西双版纳地区流苏石斛遗传多样性的ISSR分析

采用ISSR分子标记技术,对西双版纳分布的兰科濒危植物流苏石斛（Dendrobium fimbriatum）5个居群共114个个体的遗传多样性进行了研究。从100条引物中筛选出了12条用于扩增,共检测到117个位点,其中105个为多态位点。分析结果表明,流苏石斛居群水平遗传多样性较低。在物种水平上,流苏石斛多态位点百分率PPB为89．74％,Nei’s基因多样性指数日为0．3227,Shannon’s多样性信息指数见。为0．4779;在居群水平上,各个居群的多态位点百分率PPB差异较大（6．84％～39．32％）,平均值为23．93％,Nei’s基因多样性指数H为0．0871,各个居群的Shannon’s多样性信息指数见平均为0．1290。AMOVA分析的结果显示,流苏石斛的遗传变异大多数存在于居群间,占总遗传变异的74．79％。基于Nei’s遗传多样性分析得出的居群间遗传分化系数Gst=0．7443。各居群间的Nei’s遗传一致度（I）范围为0．5882～0．8331。Mantel检测发现,居群间的遗传距离和地理距离之间无显著的正相关关系（r=0．2419,P=0．2416）。鉴于流苏石斛的遗传多样性现状和居群遗传结构,我们建议对流苏石斛居群所有个体实施及时的就地保护,同时建立迁地保护居群,促进基因交流。     

古尔班通古特沙漠荒漠肉苁蓉遗传多样性分析

为了全面了解古尔班通古特沙漠荒漠肉苁蓉居群分布的遗传多样性特点,本研究通过ISSR分子标记技术,利用Nei和Shannon等多样性指数对古尔班通古特沙漠中5个居群166个个体的荒漠肉苁蓉遗传多样性、荒漠肉苁蓉种群和种内的遗传多样性进行分析。在供试材料中,8个引物共扩增出144个多态位点,多态位点百分率达100%,5个居群的多态位点百分率差异在46.53%～77.78%之间。在物种水平上,Nei基因多样度(h)为0.260 4,Shannon多样性指数(I)是0.411 0。遗传变异分析表明,物种水平的居群间遗传分化系数Gst为0.222 2,居群间的基因流Nm为1.750 7。研究显示古尔班通古特沙漠中荒漠肉苁蓉多态位点比例高,各居群基因交流较多,不同居群间遗传变异并不明显,这些对肉从蓉资源有效地保护和利用具有重要意义。     

利用ISSR标记对新疆梭梭遗传多样性的研究

利用ISSR分子标记对新疆梭梭8个居群、218个个体进行了遗传多样性的比较分析,在供试材料中,11个引物共扩增出222个多态位点,多态位点百分率为89.23%,8个居群的多态位点百分率差异在23.42%~45.05%之间,多态位点百分率最高的是乌苏居群,最低的为托克逊居群.遗传变异分析表明,物种水平的基因分化系数Gst为63.78.居群间的基因流Nm为0.284 0,Shannon多样性指数(I)为0.506 0,物种水平的Nei s基因多样度(H)为0.336 2.遗传分析表明乌苏居群和莫索湾居群有较近的遗传距离.     

黄河三角洲柽柳居群的遗传结构和遗传分化

作为黄河三角洲关键建群物种之一,柽柳（Tamarixchinensis）在维持当地湿地生态系统平衡中起着重要作用。为更好地了解黄河三角洲柽柳居群的遗传结构和分化水平,本文利用10个ISSR分子标记,对来自三个柽柳居群的90个个体的遗传多样性进行了对比分析,结果表明：黄河三角洲的柽柳在物种水平存在较高的遗传多样性,总的多态位点百分率（P）达85％,Nei’s基因多样度（H）和Shannon’s多样性指数（I）分别为0．276和0．419;遗传变异主要存在于居群之内,居群间遗传分化程度低（Gst=0．077,φst=0．072）。这种遗传结构和分化格局的形成除了和柽柳的生活型、交配体系以及种子传播模式紧密相关外,可能还与其生境,特别是土壤的含盐量具有一定的关系。     

