广西梨种质资源遗传多样性和群体结构分析
S661.2; [目的]阐明广西地方梨种质的遗传多样性、亲缘关系及群体结构,加快梨种质的鉴定、评价和保护,促进地方优质梨种质资源的合理有效利用,助推品种改良和种质创新.[方法]利用筛选获得的15个SSR分子标记对71份广西地方梨种质和48份外地梨种质进行遗传多样性和群体结构分析.[结果]共检测出190个等位基因(Na),平均等位基因数(Na)为12.667,平均有效等位基因数(Ne)为5.454,位点多态性信息指数(PIC)平均值为0.762,较好地揭示了梨的遗传多样性;观测杂合度(Ho)和期望杂合度(He)平均值分别为0.682和0.788,说明梨群体内存在近缘交配;香农指数(I)平均值为1...
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          | Published in | 果树学报 Vol. 41; no. 3; pp. 379 - 391 | 
|---|---|
| Main Authors | , , , , , , | 
| Format | Journal Article | 
| Language | Chinese | 
| Published | 
            广西桂北特色经济作物种质创新与利用重点实验室·广西特色作物研究院,广西桂林 541004%江苏省梨工程研究中心·南京农业大学园艺学院,南京 210095
    
        2024
     | 
| Subjects | |
| Online Access | Get full text | 
| ISSN | 1009-9980 | 
| DOI | 10.13925/j.cnki.gsxb.20230416 | 
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| Abstract | S661.2; [目的]阐明广西地方梨种质的遗传多样性、亲缘关系及群体结构,加快梨种质的鉴定、评价和保护,促进地方优质梨种质资源的合理有效利用,助推品种改良和种质创新.[方法]利用筛选获得的15个SSR分子标记对71份广西地方梨种质和48份外地梨种质进行遗传多样性和群体结构分析.[结果]共检测出190个等位基因(Na),平均等位基因数(Na)为12.667,平均有效等位基因数(Ne)为5.454,位点多态性信息指数(PIC)平均值为0.762,较好地揭示了梨的遗传多样性;观测杂合度(Ho)和期望杂合度(He)平均值分别为0.682和0.788,说明梨群体内存在近缘交配;香农指数(I)平均值为1.876,反映梨群体的遗传多样性丰富.广西地方种质的平均等位基因数为11.53,平均有效等位基因数为5.606,香农指数(I)为1.894,均高于外地种质,说明广西地方种质的遗传多样性更丰富.聚类分析显示大部分广西地方种质与外地种质的亲缘关系较远,隶属两个不同类群,但二者存在少量的相互交叉,少数的广西梨和外地梨聚为一类,有较近的亲缘关系.群体遗传结构分析也表明大部分广西梨和外地梨的遗传结构差异较大,并且2个居群的近交系数(Fis)均值都大于0,存在近缘交配.进一步研究发现,71份广西地方种质聚为3个类群,从群体遗传结构上可划分为4个不同群体,但群体间未表现明显的区域分化特征.分子方差分析结果表明,供试梨种质的变异主要来源于个体内,群体间和个体间的遗传分化程度较低,应关注对群体内个体的选择和保护.[结论]广西地方梨种质遗传多样性相对丰富,居群内普遍存在近缘交配,没有明显的区域分化特征,其遗传背景和外地一些栽培种或杂交种差异较大,建议加强对广西地方梨种质的保护和利用. | 
    
|---|---|
| AbstractList | S661.2; [目的]阐明广西地方梨种质的遗传多样性、亲缘关系及群体结构,加快梨种质的鉴定、评价和保护,促进地方优质梨种质资源的合理有效利用,助推品种改良和种质创新.[方法]利用筛选获得的15个SSR分子标记对71份广西地方梨种质和48份外地梨种质进行遗传多样性和群体结构分析.[结果]共检测出190个等位基因(Na),平均等位基因数(Na)为12.667,平均有效等位基因数(Ne)为5.454,位点多态性信息指数(PIC)平均值为0.762,较好地揭示了梨的遗传多样性;观测杂合度(Ho)和期望杂合度(He)平均值分别为0.682和0.788,说明梨群体内存在近缘交配;香农指数(I)平均值为1.876,反映梨群体的遗传多样性丰富.广西地方种质的平均等位基因数为11.53,平均有效等位基因数为5.606,香农指数(I)为1.894,均高于外地种质,说明广西地方种质的遗传多样性更丰富.聚类分析显示大部分广西地方种质与外地种质的亲缘关系较远,隶属两个不同类群,但二者存在少量的相互交叉,少数的广西梨和外地梨聚为一类,有较近的亲缘关系.群体遗传结构分析也表明大部分广西梨和外地梨的遗传结构差异较大,并且2个居群的近交系数(Fis)均值都大于0,存在近缘交配.进一步研究发现,71份广西地方种质聚为3个类群,从群体遗传结构上可划分为4个不同群体,但群体间未表现明显的区域分化特征.分子方差分析结果表明,供试梨种质的变异主要来源于个体内,群体间和个体间的遗传分化程度较低,应关注对群体内个体的选择和保护.[结论]广西地方梨种质遗传多样性相对丰富,居群内普遍存在近缘交配,没有明显的区域分化特征,其遗传背景和外地一些栽培种或杂交种差异较大,建议加强对广西地方梨种质的保护和利用. | 
    
