四膜虫S1株——上海四膜虫,新种

四膜虫S1是一株自接型四膜虫,根据形态特征应属梨形四膜虫复合种。本种除克隆内接合外,和其它十二种四膜虫均不接合。本种的异柠檬酸脱氢酶,四唑氧化酶,谷氨酸脱氢酶和乙酸酯酶的同功酶谱和其它十二种四膜虫相比,差异明显。此外,金亦石等(1987)所提供的S1和其它十种四膜虫的rDNA分子的四种限制性内切酶图谱也说明,S1株与除T.australis以外的其它九种的酶切图谱是显著不同的。据此,作者认为本种应是梨形四膜虫复合种中一新种,并定名为上海四膜虫。     

川中丘陵地区大豆根瘤菌遗传多样性与系统发育关系

【目的】研究分离自川中丘陵地区大豆根瘤菌的遗传多样性和系统发育。【方法】采用16S rDNA PCR-RFLP和16S rRNA基因、glnII、共生基因(nodC)系统发育分析的方法进行研究。【结果】供试未知菌的16S rDNA用4种限制性内切酶(HaeⅢ、HinfⅠ、MspⅠ及TaqⅠ)酶切后获得5种16S遗传图谱类型。16S rDNA PCR-RFLP结果表明,所有供试菌株在83%水平分为慢生根瘤菌属(Bradyrhizobium)和中华根瘤菌属(Sinonrhizobium)两大类群,而75%的菌株为中华根瘤菌。6个代表菌株的16S rDNA、glnII和nodC三个位点基因的系统发育结果基本一致,4株与S.fredii USDA205T相似度最高;有2株分别与B.yuanmingense CCBAU10071T、B.diazoefficiens USDA110T相似度最高。4个Sinonrhizobium代表菌株16S rDNA、glnII序列相似度分别为98.3%-99.9%、98.2%-100%,但它们的nodC基因序列完全相同。【结论】川中丘陵地区大豆根瘤菌具有较丰富的遗传多样性,S.fredii为优势种。     

安徽某淡水龙虾养殖群体分类的分子标记筛选

为筛选可用于淡水龙虾养殖群体物种分类的分子标记,对安徽省某水产养殖有限公司采集的淡水龙虾样本进行了线粒体COⅠ、16S rDNA、D-loop、Cyt b及12S rDNA基因的测序分析,并与GenBank中30个滑螯虾属(Cherax)物种的相应基因序列比对,同时,进行上述5种分子标记在种内个体间、属内种间、科内属间和目内科间的同源性变异范围比对分析。结果显示,本研究所采集淡水龙虾样本与四脊滑螯虾(C. quadricarinatus)的相似性最高,其中,1 113 bp的Cyt b相似性100%,COⅠ、16S r DNA及12S rDNA相似性都在99%以上;在以克氏原螯虾(Procambarus clarkii)为外类群构建的邻接系统发育树中,本研究样本与四脊滑螯虾聚为一支,然后与其他物种聚合构成系统树,确定本研究采集的淡水龙虾样本为四脊滑螯虾;通过同源性变异范围比对分析,在淡水龙虾养殖群体的分子分类工作中,16S rDNA、Cyt b及12S rDNA比COⅠ和D-loop这2种分子标记具有较强优势。本研究结果可为今后淡水龙虾养殖场中物种的分类鉴定工作提供参考。     

东寨港红树林土壤芽胞杆菌分离及其多样性分析

采用热处理法从海南省东寨港红树林海漆林区土壤中分离到276株芽胞杆菌,利用PCR-RFLP与序列分析技术对其16S rDNA遗传多样性进行了研究。16S rDNA PCR-RFLP酶切图谱的聚类分析表明,在100%的相似性水平上,分离的276株芽胞杆菌分属于15个遗传类群,表明存在较为丰富的遗传多样性。15种遗传类型的26株代表芽胞杆菌的16S rDNA序列分析可知,这些芽胞杆菌主要分布于Bacillus(69.2%)、Halobacillus(3.8%)、Virgibacillus(7.7%)、Gracilibacillus(3.8%)、Oceanobacillus(7.7%)和Lysinibacillus(7.7%)6个属,其中Bacillus为优势属。有3株芽胞杆菌的16S rDNA序列与数据库中相应模式菌株的最大相似性在98.O%~98.9%之间,可能为潜在的新分类单元。     

