应用5.8S rDNA及ITS区序列分析链格孢种级分类*

对9个链格孢小孢子种和3个大孢子种共20个链格孢菌株的5.8S rDNA及其两侧的ITS1区和ITS2区进行了序列分析。聚类分析结果表明形态差异大的种可以明确加以区分,而供试的9个小孢子种之间差异很小,不能根据对所选区段的序列分析加以区分。传统分类上的滨菊链格孢不属于Alternaria, 其分类地位需进一步研究。     

应用5．8SrDNA及ITS区序列分析链格孢种级分类

对9个链格孢小孢子种和3个大孢子种共20个链格孢菌株的5．8SrDNA及其两侧的ITS1区和ITS2区进行了序列分析。聚类分析结果表明形态差异大的种可以明确加以区分,而供试的9个小孢子种之间差异很小,不能根据对所选区段的序列分析加以区分,传统分类上的滨菊链格孢不属于Alternaria,其分类地位需进一步研究。     

小孢子链格孢endoPG基因核苷酸序列分析及系统发育研究

对供试小孢子链格孢菌株的内聚半乳糖醛酸酶(endoPG)基因进行扩增,大部分菌株都可获得PCR产物。核苷酸和氨基酸序列比较表明:不同种小孢子链格孢endoPG基因核苷酸序列存在明显差异,甚至表现在氨基酸水平,这些差异可以作为一些种如梨黑斑链格孢、长柄链格孢区分的分子性状。利用邻近结合法构建系统发育树,所有菌株被分为8个聚类组。在系统发育树上,链格孢的一些不同分离物被聚在不同组中,而细极链格孢、链格孢的部分菌株、苹果链格孢、柑橘链格孢、粗柠檬褐斑链格孢、橘树链格孢被聚为一组,显示根据形态学特征划分的这些种与分子性状的不一致性。endoPG基因核苷酸序列富于变化,为小孢子链格孢系统发育研究提供了一种有用的手段。     

小孢子链格孢endoPG基因核苷酸序列分析及系统发育研究

对供试小孢子链格孢菌株的内聚半乳糖醛酸酶(endoPG)基因进行扩增,大部分菌株都可获得PCR产物。核苷酸和氨基酸序列比较表明:不同种小孢子链格孢endoPG基因核苷酸序列存在明显差异,甚至表现在氨基酸水平,这些差异可以作为一些种如梨黑斑链格孢、长柄链格孢区分的分子性状。利用邻近结合法构建系统发育树,所有菌株被分为8个聚类组。在系统发育树上,链格孢的一些不同分离物被聚在不同组中,而细极链格孢、链格孢的部分菌株、苹果链格孢、柑橘链格孢、粗柠檬褐斑链格孢、橘树链格孢被聚为一组,显示根据形态学特征划分的这些种与分子性状的不一致性。endoPG基因核苷酸序列富于变化,为小孢子链格孢系统发育研究提供了一种有用的手段。     

小孢子链格孢OPA2-1核苷酸序列分析及系统发育研究

本研究采用引物对OPA2-1L/OPA2-1R对供试小孢子链格孢菌株OPA2-1区段进行扩增,所有菌株都可获得PCR产物。核苷酸序列分析表明:不同小孢子链格孢种OPA2-1核苷酸序列存在明显差异。利用邻近结合法构建系统发育树,供试菌株被分为8个组,梨黑斑链格孢Alternaria gaisen、长柄链格孢A.longipes、树状链格孢A.arborescens明显被归于不同分支,显示OPA2-1核苷酸序列对这些种均具有区分能力;链格孢A.alternata的一些不同分离物被聚在不同组中,说明链格孢A.alternata存在明显遗传差异,可能为一个复合体。OPA2-1核苷酸序列富于变化,可作为小孢子链格孢系统发育研究的一种有用的手段。     

