941 resultados para 12S rRNA
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冷泉是指温度接近于海水,而以高于周围水环境浓度的烃类化合物(主要为甲烷)、硫化物或二氧化碳为主要成分,受地质构造或压力梯度作用渗出沉积物表层的流体。对冷泉沉积物中微生物群落的调查,有助于认识该极端环境中某些生理未知微生物类群的功能并理解微生物活动对整个系统的影响。 本文对从鄂霍次克海冷泉区采集获得的沉积物样品按深度划分得到的11个断层中的6个断层进行了总基因组的提取,利用16S rDNA作为分子标记,构建克隆文库并结合总有机碳、总氮、硫等环境因子对该样品中的细菌和古菌群落结构沿沉积物断层的分布情况进行研究,结果显示该沉积物中的细菌和古菌均具有高度多样性且显示出明显的成层分布: 1.细菌群落主要来自10个细菌门,优势门类为绿弯菌、未定门JS1、γ-、δ-变形菌,同时还发现浮霉菌、未定门OP8、放线菌、酸杆菌、拟杆菌、疣微菌的存在。我们还在分布于表层沉积物δ-变形菌类群中发现了占该层群落15%以上的SRB(硫酸盐还原菌)类群,这强烈提示着该沉积物环境中存在着AOM(甲烷厌氧氧化)过程。 2.古菌类群主要划分为DSAG、MBG-D、MCG、MGI、MBG-A和MHVG等类群。其中MBG-D类群沿断层的垂直分布与沉积物中硫含量表现出相似的变化趋势,这提示MBG-D类群可能参与该环境中硫相关的地质化学过程。
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本研究以双壳纲、翼形亚纲、珍珠贝目、扇贝超科的栉孔扇贝(Chlamys farreri )、海湾扇贝(Argopecten irradians)和牡蛎超科巨蛎属(Crassostrea)的长牡蛎(C. gigas)、葡萄牙牡蛎(C. angulata)、熊本牡蛎(C. sikamea)、香港巨牡蛎(C. hongkongensis)和近江牡蛎(C. ariakensis)5种牡蛎及异齿亚纲、帘蛤目、帘蛤科的紫斑文蛤(Meretrix pethechialis)为研究对象,系统的研究了以上物种的线粒体基因组全序列的特点。并以线粒体12个蛋白质编码基因的序列,在氨基酸和核苷酸水平上构建了软体动物的分子系统发生树。本研究旨在为利用线粒体基因组全序列全面构建软体动物分子系统发生树,为软体动物的系统发生和进化研究提供一种新的思路和前期基础工作,本研究主要内容分为以下三个部分: 一、栉孔扇贝和海湾扇贝线粒体基因组序列分析及分子系统发生研究 采用Long-PCR技术扩增了栉孔扇贝和海湾扇贝线粒体全基因组,利用步移法结合文库构建的测序策略获得了线粒体基因组的序列。海湾扇贝线粒体全基因组长度为16,211 bp,栉孔扇贝接近全序列长度为20,789 bp。两个基因组都编码35个基因,包括12个蛋白质编码基因,2个rRNA和21个tRNA。与典型的动物线粒体基因组相比,两个基因组都缺少一个蛋白质编码基因atp8和2个trnS, 在海湾扇贝基因组中有1个trnF的重复,而在栉孔扇贝基因组中有1个trnM的重复。基因排列比较显示,尽管海湾扇贝、栉孔扇贝和巨扇贝分类学上属于同一扇贝科,但是它们的线粒体基因排列非常不同。在四种扇贝中,虾夷扇贝与栉孔扇贝的基因排列顺序非常相似;即使排除tRNA的比较,栉孔扇贝和海湾扇贝基因组仅仅共享三个小的基因块;而海湾扇贝与巨扇贝仅有一个相同的基因块。在所有的系统发生分析中,四种扇贝稳定的系统发生关系得到强有力的支持,海湾扇贝较其他三种扇贝较早的分化出来;栉孔扇贝比其他两种扇贝与虾夷扇贝亲缘关系更近。贝叶斯法和最大似然法分析都支持扇贝超科的单系发生。 二、巨蛎属牡蛎线粒体基因组全序列分析及分子系统发生研究 采用Long-PCR扩增技术和步移法结合文库构建的技术策略获得了巨蛎属C. gigas、C. angulata、C. sikamea、C. hongkongensis和C. ariakensis 5种牡蛎线粒体全基因组序列,并于GenBank已公布的美洲牡蛎C.virginica序列进行比较研究。C. gigas、C. angulata、C. sikamea、C. hongkongensis和C. ariakensis线粒体全基因组长度分别为18,225 bp、18,225 bp、18,243 bp、18,622 bp和18,414 bp,都长于C. virginica基因组17,244 bp的长度。