基于SSR标记分析大豆疫霉根腐病抗源的遗传多样性

丰富的遗传多样性可为大豆育种提供宽阔的遗传基础,本研究基于35对SSR标记,对60份东北地区大豆疫霉根腐病抗性品种进行了遗传多样性分析,共检测到189个等位基因,平均每个位点等位变异数5.4个,多态性信息含量指数(PIC)为0.1550~0.8195,平均为0.6636;遗传相似系数的变异范围为0.31~0.74。利用5对高多态性SSR引物构建了60份抗性材料的指纹图谱,这5对SSR引物构建的指纹图谱可以将60份疫霉根腐病抗性材料逐一区分开。采用NTSYS2.10基于遗传距离的聚类分析,将60份抗性材料分为7个类群,其中78.33%的抗性品种(系)的遗传相似系数在0.45~0.74间,表明遗传差异相对较窄,品种间遗传多样性水平较低。聚类分析与群体遗传结构分析结果有部分重合,均反映出不同地区的抗性材料间存在一定的渗透和交流。     

大豆品种早熟18抗疫霉根腐病基因的SSR分子标记

大豆品种早熟18是抗疫霉根腐病的有效抗源。本研究鉴定和分子标记早熟18的抗疫霉根腐病基因,以期为该品种的有效利用及分子辅助育种奠定基础。以感病大豆品种Williams与早熟18杂交建立分离群体。抗性遗传分析表明,早熟18对大豆疫霉菌抗性由1个显性单基因控制,该基因被定名为RpsZS18。SSR标记连锁分析表明,RpsZS18位于大豆分子遗传连锁群D1b上的SSR标记Sat_069和Sat_183之间,与这两个标记的遗传距离分别为10．0cM和8．3cM。RpsZS18是D1b连锁群上鉴定的第一个抗疫霉根腐病基因。     

部分耐盐小麦品种(系)SSR位点遗传多样性研究

选择有多态性的32对SSR引物对80个小麦耐盐品种(系)进行遗传差异研究,共检测出155个等位变异,平均每个位点上有4.75个等位变异;供试80份耐盐小麦品种(系)来源广泛,遗传基础丰富,表现出较高的遗传多样性,遗传相似系数范围在0.26～0.81;聚类分析结果显示,冬性小麦品种(系)聚为一大类;春性小麦品种(系)也聚为一大类;一些系谱相同或相近的品种(系)遗传相似系数较大;A、B、D基因组中SSR位点平均等位变异差异不大,以B基因组较高.     

大豆疫霉根腐病抗源筛选

由大豆疫霉菌引起的大豆疫霉根腐病是大豆生产的重要病害,该病已在我国大豆主要产区发生,并在局部地区造成较大产量损失。利用抗病品种是防治大豆疫霉根腐病最有效的方法。本研究目的是筛选大豆疫霉根腐病抗源,为病害防治和抗病品种的选育提供参考。用下胚轴创伤接种方法对120个栽培大豆品种（系）进行接种,鉴定其对10个具有不同毒力大豆疫霉菌菌株的抗性。有110个品种（系）分别抗1～10个大豆疫霉菌菌株,其中以河南大豆品种（系）对疫霉菌的抗性最丰富,安徽、湖北和山西大豆品种（系）也具有抗性多样性。120个大豆品种（系）对10个大豆疫霉菌菌株共产生57个反应型,有4个抗性反应型分别与单个抗病基因的反应型一致,有7个抗性反应型与2个已知基因组合的反应型相同,其他抗性反应型为新的类型。一些大豆品种（系）中可能存在有效的抗大豆疫霉根腐病新基因。     

安徽和黑龙江省大豆疫霉群体遗传结构的SSR分析

采用简单重复序列(SSR)的分析方法,对来自安徽和黑龙江省的大豆疫霉群体进行了遗传多样性分析。通过使用20对SSR引物对供试的83株大豆疫霉菌株进行PCR扩增,共得到109个SSR标记,全部为多态性标记,平均每对引物扩增出5.5条带。遗传变异与相似性分析表明,安徽群体具有更高的遗传变异度,安徽群体与黑龙江群体间遗传相似性较低;聚类分析显示,供试菌株在80%的相似性水平上可被区分为7个类群,且安徽群体分布于更多的聚类组中;Shannon-Wiener多样性指数也表明安徽群体的遗传多样性较黑龙江群体丰富。综合分析表明,本研究的结果不支持关于安徽的大豆疫霉可能来源于黑龙江的推测。     

