大亚湾海域可培养细菌鉴定及系统发育分析

对大亚湾海域表层水体的可培养细菌进行分离,测定了分离培养细菌的16S rRNA 基因V3 区序列,并采用该研究中的35 个序列与从GenBank 下载的46 个序列构建了系统树,对细菌进行了分子鉴定。在9 个站点的表层水体中共分离得到70株菌株,分属35 个种。其中α-变形菌纲(Alphaproteobacteria)和放线菌纲(Actinobacteria)为分离菌株最多的两个菌纲,分离率分别为40%和35.7%;而β-变形菌纲(Betaproteobacteria)仅分离到1 株(1.4%)。此外,还分离得到盖球菌属(Kytococcus)、间胞囊菌属(Intrasporangium)等非常见菌株。大亚湾海域细菌的Shannon-Wiener's 多样性指数为3.21。大亚湾海域表层水体可培养细菌丰富的种类多样性以及较高的α-变形菌分离率,说明了该海域具有良好的水质,同时也是潜在的微生物菌种资源库。     

宜宾浓香型白酒酿造过程中可培养细菌的系统发育多样性

【目的】为较系统地了解宜宾浓香型白酒酿造过程中可培养细菌的多样性,得到一些潜在的微生物资源。【方法】采用改良的NA培养基和高氏I号培养基分离、去除冗余,测定所得细菌纯培养物的16S rRNA基因,进行系统发育分析。【结果】分离得到603株细菌,4株菌的序列与GenBank中典型菌株序列相似性低于97%,代表着潜在新类群;599株菌与GenBank中34个属、101个种的典型菌株序列相似性大于97%,其中以Bacillus为绝对优势菌(315株),Streptomyces(121株)、Lysinibacillus(35株)、Staphylococcus(45株)为次优势菌,其余各属菌株均在10株以下。而且有16个属均只检测到1株菌。【结论】宜宾浓香型白酒发酵过程中的细菌呈现出较为丰富的多样性和一定的稳定性。     

九香虫(椿象)体内可培养细菌的多样性分析

【目的】认识药用昆虫九香虫(Aspongopus chinesis Dallas)成虫体内可培养细菌资源多样性。【方法】运用纯培养法、反转录重复因子扩增(BOXA1R-PCR)分析技术、16S r RNA基因测序和系统发育分析对样品中可培养细菌进行多样性研究,测定了分离菌株的抗菌特性、吲哚乙酸(IAA)含量和产淀粉酶活性等指标。【结果】通过6种不同培养基共分离得到52株菌落特征不同的细菌菌株。基于菌落特征和BOXA1R-PCR图谱选取12株代表菌株用于16S r RNA基因序列测定。16S r RNA基因序列系统发育分析显示,52株菌株分属于芽孢杆菌属(Bacillus)、假单胞菌属(Pseudomonas)、寡养单胞菌属(Stenotrophomonas)和伯克霍尔德氏菌属(Burkholderia)4个属,其中芽孢杆菌属(Bacillus)为优势菌属。分离到的52株细菌有44株(占总分离菌株的84.6%)表现出对供试病原菌具有较好的抑制作用,高达94.2%的分离菌株能产IAA,有43株(占总分离菌株的82.7%)表现出淀粉酶活性。【结论】九香虫内细菌种群较为多样,具有潜在应用价值。     

野生及温室盆栽蕙兰可培养根内生细菌的遗传多样性

惠兰(Cymbidium faberi)是中国兰属代表种之一,具有很高的观赏价值和经济价值,对其内生细菌进行研究不仅可以丰富植物内生细菌资源,还可以为探讨兰花与微生物之间的相互作用关系提供基础数据。本研究采用分离培养方法及16S r RNA基因序列测定对天目山野生蕙兰、在温室培养1年后的蕙兰根内生细菌遗传多样性进行了研究。结果表明:从野生蕙兰根内分离得到的97株细菌分属于变形菌门的α-变形菌纲、β-变形菌纲、γ-变形菌纲及厚壁菌门的13个属,其最优势类群为γ-变形菌纲(86.60%),Lelliottia(26.80%)为最优势菌属。从温室盆栽蕙兰根内分离得到的52株细菌分属于变形菌门的α-变形菌纲、β-变形菌纲、γ-变形菌纲及放线菌门的9个属,优势类群为β-变形菌纲(48.08%),优势菌属为草螺菌属(Herbaspirillum)(34.62%),其中菌株eh R17为潜在的新种。这些结果表明天目山野生蕙兰可培养根内生细菌多样性较其在温室培养1年后更为丰富,同时也说明植物内生细菌的群落结构与生长环境密切相关。     

