细胞壁类型均符合链霉菌的特征,最适生长pH均为4．5—5．5。结果表明应用DDC方法分离非常见的嗜酸和耐酸链霉菌是可行的。     

嗜酸丝状放线菌的选择性分离与多样性

摘要:【目的】针对酸性土壤中的嗜酸丝状放线菌,建立有效的选择性分离方法,并了解其多样性。【方法】用不同的样品预处理方式和分离培养基,并添加不同的抑制剂进行分离;根据放线菌的菌落数和出菌率确定最佳分离方法组合。采用最佳分离方法对从江西采集的17份酸性土壤样品进行分离;根据培养特征对分离菌株进行分群,进一步通过对各类群的显微形态观察和pH梯度生长实验确定代表菌株;对代表菌株进行16S rRNA基因序列分析研究其多样性。【结果】嗜酸丝状放线菌的最佳分离方法为：土壤样品经分散差速离心预处理后,涂布添加了放线菌酮、制霉菌素和萘啶酮酸（各50 mg/L）的GTV培养基。用此方法共分离到放线菌369株,归为10个不同的颜色类群,其中6.6%为严格嗜酸放线菌,72.4%为中度嗜酸放线菌,21.0%为耐酸放线菌。52株嗜酸放线菌代表菌株分布于放线菌目中的12个属：链霉菌属(Streptomyces)、小单孢菌属(Micromonospora) 、诺卡氏菌属(Nocardia)、野野村菌属(Nonomuraea) 、韩国生工属(Kribbella) 、小双孢菌属(Microbispora)、马杜拉菌属(Actinomadura)、拟无枝菌酸菌属(Amycolatopsis)、指孢囊菌属(Dactylosporangium)、伦茨氏菌属(Lentzea)、游动四孢菌属(Planotetraspora) 和链嗜酸菌属(Streptacidiphilus),其中链霉菌分离菌株在系统发育树上形成12个不同的进化类群。【结论】所建立的选择性分离方法可用于土壤嗜酸丝状放线菌的高效分离;江西酸性土壤含有丰富多样的嗜酸丝状放线菌种属。     

盐地碱蓬内生中度嗜盐菌的分离与系统发育多样性分析

为了了解东营滨海盐地碱蓬植株内生中度嗜盐菌的多样性,采用传统分离鉴定技术和基于16S rRNA序列分析对样品中可培养细菌的多样性进行研究。根据其生理生化特征、16S rRNA序列测定和系统发育分析,分离获得的15株内生菌可分为4个类群,涉及Halomonadaceae科的Chromohalobacter属、Kushneria属、Halomonas属以及Bacillaceae科的Bacillus属。类群I中4菌株的16S rRNA序列与Chromohalobacter israelensis的最高相似性为95%。类群II共7株菌,归属于Kushneria属,是碱蓬内生中度嗜盐菌中的优势类群。类群III菌株的16S rRNA序列与一株尚无明确分类地位的Gammaproteobacteria亚门耐盐固氮细菌Haererehalobacter sp.JG11的相似性为99%。类群IV中的芽孢杆菌的16S rRNA序列与已知细菌的相似性为96%,很可能代表了Bacillus属的新种。各种水解酶类的分析表明,在分离的15株菌中有3株菌产蛋白酶,14株产酯酶,8株产DNA酶,11株产半乳糖苷酶,14株产脲酶。研究结果揭示,盐地碱蓬中存在较为丰富的中度嗜盐菌多样性和系统发育多样性,并且潜藏着较多的新的微生物类群。     

