槭叶小牵牛——中国大陆一新归化种

走马胎(Ardisia gigantifolia)是紫金牛科(Myrsinaceae)紫金牛属(Ardisia)多年生小灌木植物。走马胎作为我国传统中药材,已有多年的药用历史。目前,走马胎不再局限于临床药用,在食疗和保健方面的开发利用崭露头角,大大扩展了其应用范围。随着走马胎市场需求量增大,野生走马胎的过度采挖,导致野生走马胎资源几近枯竭。人工栽培走马胎逐渐成为供应药用市场的主力军,但是人工栽培走马胎种质、种子来源混杂,常会造成质量和疗效的不稳定,利用分子标记技术可以从分子水平上对走马胎进行种质的区分和评价。该研究利用ISSR分子标记技术,对来自广西地区的36份走马胎种质资源进行了遗传多样性分析,采用 POPGEN32 进行数据分析,UPGMA 绘制聚类图。结果表明：14条ISSR引物共检测到136个清晰的扩增位点,多态性位点112个,多态位点百分率为82.35%;Nei’s基因多样性指数(H)为0.296 5,Shannon多样性指数(I)为0.441 7,基因分化系数(Gst)为0.855 8。个体间的遗传相似系数为0.667 8～0.838 2,平均为0.739 1。基于聚类分析可知,所有的个体被划分为5类,其中绝大多数来自相同或者邻近地区的个体严格按照地理位置聚为相同的一类或者亚类,只有少数个体在归类上与地理位置相悖。研究证明ISSR分子标记技术在评价走马胎种质资源亲缘关系和遗传变异等方面有很好的适用。该研究结果可为该药用植物的种质资源评估和引种栽培提供科学依据。     

走马胎种质资源遗传多样性的ISSR分析（英文）

走马胎(Ardisia gigantifolia)是紫金牛科(Myrsinaceae)紫金牛属(Ardisia)多年生小灌木植物。走马胎作为我国传统中药材,已有多年的药用历史。目前,走马胎不再局限于临床药用,在食疗和保健方面的开发利用崭露头角,大大扩展了其应用范围。随着走马胎市场需求量的增大,野生走马胎植物被过度采挖,导致野生走马胎资源几乎枯竭。人工栽培走马胎逐渐成为供应药用市场的主力军,但是人工栽培走马胎种质、种子来源混杂,常会造成质量和疗效的不稳定,而利用分子标记技术可以从分子水平上对走马胎进行种质的区分和评价。该研究利用ISSR分子标记技术,对来自广西地区的36份走马胎种质资源进行了遗传多样性分析,采用POPGEN32软件进行数据分析,用UPGMA软件绘制聚类图。结果表明:14条ISSR引物共检测到136个清晰的扩增位点,多态性位点112个,多态位点百分率为82.35%;Nei’s基因多样性指数(H)为0.296 5,Shannon多样性指数(I)为0.441 7,基因分化系数(Gst)为0.855 8。个体间的遗传相似系数为0.667 8~0.838 2,平均为0.739 1。基于聚类分析可知,所有的个体被划分为5类,其中绝大多数来自相同或者邻近地区的个体严格按照地理位置聚为相同的一类或者亚类,只有少数个体在归类上与地理位置相悖。研究证明ISSR分子标记技术在评价走马胎种质资源亲缘关系和遗传变异等方面有很好的适用。该研究结果为该药用植物的种质资源评估和引种栽培提供了科学依据。     

广东省五节芒遗传多样性的ISSR分析

采用ISSR分子标记技术,对广东省内分布的能源植物五节芒(Miscanthus floridulus)13个野生居群共215个个体的遗传多样性进行了研究.9个ISSR引物共扩增到了81个位点,其中76个是多态性位点.结果表明,广东五节芒的遗传多样性水平很高,物种水平上,多态位点百分率(PPB)为93.83％,Nei's...     

