Genetic Diversity Analysis of 13 Maize Inbred Lines by SSR Molecular Markers

This paper used SSR molecular markers to perform the genetic diversity analysis on 13 ordinary inbred lines of maize of different sources in order to divide heterotic groups of maize inbred line and predict heterosis. Using 12 pairs of SSR primers,a total of 47 allelic variants were detected in 13 inbred lines,2-5 alleles were detected for each pair of primers,an average of 3. 9,and polymorphism information content varied from 0. 379 to 0. 828. According to the cluster analysis,the 13 inbred lines could be divided into 5 groups.

Identification and Purity Test of Super Hybrid Rice with SSR Molecular Markers

Five super hybrid rice combinations, i.e. HYS-1/R105, Pei'ai 64S/E32, Liangyoupeijiu (Pei'ai 64S/9311), 88S/0293, and J23A/Q611, and their parental lines were tested by means of SSR analysis. A total of 144 SSR primer pairs distributed on 12 rice chromosomes were used, out of which 47 detected polymorphism among the tested rice lines. Among all these primers, RM337 and RM154 produced polymorphic patterns in four or more of the tested experimental materials respectively, and they could distinguish among most rice genotypes tested. Twenty-four primer pairs, two on each rice chromosome, were selected to make a reference SSR marker-based fingerprinting for the rice lines. For most of the primer pairs, F1 hybrids mainly showed complementary pattern of both parents, which could be very useful to distinguish the F1 from its parental lines. In addition, 5 primer pairs were selected as special primer pairs for five hybrid rice combinations respectively. By combining the rapid, simple method on DNA extraction, it is suggested that SSR technique has wide prospective in variety authentication and purity identification.

Development of Specific SSR Molecular Marker of "Huangzhou Radish" Based on Purity Identification

As an excellent local crop variety of Huanggang,"Huangzhou radish" has been widely promoted and its market influence is increasing day by day.Recently,the purity of "Huangzhou radish" has declined deeply,so it is urgent to improve and strengthen the purity and viability of "Huangzhou radish" including bad phenomena such as degeneration of varieties after self-pollination.At present,there was no SSR molecular marker can be used for genetic diversity identification of "Huangzhou radish".SSR molecular marker can provide a favorable tool to study "Huangzhou radish".In this study,"Xiakang","Hongbao"and "Huangzhou radish" were used as experimental materials,100 SSR primers were screened,and 25 pairs of SSR primers were selected.Finally,two pairs of primers were selected for identification of the purity of "Huangzhou radish" by non-denatured polyacrylamide gel electrophoresis (PAGE).The results showed that R-102 and R-112 primer pairs could amplify the special bands for "Huangzhou radish" from above three kinds of radishes.These two pairs of primers could be developed as SSR markers to identify the specificity and purity of "Huangzhou radish".Furthermore,this study provides convenient conditions for promoting the economic and social value of "Huangzhou radish".

Genetic Diversity of Jinsha Pomelo and Its Closely-related Germplasms Assessed by SSR Molecular Markers

SSR molecular markers were used to analyze the genetic diversity of 8 Jinsha pomelo germplasm and its closely-related varieties from main planting area in Jiangxi Province. A total of 92 alleles were detected from 26 pairs of selected primers with 53. 68% of polymorphism. The alleles detected per locus were ranged from 2 to 8. On average,3. 54 alleles were amplified from per pair of primers. The similarity coefficients of the 8 varieties were in the range of 0. 729-0. 924.According to the genetic similarities based on UPGMA method,all materials were divided into two groups of Jinlan pomelo and Shatian pomelo at the similarity coefficient of 0. 738.