酸性土壤中嗜酸稀有放线菌的多样性研究

从江西、云南、北京采集的10份酸性土样中分离出嗜酸放线菌252株,其绝大部分为链霉菌。通过形态观察、pH梯度生长实验和细胞壁化学组分分析筛选出稀有放线菌代表菌株20株。ARDRA分析表明,它们呈11种不同的图谱类型,其中9株的图谱相同,另外4株的图谱与之差异不大,而其余7株的图谱与之差异很大且各不相同。16S rDNA序列分析表明,20株稀有放线菌中的18株分别属于6个已知属,其中13株属于诺卡氏菌属(Nocordia),它们在系统发育树上处于多个进化分枝;各有1株分别属于壤球菌属(Agrococcus)、节杆菌属(Arthrobacter)、北里孢菌属(Kitasatospora)、考克斯菌属(Kocuria)和嗜酸链霉菌属(Streptacidiphilus);其余2株是迄今尚未定名的一个新科(“Ellin5034 group”)中的成员。实验结果显示,酸性土壤中的嗜酸稀有放线菌具有较丰富的种属多样性,其中诺卡氏菌属(Nocardia)是一优势菌群。     

一株中度嗜热嗜酸硫氧化杆菌的分离和系统发育分析

从云南腾冲温泉酸性水样分离得到一株中度嗜热嗜酸硫氧化杆菌MTH 0 4 ,对分离菌株进行了形态、生理生化特性研究及 1 6SrDNA序列分析。该菌株为革兰氏阴性细菌 ,短杆状 ,菌体大小 (0 6～ 0 8) μm× (1～ 2 ) μm ,化能自养 ,可利用硫磺、四硫酸盐、硫代硫酸盐为能源生长 ,不能利用蛋白胨、葡萄糖、酵母粉 ,也不能进行混合型生长。最适生长温度在 4 0℃～ 4 5℃之间 ,最适生长pH 2 0～ 3 0 ,代时 8h。以 1 6SrDNA序列同源性为基础构建了包括 1 3株相关种属在内的系统发育树 ,结果表明 ,MTH 0 4与喜温硫杆菌 (Thiobacilluscaldus)处于同一进化树分支中 ,相似性达 99 5 %以上     

酸性和碱性土壤新分离的放线菌中线型和环型质粒的检测

从湖南、云南采集的19份酸性土壤样品分离到50株放线菌,在pH4.5和pH7.0的培养基上都能生长.从新疆、青海、云南的14份碱性土壤样品中分离到38株放线菌,在pH10.0和pH7.0的培养基上均能生长.因此,这些菌株属于中度嗜酸或中度嗜碱放线菌.利用脉冲电泳技术和普通凝胶电泳在其中12株放线菌中检测到线型质粒,其中3株放线菌中检测到环型质粒.这是首次在中度嗜酸和中度嗜碱的放线菌中报道线型和环型质粒.     

小溪自然保护区非盐环境土壤中嗜盐和耐盐菌多样性

【目的】研究湖南小溪国家级自然保护区普通非盐环境(ordinary non-saline environment)土壤样品中可培养嗜盐及耐盐细菌(含放线菌)多样性。【方法】采用纯培养法和基于16S rRNA基因序列的系统发育分析对样品中嗜盐及耐盐细菌多样性进行研究。【结果】用补充5%-20%(w/v)NaCl的MA、ISP2、ISP5、NA和HAA培养基从土壤样品中分离到114株细菌,其中8株为中度嗜盐菌,19株为轻度嗜盐菌,87株为耐盐菌。根据形态观察和部分生理生化实验结果去冗余,选取61个代表性菌株进行基于16S rRNA基因序列的系统发育多样性分析。结果表明,这些菌株属于细菌域(Bacteria)的3个大的系统发育类群(门;phylum)(Actinobacteria,Firmicutes,Proteobacteria)的16个科、18个属,代表了41个物种。多数菌株属于Firmicutes门(38株,62.3%)和Actinobacteria门(18株,29.5%)。大多数菌株与其系统发育关系最密切的已知物种的典型菌株之间存在一定的遗传差异(16S rRNA基因序列相似性为96.9%-99.8%),其中有7个菌株(JSM070026,JSM081004,JSM081006,JSM081008,JSM083058,JSM083085,JSM084035)代表7个潜在新种(potential novel species)。【结论】研究结果表明,湖南小溪国家级自然保护区普通非盐环境土壤中存在较为丰富的可培养嗜盐及耐盐细菌多样性,并且潜藏着较多新的微生物类群(物种)。     