黄芩种质资源ISSR遗传多样性的分析及评价

采用ISSR分子标记技术对6个野生或栽培居群共147份黄芩种质进行遗传多样性分析和评价。分析结果表明,51个ISSR引物中筛选出18条扩增条带清晰、重复性好和多态性高的引物,共扩增出485条清晰的条带,其中466条具有多态性,平均多态性位点比率为96.08%,平均Nei’s基因多样性指数和Shannon’s信息指数分别为0.244 4和0.388 9,等位基因数（Na）和有效等位基因数（Ne）分别为1.993 8和1.383 9,遗传分化指数G_st=0.122 3,遗传一致度（I）和遗传距离（D）分别为0.951 5和0.050 1,说明收集的黄芩种质资源在总体上具有较高的遗传多样性,不同居群间存在一定的遗传分化和基因交流,遗传变异主要存在于居群内。分子聚类结果表明,同一地区的种质并没有按照收集来源完全聚类,可能与种质不同起源或民间栽培引种有关。在DNA分子水平揭示黄芩种质资源的遗传多样性水平,将为进一步黄芩种质资源评价、保存和新品种选育等利用提供依据。     

基于ISSR标记的中国芋种质资源遗传多样性分析

本研究利用ISSR分子标记技术,对国家种质武汉水生蔬菜资源圃收集并保存的来自全国各地的72份芋种质资源进行遗传多样性检测。研究结果表明,13条ISSR引物在72份芋种质资源中共扩增出109条带,其中85条带具有多态性,平均多态性位点比率为78.51%;不同芋种质资源间遗传相似系数的变幅为0.56~1,说明ISSR标记能够揭示芋种质资源之间较高的遗传多样性;在遗传系数0.725处,72份芋种质资源被聚为3大类,为进一步研究芋种质资源分类、起源、保存和利用奠定了基础。     

抗风桐(Pisonia grandis)的生态生物学特征

对收集于广西桂林的17份野生毛葡萄种质和24份栽培葡萄种质,分别使用12条ISSR和12条SCoT引物进行了遗传多样性和亲缘关系检测。结果表明：两种分子标记均能产生较丰富的多态性片段,可有效应用于葡萄的遗传多样性检测,但在聚类分析结果上表现出一定的差异性,SCoT分子标记能更好地区分野生种质和栽培品种,说明SCoT分子标记在葡萄遗传多样性检测和系统进化研究上可能更有优势。从SCoT聚类结果上看,广西植物研究所收集的3个野生毛葡萄种质zws1、zws2和zws3相对其它野生种质而言,更偏向于与栽培种质聚为一类,说明这一类野生毛葡萄可能是这些栽培品种的原始亲本来源之一。不同的野生种质聚为多个类群,并表现出明显的地域特性,但遗传距离相对较远,说明桂林野生毛葡萄资源具有丰富的遗传变异。栽培品种没有明显的聚类特点,可能因为所选用的栽培品种的地域代表性并不是很强,也可能是因为栽培品种在不断的人工杂交选育过程中,遗传背景趋向一致,遗传多样性降低。该研究证明SCoT分子标记在葡萄遗传多样性研究上具有一定的优势。该研究结果为桂林毛葡萄资源的保护、利用和品种选育提供了理论依据,也为葡萄的系统进化研究提供了参考。     

41份葡萄种质遗传多样性的ISSR和SCoT对比分析

对收集于广西桂林的17份野生毛葡萄种质和24份栽培葡萄种质,分别使用12条ISSR和12条SCoT引物进行了遗传多样性和亲缘关系检测。结果表明:两种分子标记均能产生较丰富的多态性片段,可有效应用于葡萄的遗传多样性检测,但在聚类分析结果上表现出一定的差异性,SCoT分子标记能更好地区分野生种质和栽培品种,说明SCoT分子标记在葡萄遗传多样性检测和系统进化研究上可能更有优势。从SCoT聚类结果上看,广西植物研究所收集的3个野生毛葡萄种质zws1、zws2和zws3相对其它野生种质而言,更偏向于与栽培种质聚为一类,说明这一类野生毛葡萄可能是这些栽培品种的原始亲本来源之一。不同的野生种质聚为多个类群,并表现出明显的地域特性,但遗传距离相对较远,说明桂林野生毛葡萄资源具有丰富的遗传变异。栽培品种没有明显的聚类特点,可能因为所选用的栽培品种的地域代表性并不是很强,也可能是因为栽培品种在不断的人工杂交选育过程中,遗传背景趋向一致,遗传多样性降低。该研究证明SCoT分子标记在葡萄遗传多样性研究上具有一定的优势。该研究结果为桂林毛葡萄资源的保护、利用和品种选育提供了理论依据,也为葡萄的系统进化研究提供了参考。     

