基于WGP物理作图法的虾夷扇贝Fosmid克隆混池策略及解码率研究

利用全基因组解析(Whole genome profiling,WGP)法进行物理图谱构建时,克隆混池策略及克隆解码率的高低是影响物理图谱构建效果的关键性因素。如何通过调控混合克隆数目,来平衡克隆解码率和测序的成本,是利用WGP法构建物理图谱的亟需解决的问题。本研究利用虾夷扇贝Fosmid文库的部分克隆,使用序列特异性标签的WGP方法,对虾夷扇贝物理图谱构建方法的混池策略及克隆解码率进行了初步研究。通过计算机分别模拟了384 N(N=1,2…24)孔培养板内的克隆混合,计算出了对应混合尺度下BsaXI和FspEI两种酶的克隆解码率。以该模拟数据作为参照,最终分别以4、8、12、16张384孔培养板内的克隆混合构建了克隆超级池;并利用2b-RAD技术构建了基于BsaXI和FspEI两种限制性内切酶的测序文库。通过对酶切标签数据的分析,成功实现了混合池内的克隆解码,且在利用两种酶对应的酶切标签联合解码后,联合解码率达到84%以上。本研究最终确定了由8张384孔培养板混合的混池策略及利用BsaXI和FspEI两种酶切标签进行联合克隆解码,为后期利用WGP方法构建虾夷扇贝物理图谱提供了参考方案。     

南沙海区沉积物中细菌和古细菌16S rDNA多样性的研究

采用细菌16SrDNA通用引物和PCR扩增等方法,构建了南海南沙海区沉积物16S rDNA文库,并通过RFLP酶切分型对所获得的70个克隆进行测序。从国际分子生物学数据库中调取相关序列,以PAUP4．0分析软件构建序列同源性矩阵和系统发育树图。结果表明,与细菌文库中克隆相似的微生物属于4个细菌类群：变形细菌(Proteobacteria)(60％)、革兰氏阳性细菌(Gram-positivre bacteria)(13％)、浮霉菌(Planetomycetes)(10％)和无硫绿细菌(Green nonsulfur bacteria)(6％),其中变形细菌(包括δ-、γ-和α-变形细菌)是明显的优势类群。采用Blast程序对所有序列基因数据库进行搜索,发现只有一个克隆与已知序列完全相似,说明文库具有极高的多样性。但是对古细菌文库中所获得的克隆子进行二级结构和序列特征分析的结果表明,这些克隆子均为海洋未获培养的细菌,因此在作者的文库中并未有古细菌的发现。     

天津近海可培养细菌多样性的初步调查

根据天津近海地理地貌特征设置了5个调查站住,分别采集不同水层的水样,进行了可培养细菌调查和多样性分析.调查结果表明,天津近海海水细菌总数为0.28×107～6.08×107cfu/L.划线培养获得的菌株经16S rDNA扩增后,用RsnⅠ、Msp Ⅰ限制性内切酶酶切,共获得27种酶切谱型.对27种谱型的细菌进行16S rDNA克隆和序列分析表明,天津近海海水可培养细菌分属于3个分类单元,即变形细菌(18种)、厚壁菌(5种)、拟杆菌(4种).对天津近海海水可培养细菌的可能代谢类型进行了比较分析,为今后开发利用海洋生物资源和修复天津近海生态环境提供了数据.     

印度尼西亚Padang Cermin热泉古菌多样性分析

通过印度尼西亚苏门答腊岛Padang Cermin热泉环境基因组DNA构建古菌16S rRNA基因文库,并利用PCR-RFLP技术对其古菌多样性和系统发育分析进行了研究.根据限制性内切酶AluⅠ和MspⅠ的特征性酶切图谱,将62个阳性克隆归类为14个分类操作单位(operational taxonomic unit,OTU),文库的覆盖度达90.32％.克隆文库的优势类群为OTU2和OTU1,分别占克隆文库的27.42％和20.96％.从每个OUT中选取一个代表性克隆进行16S rRNA基因的序列测定与系统发育分析,结果表明,测定的Padang Cermin热泉中的古菌均属于泉古菌门,包括热变形菌目(Thermoproteales)、硫还原球菌目(Desulfurococcales)、杂色泉古菌(miscellaneous crenarchaeotic group,MCG)和未培养泉古菌(uncultured Crenarchaeota,UC),该热泉代表性克隆与GenBank数据库已有16S rRNA序列的相似性为91.9％～97.8％,而且与其相似性最高的序列均来自未培养的古菌克隆,由结果可见,Padang Cermin热泉古菌群落与已报道的其他热泉古菌群落的相似性较低,表明该热泉可能具有某些独特的特征,存在着特殊的古菌生态类群.     