新疆塔里木盆地可培养嗜盐放线菌系统发育多样性

应用纯培养手段和基于16S rRNA基因序列的系统发育分析,对从塔里木盆地高盐环境土壤样品中分离的18株可培养嗜盐放线菌多样性进行了研究.实验结果表明,18株嗜盐放线菌可3个(GlycomycetaceaePseudonocardineae和Nocardiopsaceae),在有效发表的5个属的嗜盐放线菌中有4个属的嗜盐放线菌被分离到.多数菌株属于Actinopolyspora属(38.9%),Nocardiopsis属(27.8%)和Streptomonospora属(22.2%),是塔里木盆地高盐环境中嗜盐放线菌的优势类群.这些分离菌株中,菌株YIM 92370与最近种的相似性为92%,在Glycomycetaceae科内形成一个独立的分支,极有可能代表Glycomycetaceae科的一个新属.研究结果表明塔里木盆地高盐环境中存在有较为丰富的嗜盐放线菌系统发育多样性,并且潜藏着新类型的放线菌资源.     

天山一号冰川底部沉积层产蛋白酶耐低温菌株的筛选及其系统发育

[目的]通过对天山一号冰川底部沉积层耐低温菌的分离和其中产蛋白酶菌株的筛选,了解冰川微生物生理多样性和系统发育多样性,为高效低温蛋白酶生物技术的研发奠定基础.[方法]采用稀浓度的R2A、TSB平板涂布分离可培养细菌,通过脱脂乳选择性培养基筛选产蛋白酶的耐低温菌株.对分离菌株表型特征、生理生化特性、最适生长温度、耐盐性、产酶性能进行了比较,结合16S rRNA基因序列同源性分析确定产蛋白酶菌株的多样性和系统进化地位,通过BOX-PCR指纹技术分析16S rRNA基因序列高相似度的近缘菌株的遗传差异.[结果]从125株分离物中筛选到27株产蛋白酶的耐低温菌株,其中21株为适冷菌,仅6株菌为专性嗜冷菌,革兰氏阴性菌居多,假单胞菌属(Pseudomonas)菌株占40.7％.产酶菌株隶属于5个系统发育类群、9个属,其中γ-Proteobacteria、Actinobacteria、CFB(Cytophaga-Flexibacter-Bacteroides)为优势类群.[结论]天山1号冰川底部沉积层冻土中产蛋白酶的耐低温细菌多样性较丰富,本研究筛选得到的同属近缘种群较多,其产酶性状存在差异,适合开展微生物种群的生物地理学研究.     

大连海域沉积物中可培养海洋链霉菌活性及其多样性

以大肠杆菌、金黄色葡萄球菌和尖孢镰刀枯萎病菌作为测试靶目标,采用9种分离培养基从大连海域13个不同采样点的海洋沉积物样品中分离到165株海洋链霉菌。从165株海洋放线菌中筛选到对金黄色葡萄球菌具有抑制活性的菌株85株,占总菌株数的51.5%;对大肠杆菌具有抑制活性的菌株27株,占总菌株数的16.4%;对尖孢镰刀枯萎病菌具有抑制活性的菌株仅有6株,占总菌株数的3.6%。因此,海洋链霉菌的活性更多地表现为对细菌的抗性,尤其对革兰氏阳性细菌具有更高的抑制活性。对其中具有抑制活性或形态独特的菌株进行了16S r DNA序列分析,并构建系统发育树,显示活性海洋链霉菌具有丰富的种类多样性和广谱抗菌活性。同种海洋链霉菌与土壤链霉菌活性比较结果也表明,海洋链霉菌多表现抗革兰氏阳性细菌活性。     

Phylogenetic diversity of acidophilic sporoactinobacteria isolated from various soils