利用RAPD和ISSR分子标记分析地黄种质遗传多样性

用RAPD与ISSR技术对地黄的8个品种和2个脱毒品系进行了种质遗传多样性分析.分别从80条RAPD引物和44条ISSR引物中筛选出适合地黄种质分析的17条RAPD引物和10条ISSR引物用于RAPD和ISSR分析.17条RAPD引物共扩增出177条带, 多态性位点数为109; 多态性位点比率为61.58%;平均多样性指数(I)为0.3135;每个位点的有效等位基因数(Ne)是1.3641; 10条ISSR引物共扩增出110条带. 多态性位点数为79; 多态性位点比率为71.58%;平均多样性指数(I)为0.3577;每个位点的有效等位基因数(Ne)是1.4037. 基于扩增条带数据库建立了各自的Jaccard遗传相关系数矩阵,构建了相似的分子树状图,将10个供试材料分为2类:一类群含组培85.5、大田85.5、组培9302、大田9302、金状元和金白6个材料;另一类群含北京1号、大红袍、地黄9104和野生地黄4个材料.两种分子标记的分析结果呈极显著正相关(r＝0.649).结果表明,RAPD与ISSR标记适合于地黄种质遗传多样性分析,ISSR标记技术是一种多态性和重复性优于RAPD技术的实用技术.     

基于ISSR与RAPD标记分析内蒙古赤芍的遗传多样性

采用ISSR和RAPD分子标记技术对28个赤芍种群进行遗传变异和亲缘关系分析,为准确地评价赤芍种质的遗传特征、资源保护及新品种选育提供理论依据。结果显示:(1)利用分别筛选的14条ISSR和RAPD引物扩增出257条和215条条带,其中多态性条带分别为251条和209条,多态性条带百分率分别为97.8%和97.2%;同时证实野生赤芍种群的遗传多样性高于栽培种群。(2)根据Shannon’s信息指数(I)和Nei’s基因多样性指数(H_e)值,发现内蒙古多伦种群(DL)的遗传多样性水平最高,建议在此地建立野生赤芍资源保护区。(3)根据遗传分化系数(G_(st)),发现野生赤芍种群的遗传分化主要发生在种群内,可能由遗传漂变引起;而栽培赤芍种群的遗传分化主要在种群间,说明栽培赤芍种群间的基因交流较少。(4)两种分子标记的聚类分析结果均将28个赤芍种群聚为5大类,遗传距离变化范围分别为0.115 1～0.343 8和0.095 5～0.286 2。研究表明,互相印证的ISSR和RAPD方法可以在DNA水平上更准确有效地分析赤芍种质资源的遗传结构和遗传多样性。     

橡胶树种质资源遗传多样性研究——Ⅰ．速生种质遗传多样性RAPD分析

应用RAPD技术对8份野生种质和12份栽培种质进行遗传多样性分析,筛选到18个具有多态性扩增的引物．共扩增出128条带。据Nei-Li相似系数将20份材料分别聚为野生种质和栽培种质两大类。5个野生种质聚为野生种质类群,12个栽培种质和3个野生种质聚为栽培种质类群。研究结果表明,RAPD技术用于橡胶树种质资源研究,能够为野生种质优良特性导入栽培种质提供分子水平的参考依据。     

Genetic diversity analysis of Cynodon dactylon (bermudagrass) accessions and cultivars from different countries based on ISSR and SSR markers

ISSR and SSR markers were used to evaluate genetic diversity among 33 Cynodon dactylon accessions and 22 cultivars from four different countries in order to provide information on how to improve the utilization of bermudagrass germplasms. Eighty eight bands were amplified by nine SSR primer combinations and 236 bands were observed from 23 ISSR primers. The results showed that 97.7% of the SSR primers and 86.9% of the ISSR primers were polymorphic. The genetic similarity coefficients (GSC), gene diversity (He) and Shannon index (I) were 0.58–0.97, 0.27 and 0.41, respectively, for ISSR and 0.52–0.97, 0.29, and 0.43 for SSR. The UPGMA analysis clustered the 55 accessions (cultivars) into three groups. The cluster results produced by the ISSR data were close to the SSR data results. Analysis based on the combined ISSR and SSR data was more closely related to the geographical distribution of the tested germplasm.     