本研究的5种牡蛎线粒体基因组都编码39个基因,包括12个蛋白质编码基因,2个rRNA和25个tRNA。与典型的线粒体基因组相比,都缺少一个蛋白质编码基因atp8,有trnM、trnK和trnQ 3个tRNA基因的重复,更特别的是基因组中的rrnL分为两段,这在其它线粒体基因组中未见报道,有一个重复的rrnS;而C. virginica基因组编码37个基因,与其他牡蛎相比,没有trnK和trnQ重复,只有一个rrnS。基因排列比较显示,巨蛎属的5种牡蛎C. gigas、C. angulata、C. sikamea、C. hongkongensis和C. ariakensis基因排列完全一致,而与C. virginica的基因排列相比仍然有较大的差别,有多个tRNA发生易位。系统发生分析显示,C. gigas和C. angulata首先聚在一起,然后与C. sikamea聚为一支。C. hongkongensis和C. ariakensis聚成一支。C. virginica为单独的一支。系统树清楚的显示出C. gigas和C. angulata以及C. hongkongensis和C. ariakensis非常近的亲缘关系,这也是长期以来,牡蛎分类学上的经典问题,有学者认为C. gigas和C. angulata为同一物种,线粒体基因组的数据显示C. gigas和C. angulata可能达到不同物种的差异。传统分类上的“近江牡蛎”的“白蚝”和“赤蚝”,线粒体序列差别明显,完全支持两种牡蛎新种名的制定。 三、紫斑文蛤线粒体基因组全序列分析及分子系统发生研究 采用Long-PCR扩增技术和步移法结合文库构建的技术策略获得了紫斑文蛤线粒体基因组全序列。该基因组全长19,567 bp,编码36个基因,包括12个蛋白质编码基因,2个rRNA和22个tRNA。与典型的线粒体基因组相比,缺少一个蛋白质编码基因atp8和1个trnS, 有1个trnQ基因的重复。基因排列比较显示,双壳类的基因排列在低的分类阶元时相对保守。在帘蛤科中,紫斑文蛤M. petechialis和菲律宾蛤仔V. philippinarum共享四个完全一致的基因块,两个大的基因块是cox1-L1-nad1-nad2-nad4L-I 和 cox2-P-cob-rrnL-nad4-H-E-S2-atp6-nad3-nad5,另两个小基因块只包括tRNA基因。在以氨基酸序列构建的分子系统树中,帘蛤科紫斑文蛤与菲律宾蛤仔首先聚在一起,然后,它们与A. tuberculata形成一个进化枝。这一枝与H. arctica结合起来,支持异齿亚纲单系发生。
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深海生物圈有着不同于陆地和浅海的典型特点,例如高压、低温、永久黑暗及寡营养,并且深海微生物具有特殊的代谢途径及庞大的生物量,这使得深海成为一个巨大的有待开发利用的生物资源宝库。 本文研究的样品分别取自东太平洋E272站位(12°36’39"N, 104°19’28"W)和西太平洋Ph05-5站位(16°04’93"N, 124º34’48"E)。E272站位距离东太平洋13°N海隆45km,水深3 191m;而Ph05-5站位地处西菲律宾海盆,在黑潮源区附近,位于西太平洋暖池区边缘,水深3 382m,并且Ph05-5岩芯一共包含了五个明显的火山灰层。 本文采用了末端限制性片段长度多态性分析(T-RFLP)和16S rRNA 基因文库分析的方法在小尺度上对东太平洋E272站位的沉积物样品进行细菌群落结构的研究。研究结果表明沉积物细菌群落结构在小尺度上存在明显的垂直变化。系统进化分析表明,该沉积物样品的细菌多样性较高,共包含9个主要的门类,包括变形菌门、绿弯菌门(绿色非硫细菌)、浮霉菌门、酸杆菌门、放线菌门(高G+C革兰氏阳性菌)、拟杆菌门、硝化螺旋菌门、以及两个待定的门类OP8和TM6。其中变形菌门细菌是一类在海洋中非常常见的细菌,广泛分布于各个海洋环境,在我们的文库当中发现了变形菌门的三个纲,包括α-、-、-变形菌纲。本项研究充分表明该沉积物环境中具有较高的细菌多样性,在小尺度上细菌群落垂直分布明显,其结果也可从侧面反映深海沉积物近表层处的环境条件在小尺度上的垂直变化显著。 