河北区试小麦品种(系)DNA指纹图谱构建及遗传差异分析

采用42个SSR标记为2009-2013年河北省区域试验的70份小麦品种(系)构建DNA指纹图谱,进行遗传差异分析,为小麦品种改良和种质资源创新提供参考。结果表明,42个SSR标记在70份品种(系)中共检测到303个等位变异,单个SSR位点的平均等位变异为7.21个,PIC值平均0.69;基因多样性平均0.73,遗传相似系数变化范围为0.05-1.00,平均0.28;表明参加河北省区域试验的品种(系)间存在不同程度的遗传差异。聚类分析把70份品种(系)划分为4大类,6个亚类,表明同一育种单位或地区品种(系)遗传背景相近,应该加大外来小麦种质资源的引进和利用力度。     

黑龙江省主要栽培大豆品种(系)对大豆疫霉根腐病的多抗性评价

用下胚轴伤口接种方法接种鉴定黑龙江省60个栽培大豆品种和育成品系对5个具有不同毒力大豆疫霉菌菌株41-4、PMCl、USAR4、PSZJ6和USAR17的抗性.有50个品种(系)抗1个或1个以上茵株或表现中间类型,其中有5个、8个、16个和21个品种(系)分别对4个、3个、2个和1个菌株表现抗性或中间类型.60个品种(系)对5个菌株共产生12种反应模式,其中呈RRSSR反应类型的品种(系)可能含有Rpslα或Rpslc基因,品系农大3861可能含有Rps3c基因,呈SSSSS反应模式的品种(系)可能含有Rps7基因,或不含抗病基因;其它9种反应模式与含有已知单基因品种或单基因组合的反应模式不同,可能具有未知抗病基因.该研究结果表明,黑龙江省具有较丰富的抗大豆疫霉根腐病大豆品种(系),大部分品种(系)的抗性是有效的,可合理地用于大豆生产和抗疫霉根腐病育种.     

陕棉抗病种质及其衍生品种的遗传多样性与群体结构研究

通过72个分布于棉花全基因组的SSR标记,对54份陕棉抗病种质及其衍生品种的遗传多样性与群体结构进行了分析。结果表明:(1)54份陕棉种质间的遗传相似系数在0.733 3~0.987 2之间,其中材料间相似系数≤0.90的占11.1%,相似系数≥0.95的占55.6%,相似系数在0.90~0.95的占33.3%。(2)72个SSR标记等位基因变异的多态性信息含量(PIC值)在0.04~0.68,平均为0.33。(3)基于遗传距离的UPGMA聚类分析显示,在遗传相似系数为0.877时将54个品种分为5类,第Ⅰ类44个品种,第Ⅲ类7个品种,第Ⅱ、Ⅳ、Ⅴ类各1个品种。(4)基于数学模型的聚类和群体结构分析显示,54份种质归属于4个组群。研究认为,54份材料间遗传相似系数较大,遗传基础比较狭窄,多样性很低。     

黑龙江省主栽大豆品种遗传多样性的SSR 分析

使用合丰25等来自13个育种单位的13份大豆(Glycine max)品种对大豆20个连锁群上的100对SSR标记进行筛选, 最终保留了扩增稳定且多态性较高的43对SSR标记, 分析了黑龙江省83个主栽大豆品种的遗传多样性。结果表明, 在所有供试材料中共鉴定出等位变异157个, 每个位点2-7个, 平均为3.65个。品种间遗传相似系数为0.216-0.937, 平均为0.638 4, 表明黑龙江省大豆品种的遗传相似性较大, 故拓宽黑龙江省大豆品种的遗传基础具有重要意义。     

92份棉花资源遗传多样性的SSR分析

选用均匀分布于棉花全基因组的132个SSR标记,对精选的92个棉花品种(系)进行分析,结果表明,共扩增出494个多态性条带,每个引物平均3.69个.等位基因变异的多态性信息含量(PIC)在0.010 0～0.871 4之间,平均为0.546 6.采用NTSYS-pc软件计算品种对间的相似系数, 92个品种之间的成对相似系数平均为0.729 2±0.135 0,变幅在0.411 8～0.957 5之间,其中陆地棉种内48.94%的品种对相似系数≤0.800 0,海岛棉种内50.91%的品种对相似系数≤0.800 0,表明此自然群体的遗传基础较为宽泛.根据Jaccard's相似系数所得的UPGMA聚类图和系谱追溯的结果显示,此群体中品种的选育过程复杂,血统来源多样,存在较高程度的遗传多样性.     