ISSR-based clustering of cultivated flax germplasm is statistically correlated to thousand seed mass

Inter-simple sequence repeat (ISSR)-polymerase chain reaction (PCR) polymorphism was generated to provide useful markers for assessment of genetic diversity within flax germplasm collections. We used nine previously selected anchored ISSR primers for fingerprinting of 53 flax cultivars or genotypes and obtained 62 scorable bands, from which 45 bands (72.6%) were polymorphic. An efficient separation of 53 flax accessions into four groups and eight subgroups was achieved using unweighted pair group method with arithmetic means (UPGMA) clustering procedure based on genetic similarity expressed by the Jaccard similarity coefficient (JSC). Clustering procedure within both groups and subgroups successfully produced smaller homogenous clusters, whereas clustering between the main four groups of flax accessions displayed only a continuous decrease of similarity with a weak clustering effect. Statistical significance of grouping and subgrouping within a cluster dendrogram was estimated by calculation of the error flag and cophenetic correlation parameter for each branch. Principal coordinates (PCO) analysis mostly confirmed the separation by UPGMA clustering. We observed a statistically significant correlation between the number of total vs polymorphic bands in ISSR patterns. A one-way analysis of variance (ANOVA) test confirmed statistically significant differences in the average thousand seed mass (TSM) between eight subclusters of flax accessions from an ISSR-PCR-based UPGMA dendrogram, which indicate statistical correlation between flax ISSR polymorphism (the structure of ISSR-based clustering) TSM.     

Genetic diversity of mango cultivars estimated using SCoT and ISSR markers

Two molecular marker systems, SCoT and ISSR were used for identification and genetic comparison analysis of 23 mango germplasm accessions collected within Guangxi province of China. Using 18 selected SCoT primers 158 bands were generated, of which 104 (65.82%) were polymorphic. Eighteen selected ISSR primers amplified 156 bands with 87 (55.77%) being polymorphic. The cultivars of Xiang Ya Mango type and their progeny have high genetic similarity with each other. The 23 cultivars were clustered into two major groups based on the SCoT analysis and three major groups based on the ISSR analysis with UPGMA. These clusters are in accordance with their known origins and main phenotypic characteristics. Our results indicated that the SCoT analysis better represents the actual relationships than ISSR analysis, although both analyses give similar results. The results also demonstrate that the SCoT marker system is useful for identification and genetic diversity analysis of mango cultivars.     

Population structure and genetic diversity in bottle gourd [Lagenaria siceraria (Mol.) Standl.] germplasm from India assessed by ISSR markers

Genetic diversity analysis was undertaken in 42 geographically distant genotypes accessions of bottle gourd (Lagenaria siceraria) from India northeastern (14) and northern region (28) using inter-simple sequence repeat (ISSR) markers. A total of 209 amplified bands were obtained from 20 ISSR primers used in this study, of which 186 were polymorphic with 89.00 % band polymorphism. Various parameters namely, observed number of alleles, effective number of alleles, Nei’s gene diversity/heterozygosity, resolving power, Shannon’s information index and gene flow were estimated under experiment. Jaccard’s similarity coefficient matrix was generated for pairwise comparisons between individual ISSR profiles and UPGMA cluster analysis based on this matrix showed clustering into six groups. Jaccard’s coefficient of similarity values ranged from 0.409 to 0.847, with a mean of 0.628 revealing a moderate level of genetic diversity. The Bayesian model-based approach to infer hidden genetic population structures using the multilocus ISSR markers revealed two populations among the 42 genotypes. This is the first report on the assessment of genetic variation using ISSR markers in this medicinal vegetable plant, and this study of diversity analysis will be helpful in analyzing future hybrid breeding strategy and devising effective germplasm exploration and conservation strategy.     

Genetic Variability and Geographic Differentiation in Thymus daenensis subsp. daenensis, an Endangered Medicinal Plant, as Revealed by Inter Simple Sequence Repeat (ISSR) Markers

Thymus daenensis is an aromatic medicinal plant endemic to Iran. We used inter simple sequence repeat (ISSR) markers to detect genetic polymorphism in this herb using 17 T. daenensis accessions collected from different geographic regions in Iran. The 15 primers chosen for analysis revealed 256 bands, of which 228 (88.9%) were polymorphic. Jaccard’s similarity indices based on ISSR profiles were subjected to UPGMA cluster analysis. The generated dendrogram revealed two major groups. The Tc group included the accessions collected from the center of the Zagros Mountains, and the Te group was collected from the extremes of the Zagros range. A principal coordinate analysis confirmed the results of clustering. The results showed that the divergence of accessions based on the Zagros Mountains is more logical in comparison with classification on the basis of provincial borders. Gene diversity and expected heterozygosity were greater in the Tc group than in the Te group, suggesting that the germplasm collected from the center of the Zagros Mountains is more variable.     