Spore forming actinobacteria (sporoactinobacteria) isolated from soils with an acidic pH in Pinus thunbergii forests and coal mine waste were subjected to taxonomic characterization. For the isolation of acidophilic actinobacteria, acidified starch casein agar (pH adjusted to 4-5) was used. The numbers of actinobacteria growing in acidic media were between 3.2 x 10(4) and 8.0 x 10(6) CFU/g soil. Forty three acidophilic actinobacterial strains were isolated and their 16S rDNA sequences were determined. The isolates were divided into eight distinctive phylogenetic clusters within the variation encompassed by the family Streptomycetaceae. Four clusters among them were assigned to the genus Streptacidiphilus, whereas the remaining four were assigned to Streptomyces. The clusters belonging to either Streptomyces or Streptacidiphilus did not form monophyletic clade. The growth pH profiles indicated that the representative isolates grew best between pH 5 and 6. It is evident from this study that acidity has played a critical role in the differentiation of the family Streptomycetaceae, and also that different mechanisms might have resulted in the evolution of two groups, Streptacidiphilus (strict acidophiles) and neutrotolerant acidophilic Streptomyces. The effect of geographic separation was clearly seen among the Streptacidiphilus isolates, which may be a key factor in speciation of the genus.     

Classification of acidophilic, neutrotolerant and neutrophilic streptomycetes by nucleotide sequencing of 5S ribosomal RNA.

Complete 5S ribosomal RNA sequences were obtained for four acidophilic actinomycetes, seven neutrophilic streptomycetes and a strain of Streptoverticillium baldaccii. All of the organisms contained RNAs belonging to the 120 nucleotide type. An evolutionary tree was generated after combining the test data with results from similar studies on representative Gram-positive bacteria. The acidophilic, neutrotolerant and neutrophilic actinomycetes were recovered in a distinct cluster that was equated with the genus Streptomyces. The sequence data support the view that the genera Chainia, Elytrosporangium, Kitasatoa and Microellobosporia should be considered as synonyms of the genus Streptomyces. The recovery of the Streptoverticillium baldaccii strain on the fringe of the Streptomyces cluster is also consistent with current trends in the taxonomy of these organisms. Further work is needed to determine the taxonomic status of the two streptomycete subgroups that comprised the streptomycete cluster.     

Influences of soil acidity on Streptomyces populations inhabiting forest soils.

The Streptomyces populations inhabiting five acidic forest soils were examined. It was found that lowering the pH of a medium selective for streptomycetes (starch-casein agar) to the pH of the particular soil horizon being plated influenced both the total numbers and types of streptomycetes that were isolated from the soils examined in this study. On the acidified medium both the numbers of streptomycetes and the percentage of total bacteria on the plates represented by streptomycetes increased (as compared with the same medium with a pH of 7.2). These differences were greatest on the isolations from the most acid soils. The largest concentrations of streptomycetes were found in the surface horizon (0 to 15 cm) and the litter layer immediately over the surface mineral horizon. Acidity tolerance tests demonstrated that random samplings of isolates contained acidophilic, neutrophilic, and acidoduric strains, with the largest numbers of acidophiles being found on the acidified media from the most acid soils. There were no differences between overall utilization of selected carbohydrates among the isolates taken from either the neutral or acidic media, although a larger proportion of the acid media isolates produced acid from the carbohydrates. Evidence is presented which indicates that different types of streptomycetes were isolated on the acid media, and possible reasons for the presence of these acid-tolerant populations are discussed.     

Influences of soil acidity on Streptomyces populations inhabiting forest soils.