新疆甜高粱种质资源遗传多样性的SSR分析

选用50对SSR引物对新疆现有72份甜高粱种质资源进行遗传多样性分析。结果表明:有20对引物在72份甜高粱种质资源中表现为多态性。共检测到91个等位基因,每对引物可检测到的等位基因数目为2～5个,平均为3.45个。多态性信息量(PIC)的变动范围为0.2859～0.6652,平均为0.5057。72份甜高粱种质间的遗传相似系数变化范围为0.2001～1.000,平均值为0.5599。UPGMA聚类分析将72份材料划分为A、B两大类群,A群包括69份材料,而A群又被分成从Ⅰ到Ⅺ共11个亚群,B群包括3份材料,农艺性状近似的大多被聚到同一类群。     

Genetic structure and a selected core set of Brazilian soybean cultivars

Soybean is one of the most valuable and profitable oil crop species and a thorough knowledge of the genetic structure of this crop is necessary for developing the best breeding strategies. In this study, a representative collection of soybean cultivars recommended for farming in all Brazilian regions was genotyped using 27 simple sequence repeat (SSR) loci. A total of 130 alleles were detected, with an average allelic number of 4.81 per locus. These alleles determined the core set that best represented this soybean germplasm. The Bayesian analysis revealed the presence of two clusters or subgroups within the whole collection (435 soybean cultivars) and the core set (31 entries). Cultivars of similar origin (ancestral) were clustered into the same groups in both analyses. The genetic diversity parameters, based on the SSR loci, revealed high similarity between the whole collection and core set. Differences between the two clusters detected in the core set were attributed more to the frequency of their ancestors than to their genetic base. In terms of ancestry, divergent groups were presented and a panel is shown which may foster efficient breeding programs and aid soybean breeders in planning reliable crossings in the development of new varieties.     

番茄栽培品种SSR标记和形态标记的遗传多样性分析

比较了SSR标记和形态标记在研究番茄栽培品种遗传多样性上的应用。用7对SSR引物检测了11个番茄栽培品种的遗传多样性,共得到53条带,每一个位点上扩增出2-9条带,平均为6条;品种间遗传相似系数在0.39-0.84之间,平均遗传相似系数为0.60。根据11个形态学性状表型值计算的遗传相似系数在0.27-0.72之间,平均遗传相似系数0.58。用UPGMA进行聚类分析,SSR标记和形态标记都可依果肉颜色和果实大小将供试材料分组,即黄色和红色果肉,樱桃小番茄和大、中果形的混合型;两种方法对番茄栽培品种遗传多样性的评价相近。     

Molecular characterization and genetic diversity analysis of soybean (Glycine max (L.) Merr.) germplasm accessions in India

Molecular characterization and genetic diversity among 82 soybean accessions was carried out by using 44 simple sequence repeat (SSR) markers. Of the 44 SSR markers used, 40 markers were found polymorphic among 82 soybean accessions. These 40 polymorphic markers produced a total of 119 alleles, of which five were unique alleles and four alleles were rare. The allele number for each SSR locus varied between two to four with an average of 2.97 alleles per marker. Polymorphic information content values of SSRs ranged from 0.101 to 0.742 with an average of 0.477. Jaccard’s similarity coefficient was employed to study the molecular diversity of 82 soybean accessions. The pairwise genetic similarity among 82 soybean accessions varied from 0.28 to 0.90. The dendrogram constructed based on genetic similarities among 82 soybean accessions identified three major clusters. The majority of genotypes including four improved cultivars were grouped in a single subcluster IIIa of cluster III, indicating high genetic resemblance among soybean germplasm collection in India.

Electronic supplementary material

The online version of this article (doi:10.1007/s12298-014-0266-y) contains supplementary material, which is available to authorized users.     

Molecular Analysis of Soybean Cultivars Differing in Response to Salinity Stress

Forty-seven soybean cultivars differing in response to sodium chloride were analyzed with 37 SSR markers for genetic diversity estimation. Thirty-two (86.5 %) out of 37 markers were polymorphic. The number of alleles ranged from 2–7 for different polymorphic markers, whereas the polymorphic information content (PIC) ranged from 0.061 to 0.793 with an average of 0.549. Average genetic similarity coefficient was 0.281. UPGMA based cluster analysis placed cultivars into five main clusters. In addition, the Mantel’s test for cophenetic correlation with r = 0.878 indicated good fit of the cultivars to a group in the cluster analysis. No clear pattern was observed between major clusters and place of release or targeted area of the cultivars. Genetically diverse cultivars were identified that could be potentially important sources of the germplasm for the development of salt tolerant cultivars in soybean.     