红泡刺藤居群的遗传多样性研究

利用ISSR分子标记对红泡刺藤的12个居群共242个个体进行了遗传多样性分析.结果表明:(1)16个ISSR引物共扩增到257个位点,其中236个是多态性位点,占91.83％.(2)红泡刺藤居群具有较高水平的遗传多样性,在物种水平上,平均每个位点的多态位点百分率为97.50％,有效等位基因数为1.267,Nei's遗传多样性为0.177,Shannon's多态信息指数为0.296;居群水平上多态位点百分率为51.43％,有效等位基因数为1.205,Nei's 遗传多样性为0.127,Shannon's多态信息指数为0.202.(3)居群间基因分化系数为0.2815,AMOVA分析居群间遗传变异占总量的34.47％,二者结果相近,说明红泡刺藤居群间存在一定程度的遗传分化.居群内的遗传变异为65.53％,基因流为1.2762.(4) Mantel检测显示居群间的遗传距离与地理距离不存在相关性.UPGMA聚类分析和二维主成分分析结果一致,红泡刺藤居群可分为2个居群组,即金沙江居群和维西居群为一个类群,其他居群为另外一大类,表明生态地理条件相似的居群优先集中.     

东俄洛橐吾遗传变异与分化的ISSR分析

应用ISSR标记对东俄洛橐吾（Ligularia tongolensis）的遗传多样性进行了研究。从100个引物中筛选出8个用于正式扩增。在所研究的8个居群共150个个体中检测到148个多态位点。在居群水平上,多态位点百分率（PPB）为50.45%,Nei′s基因多样性指数（H）和Shannon信息指数（I）分别为0.1595和0.2440。在物种水平上,多态位点百分率（PPB）为88.10%,Nei′s基因多样性指数（H）和Shannon信息指数（I）分别为0.2811和0.4279。居群间的遗传分化系数（Gst）达0.4355。研究结果表明东俄洛橐吾的遗传多样性水平很高,居群间遗传分化较大。这与其多样化的生态环境是有必然联系的。因适应其多样化的生态环境而形成了遗传多样性;且因其生态环境的不连续性阻碍了居群间的基因交流而产生了遗传分化,即东俄洛橐吾高水平的遗传多样性和遗传分化是适应其分布区多样化生态环境的结果。     

云南穗花杉的遗传多样性研究

采用随机扩增多态DNA(RAPD)方法对云南穗花杉(Amentotaxus yunnanensis)4个居群和台湾穗花杉似(Amentotaxus for9rmosana)1个居群共104个个体进行了遗传多样性分析。9个随机引物共扩增出清晰谱带143条。云南穗花杉在物种水平上遗传多样性较高(多态位点百分率P为79．0％,基因多样性指数He为0．2718),但云南穗花杉和台湾穗花杉居群内遗传多样性均较低(P为18．0％、6．9％;He为0．0688、0．0198)。云南穗花杉居群间遗传分化强烈(AMOVA,GST和Shannon多样性指数分别为0．7611,0．7503和0．7526)。据推测,第四纪冰川引起的瓶颈效应,小规模居群引起的遗传漂变及幼苗成活率低等因素都加剧了居群间的遗传分化。建议对所研究的云南穗花杉全部居群予以保护,特别是对云南西畴和贵州兴义市七舍两个具有相对较高遗传多样性的居群应该优先建立就地保护点,以达到最大限度保存云南穗花杉遗传多样性的目的。     

金花茶遗传多样性的ISSR分析

采用ISSR分子标记对金花茶的4个自然分布居群的126份样品的遗传多样性水平进行了研究。用12条引物,共检测到105个清晰的扩增位点,其中多态性位点79个,多态位点百分率(PPB)为75．24％。采用POPGENE软件进行分析,结果表明：居群总的Nei’s基因多样性指数为0．2302,Shannon信息多态性指数为0．3502,金花茶总的遗传多样性水平较高。但金花茶居群内的遗传多样性相对较低。基因分化系数为0．5752,遗传变异主要存在于居群间。用NTSYS软件对样品进行UPGMA聚类分析,结果4个居群的样品各自聚在一起,而金花茶两间断分布区区内的居群又各自聚在一起。金花茶4个居群间的遗传距离与地理距离呈显著的正相关(r=0．68261,P=1．0000)。     