厦门近岸水域海洋附着细菌的群落结构及其动态变化

为研究海洋附着细菌的群落结构及动态变化,在厦门近岸海区进行挂板实验.将无菌玻璃板浸没于海水中,连续放置14 d.分别于放置1 h和7、14 d后取玻璃板上附着生物样品.用细菌通用引物构建16S rRNA基因克隆文库,每个克隆文库随机挑选约40个克隆子测序,序列同源性分析和系统进化分析结果表明,所有的克隆子可分为六大类群:γ-变形菌纲(γ-Proteobacteria)、拟杆菌门(Bacteroidetes)、厚壁菌门(Firmicutes)、α-变形菌纲(α-Proteobacteria)、蓝细菌门(Cyanobacteria)和真核硅藻类叶绿体,各类群分别占42.0%、4.5%、2.2%、2.2%、1.1%和45.0%.γ-变形菌纲变形斑沙雷氏菌(Serratia proteamaculans)为优势附着细菌,占测序克隆子的31.5%.这类细菌在1 h样品中的比例超过一半,说明变形斑沙雷氏菌在生物膜形成初期发挥着重要作用.随着挂板时间延长,检测到的细菌类群有所增加:附着7 d后检测到拟杆菌门细菌,附着14 d后检测到厚壁菌门细菌.γ-变形菌纲细菌所占比例随挂板时间的延长而逐渐降低,从挂板1 h的81%降至7 d的21%,14 d的18%.另外,在各阶段的附着样品中,都检测到较多的真核克隆子序列,约占16%～64%.本研究为进一步阐明海洋附着细菌的附着动态及其在生物膜形成过程中的作用奠定了基础.     

三疣梭子蟹(Portunus trituberculatus)微卫星位点的分离和序列分析

采用磁珠富集法,利用生物素标记的(GT)15寡核苷酸探针从三疣梭子蟹基因组DNA的Sau3A1酶切的500-1000bp片段中筛选微卫星序列.洗脱的杂交片段克隆到PMD18-T载体上构建富集微卫星基因组文库后,通过PCR筛选检测出阳性克隆进行测序.在56条测序序列中有49条非冗余序列包含有重复次数不少于5次的微卫星位点,阳性序列比例达到87.5%.其中perfect类型微卫星最大的重复次数为47次.在47条非冗余序列中,共有40条(85.1%)微卫星重复序列两端有侧翼序列能够进行引物设计.本研究中筛选的微卫星位点将为下一步的三疣梭子蟹种群遗传结构分析、经济性状的QTL定位提供遗传标记.     

细角螺微卫星DNA 富集文库构建及特征分析

采用生物素磁珠富集法,用生物素标记的(GT)15和(CT)15两种探针与细角螺基因组 MseI 酶切的300~1200bp 片段杂交,杂交复合物与链霉亲和素磁珠结合,捕获含有重复序列的微卫星片段。最后将磁珠捕获到的重复序列与PMD19-T载体连接后克隆到DH5α中构建微卫星基因组文库。通过PCR检测出354个阳性克隆,从中随机选取248个片段大于500bp的阳性克隆进行测序,结果显示,在220个成功测序的阳性克隆中共获得278个微卫星序列,其中完美型171个,占61.5%;非完美型81个,占29.1%;复合型26个,占9.4%。除探针使用的GT和CT的重复序列外,还筛选到三碱基GTT、TGG、GAA、CAA;四碱基TCTA、ACAG、TAGA、GTGA、GTCT、GATA及五碱基TTTTG的重复序列。在278条序列中共有82条可以设计引物。     

使用反应器培养钝顶螺旋藻(Spirulina plarensis)过程中细菌群落的组成变化

使用气升式光生物反应器培养钝顶螺旋藻25天,发现随螺旋藻生物量的增长,细菌生物量有一定的增长趋势.应用PCR-DGGE技术分析螺旋藻培养过程中细菌种类组成,发现在不同时期细菌群落组成变化明显.通过DGGE图谱中18条特征条带的克隆、测序及系统进化分析,发现其中有8条序列与а变形菌纲序列相似,3条与拟杆菌纲序列相似,2条...     

