云南山茶(Camellia reticulata) nrDNA ITS序列多态性分析

对云南山茶 (Camellia reticulata) 8个品种的核核糖体DNA内转录间隔区(nrDNA ITS)进行克隆测序,将获得的ITS序列进行GC含量、 5.8S区二级结构的稳定性、替代模式、核苷酸多样性及系统发育关系的相关分析.实验结果显示,云南山茶8个品种的ITS序列存在丰富的基因组内多态性,同时包含中性进化的假基因,表明其ITS序列逃离了一致性进化.云南山茶ITS序列多态性的原因可能来自广泛的种间杂交,以及rDNA位点在基因组中有不确定的物理位置.ITS假基因为品种的物种形成研究提供了更全面的遗传证据,同时也提示了利用ITS假基因进行系统发育分析可能会对其真实的系统关系造成影响.     

山茶属植物ITS的扩增及其序列特征分析

以山茶属(Camellia)植物为实验材料,通过在PCR反应液中加入二甲基亚砜(DMSO)来改进ITS区的扩增效果,并对获得的序列进行了相关的比较分析以及系统发育分析。分析结果表明:(1)PCR反应液中添加4%的DMSO能明显提高ITS的扩增效率,并能有效防止ITS假基因的扩增;(2)与功能拷贝相比,ITS假基因序列的ITS1和ITS2区存在多处碱基缺失,GC含量明显偏低,5.8S区二级结构稳定性降低;(3)应用ITS假基因进行种水平的系统发育分析会对其真实的系统关系造成影响,提示进行系统进化研究时应警惕假基因的干扰。     

四照花亚属的nrDNA ITS致同进化不完全

四照花亚属(Cornus subg.Syncarpea)隶属于山茱萸科山茱萸属(Cornus),我国该亚属共有5种8亚种。为探讨四照花亚属nrDNA ITS序列的致同进化不完全现象及假基因产生的可能原因,分析了该亚属4种(每种1~2个居群)共21个个体的nrDNA ITS序列。结果表明,这些类群的nrDNA ITS存在多态性,通过分析这些nrDNA ITS克隆序列的G+C含量、5.8S保守基序和二级结构最小自由能,推测其可能存在假基因。系统发育研究结果显示所有nrDNA ITS序列分成5个分支,同一个体的不同拷贝被分别置于两个甚至多个分支中,且不同分支显示了不同种间关系。四照花亚属物种个体内部存在nrDNA ITS不完全致同进化,可能归咎于不完全的世系分选(incomplete lineage sorting)、种间杂交或多倍化等进化事件,从而导致基因组内nrITS区序列出现多态性,同时也导致难以通过外部形态来划分亚属内种间界限。     

长毛红山茶和长尾红山茶的核型分析

<正> 长毛红山茶(Camelliav uillosa Chang et S.Y.Liang)和长尾红山茶(C.longicaudata Chang et S.Y.Liang)均为张宏达教授定的新种,分别隶属于山茶属(Camellia)红山茶组(Sect.Camellia)的滇山茶亚组(Subsect.Reficulala)和光果红山茶亚组(Subsect.Lucidissima),前者分布在我国的湖南、广西和贵州,后者分布在广东和广西。 红山茶组共有33个种、1个亚种,7个变种。根据文献资料统计,该组作过染色体计数的有10个种,1个亚种和6个变种,作过核型分析的有4个种、1个亚种和2个变种。本文对该组的长毛红山茶和长尾红山茶的核型作首次报道,并与该组的10个种,1个亚种和6个变种的染色体数目或核型作了比较。     

樟属植物ITS序列多态性分析

对樟科樟属(Cinnamomum Schaeffer) 17个代表样本的核糖体DNA内转录间隔区(nrDNA ITS)进行克隆测序。对获得的87条不同ITS序列的长度变异、GC含量、5.8S区二级结构的稳定性、遗传距离、进化模式以及系统发育关系进行了相关分析。研究结果显示, ITS序列在樟属植物内存在明显的多态性, 87条序列中的22条序列被鉴定为假基因序列, 其余65条序列为功能基因序列; 假基因序列采用中性进化模式, 变异明显大于功能序列。ITS序列在樟属植物中出现一致性进化不完全和假基因现象也可能发生在樟科其它类群中, 这可能是导致樟科植物ITS序列直接测序方式成功率低的重要原因。     