二色胡枝子种子储藏蛋白多样性研究

采用SD-PAGE方法对二色胡枝子14个居群147个个体单粒种子盐溶蛋白进行了电泳检测,共检测到28个蛋白单体,其中多态性单体23个,多态百分率为82．14％,各居群内多态百分率平均为33％。各居群间的遗传分化系数（Gst）为0．4669。居群间基因流（Nm）为0．5709。种群内的基因多样性占总群体的53．3％,表明二色胡枝子种群具有丰富的遗传多样性,居群内变异是二色胡枝子遗传多样性的主要来源。聚类分析结果将14个二色胡枝子居群分为3类,居群间地理距离和遗传距离相关性不显著。     

华中特有珍稀植物裸芸香的AFLP遗传多样性分析

采用选择性扩增片段多态性(AFLP)方法对华中特有单种属植物裸芸香(Psilopeganum sinense)的8个自然居群的遗传多样性进行了检测与分析。结果表明:裸芸香的遗传多样性较低,且居群内遗传多样性显著低于物种水平遗传多样性。筛选出的5对引物共得到180个位点,76个为多态位点,多态位点百分率为42.2%,8个居群多态位点百分率为:3.3%～16.7%,居群平均多态位点百分率为9.4%;8个居群Nei多样性指数为0.01987～0.06987,Shannon’s多样性指数为0.0197～0.0816。居群间分化系数Gst=0.5069,居群间基因流为0.2432,不足以维持居群间的基因交流及现有的遗传结构。AMOVA分析表明总遗传变异的13.17%存在于4个地理区域之间,50.45%存在于地理区域内的居群间,36.38%的遗传变异存在于居群内个体间。NTSYS分析表明遗传距离与地理距离不存在相关关系。UPGMA聚类结果表明长江南北两岸的居群并没有产生明显分化。最后,分析了裸芸香的濒危原因并提出了有效的保育措施。     

广西地不容种质资源的ISSR分析

采用简单序列重复区间扩增(ISSR)分子标记技术对广西地不容3个野生居群和1个引种居群共92个个体进行了遗传多样性研究。10个引物共扩增出61条带,其中60条具多态性,多态性位点百分率为98.36%。4个居群多态性百分率在73.77%～86.89%。Nei’s基因多样性指数(H)为0.3379,Shannon信息多样性指数(Ⅰ)为0.5055。3个野生居群Nei’s遗传分化系数(Gst)表明:83.87%遗传变异分布在居群内,16.13%的遗传变异分布在居群间。引种居群与3个野生居群间的遗传一致度达0.8846。引种居群有效地保护了广西地不容的遗传多样性。     

利用AFLP分子标记探讨蜡梅种质资源的遗传多样性

利用AFLP分子标记技术,对中国蜡梅种质资源7个野生种群的遗传多样性进行了研究。利用筛选出的3对引物,共扩增出253条谱带,其中218条多态带,多态位点占86.17% ;种群间的基因分化系数为0.2906,说明蜡梅基因多样性主要存在于种群内;种群总的Nei s基因多样性指数为0.2933,Shannon信息多态性指数为0.4487,蜡梅总的遗传多样性水平较高。蜡梅不同种群遗传多样性水平差异较大,种群多态位点百分率在65.44% ～87.16%之间,Nei s基因多样性指数为0.1653 ～0.4012,Shannon信息多态性指数为0.3132 ～0.5603。神农架种群(SN)和保康种群(BK)的遗传多样性水平较高。用NTSYS2.01版软件对样品进行UPGMA聚类分析,结果7个种群并没有按地理距离进行聚类。最后提出要对各蜡梅野生群体采取相应的迁地和就地保护措施。     

中华水韭遗传多样性的RAPD分析

采用RAPD方法对珍稀濒危植物中华水韭(Isoetes sinensis)4个自然居群的48个样品进行了DNA多态性分析。从60个随机引物中筛选出14个有效引物,共产生124条DNA片段,其中72条为多态性条带,总的多态位点百分率(PPB)为58．06％。各居群间多态位点百分率差异显著(0．81％-12．90％)。AMOVA分析结果表明,4个居群间基因分化系数Фst=0．5894,即遗传变异中有相当一部分来源于群体间(58．94％)。日益缩小的种群规模而导致的居群内近交和遗传漂变的发生以及居群间有限的基因交流可能是中华水韭目前遗传结构的主要成因。鉴于目前中华水韭居群内个体数偏少、遗传多样性较低的现状,建议对其进行就地保护并保护尽可能多的生境,对不同自然居群内的个体进行植株相互移栽和育苗移栽,以提高不同居群间的基因交流,尽可能地保护中华水韭的遗传多样性。     