宁波北仑港冬季浮游细菌多样性研究

采用分子生物学方法对宁波北仑港冬季水体中的浮游细菌多样性进行了研究.提取水样中细菌基因组总DNA,以细菌16S rDNA通用引物进行PCR扩增,扩增产物经分子克隆、测序与序列分析,对水样中的细菌建立了16S rDNA克隆文库和系统发生树.结果表明,浮游细菌群落具有较高的多样性,34个克隆子分属2个不同的细菌类群,6个克隆子属于未知类群,优势细菌类群为Pro-teobacteria类群（变形菌类群）,占80%;细菌优势类群顺序为β-Proteobacteria类群（32.5%）、γ-Proteobacteria类群（25%）、α-Proteobacteria类群（15%）、ε-proteobacteria类群（7.5%）、Firmicutes类群（厚壁菌类群）（5%）.这一结果与近年来国内外有关港口微生物多样性的报道较为一致.用DNAStar中Clustalw程序从测序的40个克隆子中选出17个OTU进行系统发育分析,同样表明浮游细菌多样性较强.     

泥蚶(Tegillarca granosa)GT微卫星位点的筛选和性质鉴定

采用磁珠富集法,利用生物素标记的(GT)15寡核苷酸探针从泥蚶基因组DNASau3A1酶切的500—1000bp片段中筛选GT/CA微卫星位点。洗脱的杂交片段克隆到PMD18-T载体上构建富集微卫星基因组文库后,通过PCR筛选检测出阳性克隆进行测序。在139条序列中有115条序列包含有重复次数不少于5次的微卫星位点,阳性序列比例达到82.7%。其中perfect类型微卫星最大的重复次数为35次。在112条非冗余序列中,共有100条(88.5%)微卫星重复序列两端有侧翼序列能够进行引物设计。     

Bacterial diversity in the sediments collected from the Shikoku Basin

Diversity of bacteria was studied in deep-sea sediments from the Shikoku Basin in the Northwest Pacific Ocean by PCR, RFLP and sequence analysis of 16S rDNA and comparing with Genbank database. Based on the RFLP profile generated, 77 clones from the 16S rDNA library were divided into 27 types. Phylogenetic analysis showed that the 27 independent clones fell into four groups: Proteobacteria (62.96%), Chloroflexi (14.81%), Planctomycetes (14.81%) and Acidobacteria (7.41%). Among all sequenced clones, 6 were related to the sulfur or sulfate metabolism bacteria and the results also demonstrated that some bacteria in deep-sea sediments had relation to matter-energy circulation.     

Microbial diversity in polluted harbor sediments I: Bacterial community assessment based on four clone libraries of 16S rDNA

Bacteria, as the most abundant sediment organism, play a major role in the fate of pollutants. Therefore, many pollutant-related bacteria have been studied in harbor sediments, yet the entire bacterial profiles have not been reported. The bacterial diversity and community structures from sediments in Victoria Harbor (Hong Kong), including two polluted (VH and VHW) and two adjacent (open oceanic, TLC; estuary discharge affected, PC) sites, were characterized by analyses of four 16S rDNA clone libraries. Upon comparisons of RFLP patterns from 254 clones in the libraries, 178 unique phylotypes were retrieved. LIBSHUFF and Rarefaction analyses indicated that the sediment bacterial communities at the four sites showed high 16S rDNA richness and were significantly different from each other. Phylogenetic analysis of full-length 16S rDNA revealed 19 bacterial phyla in Victoria Harbor sediments. γ- and δ-proteobacteria, holophaga/acidobacteria, and planctomycetales were recorded in all the libraries. In addition, γ- and δ-proteobacteria were dominant at all sites (33.33–11.67%). Besides these two phyla, ε-proteobacteria, firmicutes, aminobacterium, holophaga/acidobacteria and bacteroidetes were judged to be major components of a given library since they constituted 10% or more of the total OTUs of the given library. The cyanobacteria, verrucomicrobia, β-proteobacteria, aminobacterium, chlorofiexi, and candidate division OP1, OP8 were detected in minor proportions in various libraries. A portion of the clones were only distantly related to sequences in the GenBank, suggesting bacteria in Victoria Harbor sediments were unique and diversified.     