中国典型冻土区土壤可培养细菌多样性

[目的]对比分析中国典型高纬度冻土区和高海拔冻土区土壤可培养细菌的多样性.[方法]采用NM、TSA 、R2A 3种培养基分离培养不同冻土区土壤可培养细菌,用通用引物扩增分离的细菌16S rRNA基因,根据系统发育分析进行鉴定.[结果]从6个样品中得到冻土土壤可培养细菌的菌落数量为4.70×103 -2.57×105 cfu/g(土壤干重),根据不同的菌落形态分离出144株可培养细菌.纯培养物的16S rRNA基因部分序列分析表明:我国高纬度冻土区土壤样品中的细菌分别属于Firmicutes分支(59.52％)、Gammaproteobacteria 分支(38.10％)、Betaproteobacteria分支(2.38％),其中假单胞菌属(Pseudomonas)、芽胞杆菌属(Bacillus)、类芽胞杆菌属(Paenibacillus)的菌株为该区域的三大优势菌群.我国高海拔冻土区土壤样品中分离细菌属于Gammaproteobacteria分支(89.22％)、Firmicutes分支(8.82％)和Bacteroidetes分支(1.96％)o优势菌群为假单胞菌属( Pseudomonas).[结论]我国高纬度冻土区和高海拔冻土区土壤具有较高的可培养细菌多样性;不同类型冻土区土壤可培养细菌群落组成不同.本文研究结果将为我国冻土区土壤细菌资源研究与利用提供理论依据.     

硇洲岛海胆可培养细菌的多样性

摘要：【目的】研究南海硇洲岛马粪海胆（Hemicentrotus pulcherrimus）可培养细菌多样性。【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细菌（含放线菌）多样性进行研究。【结果】用补充0～2.0 mol/L NaCl的MA、ISP 2、NA、SWA和HAA培养基从海胆样品中分离到106株细菌菌株,根据形态观察和部分生理生化实验结果去冗余,选取34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,这些分离菌株代表21个物种,属于3个大的系     

一平浪盐矿古老岩盐沉积中可培养细菌的系统发育多样性研究

运用纯培养法和基于16S rRNA基因序列的系统发育分析对云南省一平浪盐矿古老岩盐沉积中可培养细菌的多样性进行了研究。用补充0.5~3.5mol/L NaCl的MBA和ISP2琼脂培养基从卤水、岩盐和盐土样品中分离到38株细菌,用细菌通用引物进行16S rRNA基因扩增和序列测定,用相关软件进行序列相似性搜索、比对和系统发育分析。结果表明,38个分离菌株可分为31个物种,属于4个大的系统发育类群(Proteobacteria,Bacteroidetes,Firmicutes,Actinobacteria)、17个科、24个属。多数菌株属于Proteobacteria门(18株,47.3%;Gamma-Proteobacteria,31.5%;Alpha-Proteobacteria,15.8%)和Firmicutes门(13株,34.2%)。这些分离菌株中,至少有3个菌株可能代表3个不同属的3个新物种:Y3、Y15和Y25分别代表Idiomarina属、Salinicoccus属和Saccharospirillum属的新物种;而菌株Y21有可能代表Staphylococcaceae科的一个新属。从以上结果可以看出,一平浪盐矿古老岩盐沉积中存在较为丰富的微生物物种多样性和系统发育多样性,并且潜藏着新的微生物资源。     