白菜种传黑斑病菌rDNA ITS区序列分析

本文以来自国内外的20株白菜黑斑病菌及近源种为研究材料,进行了5.8SrDNA及其侧翼ITS区的克隆、测序、序列变异及遗传进化关系分析。黑斑病菌及其近源种真菌核糖体5.8SrDNA及其侧翼ITS区序列比对结果显示,不同种菌株ITS1比ITS2在碱基构成上有更大变异,而且ITS1的序列长度变异比ITS2的大;而种内虽然各菌株的寄主和地理来源不同,但ITS1和ITS2在长度上均没有变异,碱基构成上存在微小的变异。对该区序列的聚类分析表明,白菜黑斑病菌3个种芸薹链格孢Alternariabrassicae、甘蓝链格孢A.brassicicola和萝卜链格孢A.japonica虽然地理来源和寄主不同,但种内的不同菌株均在一个独立的聚类组中,种之间以及其和链格孢属内其它种在聚类关系上能明显分开,可基于该区进行黑斑病菌的分类鉴定。     

链格孢属小孢子种的RAPD分析*

用筛选出的12个随机引物,对链格孢属Alternaria13个小孢子种和作为对照的3个大孢子种共55个分离系(isolates)进行RAPD分析。大孢子种Alternariasolani、A.porri和形态独特的A.leucanthemi在树状聚类图上遗传距离0.44处与所有供试小孢子种区分开,它们彼此之间在遗传距离0.25处相区分,表明所采用的RAPD分析方法适于链格孢种间亲缘关系的研究。所有供试的链格孢小孢子种在遗传距离0.31水平上被聚在一起,表明它们之间的亲缘关系较近。A.infectoria与其它链格孢小孢子种之间遗传距离较远;A.longipes的3个分离系和A.brassicicola的7个分离系在较低的遗传距离上被聚在一起,表明它们是独立的种。其它供试链格孢小孢子种的不同分离系在树状聚类图上未显示明确区分。     

链格孢属小孢子种的RAPD分析

用筛选出的12个随机引物,对链格孢属Alternaria13个小孢子种和作为对照的3个大孢子种共55个分离系(isolates)进行RAPD分析。大孢子种Alternariasolani、A.porri和形态独特的A.leucanthemi在树状聚类图上遗传距离0.44处与所有供试小孢子种区分开,它们彼此之间在遗传距离0.25处相区分,表明所采用的RAPD分析方法适于链格孢种间亲缘关系的研究。所有供试的链格孢小孢子种在遗传距离0.31水平上被聚在一起,表明它们之间的亲缘关系较近。A.infectoria与其它链格孢小孢子种之间遗传距离较远;A.longipes的3个分离系和A.brassicicola的7个分离系在较低的遗传距离上被聚在一起,表明它们是独立的种。其它供试链格孢小孢子种的不同分离系在树状聚类图上未显示明确区分。     

链格孢属小孢子种的RAPD分析

用筛选出的12个随机引物,对链格孢属Alternaria13个小孢子种和作为对照的3个大孢子种共55个分离系(isolates)进行RAPD分析。大孢子种Alternaria solani,A.porri和形态独特的A.leucanthemi在树状聚类图上遗传距离0．44处与所有供试小孢子种区分开,它们彼此之间在遗传距离0．25处相区分,表明所采用的RAPD分析方法适于链格孢种间亲缘关系的研究。所有供试的链格孢小孢子种在遗传距离0．31水平上被聚在一起,表明它们之间的亲缘关系较近。A.infectoria与其它链格孢小孢子种之间遗传距离较远;A.longipes的3个分离系和A.brassiciola的7个分离系在较低的遗传距离上被聚在一起,表明它们是独立的种。其它供试链格孢小孢子种的不同分离系在树状聚类图上未显示明确区分。     