Research Progress on Application of Molecular Markers in Breeding of Camellia oleifera

Camellia oleifera is an important woody oil tree species unique to China.It is known as the world s four major woody oil crops along with olive,oil palm and coconut.It is known as the‘king of oil’because of its high oil content.With the increase of people's attention to the yield of Camellia oleifera,its high yield has become the focus.In traditional breeding model,judgment is performed by phenotypic traits,but this method is single and easily affected by the environment,and can no longer meet the demand.In contrast,molecular marker breeding is not affected by the environment,and is stable and efficient and capable of accurately mapping target genes,so it has attracted much attention.In this paper,the research progress on C.oleifera germplasm resources diversity,DNA fingerprinting construction,genetic linkage map construction and QTL mapping was summarized,and the application of SSR molecular marker technique combined with association analysis in C.oleifera breeding in recent years was discussed,in order to provide new ideas for high-yield breeding of C.oleifera.

Databasing Molecular Identities of Sugarcane (Saccharum spp.) Clones Constructed with Microsatellite (SSR) DNA Markers

This paper reports the development of the first SSR marker-based sugarcane (Saccharum spp.) molecular identity database in the world. Since 2005, 1,025 sugarcane clones were genotyped, including 811 Louisiana, 45 Florida, 39 Texas, 130 foreign, and eight consultant/seed company clones. Genotyping was done on a fluorescence-capillary electrophoresis detection platform involving 21 highly polymorphic SSR markers that could potentially amplify 144 distinctive DNA fragments. Genotyping data were processed with the GeneMapper? software to reveal electrophoregrams that were manually checked against the 144 fragments. The presence (A) or absence (C) of these 144 fragments in any sugarcane clone was recorded in an affixed sequence order as a DNAMAN? file to represent its molecular identity being achieved into a local molecular identity database. The molecular identity database has been updated annually by continued genotyping of newly assigned sugarcane clones. The database provides molecular descriptions for new cultivar registration articles, enables sugarcane breeders to identify mis-labeled sugarcane clones in crossing programs and determine the paternity of cross progeny, and ensures the desired cultivars are grown in farmers’ fields.

The Construction of Heat-resistant Near Isogenic Line (NIL) of Bombyx mori and the Development of Molecular Marker Breeding Technique

[Objective] The study aimed to provide theoretical basis for development and application of molecular marker breeding technique to obtain Bombyx mori near-isogenic lines （NILs）. [Method] Thermotolerance gene was introduced into sensitive variety Ou17 by developing NILs and recurrent backcross,then through six generations of backcross,thermotolerance-assisted selection,and two generations of self-cross. [Result] Bombyx mori NILs carrying thermotolerance gene （new germplasm） were produced. Meanwhile,thermotolerance level of progenies of each backcross and molecular markers of NILs were determined,and then attempts were made to produce practical thermotolerance hybrids by using thermotolerance varieties whose thermotolerance gene is linked to SSR markers. [Conclusion] The study successfully construct thermotolerance NILs,monitor thermotolerance level and breeding results of progenies of each backcross,and determine molecular marker of NILs.

Molecular Diversity Analysis of Some Chilli (<i>Capsicum</i>spp.) Genotypes Using SSR Markers

Chilli belongs to the genus Capsicum which possesses enormous wealth of genetic diversity. Extent of genetic diversity determines the success level of crop improvement programme. Simple sequence repeats (SSRs) are the most widely used marker system for molecular diversity analysis especially in cultivated species. The aim of our present study was to assess the molecular genetic diversity of 20 local chilli genotypes of Bangladesh using SSR markers. Genomic DNA was extracted from young leaves and PCR reactions were performed. Eleven SSR primers were used in PCR amplification. Total 10 alleles were detected for the five polymorphic SSR loci, with a mean of 2.00 alleles per primer. Gene diversity ranged from 0.333 to 1.00 with an average of 0.567. Polymorphic Information Content (PIC) values of the SSR primers ranged from 0.255 to 0.500 with an average value of 0.371. The similarity index matrix ranged from 0.00 to 1.000. It was highest in several germplasms viz. Pop-2 vs Pop-18;Pop-3 vs Pop-5 vs Pop-19 vs Pop-20 and the lowest in the germplasm Pop-8 vs Pop-18. Dendrogram based on Nei’s genetic distance using Unweighted Pair Group Method of Arithmetic Means (UPGMA) indicated the segregation of 20 chilli genotypes into two main clusters. The SSR markers showed genetic variability in the studied pepper genotypes and they are powerful tools for estimating molecular diversity of chilli. The findings of the present study have potential applications in future breeding programme for the genetic improvement of chilli.