Genetic diversity and relationship of global faba bean (<Emphasis Type="Italic">Vicia faba</Emphasis> L.) germplasm revealed by ISSR markers

Genetic diversity and relationships of 802 faba bean (Vicia faba L.) landraces and varieties from different geographical locations of China and abroad were examined using ISSR markers. A total of 212 repeatable amplified bands were generated with 11 ISSR primers, of which 209 were polymorphic. Accessions from North China showed highest genetic diversity, while accessions from central China showed low level of diversity. Chinese spring faba bean germplasm was clearly separated from Chinese winter faba bean, based on principal component analysis and UPGMA clustering analysis. Winter accessions from Zhejiang (East China), Jiangxi (East China), Sichuan (Southwest China) and Guizhou (Southwest China) were quite distinct to that from other provinces in China. Great differentiation between Chinese accessions and those from rest of the world was shown with a UPGMA dendrogram. AMOVA analyses demonstrated large variation and differentiation within and among groups of accessions from China. As a continental geographic group, accessions from Europe were genetically closer to those from North Africa. Based on ISSR data, grouping results of accessions from Asia, Europe and Africa were obviously associated with their geographical origin. The overall results indicated that the genetic relationship of faba bean germplasm was closely associated with their geographical origin and their ecological habit.     

苏州东山茶树种质资源遗传多样性的ISSR分析

利用ISSR分子标记对苏州洞庭地区的51份茶树(Camellia sinensis)种质资源进行遗传关系研究。结果表明,从12条引物中筛选出6条引物,共扩增出76个位点,其中多态性位点70个,占92.11%。51份茶树种质资源遗传相似性(GS)变化范围0.37～0.89;其中白沙和东灵1号GS值最大、遗传相似程度最高、遗传距离最近。通过类平均聚类(UPGMA)法,可将51份材料分为2个大类,每一大类又分为4个亚组,相同亚组下的亲缘关系较近。其中,部分来自同一品种的不同品系具有较高的遗传相似性系数。ISSR标记可有效评价苏州茶树种质的遗传多样性,为更有效地保护和利用茶树种质资源和茶树优良品种的选育提供遗传信息。     

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）。     

利用ISSR分子标记检测空间诱导罗汉果DNA突变

为探究太空环境对罗汉果造成的诱变效应,筛选罗汉果新品种培育优异种质,该研究运用ISSR分子标记技术,对28个航天诱变罗汉果及主栽品种进行了全基因组多态性检测和聚类分析。结果表明:从100个ISSR引物中筛选得到17个引物,共扩增出157个条带,其中83条具有多态性,多态条带百分率为52.87%,遗传相似系数范围为0.707~0.987。根据UPGMA聚类图,28个罗汉果样本可以分为3类:聚类Ⅰ为航天种质B6♂和B3♀;聚类Ⅱ为航天种质A1♀、A14、A18♂与主栽品种;聚类Ⅲ中都为航天罗汉果种质。上述结果暗示A1♀、A14、A18♂与其他航天种质已经产生了一定的遗传分化,具有与主栽品种相似的遗传背景,可能获得了有益突变。该研究结果为罗汉果新品种培育和杂交亲本选配提供了科学依据。     

利用ISSR和SRAP标记分析细辛资源遗传多样性与亲缘关系

采用ISSR、SRAP分子标记对61份细辛资源进行遗传多样性与亲缘关系进行分析,结果表明:(1)ISSR标记平均每条引物可获得8.35个DNA片段,多态性比率为86.3%,SRAP标记平均每对引物可获得7.85个DNA片段,多态性比率为86.0%。(2)利用相同数量的引物,ISSR标记揭示的多态性略高于SRAP标记。(3)按照种质间相似系数得出聚类图,可将所有细辛资源分开,在依据ISSR标记聚类分析中,生物学上北细辛和汉城细辛的划分,其作用不如地域来源的效应。SRAP分子标记中,大部分资源的聚类与地域性有关,但有4份汉城细辛优先聚类,SRAP分子标记在揭示基因组差异方面有一定的优势。(4)2种分子标记的聚类图中,来自同一产地的北细辛和汉城细辛优先聚类,其亲缘关系更近。聚类图中未出现北细辛与汉城细辛分别聚类。分子标记分类与传统植物学分类不一致。