链格孢菌酯酶同工酶分析及其分类学意义

分析了20株链格孢菌的酯酶同工酶聚丙烯酰胺凝胶电泳图谱,并将酶谱进行聚类分析。结果发现:20株链格孢菌在37%的相似系数处明显分为大孢子组和小孢子组;大孢子组在52%的相似系数处分为6组,每组代表1个种,小孢子组在较高的相似性水平上分组与形态分组结果基本一致。本试验结果还表明:酯酶同工酶电泳方法简单易行,能准确反映种间的微小差异,适用于链格孢属真菌的种级分类,可作为传统形态学分类的一个重要辅助手段。     

基于rDNAITS序列分析Alternaria与相似属的关系及A.leucanthemi的分类地位

对Alternaria,Stemphylium,Ulocladium,Nimbya,Embellisia等五个形态相似属的代表性种进行了5.8S/ITS区段序列测定,连同从GenBank下载的相关有性型Pleospora,Lewia的同项资料,由Neighbor-joining方法构建系统发育树。序列对比结果显示,所有参试的菌株/种的5.8SrDNA序列保守程度较高,ITS序列变化较大,ITS1比ITS2变化更大。由5.8S/ITS构建的系统发育树可以足够将供试菌区分到属;系统发育树显示Alternaria,Ulocladium,Nimbya和Embellisia系统学关系较近,又存在一定的分化;Stemphylium聚在相对较远的分支上,与上述四属关系较远,相对独立进化;有性型的Pleospora与无性型的Stemphylium被聚到一个分支,这种不同阶段菌株在遗传基础上的一致,充分证明所用方法及所选测序的rDNA区段对本类群真菌的分类很有价值。Alternarialeucanthemi位于系统发育树的外侧,较为独立进化,与Alternaria的其它种亲缘关系较远,却与Stemphyliumspp.和Bipolarisspp.关系较近,对其目前的分类地位提出质疑。     

Amazonian malaria vector anopheline relationships interpreted from ITS2 rDNA sequences

Species identification of anopheline mosquitoes (Diptera: Culicidae) can be problematic because many of them belong to complexes of morphologically similar species, often with contrasted ecology, behaviour and vectorial importance. The application of DNA-based diagnostics has proved to be useful for distinguishing between such species. We determined ribosomal DNA sequences of the second internal transcribed spacer (ITS2) from samples of 16 species of Anopheles captured in the Amazon Basin, Brazil. Length of the ITS2 varied from 323 to 410 base pairs, with GC content ranging from 50.7% to 66.5% and sequence identity from 25% to 99% between species. Maximum-likelihood paup analysis separated two distinct groups of species conforming with the recognized subgenera Anopheles (represented by eiseni, mattogrossensis, mediopunctatus and peryassui) and Nyssorhynchus (represented by 12 spp.). For the latter group, the neighbour-joining tree generated from rDNA sequence ITS2 relationships is compatible with the morphological taxonomic key established for these Amazonian species: albitarsis, aquasalis, benarrochi, braziliensis, darlingi, deaneorum, dunhami, evansae, nuneztovari, oswaldoi, rangeli and triannulatus. These ITS2 sequence data proved to be a useful tool for species identification and, potentially, to solve taxonomic problems.     