白三叶杂交F1代群体的表型鉴定及SSR分析

早期快速鉴定白三叶(Trifolium repens L.)F1杂交子代,获取真杂种对白三叶优良品系的培育和遗传学研究具有重要的意义。本文针对两个白三叶亲本及55个杂交F1的6个表型性状进行分析,绘制聚类热图,再选用3对特异性SSR引物鉴定杂交F1代的真实性。结果表明,在聚类热图中57个株系可以根据亲本的表型性状划分为父本型和母本型。筛选出的19对SSR引物共扩增共得到清晰可辨条带281条,多态性条带137条,多态位点占比为48.41%,每个SSR位点的PIC在18.49%~43.58%之间,平均值为34.73%。其中3对特异性引物在55个杂交后代中共鉴定出53个真杂种,真杂种比率为96.36%,与UPGMA聚类分析结果基本一致。19对SSR分子标记引物具有较高的多态性,可直接用于白三叶遗传多样性分析、杂种鉴定等相关研究,鉴定到的白三叶F1代真杂种为后续育种工作奠定重要基础。

基于SSR的云南野生猕猴桃种质资源亲缘关系分析

为探讨云南猕猴桃属种质资源的亲缘关系,采用SSR分子标记方法对70份云南野生猕猴桃种质资源的亲缘关系进行分析。UPGMA聚类分析结果表明,70份猕猴桃种质资源在遗传相似系数0.17水平上可分为4个类群,类群Ⅰ共6份材料,包括滇东南麻栗坡的中越猕猴桃MLP001和MLP010、西畴的中越猕猴桃TSH-1和TSH-4,以及滇南屏边的中越猕猴桃PB001和PB005;类群Ⅱ共31份材料,主要包括滇东北的18份材料,滇西北的3份紫果猕猴桃TC-8、TC-1、TC-10,以及5份贡山猕猴桃CJ-11、CJ-13、CJ-7、CJ-3、CJ-2;类群Ⅲ共14份材料,主要包括滇东北的10份美味猕猴桃和中华猕猴桃系列材料,滇东的JZS-5、JZS-9及JZS-7,以及滇东南西畴的黄毛猕猴桃XPS-1;类群Ⅳ共19份材料,主要包括滇东北的16份材料,滇东南西畴的京梨猕猴桃XCFD-1及革叶猕猴桃XCFD-3,果实无被毛且果皮带斑点,果实较小,与其他类群具有较远的亲缘关系。SSR分子标记反映了云南猕猴桃属70份种质资源间的遗传亲缘关系,其中一些材料按种类、资源分布地及形态学性状特征形成明显有规律的聚类关系。

黄精转录组SSR分子标记开发及种质遗传多样性分析

为丰富可用于黄精属鉴定的SSR分子标记,开发可用于黄精属(Polygonatum sp.)种质资源鉴定与遗传多样性分析的简单重复序列(simple sequence repeat,SSR)分子标记,为药材黄精正品和伪品的鉴定及遗传多样性分析提供基础。通过对3种黄精属植物进行转录组测序,从60836967个Unigenes鉴定出19630个包含1~6个碱基重复类型的SSR位点,设计和筛选获得了9对SSR有效性引物,并对来源于5个省份共计31份种质资源进行鉴定与遗传多样性分析。9对SSR引物不仅能够将长梗黄精与其他3种药材黄精划分开,还能够较好地区分不同基源黄精(滇黄精、黄精、多花黄精),并且31份资源遗传相似系数范围为0.0769~0.75。此外,构建了31份黄精属种质资源的DNA指纹图谱数据库,开发了相对应的指纹图谱。本研究结果为黄精属种质资源的分类鉴定、遗传多样性分析和品种选育提供了可用的分子标记以及参考依据。

