中国栽培糙皮侧耳品种体细胞不亲和性实验与RAPD分析结果的比较

对收集的糙皮侧耳Pleurotus ostreatus19个栽培菌株在贫营养的半PDA培养基中配对进行拮抗线实验,考察其相互间体细胞不亲和性。结果表明,此19个菌株间出现拮抗线的比率是100%,形成的拮抗线类型可分为菌丝集结型(A型)、隔离带型(B型)和暗线型(D型)三类,出现的比例分别是24.9%、23.7%和51.4%。显微观察暗线型拮抗线区域有菌丝自融形成的溶菌沟,另2种拮抗线中没有菌丝自溶。以拮抗线类型分别作为变量进行NTSYS-PC聚类分析,从相似性系数0.48处截断可将其分为3大类,第一类包括802和黑平王等9个菌株;第二类包括苏引6号和江都71等6个菌株;第三类包括夏王40和早秋高丰等4个菌株。应用13条随机引物扩增此19株糙皮侧耳菌株总DNA,共扩增出917条不同分子量的DNA条带。RAPD聚类分析表明,这些菌株的遗传相似性高达85%以上。从相似性系数0.86处截断,也可将这些菌株分为3大类,第一类包括了802和黑平王等17个菌株;第二类仅包括推广一号和夏王40两个菌株;第三类只有831一个菌株。两种方法的聚类分析结果没有相关性。因此,拮抗反应可以作为评价糙皮侧耳栽培菌株之间遗传多样性的方法之一,但与基因组DNA指纹多样性分析结果并不完全吻合,更不能代替分子指纹分析。     

一种快速辨别糙皮侧耳和肺形侧耳的方法

目的：建立一种快速、经济的方法辨别糙皮侧耳（P.ostreatus）和肺形侧耳（P.pulmonarius）。方法：在GenBank下载糙皮侧耳和肺形侧耳的ITS序列,经ClustalX序列比对,利用Primer 3设计特异引物组合1F（5′-GATAGATCTGTGAAGTCGTC-3′）、1R（5′-TCACAATTGGAAAGAAACC-3′）和2R（5′-TGCGTGCTATTGATGAGTGA-3′）,最后经PCR扩增和琼脂糖凝胶电泳检测。结果：5个糙皮侧耳菌株均能得到2条带,分别为342bp和459bp。4个肺形侧耳菌株均能扩增到一条446bp的片段。结论：该组引物适合辨别糙皮侧耳和肺形侧耳。     

AFLP在橡胶树优异种质研究中的应用

采用377DNA测序仪（P.E.Corp.)用AFLP技术对25种分别具有高产／低产、抗白粉病／感白粉病、抗寒／不抗寒、死皮／不死皮性状的橡胶树（Hevea brasiliensis Mull.Ary)无性系（其中Wickham种质15种,Amazon野生橡胶树种质10种）进行了指纹图谱分析,从64对引物组合中选出2对引物组合构建了所有被研究种质的指纹图谱。2对引物共扩增出518条带,多态性比率超过98．6％。遗传多样性分析表明,橡胶树种质间遗传距离为0．25－0．81,RRIM600种质内遗传距离为0．07－0．17。通过基因分型分析获得一条大小为320bp的抗白粉病种质特有的片段。根据以上的AFLP数据进行了聚类分析,结果表明所有被研究种质几乎是依次聚成一个大类。     

ISSR分子标记技术在金针菇菌株鉴别中的应用

利用简单重复序列区间扩增多态性（ISSR）分子标记对来源不同的6种金针菇（Flammulina velutipes）菌株进行了分子鉴定。从20条ISSR引物中筛选出8条可用引物,共获得136条DNA片段,其中多态性条带111个（占总条带数的81．6％）。供试菌株间遗传相似系数从0．5674（农大04—1和全禾04—1）至0．8947（太行05—1和河北03-1）不等。利用UPGMA软件据此进行聚类分析,可将供试金针菇菌株分为3个组群。结果表明,ISSR分子标记可以有效地用于金针菇生产菌株快速准确鉴别,是金针菇指纹图谱分析的有效工具。     

华南瓜类疫霉的RAPD遗传多样性分析

为了解来自广东和广西的瓜类疫霉的遗传多样性,利用从180条RAPD引物中所筛选出的多态扩增性强、重复性好的12条引物,对分离自两省区的96株瓜类疫霉进行了全基因组DNA遗传多样性分析和指纹图谱构建。通过对供试菌株的RAPD-PCR扩增,共获得135条DNA标记谱带,其中124条为多态性谱带,多态检测率为91.9%。利用NTSYSpc Version2.1软件对供试菌株间的遗传距离进行聚类分析并构建系统树,以遗传相似系数0.81为阈值,将96个供试菌株划分为12个RAPD群,多数分离物之间遗传相似性较低,在DNA水平上存在显著的遗传变异,具有较丰富的遗传多样性。不同地区间菌株的遗传分化程度不同,分离自黄瓜的菌株遗传分化明显高于分离自冬瓜的菌株。RAPD群与菌株地理来源、分离寄主、致病力、交配型及甲霜灵抗性均无明显的相关性。     