可产生铁载体的春兰根内生细菌多样性

摘要：【目的】了解可产生铁载体的春兰根内生细菌的多样性,以便筛选到高效的植物促生细菌。【方法】采用CAS检测法测定了189株春兰根内生细菌产生铁载体的能力,并结合16S rRNA基因系统发育分析对可产铁载体的春兰根内生细菌多样性进行了研究。【结果】从189株春兰内生细菌中筛选到47株可产生铁载体的细菌,占菌株总数的24.9%。16S rRNA基因系统发育分析结果表明,47株细菌分属于4个系统发育类群（Alphaproteobacteria,Betaproteobacteria,Firmicutes,Actinobacteria）,17个属的31个种。其中放线菌门为最优势类群（42.6%）,芽孢杆菌属（Bacillus）和贪噬菌属（Variovorax）为优势菌属,且贪噬菌属为高产铁载体的主体菌属。另外有2个菌株可能代表两个不同属的新物种。【结论】春兰根中可产生铁载体的内生细菌具有丰富的多样性。     

中国主要矿区油页岩可培养细菌的分离与鉴定

【目的】研究油页岩本源环境中可培养细菌多样性,对于发掘利用尚未开发的油页岩细菌资源具有重要意义。【方法】以野外采集的吉林桦甸、广东茂名和辽宁抚顺3个中国主要矿区的油页岩作为研究对象,采用稀释平板培养法,以营养琼脂培养基对油页岩中的细菌进行分离纯化,并对分离菌株进行基于16S rRNA基因的序列测定和系统发育分析。【结果】3个矿区共鉴定出10属,其中抚顺矿的9个操作分类单元(Operational taxonomic units,OTUs)属于Pantoea、Brevibacillus、Paenibacillus、Microbacterium、Arthrobacter、Pseudomonas和Bacillus菌属;茂名矿的5个OTUs属于Bacillus和Sinomona菌属,桦甸矿的5个OTUs属于Staphylococcus、Acinetobacter、Bacillus和Arthrobacter菌属。【结论】3个矿区可培养细菌群落组成均较简单,且在门的分类层次上相似,即均具有厚壁菌门和放线菌门,抚顺矿和桦甸矿还存在部分变形菌门细菌。在属的分类层次上,各矿区差异较大。     

浓香型白酒窖泥中可培养细菌的分离鉴定及产酸研究

为系统了解浓香型白酒窖泥中可培养细菌的多样性,采用平板稀释涂布法分离筛选窖泥中可培养菌株。扩增纯培养细菌的16SrRNA基因,测序并与EzBioCloud数据库比对,所有序列已在GenBank中注册。结果共从窖泥中筛选出42株差异性较大的菌株,其中5株与模式菌株相似性低于97％,共包括14个属,以Bacillus、Lysinibacillus、Sporosarcina、Staphylococcus四个属为主;高效液相色谱检测各个菌发酵液结果表明,有机酸包括乙酸、乳酸、酒石酸、苹果酸、柠檬酸、琥珀酸、α-酮戊二酸、草酸;其中尤以乙酸、乳酸的产量较高。     

应用高通量技术分析F446饱水木漆器中微生物群落结构多样性

【背景】饱水保藏木漆器的环境中,微生物数量多、种类丰富,木漆器易受到微生物的腐蚀。【目的】研究木漆器上的微生物群落结构,分析饱水木漆器的微生物病害信息。【方法】采用Illumina MiSeq高通量测序技术对木漆器和保藏水样中的细菌进行群落结构分析。【结果】木质样品与水样品中的微生物群落多样性较丰富并在分布上存在一定差异。门水平上,木质样品共有7个优势菌门(相对丰度1%),分别为Proteobacteria(64.00%)、Acidobacteria(14.70%)和Actinobacteria(3.83%)等;水样共有6个优势菌门,分别为Proteobacteria(61.26%)、Acidobacteria(8.25%)和Planctomycetes(4.88%)等。属水平上木质样品共有8个优势菌属(相对丰度1%),分别为Phenylobacterium(16.24%)、Acidobacteria-Gp6(9.68%)和Rhodoplanes(6.45%)等;水样共有10个优势菌属,分别为Naxibacter(9.03%)、Acidobacteria-Gp6(3.84%)和Nevskia(3.27%)等。未分类菌在门和属上,木质样品分别占8.70%和50.68%;水样品分别占12.83%和59.35%。【结论】木漆器饱水保藏环境中木质样品与水样品的微生物群落结构均比较丰富,在门和属水平上水样品比木质样品复杂。另外,被测样品中可能含有大量潜在新菌。     

可可西里碱性土壤样品细菌的分离和生物学特性

可可西里是位于青海玉树藏族自治州的自然环境保护区,由于当地的恶劣气候特点,其土壤微生物多样性很少被研究.采用5种分离培养基对来源于可可西里的12个盐碱土壤样品进行选择性分离,共分离得到5株细菌.其中4株菌分别属于游动微菌属(Planomicrobium)、库克菌属(Kocuria)、气球菌属(Aerococcus)和芽...     