猫科动物DNA条形码及线粒体假基因对物种鉴定的影响

在多种动物类群中,基于线粒体细胞色素c氧化酶亚基Ⅰ(COⅠ)基因的DNA条形码是一种高效的物种鉴别手段,然而猫科Felidae动物中广泛存在的线粒体假基因可能影响DNA条形码的有效性。本研究共涉及猫科动物12属25种119个样本。采用3对条形码通用引物对6属11种29个猫科动物样本进行了扩增及测序。结果3个样本扩增失败,8个样本得到假基因,18个样本获得了条形码序列。结合另外93条猫科动物条形码序列(源自BOLD Systems),采用Kimura 2-parameter模型计算遗传距离,构建Neighbor-Joining(NJ)树。结果显示,遗传距离种内为0%~8.1%,平均0.8%;种间为1.4%~13.1%,平均8.7%;属间为8.2%~21.8%,平均15.1%。NJ树显示,除3个种外,其余物种均以极高的置信度(99%)形成单系分支。而假基因序列有些可以单独形成分支,有些夹杂在COⅠ序列形成的分支中,对物种鉴定产生干扰。     

四个DNA 片段在山茶属分子系统学研究中的应用

选取山茶属14 个组中的10 组21 种植物对目前常用于属内种间的4 个DNA 片段( ITS、waxy 、trnLF
、rpL16) 进行序列测定。结果表明: ( 1) 来自叶绿体基因组的2 个片段( trnL- F、rpL 16) 其PCR 扩增和
测序都很容易, 但两者的进化速率都非常慢, 序列矩阵只有很少信息位点( trnL-F 含9 个, rpL16 为20
个) , 不能提供必要的系统发育信息。( 2) 来自核基因组的ITS 片段其PCR 产物比较容易获得, 但其序列
的测定存在较多问题。( 3) waxy 是来自核基因组的另一个片段, 其PCR 扩增因受模板DNA 的数量和质量
的影响很大而有一定难度, 但其进化速率较快, 序列矩阵具有较多信息位点( 92 个) , 并且在山茶属是单
拷贝, 这对于解决山茶属这类具有许多近缘物种的类群的系统关系有重要价值。基于tsnL- F、rpL16 和
waxy 三组数据所建分子系统树支持山茶属为一单系, 但属下系统由于取样等原因有待进一步研究。     

假基因的组成、分布及其分子进化

假基因(pseudogene)是指基因组中与正常基因序列相似, 但是缺乏功能的DNA 序列。通过序列同源性搜索, 可以收集基因组中假基因的群体特性、染色体分布和同源家族等特性。假基因很好地保留了数百万年前基因组中祖先基因的分子记录, 被视为“基因化石”, 因此假基因在进化和比较基因组学中是重要的资源。应用假基因和基因比较体系, 可以探究生物基因的进化史和基因组稳定性。如: 用Ka/Ks比值确定假基因的自然选择压、物种亲缘关系和进化距离, 分析假基因自身的进化趋势, 探讨DNA 突变的成因等。     

ITS 假基因对栎属系统学研究的影响及其对分子系统学研究的启示*

核糖体rDNA ITS 是被子植物系统发育研究中应用最广泛的分子标记之一。以前人们认为同一物种
中的ITS 序列因致同进化而使不同拷贝高度一致, 在分子系统学研究中常以ITS1- 518S- ITS2 序列作为构建
系统进化树的基础。近年来, 在对一些被子植物的研究中发现这段序列在同一物种中具有多态性, 有些拷
贝中的518S 区不具编码功能, 人们把含有不具编码功能518S 区的ITS1-51 8S- ITS2 序列定义为ITS 假基因序
列, 它对同源基因致同进化的假设形成了新的挑战。在诸多应用ITS 序列重建系统进化关系的研究中, 栎
属系统学研究因ITS 假基因的发现而倍受关注。本文以栎属为例回顾了ITS 假基因的发现过程, 分析了其
对该属系统学研究的影响, 为分子生物学在植物系统进化研究中的应用提供一些新的参考。     