黑水虻幼虫肠道和体表产酶细菌的分离和鉴定

从野外收集和室内饲养的黑水虻Hermetia illucens L.幼虫体表和肠道分离出同时具蛋白质和有机磷分解能力的细菌10株,其中编号为T2、T4、T6、T7和T8的菌株分离自体表,编号为S14、S15、S16、S19和S20的菌株分离自肠道。克隆细菌的16S rDNA和DNA促旋酶B亚基编码基因gyrB对10株细菌进行了鉴定。通过16S rDNA序列确定10株菌为芽孢杆菌属,根据gyrB基因以及BLAST结果构建系统发育树,将10株细菌鉴定为枯草芽孢杆菌。然后将10株菌的gyrB基因以B.subtilis subsp.subtilisstr.168和模式菌株B.subtilis subsp.subtilis BCRC10255相应基因序列为参照构建系统发育树,分析10株菌在种的水平上的亲缘关系,发现10株菌存在亲缘关系差异,没有重复菌株。     

波兰小麦和矮兰麦45S rDNA和5S rDNA基因位点FISH分析

采用双色荧光原位杂交技术, 以45S rDNA和5S rDNA基因为探针, 对波兰小麦(Triticum polonicum L.)和矮兰麦(T. turgidum L. cv. Ailanmai)进行了分析。结果表明, 高秆波兰小麦(T. polonicum L. High)和矮兰麦的45S rDNA和5S rDNA基因位点高度一致, 都显示4个45S rDNA和6个5S rDNA基因位点; 矮秆波兰小麦(T. polonicum L. Dwarf)的45S rDNA基因位点与高秆波兰小麦和矮兰麦也一致表现出4个位点, 而其5S rDNA基因位点有8个。同时讨论了rDNA基因位点的数目和分布位置在种间和种内存在差异的原因。     

人乙型肝炎病毒(HBV)adr亚型基因组的多态性

由乙型肝炎adr亚型病毒(HBVadr)携带者26人的混合血清,得到了HBVadr基因组克隆株(PADR)158株,对这些克隆株进行四种限制性内切酶(BglⅡ,HindⅢ,PstⅠ,XhoⅠ)切点测定,并对其中S株的13种限制性内切酶图谱进行比较研究,发现同为adr亚型病毒,其基因组的限制性酶切图谱存在差异。另外,通过HindⅢ)切点得到的12个克隆株(PADR-H),也进行了酶切图谱分析。在这170个克隆株中,已经发现了5种类型的HBVadr基因组限制性酶切图谱,其中有6种酶(AvaⅠ,EglⅠ,BglⅡ,HincⅡ,HindⅢ,HpaⅠ)的7个变异点。本文报道了HBVadr基因组的多态性现象。     

泥河湾大长梁遗址和马圈沟Ⅰ文化层放线菌的分离及系统发育分析

为分析泥河湾盆地大长梁遗址和马圈沟Ⅰ文化层中可培养放线菌的物种多样性,本实验通过平板稀释涂布法对该区域土样进行放线菌的物种分离,得到197株放线菌纯培养物。采用链霉菌属特异引物对放线菌纯培养物进行初步鉴定,确定143株放线菌归属于链霉菌属。对未被鉴定的54株放线菌进行16S rDNA全序列测定并分析其系统发育关系。最终,将197株放线菌归属于放线菌纲下的5个亚目,6个科,10个属。其中,马圈沟Ⅰ文化层的分离菌株12-9与Nocardioides albus KCTC 9186T之间的16S rDNA序列相似性是93.73%,可能是一个潜在新属;大长梁遗址的分离菌株18-64与Haloglycomyces albus YIM 92370T的16S rDNA序列相似性是93.64%,可能是一个潜在新属。     

蓖麻蚕核糖体RNA基因在大肠杆菌中的无性繁殖

用pBR322作运载体,构建了含有蓖麻蚕核糖体RNA基因(rDNA)完整重复单位的重组质粒-pAR3。pAR3含有11.1Kb rDNA完整重复单位,包含有pAR1和pAR2所携带的rDNA片段。制作了pAR3和rDNA的限制性内切酶图谱。发现限制酶图谱与郑仲承等报道的一致,而与家蚕的rDNA的图谱不同。     

