216 resultados para 5S rRNA


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从采集的土壤样品中分离筛选出一株碱性蛋白酶产生菌G-41,经16S rRNA分子鉴定为芽孢杆菌属菌株。该菌株在发酵培养基中能产生较高产量的胞外碱性蛋白酶(1.7×104U/mL)。以G-41为出发菌株,对其进行重离子辐照诱变处理,获得突变株G-41-68,将该突变株再次经重离子诱变,从大量突变株中筛选出碱性蛋白酶高产菌株15Gy-54,其酶活力达到6.22×104U/mL。与出发菌株相比较,突变株G-41-68和15Gy-54的酶活力分别提高了1.58倍和2.65倍。对突变株15Gy-54的发酵条件进行了优化研究,结果表明,该菌株的碱性蛋白酶活力得到进一步提高,达到7.18×104U/mL,其最适发酵条件为:培养基(g/100mL)为胰蛋白胨1、酵母膏0.5、乳糖5、Na2HPO4·12H2O0.4、KH2PO40.03、Na2CO30.1、MgSO40.0481(4×10-3mol/L)、pH8.0,培养温度41℃,振荡培养时间42-48h。实验结果表明,重离子辐照诱变技术是一种非常有效的微生物诱变育种新技术。

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采用半定量反转录聚合酶链式反应(RT-PCR)技术研究了Cd胁迫对拟南芥(Arabidopsis thaliana)幼苗错配修复和增殖细胞核抗原基因表达的影响,并结合幼苗的形态和生理指标,选取Cd胁迫敏感的生物标记物。结果表明:不同浓度(0.25、0.5、1.0 mg.L-1)Cd处理对拟南芥幼苗叶片数、地上部鲜质量影响不大;Cd浓度为0.25 mg.L-1时,地上部分可溶性蛋白质含量明显升高(P<0.05),Cd浓度为0.5和1.0 mg.L-1时,可溶性蛋白质含量明显降低(P<0.05);叶绿素含量随着Cd浓度的增加而微弱增加(P>0.05)。Cd浓度为0.25 mg.L-1时,以18S rRNA为内参照,PCNA1、PCNA2、MSH2、MSH3、MSH6、MSH7 6个基因均出现了诱导表达,当Cd浓度增加到1.0 mg.L-1时,除了MSH6持续表达诱导及MSH3基因与对照相比表达抑制外,其他基因的表达依然出现诱导,但都低于0.5 mg.L-1Cd处理下的基因表达水平。以上结果表明,基因表达的改变可作为检测Cd污染对植物遗传毒性效应潜在有用的生物标记物。

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从南海红树林木榄(Bruguiera gymnorrhizo)根际土壤中分离到一株具有拮抗杉木致害菌尖孢镰刀菌萎蔫专化型SF2(Fusariumoxysporum f.sp.vasinfectum)活性的海洋细菌3728菌株,对分离菌株的形态特征、培养特征、生理生化特征和16S rRNA基因序列进行了系统的研究。发现细菌3728与枯草芽孢杆菌(Bacillus subtilis)序列相似性最高,达到100%,在系统进化树中与枯草芽孢杆菌(Bacillus subtilis AJ276351)处于同一分支上,结合形态和生理生化分析结果,将其鉴定为枯草芽孢杆菌。

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The most biological diversity on this planet is probably harbored in soils. Understanding the diversity and function of the microbiological component of soil poses great challenges that are being overcome by the application of molecular biological approaches. This review covers one of many approaches being used: separation of polymerase chain reaction (PCR) amplicons using denaturing gradient gel electrophoresis (DGGE). Extraction of nucleic acids directly from soils allows the examination of a community without the limitation posed by cultivation. Polymerase chain reaction provides a means to increase the numbers of a target for its detection on gels. Using the rRNA genes as a target for PCR provides phylogenetic information on populations comprising communities. Fingerprints produced by this method have allowed spatial and temporal comparisons of soil communities within and between locations or among treatments. Numerous samples can be compared because of the rapid high throughput nature of this method. Scientists now have the means to begin addressing complex ecological questions about the spatial, temporal, and nutritional interactions faced by microbes in the soil environment.