ITS假基因对栎属系统学研究的影响及其对分子系统学研究的启示

核糖体rDNA ITS是被子植物系统发育研究中应用最广泛的分子标记之一。以前人们认为同一物种中的ITS序列因致同进化而使不同拷贝高度一致,在分子系统学研究中常以ITS1-5.8S-ITS2序列作为构建系统进化树的基础。近年来,在对一些被子植物的研究中发现这段序列在同一物种中具有多态性,有些拷贝中的5．8S区不具编码功能,人们把含有不具编码功能5．8S区的ITS1-5．8S-ITS2序列定义为ITS假基因序列,它对同源基因致同进化的假设形成了新的挑战。在诸多应用ITS序列重建系统进化关系的研究中,栎属系统学研究因ITS假基因的发现而倍受关注。本文以栎属为例回顾了ITS假基因的发现过程,分析了其对该属系统学研究的影响,为分子生物学在植物系统进化研究中的应用提供一些新的参考。     

A yeast clade near Candida kruisii uncovered: nine novel Candida species associated with basidioma-feeding beetles

Yeasts similar to Candida kruisii were isolated repeatedly from the digestive tracts of basidioma-feeding beetles, especially nitidulids inhabiting and feeding on a variety of agarics in the southeastern USA and Barro Colorado Island, Panama. Based on the identical sequences of the D1/D2 domains of the LSU rRNA gene (rDNA) and host beetle information, the isolates were grouped into 19 genotypes which varied from C. kruisii by up to 38 nucleotide differences in the D1/D2 region. Phylogenetic analysis of rDNA sequences and phenotypic traits placed the isolates in C. kruisii and in nine undescribed taxa. The new species and type strains are designated as Candida pallodes (NRRL Y-27653^T), C. tritomae (NRRL Y-27650^T), C. panamensis (NRRL Y-27657^T), C. lycoperdinae (NRRL Y-27658^T), C. atbi (NRRL Y-27651^T), C. barrocoloradensis (NRRL Y-27934^T), C. aglyptinia (NRRL Y-27935^T), C. stri (NRRL Y-48063^T), and C. gatunensis (NRRL Y-48064^T). A phylogeny based on analysis of a combined database of sequences of SSU and LSU rDNA and the ITS region showed that the nine new species formed a novel sister clade to C. kruisii that was strongly supported by bootstrap analysis. Candida pallodes, C. tritomae, C. panamensis, and C. lycoperdinae formed one subclade, while C. atbi, C. barrocoloradensis, C. aglyptinia, C. stri, and C. gatunensis formed a second distinct subclade within the larger clade. Candida pallodes and C. atbi showed a strong host specificity to beetle species in the genus Pallodes (Coleoptera: Nitidulidae) collected from a variety of agarics. On the other hand, C. panamensis, C. tritomae, and C. lycoperdinae were associated with several unrelated beetles in Erotylidae, Scarabaeidae, Tenebrionidae, and Curculionidae as well as Lycoperdina ferruginea (Nitidulidae). Candida pallodes, C. tritomae, C. lycoperdinae, and C. atbi have been isolated repeatedly in the USA, while the other five new species have been found only at Barro Colorado Island, Panama.     

Molecular identification and phylogenetic analysis of nuclear rDNA sequences among three opisthorchid liver fluke species (Opisthorchiidae: Trematoda)

In this study, we describe the development of a fast and accurate molecular identification system for human-associated liver fluke species (Opisthorchis viverrini, Opisthorchis felineus, and Clonorchis sinensis) using the PCR-RFLP analysis of the 18S-ITS1-5.8S nuclear ribosomal DNA region. Based on sequence variation in the target rDNA region, we selected three species-specific restriction enzymes within the ITS1 regions, generating different restriction profiles among the species: MunI for O. viverrini, NheI for O. felineus, and XhoI for C. sinensis, respectively. Each restriction enzyme generated different-sized fragments specific to the species examined, but no intraspecific polymorphism or cross-reaction between the species was detected in their restriction pattern. These results indicate that PCR-linked restriction analysis of the ITS1 region allows for the rapid and reliable molecular identification among these opisthorchid taxa. In addition, phylogenetic analysis of rDNA sequences using different methods (MP, ML, NJ, and Bayesian inference) displayed O. viverrini and O. felineus as a sister group, but this relationship was not strongly supported. The failure of recovering a robust phylogeny may be due to the relatively small number of synapomorphic characters shared among the species, yielding weak phylogenetic signal. Alternatively, rapid speciation within a very short period time could be another explanation for the relatively poorly resolved relationships among these species. Our data are insufficient for discriminating between sudden cladogenesis and other potential causes of poor resolution. Further information from independent loci might help resolve this phylogeny.     