基于SSR标记的江苏地区乌桕天然群体遗传多样性分析

目的:为江苏沿海造林所需乌桕(Sapium sebiferum)树种的保护和利用提供基础。方法:以江苏省内5个地区天然群体的146个个体为对象,选用14对SSR引物进行群体的遗传多样性和遗传结构分析。结果:基于乌桕转录组序列搜索SSR位点并设计引物,筛选出47对扩增特异性较好的SSR标记(78.33%),仅有8对引物检测到多态性产物,多态性扩增比例为13.33%。结合已公布的6对多态性SSR标记,使用14对引物对146个样本共检测出78个多态性位点,平均观测杂合度为0.6726;平均期望杂合度为0.5827;Nei基因多样度平均为0.4748;Shannon指数平均为1.1541,筛选出的14对SSR引物具有丰富的多态性。5个群体中遗传距离为0.0387~0.5193,遗传相似度为0.5950~0.9621,基因流(Nm)平均为0.836。遗传变异主要存在于群体内部,占比76.97%,23.03%的变异来自群体间。赣榆大吴山(W)群体表现出明显的遗传分化,说明该地的乌桕群体与其他地区群体有着不同来源。结论:赣榆大吴山的乌桕群体遗传多样性水平较高,并有着独特的遗传背景,应对其进行充分保护及合理利用。

基于SSR分子标记吉安地区的水稻亲缘关系鉴定分析

稻种亲缘关系分析是生产优质杂交水稻的必要条件。本研究选取均匀分布于水稻基因组12条染色体的SSR分子标记,对8份水稻样品进行SSR分子标记分析,通过聚类分析法将其归类并计算得出遗传相似系数后,对8份水稻样品的亲缘关系进行了鉴定。结果表明:所选取的8份水稻样品中,其相似系数为0.65~1.00,在遗传相似系数0.65处,8份水稻样品聚为两大类群,其中5号‘赣迟A04’单独为一类,其他水稻样品聚为一类。在遗传相似系数0.80处,可划分为三大类群:第一类囊括了6种样品,表明这6个品种亲缘关系较近,其中6号‘赣早A02’与7号‘吉安早A07’疑似同一样品,3号‘井冈山迟A03’与4号‘井冈山早A05’的亲缘关系最近,而6号、7号同时与8号‘吉安迟A09’保持有最近的亲缘关系;第二类只含有2号‘迟-2’样品株;第三类则仅有5号稻株‘赣迟A04’,说明其与其他7份水稻样品的亲缘关系最远。本研究结果为杂交水稻的应用提供重要信息。

基于转录组测序的油茶SSR、SNP和InDel位点特征分析

基于油茶转录组测序数据,利用MISA和GATK3软件对SSR、SNP和InDel位点进行搜索。结果表明:在169652条unigene序列中共发现92228个SSR位点,出现频率54.37%,平均分布距离1.61 kb。油茶转录组SSR位点中,单核苷酸和二核苷酸是主要的重复类型,A/T和AG/CT是主要的重复基元类型,基元重复次数主要集中在5~11次,基序长度主要集中在12~20 bp。共得到1912501个SNP位点,转换类型SNP数量多于颠换类型SNP数量,转换类型中A/G数量最多,而颠换类型中A/T数量最多。共筛选出298984个InDel位点。油茶转录组SSR、SNP和InDel位点数量多、类型丰富,能够为油茶分子标记开发、种质资源评价、亲缘关系鉴定等研究提供支撑。