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Labyrinthulomycetes (Labyrinthulea) are ubiquitous marine osmoheterotrophic protists that appear to be important in decomposition of both allochthonous and autochthonous organic matter. We used a cultivation-independent method based on the labyrinthulomycete-specific primer LABY-Y to PCR amplify, clone, and sequence 68 nearly full-length 18S rDNA amplicons from 4 sediment and 3 seawater samples collected in estuarine habitats around Long Island, New York, USA. Phylogenetic analyses revealed that all 68 amplicons belonged to the Labyrinthulea. Only 15 of the 68 amplicons belonged to the thraustochytrid phylogenetic group (Thraustochytriidae). None of these 15 were similar to cultivated strains, and 11 formed a novel group. The remaining 53 amplicons belonged either to the labyrinthulid phylogenetic group (Labyrinthulidae) or to other families of Labyrinthulea. that have not yet been described. Of these amplicons, 37 were closely related to previously cultivated Aplanochytrium spp. and Oblongichytrium spp. Members of these 2 genera were also cultivated from 1 of the sediment samples. The 16 other amplicons were not closely related to cultivated strains, and 15 belonged to 5 groups of apparently novel labyrinthulomycetes. Most of the novel groups of amplicons also contained environmental sequences from surveys of protist diversity using universal 18S rDNA primers. Because the primer LABY-Y is biased against several groups of labyrinthulomycetes, particularly among the thraustochytrids, these results may underestimate the undiscovered diversity of labyrinthulomycetes.

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研究了 Ba Li F3中 Gd3+和 Eu2 +的光谱性质及 Gd3+对 Eu2 +的能量传递过程 ,讨论了传递机理 .Gd3+的含量 (物质的量分数 )为 0 .3 %时 ,传递效率最高 ,传递几率 PSA=1 .3 5× 1 0 5s- 1 .当 Gd3+的含量高于 0 .3 %时 ,由于 Gd3+ 和 Eu2 + 竞争吸收 Gd3+ 占优势 ,增加 Gd3+ 含量 ,竞争吸收比相应增加 ,Eu2 + 自身吸收光子数目减少 ,发射强度降低

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通过高温固相法首次合成并报道了兰紫色ZnO Al2O3 SiO2长余辉陶瓷,系统地研究了其发光和缺陷性质。在强度0.6mW·cm-2,主峰254nm的UVP紫外灯下激发15min,然后关闭激发源,样品发射兰紫色长余辉。撤去激发源以后5s,余辉初始强度为230mcd·m-2,色坐标为(0.1292,0.0984)。暗视场中,8h以后余辉仍然肉眼可辨。样品的紫外可见发射和不同时间的余辉发射光谱显示:荧光发射位于390nm,来源于基质的自致发光;而余辉有两个发射峰,主峰位于390nm,肩峰位于520nm。这表明样品中存在两种余辉发射中心。由余辉衰减曲线可以看出,这两种余辉发光都由一个快过程和一个慢过程组成。其中,慢过程决定了材料的长余辉时间。从时间依赖的余辉强度倒数曲线可以看出,余辉强度与时间成反比,这表明余辉发光的机理为电子空穴复合过程。热释光谱显示:样品分别在92和250℃附近出现两个宽的热释峰,说明材料中至少存在两种具有不同陷阱深度的电子或空穴缺陷中心。

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以分子量为550的聚乙二醇单甲醚为侧链,苯乙烯/马来酸酐共聚物为骨架,合成了苯乙烯/马来酸酐共聚物多缩乙二醇酯,用红外光谱、元素分析、DSC、热失重等方法,对合成条件、产物结构和性能进行了研究。结果表明:反应严格按照反应方程进行,精制产物是非晶的梳状聚合物。玻璃化温度为30.68℃,分解温度为120℃。对动态力学性能及其锂盐复合物离子导电性进行研究表明α转变温度和β转变温度分别是28℃和-47.7℃。电导率与温度的依赖关系符合VTF方程。室温电导率最高可达4.2×10-5S/cm。

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用辐射接枝工艺合成了功能高分子膜活性材料,并对其进行了表征,测定了以此为活性材料的离子选择电极性能。结果发现,硫酸根电极在10~(-1)—10~(-3)mol/L Na_2SO_4溶液中响应时间<70s,斜率为52mV/PSO_4~(2-);氯离子电极的线性范围1×10~(-1)—2×10~(-4)mol/L,检测下限为8×10~(-5)mol/L,稳定性好,寿命长,响应时间<5s,内阻<60kΩ,抗毒化能力强。从稀土离子选择电极中发现,以辐射接枝工艺合成的材料比化学法合成的好,前者斜率为53 mV/PGd,后者斜率为46 mV/PGd;预辐照接枝工艺合成的材料比共辐照接枝工艺的好些。