Cryptococcus zeae, a new yeast species associated with Zea mays

A new yeast, Cryptococcus zeae (type strain HB 1207^T) is described. Six strains were isolated from corn and pests of corn in Austria. Microsatellite-primed polymerase chain reaction (MSP-PCR) fingerprints showed that the strains are members of the same species. Phylogenetical analyses of domains D1/D2 26S rDNA and ITS 1-5,8S–ITS 2 sequences showed C. zeae to have the closest relationship to C. luteolus. The D1/D2 sequences of C. zeae fit with three Korean Cryptococcus sp. strains (AF459690, AF459691, AF459692). The new species is separable from the closest relative C. luteolus using only two physiological tests.     

Analysis of nucleotide sequences polymorphism of its regions of ribosomal genes of diploid Aegilops (L.) species

rDNA sequences of ITS region including full sequences of ITS1, 5.8S and partly sequenced ITS2 of 22 accessions of 5 diploid Aegilops species, were determined. The full alignment length was 524 bp. The analysis of ITS sequences shows a number of species-specific nucleotide changes. For the first time for diploid Aegilops species an interspecific polymorphism was shown. In some positions the polymorphism within accessions was determined. It can be differences either between or within individual plants. In general both inter- and intraspecific polymorphism of ITS sequences was very low. Nucleotide polymorphism was determined only in 25 sites, 12 of which were informative.     

油茶栽培历史与长江流域油茶遗传资源

普通油茶(Camellia oleifera)是我国第一大木本油料作物。普通油茶作为油料作物的栽培历史, 现存确切记载不到1,000年, 长江流域可能是最早栽培油茶的地区之一。普通油茶的野生近缘种是油茶育种宝贵的遗传资源。普通油茶属于山茶科山茶属(Camellia)油茶组(Sect. Oleifera), 其野生近缘种应包括山茶属油茶组和短柱茶组(Sect. Paracamellia)的物种, 但油茶组和短柱茶组的划分仍有争议, 物种间的系统发育关系仍不清楚。油茶组和短柱茶组是山茶属中多倍体出现频率最高的类群, 而且存在突出的种内多倍性现象, 人工选择和种间杂交可能在其中起到促进作用。长江流域是普通油茶的主产区, 也是最主要的野生普通油茶分布区, 拥有丰富的野生普通油茶遗传资源。本研究统计了山茶属油茶组和短柱茶组物种的分布地, 并与野生普通油茶的潜在分布区进行了比较。分析结果显示, 长江流域与珠江流域的分水岭——南岭、苗岭及附近地区是油茶组和短柱茶组物种多样性最高的地区, 同时也是野生普通油茶潜在的高适生区, 可能是普通油茶及其野生近缘种潜在的种间杂交带。物种多样性从南向北呈下降趋势, 可能反映了从南向北的扩散方向。普通油茶及其野生近缘种间的潜在杂交带可能蕴含着丰富的遗传多样性, 为选择育种提供了天然的育种场, 应对这些地区优先开展研究和保护, 挖掘与利用有重要经济价值的遗传资源。     

Rapid differentiation of phenotypically similar yeast species by single-strand conformation polymorphism analysis of ribosomal DNA

Single-strand conformation polymorphism (SSCP) analysis of ribosomal DNA (rDNA) was investigated for rapid differentiation of phenotypically similar yeast species. Sensitive tests indicated that some yeast strains with one, most strains with two, and all strains with three or more nucleotide differences in the internal transcribed spacer 1 (ITS1) or ITS2 region could be distinguished by PCR SSCP analysis. The discriminative power of SSCP in yeast species differentiation was demonstrated by comparative studies of representative groups of yeast species from ascomycetes and basidiomycetes, including Saccharomyces species, medically important Candida species, and phylloplane basidiomycetous yeast species. Though the species within each group selected are closely related and have relatively similar rDNA sequences, they were clearly differentiated by PCR-SSCP analysis of the ITS1 region, given the amplified fragments were less than 350 bp in sizes. By using SSCP analysis for rapid screening of yeast strains with different rDNA sequences, species diversity existing in a large collection of yeast strains from natural sources was effectively and thoroughly investigated with substantially reduced time and cost in subsequent DNA sequencing.     