基于SSR分子标记的枣品种鉴定及DNA分子身份证构建

【目的】利用荧光SSR分子标记对北京枣主栽品种的亲缘关系及遗传多样性分析并构建枣品种DNA分子身份证,为枣新品种选育、生产利用奠定基础。【方法】收集103个枣品种材料,筛选SSR荧光标记引物,采用多重荧光毛细管电泳检测技术分析扩增条带分子量和等位基因,获得相应的扩增带型,从而对每个枣种质材料进行标记并构建供试样品的DNA分子身份证。【结果】基于SSR分子标记技术,筛选出19对SSR引物用于103个枣品种遗传多样性分析,并筛选了7对核心基因组合构建DNA分子身份证。结果表明:19对引物对103个枣品种样品经SSR-PCR扩增后共检测到了156个等位标记点,每对引物平均8.211个,有效等位基因(Ne)变化范围为1.263~12.568,平均为3.467;Shannon’s信息指数(I)分布范围0.547~2.664,平均为1.351;多态信息含量PIC值变幅在0.32~0.917,平均值为0.603,观测杂合度(Ho)和期望杂合度(He)范围分别为0.208~0.920和0.133~0.990,Ho和He的平均值为0.639和0.637,显示出有较高的杂合度;遗传相似系数为0.85~0.98,且在相似系数为0.85处时被分为两大类。【结论】北京地区京枣31和京枣311、马牙枣和牙枣等栽培品种的遗传背景较狭窄,遗传相似度较高,不同品系间基因交流较少;京枣60、朗家园枣、北京蜂蜜罐、北京泡泡枣、京枣28等枣的亲缘关系较远,遗传多样性丰富。本研究结果为枣品种鉴定和培育新品种提供了重要依据。

基于大球盖菇基因组的SSR分子标记开发及指纹数据库应用

以13个大球盖菇菌株及其已公布的基因组为试材,采用生物信息学和试验验证相结合的方法,研究了大球盖菇基因组上的SSR类型及分布,设计了100对SSR引物开展试验验证,以期为大球盖菇的种质资源鉴定、品种选育、分子标记辅助育种等研究提供参考依据。结果表明:总计检索到6种SSR类型的2 124条序列,其中主要以三核苷酸类型为主,共计704,占SSR总数的33.15%;五、六碱基重复类型较多,但总和只占全部SSR数量的14.59%。由验证试验获得16对引物,其中引物DQGSSR020、DQGSSR031、DQGSSR077的多态性较高、特异性好、无杂峰、荧光亮度高、区分度好。同时,基于16对SSR引物进行大球盖菇DNA指纹编码构建,获得了13个大球盖菇菌株的32位数分子指纹数据库编码。

基于转录组测序的花斑裸鲤SSR、SNP和InDel位点特征分析

为利用分子标记规模化开发与辅助花斑裸鲤(Gymnocypris eckloni)良种选育,以花斑裸鲤(2+龄)的鳃、肾脏和肝脏组织为材料,经总RNA提取和cDNA文库构建后采用Illumina Novaseq 2000平台进行转录组测序,并采用MISA和GATK3软件分析转录组的SSR、SNP和插入缺失标记(InDel)位点特征。结果表明:在486221条Unigenes序列中共发现了128727个SSR,出现频率为26.47%,平均每3.76 kb出现1个SSR;花斑裸鲤SSR包括6个重复类型,以单碱基和二碱基重复基元类型为主,分别占总SSR位点数的46.53%和42.45%,重复基元类型共77种,其中,A/T和AC/GT两种基元的出现频率最高,是花斑裸鲤SSR的优势重复基元;所有重复次数中出现次数最多的为5~15次,占所有SSR位点的87.52%;通过GATK3软件搜索得到399080个SNP位点,转换类型多于颠换类型,分别占总SNP的56.29%和43.71%,转换类型中A/G发生频率略高于C/T,而颠换类型中A/T发生频率最高,C/G发生频率最低;InDel分析显示,从花斑裸鲤转录组Unigenes中共筛选出254065个InDel位点,平均每1903 bp出现1个InDel位点,且SNP位点和InDel位点均以含1个位点的Unigenes数最多。研究表明,花斑裸鲤转录组中SSR、SNP和InDel位点非常丰富,这些位点对花斑裸鲤种质资源鉴定、种群遗传学研究及保护管理具有重要价值。