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聚萘是一种新型的高分子,掺杂后具有导电性能,是一种导电聚合物。本文用裂解色谱法(PGC)研究了它的热裂解行为,分离鉴定了主要和特征裂解产物,并在此基础上,对其分子链结构和裂解机理进行了讨论。 实验部分 (一)样品 聚萘(PN):由本实验室直接从萘合成,使用前在100℃下真空热处理48小时加以提纯。 (二)仪器和实验条件 裂解器:美同CDS Py-ro-Probe 190型(丝式);裂解温度300-800℃,裂解时间5s。色谱仪:北分厂-2305E型,氢火焰离子化检

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聚乙快的不稳定性及难以加工影响了其应用.最近,Naarmann通过陈化在硅油中的Ti(OBu)_4~-AlEt_3催化体系及加入不同量的Li-(n-Bu)制得了拉伸后电导率达10~5S/cm的聚乙炔膜,此膜的电导和形态在空气中几个月几乎不发生改变.我们曾报导用加热的甲苯-Ti(OBu)_4~--AlEt_3催化体系合成高性能聚乙炔膜.本文进一步讨论不同溶剂对高性能聚乙炔(HPPA)合成及性能的影响.

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稀土离子4f轨道是否参与成键是一个引入注目的课题,多年来一直存在不同见解。一种认为不参与成键,理由是由于5s,5p壳层的屏蔽,4f轨道位于内壳层,并且到目前为止,分子轨道理论计算结果表明4f轨道不参与成键。另一种认为可以形成较弱的共价键,并发展了一种角重迭模型利角参数来研究共价行为,但是具体共价行为的数量级尚未有明确结论。我们在

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Karyotype and chromosomal location of the major ribosomal RNA genes (rDNA) were studied using fluorescence in situ hybridization (FISH) in five species of Crassostrea: three Asian-Pacific species (C. gigas, C. plicatula, and C. ariakensis) and two Atlantic species (C. virginica and C. rhizophorae). FISH probes were made by PCR amplification of the intergenic transcribed spacer between the 18S and 5.8S rRNA genes, and labeled with digoxigenin-11-dUTP. All five species had a haploid number of 10 chromosomes. The Atlantic species had 1-2 submetacentric chromosomes, while the three Pacific species had none. FISH with metaphase chromosomes detected a single telomeric locus for rDNA in all five species without any variation. In all three Pacific species, rDNA was located on the long arm of Chromosome 10 (10q)-the smallest chromosome. In the two Atlantic species, rDNA was located on the short arm of Chromosome 2 (2p)-the second longest chromosome. A review of other studies reveals the same distribution of NOR sites (putative rDNA loci) in three other species: on 10q in C. sikamea and C. angulata from the Pacific Ocean and on 2p in C. gasar from the western Atlantic. All data support the conclusion that differences in size and shape of the rDNA-bearing chromosome represent a major divide between Asian-Pacific and Atlantic species of Crassostrea. This finding suggests that chromosomal divergence can occur under seemingly conserved karyotypes and may play a role in reproductive isolation and speciation.

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Cultivation of the endophytic fungus Penicillium commune, which was isolated from the semi-mangrove plant Hibiscus tiliaceus, afforded one new compound 1-O-(2,4-dihydroxy-6-methylbenzoyl)-glycerol (1) along with thirteen known products, including 1-O-acetylglycerol (2), N-acetyltryptophan (3), 3-indolylacetic acid methyl ester (4), 1-(2,4-dihydroxy-3,5-dimethylphenyl)ethanone (5), 2-(2,5-dihydroxyphenyl)acetic acid (6), (4R,5S)-5-hydroxyhexan-4-olide (7), thymidine (8), uracil (9), thymine (10), ergosterol (11), beta-sitosterol (12), beta-daucosterol (13), and ergosta-7,22-dien-3 beta,5 alpha,6 beta-triol (14). The structures of these compounds were established by detailed NMR spectroscopic analysis, as well as by comparison with literature data or with authentic samples.