Phylogenetic analysis of bacterial community in deep-sea sediment from the western Pacific “warm pool”

A depth profile of bacterial community structure in one deep-sea sediment core of the western Pacific ＂warm pool＂ （WP） was investigated and compared with that in a sediment sample from the eastern Pacific （EP） by phylogenetic analysis of 16S rDNA fragments. Five bacterial 16S rDNA clone libraries were constructed, and 133 clones with different restriction fragment length polymorphism （RFLP） patterns were sequenced. A phylogenetic analysis of these sequences revealed that the bacterial diversity in a sample from the WP was more abundant than that in the EP sample. The bacterial population in the sediment core of WP was composed of eight major lineages of the domain bacteria. Among them the γ-Proteobacteria was the predominant and most diverse group in each section of WP sediment core, followed by the α-Proteobacteria. The genus Colwellia belonging to γ-Proteobacteria was predominant in this sample. The shift of bacterial communities among different sections of the WP sediment core was δ-, ε-Proteobacteria, and Cytopahga-Flexibacteria-Bacteroides （CFB） group. The ratios between them in the bacterial communities all showed inversely proportional to the depth of sediment. The sequences related to sulphate reducing bacteria （SRB） were detected in every section. The bacterial community structure in this sediment core might be related to the environmental characteristics of the surface seawater of the western Pacific WP.     

印度洋深海沉积物样品纯培养细菌的分离鉴定

为探索印度洋深海沉积物中纯培养细菌的多样性,本文对采自印度洋12个沉积物样品进行细菌纯培养分离,共获得343株细菌.所有细菌采用16S?rRNA基因进行比对分析,鉴定为4个门:厚壁菌门(Firmicutes)、变形菌门(Proteobacteria)、放线菌门(Actinobacteria)和拟杆菌门(Bacteroi...     

高压技术在深海沉积物兼性嗜压菌的筛选和鉴定中的应用

通过自行改进的高压培养罐及高压设备,对深海沉积物进行可培养微生物的筛选,获得6株具有较强耐受压力的细菌.16SrDNA的测序结果表明这些细菌分别属于6个不同的菌属.压力生长试验的结果表明这6株细菌在40MPa的条件下仍然具有较强的生长能力,属于兼性嗜压菌.对不同压力下生长的细菌做显微镜检,结果显示,除了一株芽孢杆菌在40MPa下的菌体形态发生了明显的变化外,其它5株细菌在压力条件下的菌体的分裂均没有受到明显的影响.     

Isolation and phylogenetic assignation of actinomycetes in the marine sediments from the Arctic Ocean

Actinomycetes in five marine sediments collected from the Arctic Ocean at depths of 43 to 3 050 m were cultivated using a variety of media. A total of 61 actinomycete colonies with substrate mycelia only were observed, and no colonies with aerial mycelia were observed under aerobic conditions at 15 ℃. From these colonies, 28 were selected to represent different morphological types.Denaturing gradient gel electrophoresis (DGGE) was used to check the purity of isolates and select representatives for subsequent sequencing. Phylogentic analyses based on nearly full-length 16S ribosomal RNA gene (rDNA) sequences indicated that the actinomycetes isolated were accommodated within genus Rhodococcus of family Nocardiaceae, genus Dietzia of family Dietziaceae,genera Janibacter and Terrabacter of family Instrasporangiaceae and genera Kocuria and Arthrobacter of family Micrococcaceae. One of the strains (P27-24) from the deep-sea sediment at depth of 3 050 m was found to be identical in 16S rDNA sequence(1474/1474)with the radiation-resistant Kocuria rosea ATCC 187T isolated from air. More than halfofthe isolates showed the similarities ranging from 99.5% to 99.9% in 16S rDNA sequence to dibenzofran-degrading, butyl 2-ethylhexanoate-hydrolysising and nitrile-metabolizing actinomycetes. All the strains isolated were psychrotolerant bacteria and grew better on the media prepared with natural seawater than on the media prepared with deionized water. Three of them (Dietzia sp. P27-10, Rhodococcus sp. S11-3 and Rhodococcus sp.P11-5)had an obligate growth requirement for salt, confirming that these strains are indigenous marine actinomycetes.     