菜豆EST-SSR分子标记开发及部分种质分子身份证构建

为开发菜豆高效新型分子标记,从分子水平解析菜豆重要种质的遗传多样性及亲缘关系,基于菜豆转录组数据,设计EST-SSR引物,建立EST-SSR标记系统.利用PCR筛选出多态性引物,结合毛细管电泳,分析81份菜豆种质的亲缘关系,并构建分子身份证.通过MISA软件,在菜豆转录组数据85276条非冗余序列中,共挖掘出11649个EST-SSR位点.菜豆转录组SSR标记主要重复单元为1~3个碱基,其中单碱基为主要类型,占总量的56.7%;其次是三碱基重复,占总量的21.1%.从128对EST-SSR引物中筛选出18对多态性高、重复性好的引物进行PCR扩增.供试种质的多态性信息量(PIC)为0.50~0.95,平均为0.88;遗传相似性系数为0.15~0.65,以0.35为阈值可将81份种质分为3大类,其中贵州种质主要分布于第Ⅰ,Ⅲ类,而省外品种仅分布在第Ⅱ类.利用核心引物TDc9和TDc66可以有效区分81份菜豆种质,并构建其分子身份证.研究开发的EST-SSR标记系统,可用于菜豆种质的鉴定及亲缘关系分析.

Research Progress of Molecular Markers in Genetic Diversity of Rapeseed

In recent years,with the continuous improvement and development of molecular technology in the application process,different types of DNA molecular markers have made rapid progress in the study of genetic diversity of rapeseed. The study of genetic diversity is conducive to the correct formulation of the strategy of collecting and in situ preservation of genetic resources of rapeseed,and it is the genetic basis for the improvement of rapeseed varieties. This article mainly starts with the three DNA molecular markers( SSR,RAPD,AFLP) widely used in the study of genetic diversity of rapeseed. By introducing the application principles and characteristics of SSR,RFPD and AFLP molecular markers,research progress of these three marker technologies in genetic diversity of rapeseed is briefly described.

基于SSR标记的紫薇分子鉴定及遗传分析

以紫薇品种Lagerstroemia‘Dynamite'(G2)、鄂薇1号(E1)、鄂薇4号(E4)以及W9互为亲本的杂交子代共40个优良单株为试材,利用14对在种内亲本间具有多态性的SSR引物对子代进行真杂种的鉴定,并利用Gene Marker、Popgene、Cervus和NTSYS等软件对紫薇亲本和子代进行遗传多样性、聚类分析、AMOVA分析和主成分分析。结果表明:(1)有38个单株被鉴定为真杂种,杂种率为95%。(2)14对引物的多态信息指数(PIC)平均值为0.5402,属于高度多态水平,群体平均等位基因数(Na)为4.5个,平均期望杂合度(He)以及Nei′s基因遗传多样性指数(H)分别为2.602 2和0.594 7,平均Shannon′s信息指数为1.107 9。(3)来源于湖北野生紫薇品种E1单独聚在一个分支;而来源于美国紫薇品种的E4、W9和G2聚在一个大的分支上,另外一个个体23有别于3个亲本G2、E4和W9,单独一个分支;群体M2的5个个体,与24(M4)和32(M5)聚在一起,总体形成了3个大的组群。其中大部分个体都与其亲本聚在同一分支,但也有部分个体单独聚成一分支,这也说明部分杂交子代发生了遗传变异,体现出较丰富的遗传多样性。(4)AMOVA分析和主成分分析都表明了不同样本个体内产生了丰富的遗传变异。综上所述,筛选出的SSR标记可以有效地鉴定紫薇种内杂种以及反映紫薇种内的遗传多样性,因此该研究为紫薇品种的分子鉴定提供科学依据,同时也为后期种质资源收集、构建核心种质以及创制种内新品种奠定了理论基础。