对西太平洋暖池区沉积物样品的细菌群落的研究也采用16S rRNA 基因文库分析的方法。系统进化分析表明该沉积物样品细菌的多样性相对较低,一共包含了六个不同的门类,包括变形菌门、浮霉菌门、放线菌门、厚壁菌门(低G+C革兰氏阳性菌)、绿弯菌门、酸杆菌门。在这个沉积物样品中也发现了变形菌门的三个纲包括α-、-和-变形菌纲。聚类分析和系统进化分析都表明表层的细菌群落同其它8层的细菌群落存在明显的差异,并且其它8层包括5个火山灰层和3个远洋粘土层的细菌群落结构差异不大,推测火山灰成分不仅对火山灰层的细菌群落产生影响,而且可能通过扩散对整个沉积物的微生物群落结构都产生影响。表层可能由于沉积时间较晚所以受影响相对较小或表层本身不同于较深层次的理化条件而使表层群落存在较大差异。 对东、西太平洋不同环境下的两个深海沉积物样品的细菌多样性进行比较,结合其它研究发现变形菌门细菌在不同深海环境中都普遍存在,是深海不同环境的广适类群。另外,两个环境中的细菌多样性存在很大差异,东太平洋沉积环境中的细菌多样性要远高于西太平洋沉积环境中的细菌多样性,推测其最可能的原因是西太平洋沉积物火山灰成分对细菌群落的影响,致使其细菌群落与东太平洋远洋粘土沉积物细菌群落产生很大差异;另外,不同洋区的环境差异也应该是造成细菌群落差异的一个重要方面。
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Two biological aerated filters (BAF) were setup for ammonia removal treatment of the circulation water in a marine aquaculture. One of the BAFs was bioaugmented with a heterotrophic nitrifying bacterium, Lutimonas sp. H10, where the ammonia removal was not improved and the massive inoculation was even followed by a nitrification breakdown from day 9 to 18. The nitrification was remained stable in control BAF operated under the same conditions. Fluorescent in situ hybridization (FISH) with rRNA-targeted probes and cultivable method revealed that Lutimonas sp. H10 almost disappeared from the bioaugomented BAF within 3 d, and this was mainly due to the infection of a specific phage as revealed by flask experiment, plaque assay and transmission electron observation. Analyses of 16S rRNA gene libraries showed that bacterial groups from two reactors evolved differently and an overgrowth of protozoa was observed in the bioaugmented BAR Therefore, phage infection and poor biofilm forming ability of the inoculated strain are the main reasons for bioaugmentation failure. In addition, gazing by protozoa of the bacteria might be the reason for the nitrification breakdown in bioaugmented BAF during day 9-18.