湖南同名地方稻资源SSR标记及表现型的比较分析

本研究以湖南种质库中保存的不同来源的同名湖南地方稻种质11组(同近名为1组)共136份为研究材料,进行SSR分子标记及农艺性状比较分析,目的是评价湖南同(近)名地方稻的遗传差异程度,为同(近)名地方稻种质资源的保存、供种以及重点利用种质遴选提供理论依据。研究结果表明,各组同名材料的表型遗传距离数值变化较大,各组最大遗传距离变幅1.25(D6/D13)~1.51(G1/G5),最小遗传距离变幅0.16(E7/E9)~0.81(B2/B11)。各组同名材料的SSR标记相似系数差异也大,最小相似系数变幅0.38~0.71,最大相似系数变幅0.86~1.00;同组内同(近)名材料交叉聚类。基于表型性状遗传距离与基于SSR标记遗传相似系数判别组内材料间遗传关系的结果有一致的,也有存在一定差异的。C8/C11、D16/D18、G1/G2、M2/M3、M2/M6、M3/M6、N2/N4、N5/N6、F2/F25、P3/P4的SSR标记相似系数达0.95以上,而其表现型却有1~3个性状存在有统计学意义的差异,说明供试同名材料有明显变异,即使同(近)名但也都值得保存。同时也证实了24对SSR标记分析同名地方稻遗传多样性的不足。     

宁夏水稻选育品种遗传多样性和亲缘关系分析

选择31份宁夏近年来育成或审定的水稻品种(系),利用分布于12条染色体的36对SSR引物进行遗传多样性和遗传距离分析.共检测到159个等位基因,品种间不同位点等位基因数目不等,平均4.4个.Nei基因多样性指数变幅为0.031 7～0.844 4,平均为0.508 8.按育成或审定年份,把31份水稻分为3组,SSR分析...     

Evaluation of Genetic Diversity in Chinese Wild Apple Species Along with Apple Cultivars Using SSR Markers

China, one of the primary centers of genetic diversity for the genus Malus, is very rich in wild apple germplasm. In this study, genetic diversity in 29 Malus accessions, including 12 accessions from 7 Chinese Malus species, 4 Chinese landraces, and 13 introduced apple cultivars, was assessed using a set of 19 single-locus simple sequence repeat (SSR) markers distributed across all 17 linkage groups of the apple genome. The number of alleles detected at each locus ranged from 2 to 11, with an average of 5.3 per SSR marker. In some accessions, 16 unique alleles were identified. Ten out of these 16 unique alleles (62.5%) were detected exclusively in wild species, indicating that these Chinese wild apple species have considerable genetic diversity and can be used in breeding programs to increase the genetic diversity of apple cultivars. Using 19 SSRs, an unweighted pair-group method with arithmetic average cluster analysis was conducted, and the resulting dendrogram revealed that all cultivars, except for E??peMeBckoe, were clustered together in the same group. The Russian cultivar E??peMeBckoe was closely related to the Chinese crabapple Baihaitang (M. prunifolia), with a high similarity coefficient value of 0.94. Of the two M. sieversii accessions used, one accession showed a close relationship to apple cultivars, while the other accession was closely related to wild apple species, suggesting the presence of a wider genetic diversity in Chinese M. sieversii species. The influence of SSR marker selection on genetic diversity analysis in this Malus collection was also discussed.     

吉林省大豆育成品种的遗传多样性特点分析

利用SSR分子标记技术对吉林省近年来新育成的56份大豆品种进行遗传多样性分析,以来自其他14个省份的16份大豆育成品种为对照,结果表明,吉林省育成品种15个SSR位点的等位变异数和特异等位变异数(76,12)均低于省外品种(78,18)。吉林省育成品种的遗传多样性指数(0.63,1.23)均极显著低于省外品种(0.76,1.55)。聚类分析与主成分分析结果都表明,四川省、山西省和内蒙古自治区的育成品种与其他品种的遗传距离较远。通过对不同年份平均遗传相似系数的比较,明确大豆育成品种的遗传基础的发展趋势,表明吉林省育成品种的遗传基础与省外品种相比,遗传变异较少,遗传基础较狭窄,应不断引入外省遗传变异大且亲缘关系较远的品种以拓宽其遗传基础。