Genetic Diversity and Genetic Structure of an Endangered Species, Trillium tschonoskii

The genetic diversity and genetic structure of Trillium tschonoskii (Maxim) were investigated using amplified fragment length polymorphism markers. Eight primer combinations were carried out on 105 different individuals sampled from seven populations. Of the 619 discernible DNA fragments generated, 169 (27.3%) were polymorphic. The percentage of polymorphic bands within populations ranged from 4.52 to 10.50. Genetic diversity (H_E) within populations ranged from 0.0130 to 0.0379, averaging 0.0536 at the species level. Genetic differentiation among populations was detected based on Nei's genetic diversity analysis (53.03%) and analysis of molecular variance (AMOVA) (52.43%). AMOVA indicated significant genetic differentiation among populations (52.43% of the variance) and within populations (47.57% of the variance) (p < 0.0002). Gene flow was low (0.4429) among populations. Species breeding system and limited gene flow among populations are plausible reasons for the high genetic differentiation observed for this species. We propose an appropriate strategy for conserving the genetic resources of T. tschonoskii in China.     

Genetic variability and differentiation of Caragana microphylla populations as revealed by RAPD markers

Genetic variability in random amplified polymorphic DNA (RAPD) was studied in 90 individuals of Caragana microphylla, an outcrossing perennial shrub species, from five natural populations sampled in Inner Mongolia steppe of China on a small scale. Nineteen selected primers were used to amplify DNA samples, and totally 225 bands were detected. The percentage of polymorphic bands within populations ranged form 58.22% to 63.56%, with an average of 60% at the population level and 71.11% at the species level, indicating relatively high genetic variations in C. microphylla species. Shannon's information index (I) and Nei's gene diversity (h) showed the similar trend with each other. According to the analysis of Nei's gene diversity, the percentage of genetic variation among populations was 7.13%, indicating a low level of genetic differentiation among populations. There existed a strong gene flow (Nm = 3.26) among populations. Although AMOVA analysis also revealed most variation was within populations (phi(ST) = 4.1%), a significant proportion was observed among populations (P<0.001) in the present study, suggesting genetic differentiation occurred among populations at a certain extent. Based on Mantel's tests and the results of previous studies, the genetic structure pattern of C. microphylla accorded with the isolation-by-distance model on a very large scale, however, on a small scale, the significant genetic differentiation among populations might be enhanced by the micro-environmental divergence among the sampling sites, rather than by geographic factors. Analysis of the genetic variations of C. microphylla populations provided useful information for the adaptive strategy of Caragana species.     

Genetic Diversity Within and Among Lepidium draba Populations from Eastern Anatolia Based on RAPD Analysis

Genetic variation and structure of six natural populations of Lepidium draba L. from Eastern Anatolia were assessed using random amplified polymorphic DNA (RAPD) markers. For RAPD analysis, 12 primers generated 218 reproducible bands across the six populations analyzed, of which 73 bands (33.3%) were polymorphic. The mean Nei’s gene diversity value for all six populations was 0.1771. Shannon’s information index varied with population (0.2278–0.3082), averaging 0.2608. Analysis of molecular variance (AMOVA) showed that genetic diversity was greater within populations (58.66%) than among populations (30.68%). In addition, the variation between groups was 10.33%. The genetic differentiation among populations (G _ST) was 0.3210, indicating that most genetic diversity occurs within populations. Gene flow (Nm) was low, at only 0.5288.     

有性生殖对栗疫病菌群体结构的影响

采用RAPD方法对来源于栗疫病菌8个不同子囊壳的子囊孢子后代和无性生殖的对照群体各23个菌株进行了群体结构的比较。从RAPD随机引物中筛选出扩增多态性丰富的4条引物,共扩增出条带73条,多态性检测率为100%。研究结果表明,在8个子囊壳和无性生殖群体中的基因多样性,64.27%由群体内部引起,只有35.73%的多样性由群体之间的基因差异引起。各子囊壳群体间存在的基因流动很小(Nm=0.8994)。有性群体和无性群体之间的遗传距离为0.1389,基因流动值为3.4212,说明子囊壳群体和无性生殖群体之间存在一定的系统关系。分析表明栗疫病菌子囊孢子后代在自然界的传播对自然界的病菌的多样性起重要的作用。     

