基于DNA拓扑异构酶Ⅱ基因部分序列的侧耳属系统发育分析

对侧耳属（Pleurotus）14个种的14个菌株,亚侧耳属（Hohenbuehelia）1个种和离褶伞属（Lyophyllum）1个种的DNA拓扑异构酶Ⅱ（EC 5．99．1．3）部分序列进行扩增分析。以灰盖鬼伞（Coprinus cinereus）、新型隐球酵母（Cryptococcus neoformans）和玉米黑粉菌（Puccinia polysora）等担子菌为外群,采用最大距离法、最大简约法和最大似然法构建侧耳属的系统发育树。结果表明：作为外群的3个物种独立于所有供试材料;侧耳属菌株作为一大类与供试的离褶伞属和亚侧耳属分开。侧耳属14个种又可细分成6支：可能为侧耳属起源最早的P．flabellatus、P．salmoneostramineus和P．djamor组成一组;P．tuberregium和P．pulmonarius均自成一组;P．abalonus和P．cystidiosus均产生束梗孢,聚为同组;P．eryngii var．eryngii、P．eryngii var．ferulae和P．nebrodensis为一组;另一组由P．ostreatus、P．columbinus、P．cornucopiae和P．citrinopileatus组成。按照侧耳属物种菌丝类型的不同,构建的系统发育树将该属14个种进行系群划分,单、二系菌丝分属于各个不同的分支中,说明单、二系菌丝均为多系起源,与用28S rDNA序列进行系统分析的结果一致。     

基于nLSU rDNA序列分析探讨侧耳属系统发育关系

以PCR产物直接测序分析了侧耳属（Pleurotus）27个种41个茵株的nLSU rDNA序列,以Hohenbuehelia serotina和Lentinula edodes为外群,运用MEGA3．1软件中的邻接法（neighbor—joining）和最大简约法（maximums parsimony）分别构建侧耳属的系统发育树。分子系统发育树表明：Coremiopleurotus组和Pleurotus属内单、二系茵丝系统均为多系起源;P．rattenburyi,刺芹侧耳种族群（P．eryngii species—complex）与被划分在Lepiotarii组的栎侧耳P．dryinus能与侧耳属其他成员明显分开;红侧耳P．djamor、桃红侧耳P．salmoneostramineus、扇形侧耳P．flabellatus与贝盖侧耳P．calyptratus关系密切;金顶侧耳P．citrinopileatus与P．euosmus聚在一起,而与黄白侧耳P．conucopiae为不同的分类单元;肺形侧耳P．pulmonarius与P．abieticale亲缘关系较近。     

基于28S rDNA序列构建侧耳属系统发育树

通过对侧耳属18个分类单元的28S rDNA序列进行分析,构建了侧耳属较为完整的系统发育树。分子系统学资料显示:Coremiopleurotus组和侧耳属内单、二系菌丝系统分别为多系起源的;Pleurotus组单系菌丝种类、被划分在Tuberregium组的具核侧耳和Lentodiellum组的P. levis能够分别与侧耳属内其他成员进行区分;红侧耳、P. calyptratus、P. opuntiae三者关系密切,而金顶侧耳应作为白黄侧耳的种下分类单元。     

基于28SrDNA序列构建侧耳属系统发育树

通过对侧耳属18个分类单元的28S rDNA序列进行分析,构建了侧耳属较为完整的系统发育树。分子系统学资料显示:Coremiopleurotus组和侧耳属内单、二系菌丝系统分别为多系起源的;Pleurotus组单系菌丝种类、被划分在Tuberregium组的具核侧耳和Lentodiellum组的P. levis能够分别与侧耳属内其他成员进行区分;红侧耳、P. calyptratus、P. opuntiae三者关系密切,而金顶侧耳应作为白黄侧耳的种下分类单元。     

侧耳属主要种类ITS序列分析

对侧耳属16个种的38个菌株进行了ITS序列测定,统计分析种内和种间序列趋异度。结果表明,16个种的ITS序列种内趋异度很小,为0-0.007,其中Pleurotus djamor不同地理来源的3个菌株的趋异度为0.007。在16个种的种间ITS序列趋异度中,P.rattenburyi和P.djamor之间趋异度最大,为0.282;P.ostreatus和P.cornucopiae之间的趋异度最小,为0.003。利用ITS序列能够对侧耳属的大多种类进行有效鉴定。ITS序列差异2%-3%作为伞菌中种的鉴定临界值在侧耳属中并不合适。而对于P.ostreatus和P.cornucopiae的准确鉴定,仍需开发新的分类鉴定标记。以香菇为外群,用贝叶斯法构建的侧耳属系统发育树表明,系统发育树的部分节点十分可靠,后验概率值为0.96-1.0。     