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We conducted this study to assess the diversity of bacteria associated with the surfaces of algae based on 16S rDNA sequence analyses. Twelve strains of bacteria were obtained from the surfaces of the following four species of algae: Gracilaria textorii, Ulva pertusa, Laminaria japonica, and Polysiphonia urceolata. The isolated strains of bacteria can be divided into two groups: Halomonas and Vibrio, in physiology, biochemical characteristics and 16S rDNA sequence analyses. The phylogenetic tree constructed based on 16S rDNA sequences of the isolates shows four obvious clusters, Halomonas venusta, Vibrio tasmaniensis, Vibrio lentus, and Vibrio splendidus. Isolates from the surface of P. urceolata are more abundant and diverse, of which strains P9 and P28 have a 16S rDNA sequence very similar (97.5%-99.8%) to that of V. splendidus. On the contrary, the isolates from the surfaces of G textorii, U. pertusa and L. japonica are quite simple and distribute on different branches of the phylogenetic tree. In overall, the results of this study indicate that the genetic relationships among the isolates are quite close and display a certain level of host species specificity, and alga-associated bacteria species are algal species specific.
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Twenty-nine marine bacterial strains were isolated from the sponge Hymeniacidon perleve at Nanji island, and antimicrobial screening showed that eight strains inhibited the growth of terrestrial microorganisms. The strain NJ6-3-1 with wide antimicrobial spectrum was identified as Pseudoalteromonas piscicida based on its 16S rRNA sequence analysis. The major antimicrobial metabolite, isolated through bioassay-guide fractionation of TLC bioautography overlay assay, was identified as norharman (a beta-carboline alkaloid) by EI-MS and NMR.
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The marine Roseobacter clade comprises one of the largest fractions of heterotrophic marine bacteria and accounts for about 16% of 16S rRNA gene clones retrieved from marine bacterioplankton. Their global distribution seems to be related to oceanic water masses and their environmental and biogeochemical properties. In this study, we report isolation and characterization of novel Roseobacter clade members from the Yellow Sea, China. Phylogenetic analysis of 16S rRNA gene sequences reveals that the new isolates (YSCB1, YSCB2, YSCB3 and YSCB4) are closely related to uncultured Arctic seawater bacterium R7967 (99.57-100% sequence identity) and to the cultured Roseobacter sp. DSS-1 (99.27-99.76% sequence identity) isolated from the southeastern coastal water of the USA. Interestingly, YSCB strains possess unique intracellular chromium-containing aggregates. Therefore, these novel Roseobacter clade members exhibit a peculiar property in mineral biogeneration. (c) 2006 Elsevier SAS. All rights reserved.
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Magnetotactic bacteria (MTB) are ubiquitous in aquatic habitats. Because of their fastidious requirements for growth conditions, only very few axenic MTB cultures have been obtained worldwide. In this study, we report a novel marine magnetotactic spirillum axenic culture, designated as QH-2, isolated from the China Sea. It was able to grow in semi-solid or liquid chemically defined medium. The cells were amphitrichously flagellated and contained one single magnetosome chain with an average number of 16 magnetosomes per cell. Phosphate and lipid granules were also observed in the cells. Both rock magnetism and energy-dispersive X-ray spectroscopy characterizations indicated that the magnetosomes in QH-2 were single-domain magnetites (Fe3O4). QH-2 cells swam mostly in a straight line at a velocity of 20-50 mu m/s and occasionally changed to a helical motion. Unlike other magnetotactic spirilla. QH-2 cells responded to light illumination. As a consequence of illumination, the cells changed the direction in which they swam from parallel to the magnetic field to antiparallel. This response appears to be similar to the effect of an increase in [O-2]. Analysis of the QH-2 16S rRNA sequence showed that it had greater than 11% sequence divergence from freshwater magnetotactic spirilla. Thus, the marine QH-2 strain seems to be both phylogenetically and magnetotactically distinct from the freshwater Magnetospirillum spp. studied previously. (C) 2010 Elsevier Masson SAS. All rights reserved.