26S rDNA单链构象多态性分析在临床酵母菌菌种鉴定中的应用

摘要： 【目的】探讨酵母菌临床分离株26S rDNA D1/D2区序列种内相似性和种间差异性的快速检测方法,为临床酵母菌菌种鉴定方法的改进奠定基础。调查北京地区临床酵母菌的种群多样性,为国内酵母菌感染的流行病学研究提供新的基础数据。【方法】用5种常见临床酵母菌种的模式和权威菌株作为标准参考菌株,从北京四家综合性医院收集临床酵母菌260余株,PCR扩增其26S rDNA D1/D2区,对扩增产物进行单链构象多态性（Single-Strand Conformation Polymorphism,SSCP）分析和序列测定分析。【结果】常见病原酵母菌26S rDNA D1/D2区的SSCP图谱具有明显的种间差异性和种内相似性,可以通过该方法对菌株进行初步的菌种鉴定。D1/D2-SSCP和序列分析相结合,对260余株临床酵母菌进行了菌种鉴定,共鉴定有10个属20个种,优势属为念珠菌属(Candida),优势种及其所占比例分别是：C. albicans (57.7%), C. parapsilosis (10.0%), C. tropicalis (9.2%), C. glabrata (6.7%)和C. krusei (5.8%),并发现过去从未或很少报道致病的酵母菌种,愈来愈多地出现在临床分离菌株中。【结论】 26S rDNA D1/D2区的SSCP图谱分析为临床酵母菌株的快速鉴定提供了新的方法;北京地区酵母菌临床分离株呈种群多样性分布,C. albicans虽然仍占优势,但其它念珠菌种的比例已达42%。     

Zygosaccharomyces kombuchaensis,a new ascosporogenous yeast from 'Kombucha tea'

A new ascosporogenous yeast, Zygosaccharomyces kombuchaensis sp. n. (type strain NRRL YB-4811, CBS 8849), is described; it was isolated from Kombucha tea, a popular fermented tea-based beverage. The four known strains of the new species have identical nucleotide sequences in domain D1/D2 of 26S rDNA. Phylogenetic analysis of D1/D2 and 18S rDNA sequences places Z. kombuchaensis near Zygosaccharomyces lentus. The two species are indistinguishable on standard physiological tests used for yeast identification, but can be recognized from differences in restriction fragment length polymorphism patterns obtained by digestion of 18S-ITS1 amplicons with the restriction enzymes DdeI and MboI.     

3 micron DNA - an extrachromosomal ribosomal DNA in the yeast Saccharomyces cerevisiae

A new class of extrachromosomal DNA which consists predominantly of covalently closed molecules with lengths around 3 micron, has been detected in Saccharomyces cerevisiae strain 6-1G-P188 from the Peterhof collection. Restriction analysis of the 3 micron DNA as well as of recombinant plasmids carrying HindIII fragments of the 3 micron DNA permitted construction of a physical map of the new extrachromosomal DNA species, and detection of two types differing by one EcoRI restriction site. Molecular hybridization, as well as comparison of the restriction maps, revealed the complete structural identity of the 3 micron DNA with a chromosomal repetitive unit of rDNA containing the genes for 25 S, 18 S, 5.8 S and 5 S rRNAs.     

Divergence of primate ribosomal RNA genes as assayed by restriction enzyme analysis

Primate ribosomal RNA (rRNA) genes have been compared by restriction endonuclease mapping. In all species examined, the restriction map of the reiterated ribosomal DNA is simple (within the limits of detection by hybridization with rRNA) and is consistent with a high degree of homogeneity among the repeats. Within a species, all members have similar rDNA restriction patterns. However, different species of primates have distinctly different rDNA restriction maps; even chimpanzee and man can be discerned by their rDNA restriction patterns. Possible mechanisms for maintenance of homogeneity of the rDNA repeats within a species, while allowing divergence among closely related species, are discussed.     

A reinvestigation of 5′→3′ polarity in 40S ribosomal RNA precursor of xenopus laevis

The 5′→3′ polarity of the 40S precursor rRNA molecule relative to the location of the 18S and 28S RNA regions in the precursor has been reinvestigated. Fragments of rDNA derived by the restriction endonuclease EcoRI and cloned in E. coli were partially digested with the exonuclease induced by bacteriophage λ and with exonuclease III from E. coli. The resulting rDNA fragments with single-stranded tails were hybridized separately with 18S and 28S rRNA, and the formation of the hybrid was monitored by determination of radioactivity and by electron microscopy. Since the location of the EcoRI sites in rDNA is known, and the specificity of the two exonucleases for 5′ and 3′ ends of DNA strands has been established, the hybridization of the different partially digested rDNA fragments with either 18S or 28S rRNA could be interpreted in terms of polarity of the coding strand of rDNA, and consequently of the RNA (see models in Figure 1). The results support the following model for the rRNA precursor molecule: 5′ end-transcribed spacer-18S gene-transcribed spacer-28S gene-3′ end.     