中国栽培白灵菇学名的订正

采用形态学方法对采集于新疆野生的阿魏蘑标本进行分类鉴定,结果表明其形态学特征符合刺芹侧耳托里变种Pleurotus eryngii var. tuoliensis的特征范围,它与欧洲已报道的Pleurotus nebrodensis有明显的差异。此外本研究还采用分子生物学方法对从该野生样品分离的菌株CCMSSC 02514进行了rDNA ITS序列分析,结果表明它与我国栽培白灵菇菌种CCMSSC 00973、KH5和AFRL 6022完全相同,以此构建系统发育树,将我国栽培白灵菇种质与意大利的Pleurotus nebrodensis、Pleurotus eryngii var. ferulae以及来自荷兰的Pleurotus eryngii等截然分为两组。因此,形态学和rDNA ITS序列分析结果支持我国栽培的白灵菇与欧洲的Pleurotus nebrodensis为不同种,我国的白灵菇是刺芹侧耳独立进化的一个分支,其名称应该为刺芹侧耳托里变种Pleurotus eryngii var. tuoliensis。     

中国无尾两栖类新记录种——朝鲜侧褶蛙北大核心CSCD

2021年9月在沈阳市蒲河湿地公园(41°41′54″N,122°52′19″E,海拔35 m)采集到3号无尾两栖类动物,经形态特征比较确认为侧褶蛙属(Pelophylax)金线侧褶蛙种组(P.plancyi species complex)的物种。基于线粒体12S rRNA和16S rRNA基因联合构建的侧褶蛙属部分物种最大似然系统发育树显示,采集到的侧褶蛙标本与朝鲜侧褶蛙(P.chosenicus)聚为一支,且具有较高的支持率(0.95)。综合形态和系统发育比较,确定采集到的标本为无尾目(Anura)蛙科(Ranidae)侧褶蛙属的朝鲜侧褶蛙,系中国两栖动物分布新记录种。     

基于ITS序列分析对我国主要栽培的侧耳品种的鉴定及评价

利用PCR产物克隆测序测定了20个我国主要栽培的侧耳品种的ITS序列,另外从GenBank获得侧耳属15个种25条ITS序列及亚侧耳属2个种的ITS序列。以Hohenbueheliagrisea和H.tremula为外群,运用PAUP软件中的简约分析法(parsimonyanalysis)构建的系统发育树表明:侧耳属Pleurotus是单起源的,20个主要栽培的侧耳品种分别聚在三个组,即Ostreatus-eryngii-populinus复合组、Pulmonarius组、Citrinopileatus-cornucopiae组。Ostreatus-eryngii-populinus组含刺芹侧耳Pleurotuseryngii、白灵侧耳P.nebrodensis、香侧耳Pleurotussp.、阿魏侧耳P.eryngiivar.ferulae、平963-1Pleurotussp.及糙皮侧耳P.ostreatus、日本秀珍Pleurotussp.、平802Pleurotussp.、姬菇Pleurotussp.、灰白侧耳P.spodoleucus、缘刺侧耳Pleurotussp.、凤尾菇P.sajor-caju;Pulmonarius组含肺形侧耳P.pulmonarius、小白平菇Pleurotussp.、平8804Pleurotussp.、平侧5Pleurotussp.、美味侧耳P.sapidus;Citrinopileatus-cornucopiae组含黄白侧耳P.cornucopiae、金顶侧耳P.citrinopileatus、鸡汁菌Pleurotussp.。系统树还显示黄白侧耳与金顶侧耳、白灵侧耳与刺芹侧耳亲缘关系密切,而凤尾菇与肺形侧耳分属于不同的组,属于两个不同的种。基于ITS序列分析,本文还针对目前我国栽培的主要侧耳品种在名称使用上的混淆和混乱进行了初步的评价和讨论。     

中国丝盖伞属凹孢亚属的分类与分子系统

结合形态学和分子系统学资料,对我国丝盖伞属凹孢亚属Inocybe subgen.Inosperma进行了分类学研究。确认该亚属8个分类群在中国的分布,并编制了分种检索表,包括3个中国新记录种:新褐丝盖伞Inocybe neobrunnescens、淀粉味丝盖伞I.quietiodor、蜡盖丝盖伞I.lanatodisca。根据采集的材料对此3种进行了形态学描述和绘图,并基于ITS序列,采用贝叶斯法分析了与之相近物种之间的系统学关系。基于n LSU序列重建了我国丝盖伞属凹孢亚属系统发育树,进一步分析和讨论了我国该亚属物种与欧洲和北美的近缘种之间的区别和联系,初步认为裂盖组为非单系群。     