Molecular systematics of citrus-associated Alternaria species

The causal agents of Alternaria brown spot of tangerines and tangerine hybrids, Alternaria leaf spot of rough lemon and Alternaria black rot of citrus historically have been referred to as Alternaria citri or A. alternata. Ten species of Alternaria recently were described among a set of isolates from leaf lesions on rough lemon (Citrus jambhiri) and tangelo (C. paradisi × C. reticulata), and none of these isolates was considered representative of A. alternata or A. citri. To test the hypothesis that these newly described morphological species are congruent with phylogenetic species, selected Alternaria brown spot and leaf spot isolates, citrus black rot isolates (post-harvest pathogens), isolates associated with healthy citrus tissue and reference species of Alternaria from noncitrus hosts were scored for sequence variation at five genomic regions and used to estimate phylogenies. These data included 432 bp from the 5' end of the mitochondrial ribosomal large subunit (mtLSU), 365 bp from the 5' end of the beta-tubulin gene, 464 bp of an endopolygalacturonase gene (endoPG) and 559 and 571 bp, respectively, of two anonymous genomic regions (OPA1-3 and OPA2-1). The mtLSU and beta-tubulin phylogenies clearly differentiated A. limicola, a large-spored species causing leaf spot of Mexican lime, from the small-spored isolates associated with citrus but were insufficiently variable to resolve evolutionary relationships among the small-spored isolates from citrus and other hosts. Sequence analysis of translation elongation factor alpha, calmodulin, actin, chitin synthase and 1, 3, 8-trihydroxynaphthalene reductase genes similarly failed to uncover significant variation among the small-spored isolates. Phylogenies estimated independently from endoPG, OPA1-3 and OPA2-1 data were congruent, and analysis of the combined data from these regions revealed nine clades, eight of which contained small-spored, citrus-associated isolates. Lineages inferred from analysis of the combined dataset were in general agreement with described morphospecies, however, three clades contained more than one morphological species and one morphospecies (A. citrimacularis) was polyphyletic. Citrus black rot isolates also were found to be members of more than a single lineage. The number of morphospecies associated with citrus exceeded that which could be supported under a phylogenetic species concept, and isolates in only five of nine phylogenetic lineages consistently were correlated with a specific host, disease or ecological niche on citrus. We advocate collapsing all small-spored, citrus-associated isolates of Alternaria into a single phylogenetic species, A. alternata.     

大豆疫霉和苜蓿疫霉rDNA ITS序列分析*

采用真菌核糖体基因转录间隔区(ITS)通用引物,PCR分别扩增了Phytophthora sojae的5个菌株(Pg1、Pg2、Pg3、CN1和S317)和1个P. medicaginis (菌株44390)的ITS1与ITS2,并对PCR产物进行了序列测定。根据Bioedit软件中的neighbour-joining methods分析法将上述序列和Genbank中已登录的P. sojae、P. medicaginis、P. megasperma和P.trifolii等4个形态学种10个登录菌株的ITS1与ITS2碱基序列进行聚类分析。结果是聚类组与形态学种有一定差别,4个种16个菌株分成7个聚类组。结果表明,分别属于同一形态学种且可聚为一组的不同个体之间的ITS碱基序列遗传相似性最高,但是也具有一定的多样性;形态学上属于不同种的个体的ITS可以聚为一组。上述结果提示L41385可能不属于P. sojae, L41380可能属于是P. trifolii,P. megasperma仍是一个复合种。同时提示ITS DNA碱基序列可以区分形态学种。     

Alternaria jesenskae sp. nov., a new species from Slovakia on Fumana procumbens (Cistaceae)

Alternaria jesenskae sp. nov. recovered from seeds of a shrubby perennial plant Fumana procumbens (Cistaceae) in Slovakia is described and illustrated. The new taxon can be clearly separated from the other related large-spored and filament-beaked Alternaria species based on sequences of the ITS1, 5.8S and ITS2 region as well as by its distinctive morphology. Even though the molecular data have shown close relatedness with A. multirostrata, the new species is morphologically most similar to A. tomatophila distinguished primarily by the pronounced colony pigmentation, conidial septation and beak branching.     

A new Alternaria species from grapevine in China

Twelve Alternaria strains were isolated from pedicels and rachis from different parts of grapevines in China. In a phylogenetic analysis, nine showed a close relationship with Alternaria longipes, and are described as a new species, A. viniferae sp. nov., but the other four clustered with A. alternata and A. arborescens within the alternata species-group. The new species can clearly be separated from other related small-spored Alternaria species based on sequences of portions of the glyceraldehyde-3-phosphate dehydrogenase (gpd) and Alternaria major allergen (Alt a 1) genes as well as by distinctive morphology.