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A new ciliate, Trimyema koreanum n. sp., isolated from hypersaline water (salinity of 293 parts per thousand) from a solar saltern in Korea, was investigated using live observation, protargol impregnation, and gene sequencing. Trimyema koreanum is about 30 x 13 mu m in vivo, has usually 23 longitudinal ciliary rows forming two distinct ciliary girdles visible both in vivo and in protargol impregnation. A third indistinct ciliary girdle as well as a girdle of mucocysts is distinguishable only in impregnated cells. We suggest T. koreanum as a new species, differing from the most similar species, T. marinum, by the presence of two distinct ciliary girdles (T. marinum usually has six ciliary girdles clearly visible in living cells and three anterior spirals that encircle the cell completely). Although the number of known 18S rRNA sequences in the genus Trimyema was limited, the Trimyema group including T. koreanum forms a strong clade. The phylogenetic position confirms that the isolate belongs to the genus Trimyema and is different from previously sequenced species. Trimyema koreanum is able to consume both prokaryotes and small eukaryotes (specifically, the alga Dunaliella sp.).
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Duplications and rearrangements of coding genes are major themes in the evolution of mitochondrial genomes, bearing important consequences in the function of mitochondria and the fitness of organisms. Yu et al. (BMC Genomics 2008, 9: 477) reported the complete mt genome sequence of the oyster Crassostrea hongkongensis (16,475 bp) and found that a DNA segment containing four tRNA genes (trnK(1), trnC, trnQ(1) and trnN), a duplicated (rrnS) and a split rRNA gene (rrnL5') was absent compared with that of two other Crassostrea species. It was suggested that the absence was a novel case of "tandem duplication-random loss" with evolutionary significance. We independently sequenced the complete mt genome of three C. hongkongensis individuals, all of which were 18,622 bp and contained the segment that was missing in Yu et al.'s sequence. Further, we designed primers, verified sequences and demonstrated that the sequence loss in Yu et al.'s study was an artifact caused by placing primers in a duplicated region. The duplication and split of ribosomal RNA genes are unique for Crassostrea oysters and not lost in C. hongkongensis. Our study highlights the need for caution when amplifying and sequencing through duplicated regions of the genome.
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Chromosomal location of the 5S ribosomal RNA gene was studied in the eastern oyster, Crassostrea virginica Gmelin. using fluorescence in situ hybridization (FISH). Metaphase chromosomes were obtained from early embryos, and the FISH probe was made by PCR (polymerase chain reaction) amplification of the 5S rRNA gene and labeled by incorporation of digoxigenin-1 1-dUTP during PCR. Hybridization was detected with fluorescein-labeled antidigoxigenin antibodies. Two pairs of FISH signals were observed on metaphase chromosomes. Karyotypic analysis showed that the 5S rRNA gene cluster is interstitially located on short arms of chromosomes 5 and 6. On chromosome 5, the 5S rRNA genes were located immediately next to the centromere, whereas on chromosome 6, they were located approximately half way between the telomere and the centromere. Chromosomes of C. virginica are difficult to identify because of their similarities in size and arm ratio, and the chromosomal location of 5S rRNA genes provides unambiguous identification of chromosomes 5 and 6. Previous studies have mapped the major rRNA gene cluster (18S-5.8S-28S) to chromosome 2. and this study shows that the 5S rRNA gene cluster is not linked to the major rRNA genes and duplicated during evolution.