养殖牡蛎体内检出坎氏弧菌的鉴定

2 0 0 3年 9月从福建近海养殖太平洋牡蛎 (Crassostreagigas)体内分离出 4株细菌 ,对它们形态、生理生化特征、盐度、温度和pH生长条件以及 16SrRNA基因序列进行了研究。结果表明 ,4株细菌均为革兰氏阴性杆菌 ,具极生单鞭毛 ,发酵葡萄糖产酸不产气 ,氧化酶阳性 ,生长需NaCl,无色素 ,不发光 ,在TCBS平板上形成中等大小圆形绿色菌落 ,对弧菌抑制剂O 12 9敏感 ,具有弧菌属的典型特征。结合 16SrRNA基因序列分析结果 ,该菌 (编号SXS1)与坎氏弧菌的亲缘关系最为接近 ,其同源性达 99 .0 % ,因此将该菌鉴定为坎氏弧菌。对该菌在环境中的分布与水产养殖动物疾病的关系进行了讨论。     

松材线虫伴生细菌多样性的宏基组分析

摘要：【目的】松材线虫是松材线虫病的病原,且与其伴生细菌之间存在互作关系,它们构成一个微生态系统。本研究旨在揭示松材线虫-伴生细菌群落细菌多样性。【方法】采用16S rRNA基因文库和454测序对伴生细菌群落的宏基因组进行初步分析。【结果】依据97％序列相似性划分OTU（Operational Taxonomic Unit）,构建的16S rRNA文库包含25个OTU,分别属于Alphaproteobacteria、Betaproteobacteria、Gammaproteobacteria和Bacter     

基于16S rRNA基因序列分析受砷和硫酸盐污染的土壤细菌多样性（英文稿）

为了了解普通耕地土壤(Nor-1)和受砷及硫酸盐污染土壤(Sul-1)中的细菌组成和多样性差异,对2个不同土壤样品直接提取总DNA,通过PCR扩增16S rRNA基因并建立文库,对文库克隆进行核糖体DNA扩增片段酶切分析(ARDRA)和测序,构建系统进化树。从Nor-1土壤样品中测序获得23个16S rRNA基因序列,分析序列系统发育关系表明,共包含Acidobacteria(12.3%,8/65)、Actinobacteria(3.1%,2/65)、Firmicutes(21.5%,14/65)、Nitrospira(3.1%,2/65)和Proteobacteria(60%,39/65)等5个不同细菌门。而从Sul-1土壤样品中测序获得19个16S rRNA基因序列,分析序列系统发育关系表明,共包含Firmicutes(29.5%,13/44)和Proteobacteria(70.5%,31/44)等2个不同细菌门。结果表明,受高浓度的砷和硫酸盐的影响,Sul-1土壤中细菌群落结构相较于普通耕地土壤(Nor-1)发生了明显的改变,多样性明显下降,但有大量具有较强的污染物降解能力的不动杆菌(Acinetobacter)相关序列在Sul-1土壤细菌群落中被发现。     

Identification of culturable bacteria present in haemodialysis water and fluid

Water used to prepare haemodialysis fluid is not sterile, and its microbiological control is important for the prevention of haemodialysis-associated illness. Bacterial populations inhabiting a distribution system for haemodialysis water were studied over an 18-month period. 203 planktonic bacteria isolated on R2A medium were identified by restriction analysis and sequencing of 16S rRNA gene. A diverse bacterial community was detected, containing predominantly Gram-negative members of the Alphaproteobacteria and Betaproteobacteria, as well as representatives of the genus Mycobacterium. Ecological and clinical consequences are discussed: bacteria from the genera Novosphingobium, Pseudomonas and Sphingomonas have been described in the build-up of biofilms, and others like Acinetobacter, Mycobacterium or Brevibacterium may represent a health risk to patients under haemodialysis treatment.     