Delineation of Chondrus (Gigartinales, Florideophyceae) in China and the origin of C. crispus inferred from molecular data

Complete nuclear ribosomal DNA (nrDNA) internal transcribed spacer (ITS) sequences were obtained for 18 Chondrus populations collected at 15 sites from eight countries worldwide. Pairwise comparisons with the multiple alignment revealed that intraspecific divergences of ITS sequences ranged from 0.3 to 1.8% in C. crispus Stackhouse (except for the entity SVLH from France) and from 0.0 to 0.6% in C. ocellatus Holmes, whereas interspecific divergences in Chondrus varied from 1.4 to 5.0%. Three phylogenetic methods (neighbour joining, maximum parsimony and maximum likelihood) confirmed three main lineages: the North Atlantic lineage containing entities of C. crispus from Canada, France, Germany, England, Portugal, Ireland and Wales; a second lineage comprising three species: C. sp. 1, C. armatus (Harvey) Yamada et Mikami, and C. pinnulatus (Harvey) Okamura from the Northern Pacific; and a third lineage containing just one species: C. ocellatus from the Northern Pacific. Chondrus yendoi Yamada et Mikami separated from other Chondrus species singly. nrDNA ITS data indicate that a previous assignment of C. sp. 2 to Mazzaella japonica (Mikami) Hommersand may be incorrect, and additional evidence is needed to resolve the generic placement of this entity. It is inferred from the nrDNA ITS data that three Chondrus species are presently known in China with two, C. ocellatus and C. nipponicus, in Qingdao and two, C. armatus and C. nipponicus, in Dalian. We hypothesize that the ancestor of North Atlantic C. crispus had a Pacific origin, and that the present distribution of C. crispus in the Atlantic Ocean correlates with a trans-Arctic dispersal and vicariance events associated with Pleistocene glaciation maxima.     

Extensive 5.8S nrDNA polymorphism in <Emphasis Type="Italic">Mammillaria</Emphasis> (Cactaceae) with special reference to the identification of pseudogenic internal transcribed spacer regions

The internal transcribed spacer (ITS) region (ITS1, 5.8S rDNA, ITS2) represents the most widely applied nuclear marker in eukaryotic phylogenetics. Although this region has been assumed to evolve in concert, the number of investigations revealing high degrees of intra-individual polymorphism connected with the presence of pseudogenes has risen. The 5.8S rDNA is the most important diagnostic marker for functionality of the ITS region. In Mammillaria, intra-individual 5.8S rDNA polymorphisms of up to 36% and up to nine different types have been found. Twenty-eight of 30 cloned genomic Mammillaria sequences were identified as putative pseudogenes. For the identification of pseudogenic ITS regions, in addition to formal tests based on substitution rates, we attempted to focus on functional features of the 5.8S rDNA (5.8S motif, secondary structure). The importance of functional data for the identification of pseudogenes is outlined and discussed. The identification of pseudogenes is essential, because they may cause erroneous phylogenies and taxonomic problems. Electronic supplementary material The online version of this article (doi:) contains supplementary material, which is available to authorized users.     

Wax plants disentangled: a phylogeny of Hoya (Marsdenieae, Apocynaceae) inferred from nuclear and chloroplast DNA sequences

Hoya (Marsdenieae, Apocynaceae) includes at least 200 species distributed from India to the Pacific Islands. We here infer major species groups in the genus based on combined sequences from the chloroplast atpB-rbcL spacer, the trnL region, and nuclear ribosomal DNA ITS region for 42 taxa of Hoya and close relatives. To assess levels of ITS polymorphism, ITS sequences for a third of the accessions were obtained by cloning. Most ITS clones grouped by species, indicating that speciation in Hoya usually predates ITS duplication. One ITS sequence of H. carnosa, however, grouped with a sequence of the morphologically similar H. pubicalyx, pointing to recent hybridization or the persistence of paralogous copies through a speciation event. The topology resulting from the combined chloroplast and nuclear data recovers some morphology-based sections, such as Acanthostemma and Eriostemma, as well as a well-supported Australian/New Guinean clade. The combined data also suggest that morphological adaptations for ant-symbiosis evolved at least three times within Hoya.