基于DNA序列信息的贞琵甲属物种界定分析（鞘翅目：拟步甲科：琵甲亚科）

贞琵甲属Agnaptoria是小琵甲亚族Gnaptorinina中第三大属和青藏高原特有类群，已知36种/亚种。本文选取3个线粒体基因（COI; Cytb; 16S rDNA）和1个核基因（28S rDNA-D2）片段，采用最大似然法（Maximum likelihood，ML）构建了该属的系统发育树；运用ASAP（Assemble Species by Automatic Partitioning）、GMYC（Generalized Mixed Yule Coalescent）和PTP（Poisson Tree Processes）3种方法对该属进行了分子物种界定分析。结果表明：综合运用3种分子物种界定方法的界定结果与形态鉴定结果基本吻合。依据形态特征与分子物种界定技术相结合的综合鉴定方法，大大提高了该类群的物种鉴定效率，为该类群未来在系统发育、地理分布格局演化等方面的研究提供了可靠的分子数据。     

Pleurotus eryngii species complex: sequence analysis and phylogeny based on partial EF1α and RPB2 genes

The Pleurotus eryngii species complex comprises at least six varieties (var. eryngii (DC.: Fr) Quel., ferulae Lanzi, elaeoselini Venturella et?al., nebrodensis (Inzenga) Sacc., tingitanus Lewinsohn et?al. and tuoliensis C.J. Mou). This species is unique among the genus Pleurotus because in nature it is found in association with certain species of the Apiaceae (Umbelliferae) and Asteraceae (Compositae) families. Sequences of partial regions of the translation elongation factor (EF1α) and RNA polymerase II (RPB2) genes were analyzed in order to detect nucleotide polymorphisms that might unequivocally distinguish varieties eryngii, ferulae, elaeoselini and nebrodensis. A phylogenetic analysis was also performed with an aim to establish phylogenetic relationships among those. Sequence analysis of the partial EF1α and RPB2 genes contained nucleotide polymorphisms able to unequivocally distinguish variety nebrodensis from the rest. However, distinction among eryngii, elaeoselini and ferulae was achieved only through the RPB2 gene. The phylogenetic analyses from the combined data sets (EF1α and RPB2) indicated that P. eryngii is a monophyletic group and that varieties eryngii, elaeoselini and ferulae are closely related. P. eryngii var. nebrodensis was placed in a distinct clade clearly differentiated from the other varieties but still monophyletic with the P. eryngii complex. The limited nucleotide variation in partial EF1α and RPB2 among varieties eryngii, ferulae and elaeoselini supports the placement of these groups as varieties and not species within the complex.     

Molecular genetic analysis of two taxa of the Pleurotus eryngii complex: P. eryngii (DC.Fr.) Quèl. var. eryngii and P. eryngii (DC.Fr.) Quèl. var. ferulae

With the use of isozymes and PCR-fingerprinting analysis molecular markers were found between the varieties Pleurotus eryngii var. eryngii and P. eryngii var. ferulae within the Pleurotus eryngii complex, which allowed the identification of the fruitbodies collected in Southern and Central Italy. The study of sympatric localities has shown that there is no gene exchange between them in the field. The post-mating barriers between these taxa are not yet completely efficient. However, in the field the gene pools of the two taxa appear isolated and associated with specific host plants: Eryngium campestre and Ferula communis . On the basis of the genetic and ecological differences observed and given the absence of gene exchange in sympatric localities, P. eryngii and P. ferulae are to be considered distinct biological species. © 2002 The Linnean Society of London, Biological Journal of the Linnean Society , 2002, 75 , 125–136.     

基于ITS序列分析对杏鲍菇菌种的鉴定

采用拮抗实验和ITS序列分析结合的方法,对供试的20株菌株进行了分析。ITS序列分析结果表明,供试菌种的ITS序列长度为624 bp,与GenBank数据库中杏鲍菇菌种的ITS序列相似度为99%以上,在种的水平上证明供试菌种为杏鲍菇,同时构建的系统发育树将供试菌种聚在了4个类群。     

Genetic Diversity of the Edible Mushroom Pleurotus sp. by Amplified Fragment Length Polymorphism