甘草亲缘关系的RAPD鉴定

以不同地区的3种15组甘草(Glycyrrhiza uralensis、G．infleta、G．glebra)种子为材料,探讨RAPD分子标记在研究、鉴定甘草亲缘关系中的可行性。从50个随机引物中筛选出9个有效引物,9个引物共扩增出961条DNA带,其中多态性条带811条,占总扩增条带的84．4％。对扩增出来的961条DNA带进行分析,结果表明：15组甘草植物的平均遗传距离为0．41,其中采自甘肃民勤野生甘草与采自新疆布尔津乌拉尔野生甘草遗传距离最小,为0．26;而采自内蒙古杭锦旗上海升袖的野生甘草与采自青海贵德的乌拉尔野生甘草遗传距离最大,为0．63。由RAPD聚类分析结果得出15组甘草植物之间的亲缘关系与形态学分类结果存在差异。     

华木莲的遗传多样性研究

利用ISSR标记对中国特有植物华木莲(Manglietia decidua Q．Y．Zheng)的遗传多样性进行了研究,从90个引物中筛选出10个引物用于正式扩增,共扩增出81条DNA带,其中多态性DNA带14条,占17．28％,平均每个引物扩增的DNA带8．1条,多态性条带1．4条。结果表明：华木莲的遗传多样性水平较低(种水平的遗传多样性Hr为0．0649,居群水平的遗传多样性Hs为0．0515,多态位点百分率P为17．28％)。与物种的遗传多样性平均水平、同科的其它种类以及其它特有植物相比,华木莲的遗传多样性极低。     

利用RAPD标记评价小豆种质遗传多样性

本研究利用10个RAPD引物对180份小豆种质的基因组DNA进行扩增,共扩增出44条带,其中35条具有多态性,比例为79．5％,平均每个引物扩增出3．5条多态性带;平均遗传距离为0．274,变异幅度为0．05－0．60,平均遗传多样性指数为0．692;基于RAPD标记,把180份小豆种质聚类划分为4个组群,该组群的划分与小豆的生态地域性似乎不存在明显的相关性。     

茄子耐盐种质资源遗传多样性的SRAP和ISSR分析

利用SRAP和ISSR分子标记,研究了14份耐盐茄子种质资源的遗传多样性,结果表明,2种标记均能揭示材料间较高的遗传多样性,其中ISSR标记多态性略高于SRAP标记。在SRAP分析中,每对引物组合可扩增出8-15条DNA片段,平均为12．12条：26对SRAP引物组合共扩增出315条DNA片段,其中263条具有多态性,多态性比率为83．49％;材料间遗传相似系数变化范围为0．212～0．923,平均值为0．755。在ISSR分析中,每个引物可获得5～16条DNA片段,平均为10．87条;15个ISSR引物共扩增出163条DNA片段,其中141条具有多态性,多态性比率为86．50％;材料间遗传相似系数变幅为0．333-0．957,平均值为0．736。聚类分析表明,2种标记都能将供试材料完全区分开来,聚类结果具有一定的相似性,但也存在明显差异。Mantel相关分析表明,SRAP分析与ISSR分析的相关性达到极显著性水平（r=0．904,P〈0．01）。     

用RAPD技术探讨中国枣的种下划分

利用随机扩增多态性DNA(RAPD)技术对14个枣Ziziphus jujuba 品种和1个野生种——泰山酸枣Z．spinosus的遗传变异进行了研究。从120个10-碱基随机引物中筛选出37个多态性引物用于正式扩增,共扩增出429条DNA带,其中多态性带214条,占49．88％。根据DNA扩增结果计算了品种及类型间遗传距离,并用UPGMA构建了聚类树状图。分析结果表明：龙爪枣 Z．jujuba var．tortuosa、葫芦枣 Z. jujuba var．lageniformis、无核枣 Z.jujuba var．anucleatus 等几个变种内的遗传距离大于变种间遗传距离,认为枣的变种划分是不自然的,宜并入其原变种;枣种下不宜设变种,对枣种下的众多品种,应根据品种间的遗传关系,直接划分品种群。     