Genetic diversity and biogeography of the traditional Chinese medicine, Gardenia jasminoides, based on AFLP markers

Gardenia jasminoides Ellis is used in traditional Chinese medicine (TCM) in China. Levels of genetic variation and patterns of population structure within and among eight wild or cultivated populations of G. jasminoides Ellis in China were investigated using amplified fragment length polymorphism (AFLP) markers. Of the 11 primers screened, four produced highly reproducible AFLP bands. Using these primers, 244 discernible DNA fragments were generated with 165 bands (67.6%), were polymorphic, indicating considerable genetic variation at the species level. In contrast, there were relatively low levels of polymorphism at the population level with the percentage of polymorphic bands (PPB) ranging from 36.89% to 59.43%. Genetic diversity within populations ranged from 0.2086 to 0.3108, averaging 0.2392 at the species level. A high level of genetic differentiation among populations was detected based on Nei's genetic diversity analysis (76.59%), Shannon's index analysis (64.8%) and AMOVA analysis (72.75%). No significant statistical differences (analysis of molecular variance [AMOVA], p = 0.0639) in AFLP variation were found between regions. However, the variance among populations and within populations differed significantly (p < 0.001). An indirect estimate of historical levels of gene flow (N_m = 1.7448) was consistent with the high mean genetic identity (mean I = 0.9263) found among populations. There is an association between geographic and genetic distances between populations. Presently gene change exists between populations.     

Analysis of the Genetic Structure of Sclerotinia sclerotiorum (Lib.) de Bary Populations from Different Regions and Host Plants by Random Amplified Polymorphic DNA Markers

The genetic diversity and genetic structure of a population of isolates of Sclerotinia sclerotiorum (Lib.) de Bary from different regions and host plants were investigated using the random amplified polymorphic DNA (RAPD) method with 20 random decamer primer pairs in order to provide some information on the phylogenetic taxa and breeding for resistance to sclerotinia stem rot. A minimum of three and a maximum of 15 unambiguously amplified bands were generated, furnishing a total of 170 bands ranging in size from 100to 3 200 bp, corresponding to an average of 8.5 bands per primer pair. One hundred and four of these 170bands (61.2%) were polymorphic, the percentage of polymorphic bands for each primer pair ranging from 0.0% to 86.7%. The genetic relationships among the isolates, based on the results of RAPD analysis, were examined. The genetic similarity of all selected isolates was quite high. At the species level, the genetic diversity estimated by Nei's gene diversity (h) was 0.197 and S hannon's index of diversity (I) was 0.300. The unweighted pair-group mean analysis (UPGMA) cluster analysis showed that most isolates from the same regions were grouped in the same cluster or a close cluster. The population of isolates from Hefei (Anhui Province, China) was more uniform and relatively distant to other populations. The Canadian population collected from carrot (Daucus carota var. sativa DC.) was relatively close to the Polish population collected from oilseed rape (Brassica napus L.) plants. There was no relationship between isolates from the same host plants. An analysis of molecular variance (AMOVA) revealed that the percentage of variance attributable to variation among and within populations was 50.62% and 49.38%, respectively. When accessions from China, Europe, and Canada were treated as three separate groups, the variance components among groups,among populations within groups, and within populations were -0.96%, 51.48%, and 49.47%, respectively.The genetic differentiations among and within populations were highly significant (P ＜ 0.001). Similarly, the coefficient of gene differentiation (Gst) in total populations calculated by population genetic analysis was 0.229 4, which indicated that the genetic variation among populations was 22.94%. The gene flow (Nm)was 1.68, which indicated that the gene permutation and interaction among populations was relatively high.     

中国桃蛀螟不同地理种群的遗传多样性

本文应用ISSR分子标记技术对中国桃蛀螟Conogethes punctiferalis 11个地理种群的基因组DNA进行了遗传多样性和遗传分化分析。从34条引物中筛选出6条用于ISSR多态性分析, 共扩增出211条带, 其中209条具多态性, 总的多态性条带百分率为99.05%。11个种群的遗传距离在0.0059~0.0237之间, Nei氏基因多样性指数为0.1750, Shannon信息指数为0.2966, 遗传分化系数为0.053, 基因流高达8.8724。结果提示中国桃蛀螟地理种群因基因流水平较高而种群遗传分化水平保持较低。