Pleurotus strains are the most important fungi used in the agricultural industry. The exact characterization and identification of Pleurotus species is fundamental for correct identification of the individuals and exploiting their full potential in food industry. The amplified fragment length polymorphism (AFLP) method was applied for genomic fingerprinting of 21 Pleurotus isolates of Asian and European origin. Using one PstI restriction endonuclease and four selective primers in an AFLP assay, 371 DNA fragments were generated, including 308 polymorphic bands. The AFLP profiles were found to be highly specific for each strain and they unambiguously distinguished 21 Pleurotus sp. fungi. The coefficient of Jaccard's genome profile similarity between the analyzed strains ranged from 0.0 (Pleurotus sp. I vs. P. sajor-caju 237 and P. eryngii 238) to 0.750 (P. ostreatus 246 vs. P. ostreatus 248), and the average was 0.378. The AFLP-based dendrogram generated by the UPGMA method grouped all the Pleurotus fungi studied into two major clusters and one independent lineage located on the outskirt of the tree occupied by naturally growing Pleurotus species strain I. The results of the present study suggest the possible applicability of the AFLP-PstI method in effective identification and molecular characterization of Pleurotus sp. strains.     

ITS-RFLP在白灵菇种质资源鉴定中的应用

为快速鉴别白灵菇种质资源的真伪,对58个供试菌株进行ITS特异性扩增,根据遗传差异选择菌株进行ITS克隆测序,经ITS-RFLP分析和ITS序列分析得知:58个供试菌株中,Pl.n0010、Pl.n0020、Pl.n0025、Pl.n0041这4个菌株为杏鲍菇;菌株Pl.n0037是糙皮侧耳;余下53个菌株为白灵菇。结果表明:ITS-RFLP可应用于白灵菇与杏鲍菇菌株间的鉴定。     

中国白灵侧耳自然群体的交配型因子分析

为了研究我国新疆白灵侧耳自然种群的遗传多样性,估测自然种群的遗传丰度,对51株新疆野生白灵侧耳的84个原生质体单核体的交配型因子进行分析。在84个单核体中存在54个不同的A因子和59个不同的B因子。x2检测表明交配型因子A和B的系列因子均为等概率分布。据此估算我国白灵侧耳自然群体中有79个A因子,100个B因子,自然群体中的单核交配型总数79×100=7,900个,双核交配型总数31,201,050个。可见,新疆白灵侧耳遗传多样性丰富,新疆是我国白灵侧耳的野生种质资源宝库。     

Oogonial biometry and phylogenetic analyses of the Pythium vexans species group from woody agricultural hosts in South Africa reveal distinct groups within this taxon

Pythium vexans fits into the internal transcribed spacer (ITS) clade K sensu Lévesque & De Cock (2004). Within clade K, P. vexans forms a distinct clade containing two enigmatic species, Pythium indigoferae and Pythium cucurbitacearum of which no ex-type strains are available. In South Africa, as well as in other regions of the world, P. vexans isolates are known to be heterogeneous in their ITS sequences and may consist of more than one species. This study aimed to investigate the diversity of South African P. vexans isolates, mainly from grapevines, but also citrus and apple using (i) phylogenetic analyses of the ITS, cytochrome c oxidase (cox) I, cox II, and β-tubulin regions and (ii) seven biometric oogonial parameters. Each of the phylogenies clustered P. vexans isolates into a single well-supported clade, distinct from other clade K species. The β-tubulin region was phylogenetically uninformative regarding the P. vexans group. The ITS phylogeny and combined cox I and II phylogenies, although each revealing several P. vexans subclades, were incongruent. One of the most striking incongruences was the presence of one cox subclade that contained two distinct ITS subclades (Ib and IV). Three groups (A-C) were subjectively identified among South African P. vexans isolates using (i) phylogenetic clades (ITS and cox), (ii) univariate analysis of oogonial diameters, and (iii) multivariate analyses of biometric oogonial parameters. Group A is considered to be P. vexans s. str. since it contained the P. vexans CBS reference strain from Van der Plaats-Niterink (1981). This group had significantly smaller oogonial diameters than group B and C isolates. Group B contained the isolates from ITS subclades Ib and IV, which formed a single cox subclade. The ITS subclade IV isolates were all sexually sterile or produced mainly abortive oospores, as opposed to the sexually fertile subclade Ib isolates, and may thus represent a distinct assemblage within group B. Although ITS subclade Ib included the P. indigoferae ex-type sequence, this group was considered to be P. vexans since South African isolates in this clade produced globose sporangia. Group C contained four apple isolates that were related to, but distinct from P. cucurbitacearum. Although P. vexans groups A-C might be distinct species, they are not described here as such due to (i) these groups only representing some of the known diversity in P. vexans, (ii) conflicting gene tree phylogenies preventing phylogenetic species identification, and (iii) sexually sterile isolates preventing the broad application of biometrical data.