The Streptomyces populations inhabiting five acidic forest soils were examined. It was found that lowering the pH of a medium selective for streptomycetes (starch-casein agar) to the pH of the particular soil horizon being plated influenced both the total numbers and types of streptomycetes that were isolated from the soils examined in this study. On the acidified medium both the numbers of streptomycetes and the percentage of total bacteria on the plates represented by streptomycetes increased (as compared with the same medium with a pH of 7.2). These differences were greatest on the isolations from the most acid soils. The largest concentrations of streptomycetes were found in the surface horizon (0 to 15 cm) and the litter layer immediately over the surface mineral horizon. Acidity tolerance tests demonstrated that random samplings of isolates contained acidophilic, neutrophilic, and acidoduric strains, with the largest numbers of acidophiles being found on the acidified media from the most acid soils. There were no differences between overall utilization of selected carbohydrates among the isolates taken from either the neutral or acidic media, although a larger proportion of the acid media isolates produced acid from the carbohydrates. Evidence is presented which indicates that different types of streptomycetes were isolated on the acid media, and possible reasons for the presence of these acid-tolerant populations are discussed.     

百部内生放线菌的分离、分类及次级代谢潜力

【目的】以对叶百部块根为材料分离内生放线菌,并对分离菌株进行分类、抗菌活性和次级代谢产物合成基因研究。【方法】样品经过严格的表面消毒,选用4种培养基分离百部内生放线菌;分离菌株通过形态观察和16S rRNA序列分析进行分类鉴定;采用琼脂移块法测试分离菌株的抗菌活性;通过PCR检测分离菌株的PKS/NPRS和卤化酶基因;使用HPLC-UV/VIS-ESI-MS/MS分析发酵产物。【结果】从6个样品中获得18株内生放线菌,分属链霉菌属(Streptomyces)、小单孢菌属(Micromonospora)、假诺卡氏菌属(Pseudonocardia)和甲基杆菌属(Methylobacterium)。分离菌株绝大部分具有抗菌活性和次级代谢产物合成基因,其中13株对耐药金黄色葡萄球菌和/或绿脓杆菌有拮抗活性,17株具有PKS/NRPS基因,8株菌具有卤化酶基因,且卤化酶阳性代表菌株的发酵产物具有抗细菌活性和卤代化合物特征。【结论】百部作为一种传统中药,其内生放线菌以链霉菌和小单孢菌为主,在次级代谢产物合成方面具有很好的潜力,可作为一类重要微生物资源进行活性产物开发。     

Acidophilic soil actinomycetes

A clear-cut dependence of the distribution of acidophilic actinomycetes on the pH value of soil was established. Acidophilic actinomycetes were found to be present in soils whose pH does not exceed 6.8 (acid forest soils, lowland peaty soil, and ordinary chernozem) and not in slightly alkaline soils (chestnut sodic and alluvial meadow soils). In the acid lowland peaty soil, the species diversity of acidophilic streptomycetes was lesser than the species diversity of streptomycetes revealed in the same soil by using neutral medium.     

Acidophilic Soil Actinomycetes

A clear-cut dependence of the distribution of acidophilic actinomycetes on the pH value of soil was established. Acidophilic actinomycetes were found to be present in soils whose pH does not exceed 6.8 (acid forest soils, lowland peaty soil, and ordinary chernozem) and not in slightly alkaline soils (chestnut sodic and alluvial meadow soils). In acid lowland peaty soil, the species diversity of acidophilic streptomycetes was lesser than the species diversity of streptomycetes revealed in the same soil by using neutral medium.     

西藏地区土壤放线菌种群多样性及拮抗活性研究

从西藏不同海拔、不同气候条件的5个地区采集的10份土样中,使用选择分离培养基、ISP 2（Yeast extract_malt extract agar）和高氏一号培养基,通过分散差速离心法（Dispersion and differential centrifugation,DDC）分离得到放线菌156株。根据形态和培养特征将其归入32个类群,并从中选出65个代表菌株进行全细胞壁氨基酸组分分析,结果表明：９株菌为非链霉菌胞壁类型,其余为链霉菌胞壁类型。16S rDNA扩增片段长度多态性（ARDRA）分析得到不同带型,对其序列分析结果表明：分离菌株分属链霉菌属（Streptomyces）和5个稀有放线菌属。同时测试了代表菌株抗耐药细菌和真菌的活性,其中38.5%的菌株具有拮抗活性。