油莎豆SRAP指纹图谱构建及遗传多样性分析

利用SRAP分子标记构建了14份不同地理来源、表型具有差异的油莎豆品系的分子指纹图谱并进行遗传多样性分析。结果表明100对引物中共有多态性引物42对,扩增出多态性带328条,平均每对引物7.8条。28对引物在12个品系上具有特征谱带,除品系4和14外,均可用1对引物进行鉴定;采用引物组合法仅用Me2/Em6和Me8/Em11这2对引物就可将14份材料区分开,并利用这2对引物构建了上述品系的数字指纹图谱。UPGMA聚类分析表明,所有参试材料间的遗传距离在0.12～0.75之间,平均为0.42,表明我国不同地理来源的油莎豆品系遗传差异较大,具有较为丰富的遗传多样性。     

24个中外猪种(群)的AFLP多态性及其群体遗传关系

利用12对AFLP引物组合检测了19个中国地方猪种（群）,1个培育猪种和4个欧美引进猪种混合基因组DNA的遗传变异,根据AFLP分析结果计算了24个猪种（群）间的遗传相似系数,据此构建了UPGMA聚类关系图,结果表明,AFLP标记有着很高的多态检测效率（Ai),平均每个引物组合检测到17.3个多态标记,非常适合于猪种（群）遗传多样性分析和品种鉴定;中国地方猪种与欧美引进猪种间的遗传分化十分明显,两类猪群间的亲缘关系较远;南昌白猪与大白猪,铅山黑猪与玉山黑猪有着极近的亲缘关系,分别与其育成历史,地理分布和RAPD分析结果相一致。另外还对部分猪种（群）的聚类分析结果与其形态学,地理分布和现行分类情况不相一致的原因进行了探讨。     

High-resolution genotyping of Salmonella strains by AFLP-fingerprinting

High resolution AFLP fingerprinting, in which subsets of genomic restriction fragments are amplified by means of PCR, was used for the identification of different Salmonella serotypes to investigate whether this technique is applicable in epidemiological studies. Seventy-eight different Salmonella strains comprising 62 serotypes were genetically identified by AFLP. Primer combination M00 ( Mse I primer without additional 3' nucleotides) and E11 ( Eco RI primer with two additional 3' nucleotides) resulted in reproducible profiles containing approximately 50 bands. All serotypes were characterized by a unique profile. In addition, AFLP fingerprinting enabled phage type identification. Different strains previously identified as identical, using typing methods with lower resolution, could be distinguished, showing that AFLP fingerprinting is well suited for bacterial epidemiology and identification.     

60份优质番茄自交系遗传多样性AFLP分析

本文以AFLP技术对60份优质番茄自交系的遗传多样性进行了分析。17对AFLP引物组合共扩增得到905条带,其中多态性条带251条,平均每对引物检测到约15个多态性位点,平均多态率为27.7%;仅用E7M4和E7M10两对引物组合就可以绘制60份番茄自交系的指纹图谱。60个自交系间的Jaccard遗传相似系数变幅为0.259-0.952,平均值为0.664。采用UPGMA方法聚类,遗传相似系数变幅为0.54-0.57时,60份番茄材料可以划分为7个类群。聚类结果与来源、果实大小、果形等性状未表现出明显的相关性。     

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.     

Use of AFLP for differentiation of Metschnikowia pulcherrima strains for postharvest disease biological control

Metschnikowia pulcherrima occurs naturally on fruits, buds and floral parts of apple trees. Some strains are effective as biocontrol agents against postharvest decay of apples and other fruits. The usefulness of the amplified fragment length polymorphism (AFLP) technique was evaluated for the genetic analysis of 26 strains of M. pulcherrima, isolated from different sources in different geographical regions. With six AFLP primer pairs, 729 polymorphic bands were scored. The technique showed a high discriminatory power. Genetic relationships between strains were also estimated using AFLP. All the isolates from the carposphere of apple, previously tested as biocontrol agents, were grouped in a single cluster with a high bootstrap value (97), indicating robustness and reproducibility. AFLP patterns could clearly distinguish the different strains and research is in progress to use some putative specific bands for single tag sequence (STS) conversion to develop isolate-specific markers.     