| Abstract_FL | [Objective]Pear,one of the most economically important temperate fruit trees,belongs to the genus Pyrus.China is one of the origin centers of Pyrus plants with a wide range of germplasm re-sources and has a long history of cultivation.As one of the important producing areas in southern Chi-na,pear cultivation area and production of Guangxi were 2.1 × 104 hm2 and 5.08 × 105 tons in 2022,re-spectively.There is a rich wild pear germplasm resources in Guangxi according to the previous investi-gation.However,the understanding of the genetic diversity and population structure of the pear resourc-es in Guangxi is still limited.It is of great significance for accelerating the identification,evaluation and conservation of the pear germplasm,and promoting the effective utilization of the local high-quality pear germplasm resources by clarifying the genetic diversity,population structure of the local pear germplasms in Guangxi,as well as its relationship with the nonlocal germplasms.[Methods]A total of 119 pear cultivars and landraces were collected and subjected to analyze the genetic diversity and the population structure using 15 pair of SSR primers reported in previous research.The genomic DNA was extracted by genomic DNA extraction kit of magnetic bead method,and the purity concentration and in-tegrity of the extracts were assessed by NanoDROP and agarose gel electrophoresis.A 10 μL PCR sys-tem was adopted,including 5.0 μL of 2×Taq PCR Master Mix,0.5 μL of each of forward and reverse primers(10 pmol·μL-1),1.0 μL genomic DNA(20 ng·μL-1),and 3.0 μL of ddH2O.The DNA was ampli-fied according to the molecular weight records using capillary electrophoresis technology.According to the polymorphic bands,the data matrix was obtained.The number of alleles(Na),the number of effec-tive alleles(Ne),the Shannon information index(I),the expected heterozygosity(He),the observed het-erozygosity(Ho),the polymorphic information content(PIC),and the inbreeding coefficient(Fis)were calculated using GenAlEx version 6.501 software.The Nei's genetic distance among between 119 ac-cessions of the germplasm resources were calculated using Powermarker software.The UMPGA cluster trees of the 119 pear germplasm resources based on the Nei's genetic distance were constructed using MEGA7.0 software.The genetic structure analysis of the populations of pear was performed using STRUCTURE 2.3.4 software.The population number(K)was set to 1-20.Each K value was simulated 20 times,and the Markov Chain Monte Carlo(MCMC)was set 100 000 times.Finally,the optimal △K value was calculated using the online tool STRUCTURE HARVESTER.The genetic linkage map was constructed using CLUMMP and DISTRUCT software.The principal coordinate analysis(PCoA)was accomplished using GenAIEx software.[Results]A total of 190 alleles were detected in the pear germ-plasm resources by the 15 polymorphic SSR markers.The average number of alleles was 12.667.The average effective allele per SSR marker was 5.454.The average polymorphic information content(PIC)was 0.762.These results showed that there was a relatively high genetic diversity within this popula-tion.The average observed heterozygosity(Ho)and expected heterozygosity(He)were 0.682 and 0.788,respectively,suggesting that the presence of inbreeding would exist within the pear population.The average Shannon information index(I)was 1.876,reflecting that there was a high genetic diversity in the local pear population.Compared with the nonlocal germplasms,the genetic diversity of the local pear was higher with an average allele of 11.53,an average effective allele of 5.606,and a Shannon in-formation index(I)of 1.894.The cluster analysis showed that the majority of the local germplasms in Guangxi and nonlocal germplasms were divided into two different groups,with a distant genetic rela-tionship.The analysis of population genetic structure also indicated that there was a significant differ-ence in the genetic structure between the majority of the local germplasms in Guangxi and the nonlocal germplasms.The Fis mean values of the two populations were over 0,indicating that there would be in-breeding within the population.Further research found that the 71 local germplasms in Guangxi were clustered into three groups,which could be divided into four different populations based on population genetic structure.However,there were no obvious regional differentiation characteristics between the populations.The result of the analysis of molecular variance(AMOVA)indicated that the genetic varia-tion in the pear germplasms mainly occurred within individuals,while the genetic differentiation be-tween the populations and individuals was relatively small.[Conclusion]The fifteen SSR primers had the characteristics of clear amplification results,good repeatability and high polymorphism,and would be suitable for pear germplasm identification,genetic linkage map construction,genetic diversity,and molecular marker-assisted breeding.Furthermore,the genetic diversity of the local pear germplasms in Guangxi was relatively rich.There would be a general inbreeding and no obvious regional differentia-tion within the populations,and the genetic background differed greatly from some cultivars or hybrids of nonlocal pear.Therefore,we proposed to strengthen the conservation and utilization of the local pear germplasm in Guangxi. | 
    
| Author | 齐开杰 易显荣 徐志美 刘珊廷 周民武 吴潇 赵碧英  | 
    
| AuthorAffiliation | 广西桂北特色经济作物种质创新与利用重点实验室·广西特色作物研究院,广西桂林 541004%江苏省梨工程研究中心·南京农业大学园艺学院,南京 210095 | 
    
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| Author_FL | LIU Shanting QI Kaijie YI Xianrong WU Xiao ZHAO Biying XU Zhimei ZHOU Minwu  | 
    
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| Keywords | Pear 遗传多样性 Guangxi SSR markers 梨 Population structure Genetic diversity 广西 SSR分子标记 群体结构  | 
    
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