Identification of thermophilic and marine bacilli from shallow thermal vents by restriction analysis of their amplified 16S rDNA

AIMS: In order to identify 73 thermophilic isolates from shallow, marine thermal vents of Eolian Islands, we compared their restriction patterns of amplified 16S rDNA with those of nine well described Bacillus species and eight Eolian Bacillus strains. METHODS AND RESULTS: This study allowed to assign 57 (78%) isolates to different Bacillus species. Nineteen field strains were recognised as representatives of four described species, namely B. thermodenitrificans, "B. caldolyticus", B. vulcani and B. stearothermophilus. The profiles of 38 isolates matched instead, those of seven Eolian strains (B. thermodenitrificans strain A2, B. licheniformis strain B3-15, and five novel species, represented by Bacillus strain 1bw, Bacillus strain 4-1, Bacillus strain 5-2, Bacillus strain 10-1, Bacillus strain 1as). Among the 16 unidentified isolates, seven restriction patterns were recognised. CONCLUSIONS: This study showed that restriction analysis of amplified 16S rDNA is useful for a rapid and reliable identification of strains belonging to described species as well as for recognition of new species. SIGNIFICANCE AND IMPACT OF THE STUDY: This work revealed a high taxonomic diversity among the thermophilic bacilli isolated from Eolian Islands and a distinct distribution of the species within the Eolian hydrothermal vent system.     

VARIATION IN RIBOSOMAL DNA AMONG BIOLOGICAL SPECIES OF ARMILLARIA,A GENUS OF ROOT-INFECTING FUNGI

Armillaria is a genus of root-infecting fungi composed of several biological species in North America and Europe. To examine relatedness among biological species, ribosomal DNA (rDNA) from one isolate was cloned and rDNAs from 30 isolates were mapped for eight restriction enzymes. The positions of the large (26S) and small (18S) rRNA cistrons were found by Northern hybridizations of total cellular RNA with rDNA subclones and by alignment of maps with conserved restriction sites present in rRNA genes of other fungi. Nine restriction-site and two length polymorphisms were observed. Eight North American (Roman numerals) and five European (species epithets) biological species could be placed in six classes with respect to rDNA maps (rDNA class 1: I and A. ostoyae; class 2: II; class 3: A. borealis; class 4: V, IX, and X; class 5: III, VII, A. lutea, and A. cepistipes; and class 6: VI and A. mellea). Most, but not all, polymorphisms were in intergenic regions.     

The organization of the ribosomal RNA genes in the fungus Mucor racemosus.

The rDNA of Mucor racemosus is contained on a 6.4 megadalton repeat unit. Two Bam H-1 restriction fragments that encompass the entire rDNA repeat, as well as two Hind III restriction fragments that lie within the region, have been cloned and analyzed. The rDNA unit has been defined with respect to eight restriction endonucleases and the position of the sequences encoding the 25S, 18S, and 5.8S rRNA species have been localized. In addition, the 55 RNA encoding sequence was found to reside within the basic repeat unit. The results indicate the organization of the rDNA of Mucor more closely resembles the arrangement observed in yeast than that observed in other eukaryotic organisms.     

RESTRICTION ENDONUCLEASE ANALYSIS OF RIBOSOMAL DNA SEQUENCE VARIATION IN LAMINARIA (PHAEOPHYTA)1

The taxonomy and evolutionary relationships of species in the genus Laminaria are poorly understood. Previous studies have demonstrated significant plasticity of morphological characters used to describe taxa, and interfertility has been reported among putative species. We analyzed nuclear ribosomal DNA (rDNA) sequence variation in eight species of Laminaria (L. agardhii Kjell., L. digitata (Huds.) Lamour., L. groenlandica Rosenv. [sensu Druehl 1968], L. longicruris De la Pyl., L. longipes Bory, L. saccharina (L.) Lamour., L. setchellii Silva, and L. yezoensis Miyabe) to elucidate evolutionary relationships in this genus. Restriction maps were constructed using a small subunit rDNA probe from Costaria costata (Turn.) Saunders, an rDNA repeat from the nematode Caenorhabditis elegans, and 11 hexameric restriction endonucleases in an annealing analysis of genomic DNA. Laminaria rDNA restriction maps were compared to each other and to that of the outgroup taxon, C. costata. rDNA restriction maps of Laminaria species and C. costata were similar. Restriction fragment length polymorphisms mapped to both the coding regions and the nontranscribed spacer of rDNA. Laminaria species were distinguished with this method. The restriction maps of L. agardhii, L. saccharina, and L. longicruris were identical, supporting a previous hypothesis that these species are conspecific. Comparison of restriction maps of Laminaria species suggested that the generic subdivision of Sections Simplices and Digitatae may be invalid.