东太平洋海隆深海热液区沉积物古菌多样性分析

采用PCR-RFLP方法对东太平洋海隆深海热液区3个站位沉积物中的古菌多样性进行了初步研究.结果显示,从古菌16S rRNA基因文库中随机挑取的296个阳性克隆分属奇古菌门（Thaumarchaeota,47.64%）、广古菌门（Euryarchaeota,44.93%）、泉古菌门（Crenarchaeota,6.77%）和未分类古菌（0.68%）,其中优势菌群为奇古菌门的亚硝化侏儒菌属（Nitrosopumilus,35.47%）和广古菌门的热原体纲（Thermoplasmata,27.03%）,DHVE3、DHVE5、DHVE6、MBGB和MBGE类群在沉积物样品中也均有发现.另外,3个站位沉积物中古菌类群组成存在差异,S5-TVG1站位样品文库的97个古菌克隆分属奇古菌门（49.48%）、广古菌门（49.48%）和泉古菌门（1.03%）,S14-TVG10站位样品文库的103个古菌克隆由奇古菌门（84.47%）和广古菌门（15.53%）组成,S16-TVG12站位样品文库的96个古菌克隆包括广古菌门（71.88%）、泉古菌门（19.79%）、奇古菌门（6.25%）和未分类古菌（2.08%）.研究结果表明,东太平洋海隆深海热液区沉积物中古菌多样性丰富,存在着许多新的古菌菌群;不同站位古菌菌群结构以及多样性存在差异,这与其所处环境的热液活动密切相关.     

黄河三角洲泥质沉积区表层沉积物古菌分布特征

通过古菌16S rDNA 基因文库技术, 在黄河三角洲泥质沉积区6 个站位共获得568 个克隆, 经处理得到73 个OUTs(Operational Taxonomic Units), 在此基础上进行系统进化树以及统计学分析。结果显示, 在本次研究的6 个站位的表层沉积物中, 古菌序列均来自于泉古菌(Crenarchaeota)和广古菌(Euryarchaeota): 其中以Marine Crenarchaeotic Group I(MGI)为主, 仅含少量的Miscellaneous Crenarchaeotic Group (MCG), Marine Benthic Group B(MBGB)等其他种属。研究结果表明, 6 个不同站位的沉积物中只有5 个古菌类群, 群落分布较为均匀, 多样性不高。研究结果揭示了黄河三角洲表层沉积物中古菌横向分布特征, 并为今后在黄海区域开展古菌生态学研究提供了数据信息, 特别是在当前古菌研究主要集中在深海区域的背景下, 对相应的近海区域古菌研究具有一定的参考意义。     

Molecular phylogenetic analysis of sulfate-reducing bacteria from deep sediment layers of the tropical West Pacific warm pool

1IntroductionThe tropical West Pacific warm pool(TWP-WP),which spans an area roughly between10°Nto10°S of the equator from Indonesia to the dateline,has the world’s warmest sea surface temperature ofbeing greater than29℃.With the increase of recog-niz…     

山口红树林根际土壤可培养细菌多样性及其活性筛选

为探讨广西山口红树林土壤可培养细菌的多样性,采用纯培养分离技术对采集的25个红树林样品进行可培养细菌多样性分析,挑选117株菌株进行16S rRNA基因测序并构建系统发育树分析。结果表明117株菌株分别属于9个纲20个目27个科35个属,9个纲包括α-变形菌纲（21.37%）、β-变形菌纲（1.71%）、γ-变形菌纲（12.82%）、δ-变形菌纲（0.85%）、噬纤维菌纲（0.85%）、鞘脂杆菌纲（0.85%）、黄杆菌纲（2.56%）、放线菌纲（27.35%）、芽孢杆菌纲（31.62%）。优势属为芽孢杆菌属,占所有菌株的28.20%,此外α-变形菌纲、γ-变形菌纲、黄杆菌纲和放线菌纲中发现了7株潜在的新物种。分离菌株的产酶活性检测表明,山口红树林根际土壤蕴含丰富的产淀粉酶、蛋白酶、葡聚糖、纤维素酶和几丁质酶等生物活性酶的菌株,其中芽孢杆菌纲的产酶菌株数最为丰富。初步研究结果表明广西山口红树林土壤可培养细菌资源丰富,新物种资源多样,是农业微生物开发应用的重要资源库。