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The jinjiang oyster Crassostrea rivularis [Gould, 1861. Descriptions of Shells collected in the North Pacific Exploring Expedition under Captains Ringgold and Rodgers. Proc. Boston Soc. Nat. Hist. 8 (April) 33-40] is one of the most important and best-known oysters in China. Based on the color of its flesh, two forms of C rivularis are recognized and referred to as the "white meat" and 11 red meat" oysters. The classification of white and red forms of this species has been a subject of confusion and debate in China. To clarify the taxonomic status of the two forms of C. rivularis, we collected and analyzed oysters from five locations along China's coast using both morphological characters and DNA sequences from mitochondrial 16S rRNA and cytochrome oxidase 1, and the nuclear 28S rRNA genes. Oysters were classified as white or red forms according to their morphological characteristics and then subjected to DNA sequencing. Both morphological and DNA sequence data suggest that the red and white oysters are two separate species. Phylogenetic analysis of DNA sequences obtained in this study and existing sequences of reference species show that the red oyster is the same species as C. ariakensis Wakiya [1929. Japanese food oysters. Jpn. J. Zool. 2, 359-367.], albeit the red oysters from north and south China are genetically distinctive. The white oyster is the same species as a newly described species from Hong Kong, C. hongkongensis Lam and Morton [2003. Mitochondrial DNA and identification of a new species of Crassostrea (Bivalvia: Ostreidae) cultured for centuries in the Pearl River Delta, Hong Kong, China. Aqua. 228, 1-13]. Although the name C. rivularis has seniority over C. ariakensis and C. hongkongensis, the original description of Ostrea rivularis by Gould [1861] does not fit shell characteristics of either the red or the white oysters. We propose that the name of C. rivularis Gould [1861] should be suspended, the red oyster should take the name C. ariakensis, and the white oyster should take the name C. hongkongensis. (C) 2004 Elsevier B.V. All rights reserved.
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Oysters are commonly found on rocky shores along China's northern coast, although there is considerable confusion as to what species they are. To determine the taxonomic status of these oysters, we collected specimens from nine locations north of the Yangtze River and conducted genetic identification using DNA sequences. Fragments from three genes, mitochondrial 165 rRNA, mitochondria! cytochrome oxidase I (COI), and nuclear 285 rRNA, were sequenced in six oysters from each of the nine sites. Phylogenetic analysis of all three gene fragments clearly demonstrated that the small oysters commonly found on intertidal rocks in north China are Crassostrea gigas (Thunberg, 1793), not C. plicatula (the zhe oyster) as widely assumed. Their small size and irregular shell characteristics are reflections of the stressful intertidal environment they live in and not reliable characters for classification. Our study confirms that the oysters from Weifang, referred to as Jinjiang oysters or C. rivularis (Gould, 1861), are C. ariakensis (Wakiya, 1929). We found no evidence for the existence of C. talienwhanensis (Crosse, 1862) and other Crassostrea species in north China. Our study highlights the need for reclassifying oysters of China with molecular data.
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Chromosomal location of the major ribosomal RNA genes (rRNA) were studied in the dwarf surfclam (Mulinia lateralis, Say) using fluorescence in situ hybridization (FISH). FISH probes for the rRNA genes were made by polymerase chain reaction (PCR), labeled with digoxigenin-11-dUTP and detected with fluorescein-labeled antidigoxigenin antibodies. Mulinia lateralis had a diploid number of 38 chromosomes and all chromosomes were telocentric. FISH with the rRNA probe produced positive and consistent signals on two pairs of chromosomes: Chromosome 15 with a relative length of 4.6% and Chromosome 19, the shortest chromosome. Both loci were telomeric. The rRNA location provides the first physical landmark of the M. lateralis genome.
Resumo:
Genetic markers are needed for rapid and reliable identification of oysters. In this study, we developed multiplex genus- and species-specific PCR markers for the identification of oysters from China. We used the mitochondrial cytochrome oxidase I (COI) and nuclear 28S ribosomal RNA genes for marker development. DNA sequences from different species were obtained from GenBank or by direct sequencing. Sequences were aligned, and genus- and species-specific nucleotides were identified. Primers were designed for genus/species-specific amplification to generate fragments of different sizes. A multiplex set of genus- and species-specific primers from the 28S gene was able to separate C. ariakensis and C. hongkongensis from other species and assign oysters to four genera. A set of species-specific COI primers provided positive identification of all five Crassostrea species from China, C. ariakensis, C. hongkongensis, C. angulata, C. gigas, and C. sikamea in a single PCR. The multiplex PCR assays do not require fluorescence-labeling or post-PCR enzyme digestion, providing a simple, fast and reliable method for the identification of oysters from China.