Genotypic characterization of bacteria cultured from duck faeces

AIMS: To characterize the bacterial composition of mallard duck faeces and determine if novel bacterial species are present that could be utilized as potential indicators of avian faecal contamination. METHODS AND RESULTS: Combined samples of fresh faeces from four ducks were serially diluted and plated onto six different media selected to allow the growth of a range of organisms at 42 degrees C under three atmospheric conditions: aerobic, microaerophilic and anaerobic. Forty-seven morphologically dissimilar isolates were purified and partial sequencing of the16S rRNA indicated at least 31 bacterial species. Twenty of these could be identified to the species level including pathogenic species of Bacillus, Campylobacter, Clostridium and Streptococcus. Other species identified included: Enterococcus, Escherichia, Megamonas, Cellulosimicrobium, Neisseria, Staphylococcus and Veillonella. Potentially novel species, which could represent bacteria specific to avian fauna included Bacillus, Corynebacterium, Macrococcus and Peptostreptococcus, while four isolates had <97% similarity to known bacterial species in the available databases. CONCLUSION: A survey of the natural microflora of the mallard duck and its hybrid with the grey duck identified both bacteria that are potentially human pathogenic and putative novel bacteria species as determined by 16S rRNA sequencing. SIGNIFICANCE AND IMPACT OF THE STUDY: This study provides further evidence that duck faeces is a potential human health hazard, and has identified bacteria potentially useful for distinguishing duck faeces from other faecal sources.     

16SrRNA sequencing of Dye decolorizing bacteria isolated from Soil

Dye׳s residues in textile effluents are hazardous for humans and animals health. Such pollutants can be degraded into non-harmful molecules using biological approaches that are considered cheaper and ecologically safer. Isolated 15 bacterial cultures from soil that could be used in biological system were showed decolorization capacity for Acid Green dye (33.9% to 94.0%) using thin layer chromatography and broth culture method. The most promising cultures (AMC3) to decolorize Acid green Dye (94.6%) was re-coded as NSDSUAM for submitting at IMTECH, Chandigarh for sequencing. The 16SrRNA sequencing suggested that it can be a variant of Pseudomonas geniculata (99.85% identical similarity) with difference of 2 base pairs to reference strain Pseudomonas geniculata ATCC 19374(T). Thus present study proposed dye decolorizing efficiency of the isolated strain of Pseudomonas geniculata that was previously unnoticed. The sequence is deposited in NCBI GenBank with the accession number {"type":"entrez-nucleotide","attrs":{"text":"KP238100","term_id":"745856746","term_text":"KP238100"}}KP238100.     

Characterization of culturable anaerobic bacteria from the forestomach of an eastern grey kangaroo, Macropus giganteus

AIM: To determine the culturable biodiversity of anaerobic bacteria isolated from the forestomach contents of an eastern grey kangaroo, Macropus giganteus, using phenotypic characterization and 16S rDNA sequence analysis. METHODS AND RESULTS: Bacteria from forestomach contents of an eastern grey kangaroo were isolated using anaerobic media containing milled curly Mitchell grass (Astrebla lappacea). DNA was extracted and the 16S rDNA sequenced for phylogenetic analysis. Forty bacterial isolates were obtained and placed in 17 groups based on phenotypic characteristics and restriction enzyme digestion of 16S rDNA PCR products. DNA sequencing revealed that the 17 groups comprised five known species (Clostridium butyricum, Streptococcus bovis, Clostridium sporogenes, Clostridium paraputrificum and Enterococcus avium) and 12 groups apparently representing new species, all within the phylum Firmicutes. CONCLUSIONS: Foregut contents from Australian macropod marsupials contain a microbial ecosystem with a novel bacterial biodiversity comprising a high percentage of previously unrecognized species. SIGNIFICANCE AND IMPACT OF THE STUDY: This study adds to knowledge of Australia's unique biodiversity, which may provide a future bioresource of genetic information and bacterial species of benefit to agriculture.