中国马铃薯晚疫病菌AFLP遗传多样性分析

应用AFLP分子标记检测了我国部分马铃薯主要产区马铃薯晚疫病菌的遗传多样性及不同地区菌株间的亲缘关系。在200对引物组合中,利用6个菌株筛选出12对多态性好、带型清晰的引物组合。利用这12对引物组合对1997-2002年间采自我国黑龙江、河北、四川和云南4省的50株菌株进行了PCR扩增,共扩增出922条谱带,其中多态性标记530条,占57.5%。利用NTSYSpc软件中UPGMA算法构建了我国马铃薯晚疫病菌的亲缘关系树状图,聚类分析结果表明我国马铃薯晚疫病菌的遗传多样性与病原菌的地理来源有一定的相关性,而与交配型、生理小种和对甲霜灵的抗性无明显的相关性。用POPGENE软件计算了各群体间的遗传多样性参数,结果表明我国马铃薯晚疫病菌的遗传多样性程度不高,不同地区种群间分化不明显。     

Changes in AFLP and SSR DNA polymorphisms induced by short-term space flight of rice seeds

Differences of both amplified fragment length polymorphism (AFLP) and simple sequence repeat (SSR) polymorphisms were compared between the 60-d-old rice (Oryza sativa L. cv. DH7) and F3 rice plants (SP3) derived from seed, which endured a 7-d-space flight in March 2002. Total leaf AFLP DNA bands amplified from 22 primer pairs were 537 in DH7, whereas 562 in SP3. From the total 267 SSR DNA bands generated by 267 primer pairs, 39 were polymorphic with 22 larger (56 %) or 17 smaller (44 %) fragment size bands. The greatest numbers of AFLP DNA bands were amplified by primer E1M1 in DH7 (33) and E3M1 in SP3 (35), whilst the least by E4M3 in DH7 (14) and E5M2 in SP3 (16).     

感病与抗病圭亚那柱花草遗传多样性的AFLP分析

圭亚那柱花草(Stylosanthes guianensts Swartz)原产中南美洲及非洲,是一种重要的热带豆科牧草,已在我国华南热带、南亚热带地区种植并利用.由胶孢炭疽菌(Colletotrichum gloeosporioides(Penz.)Sacc.)引起的炭疽病是柱花草的主要病害.采用扩增片段长度多态性(AFLP)技术分析了42个圭亚那柱花草品系的遗传多样性,同时对其抗病性进行了接种鉴定.从96个选择性引物对中筛选出较好的4个,分别对42个圭亚耶柱花草品系进行扩增,共获得出225条带,其中多态性带215条,平均多态性水平为95.5%,表现出高度的多态性.采用NTSYS-pc软件计算了品系间的遗传相似系数,其变化范围为0.31～0.95.根据非加权成对平均数法(uPGMA)进行聚类分析,建立了42个品系的聚类树系图,以所有品系的平均遗传相似系数0.48为阈值,共分为5类.主成分分析表明:第一主成分和第二主成分对全部品系间遗传变异的贡献率分别为56.04%和6.40%,并建立了品系间相互关系的二维图,各品系在二维图中的分布与UPGMA分类相吻合.抗病性鉴定结果表明:各品系对两种典型的病原菌的抗性有差异,其中抗病品系对两种病原菌的抗病相关系数达到0.904,表明抗病品系对两种病原菌有共同抗性.此外,抗病品系在UPGMA聚类中呈随机分布.这些结果表明,AFLP技术是分析圭亚那柱花草遗传多样性的有效方法.     

Genetic characterization of Erwinia amylovora strains by amplified fragment length polymorphism

AIMS: Erwinia amylovora is one of the most important pathogens of pear and apple and is subject to strict quarantine regulations worldwide, although its patterns of dispersal are largely unknown. Previous attempts to fingerprint E. amylovora strains by molecular techniques have detected very little polymorphism because of the high genetic homogeneity of this bacterium. Our aim was to establish and test a typing method to quantify genetic diversity among strains of this plant pathogen. METHODS AND RESULTS: Twenty-two strains from different hosts and geographical locations were examined by PCR fingerprinting with four primers and by amplified fragment length polymorphism (AFLP) with four selected combinations of primers with a single base extension. PCR fingerprinting revealed little polymorphism producing the same amplification patterns for 17 strains, while the combined AFLP patterns yielded 78 polymorphic bands (34% of total bands) and allowed the differentiation of all but two strains. Clustering of strains in the resulting dendrogram was not correlated with host, year or country of isolation, and questions previous genealogies based on PFGE patterns. CONCLUSIONS: The AFLP technique allowed the detection of an unprecedented number of genetic markers in E. amylovora and proved to be the most useful tool so far for discriminating among strains of this pathogen. The results obtained in this study strongly suggest the occurrence of multiple introductions of the pathogen in Spain and other European countries. SIGNIFICANCE AND IMPACT OF THE STUDY: A major limitation in understanding the ecology of fire blight is the lack of typing techniques with a high power of discrimination. This study demonstrates the high resolution and the usefulness of the AFLP technique to differentiate among E. amylovora strains.