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1.
为了开发铁皮石斛EST-SSR分子标记,利用SSRIT软件对铁皮石斛近缘物种-金钗石斛的15 383条EST序列进行SSR位点查找,利用Primer 5和Oligo 7软件进行引物设计和评价,之后经PCR扩增和琼脂糖凝胶电泳对引物进行初步筛选,并通过聚丙烯酰氨凝胶电泳对所筛选的引物进行有效性检测。结果表明,SSRIT软件共查找到370条SSR位点序列,共有379个SSR位点,候选SSR位点出现的频率为2.46%。二核苷酸、三核苷酸和六核苷酸重复是最主要的重复类型,分别占41.42%、26.91%和27.44%,其中二核苷酸重复中AG/CT(20.84%)和GA/TC(18.73%)最丰富;三核苷酸重复中TCT/AGA(4.22%)和GA/TC(3.96%)最丰富;而六核苷酸重复基元较多。EST-SSR平均长度为24 bp,平均每8.5条EST序列包含1个SSR位点。设计的106对EST-SSR引物中有50对能扩增出理想的PCR产物,引物有效扩增率为47.17%,其中有43对能够扩增出多态性条带,占可扩增引物的86%。本研究开发的43对引物为铁皮石斛遗传多样性分析、种质鉴定、遗传图谱构建和功能基因研究等提供了重要的参考价值。 相似文献
2.
为了明确菠菜EST序列中SSR的总体特点,开发菠菜EST-SSR引物;为利用EST-SSR引物进行菠菜性别相关特异序列的克隆奠定基础,本文从NCBI上获得1093条EST,利用在线软件SSRIT检测所含SSR序列,并进行分析。共检索出68条SSR序列,分布于64条EST中,检出率为6.22%,包括22种重复基元。其中二核苷酸重复基元的EST-SSR占主导地位,占总SSR数目的32.3%。利用在线引物设计软件Primer3.0设计了7对EST-SSR引物,在适合的PCR反应体系下,分别以雌、雄菠菜DNA基因组为模板,对设计的EST-SSR引物进行筛选,结果显示以EST序列HS097148设计的一对引物从菠菜雌雄基因组中扩增出一条雄性特异的条带,表明通过菠菜EST-SSR引物获得菠菜性别相关特异序列是可行的。 相似文献
3.
本文利用从NCBI下载的21590条银杏EST序列,分析了银杏(表达序列标签微卫星)EST-SSR在银杏EST序列的分布和比较了在不同长度EST序列中的SSR特性。在剔除冗余和低质量序列后,得到总长为5708.385kb的无冗余EST序列7961条,发现了405个EST序列(5.09%)含有475个SSR,长度400~1000bp的EST序列含SSR位点数为445个,占SSR总数的93.68%。二核苷酸和三核苷酸基元类型是银杏EST-SSR的主要类型,分别占SSR总数的73.89%和24.00%,最常见的SSR基元是:(AT)n、(AG)n、(AC)n、(AAG)n和(AAT)n。通过对银杏EST序列中SSR位点信息的发掘分析,为有针对性地设计EST-SSR引物,开发银杏EST-SSR分子标记奠定基础。 相似文献
4.
人参EST-SSR标记的建立 总被引:3,自引:0,他引:3
从7055条人参EST序列中共搜索出791个SSR。根据引物设计标准,设计了68对EST-SSR引物。在合适的PCR反应体系下,分别以人参品种集安长脖、抚松二马牙的DNA为模板,对设计的EST-SSR引物进行筛选,发现有43对EST-SSR引物能扩增出产物。在9个人参品种、2个西洋参品种和2个刺五加品种中进一步对这些可扩增的引物对进行多态性检测,发现有26对引物显示多态性,占可扩增引物的60.47%,占设计引物总数的38.23%。本研究结果表明,根据人参EST建立EST-SSR标记是一种行而有效的的方法。 相似文献
5.
为了解人参属植物EST中SSR分布特点及其在三七SSR标记中的应用,利用生物信息学方法,用primer3软件对dbEST数据库中人参属植物人参、西洋参和三七的EST序列进行搜索,发现人参属植物EST-SSR出现频率为11.54%,平均每4.39kb出现1个SSR。人参属植物单核苷酸重复基元占主导地位,其次为三核苷酸重复基元和二核苷酸重复基元,分别占总SSR的54.48%、17.31%和16.36%。人参属EST-SSR的优势类型为A/T和AT/TA,分别占54.73%和8.21%。根据人参属植物EST中的SSR设计48对引物,在合适的PCR扩增体系下,用5个三七样品的DNA为模板进行PCR扩增,引物有效扩增率85.42%,其中多态性引物占可扩增引物的70.73%。结果表明,利用人参属EST序列开发三七EST-SSR标记是可行的。 相似文献
6.
竹类植物EST-SSRs分布特征及应用 总被引:2,自引:0,他引:2
本研究利用毛竹已有的EST序列,开发竹类植物EST-SSR标记,旨在对竹子的分子分类进行研究。通过对3087条毛竹(Phyllostachys pubescens)EST序列进行筛选,获得了408条含有SSR的毛竹EST,在所有的EST-SSR中,三核苷酸重复类型(49.75%)最多,其次是二核苷酸重复类型(43.14%)、五核苷酸重复类型(4.41%)、四核苷酸重复类型(1.72%)和六核苷酸重复类型(0.98%)。不同基序类型中,GAG/CTC基序和AG基序分别是三核苷酸重复类型和二核苷酸重复类型中含量最高的重复基序,分别占18.72%和71.02%。当SSR长度等于18bp时,所检测到的SSR数量最多,达140条。随着SSR长度的增加,所检测到的SSR数量呈下降的趋势。根据搜索出的EST序列,共设计出25对引物,对12个竹类植物进行了扩增效率、多态性及通用性检测。其中18对引物能够扩增出稳定且清晰的条带,16对引物扩增具有多态性,扩增片段长度主要集中在100~500bp,引物有效率达64%。依据扩增结果进行遗传相似性分析,12种竹类植物可分为两大类群:丛生竹类群(clump bamboos)和散生竹类群... 相似文献
7.
为开发菊花EST-SSR标记并用于万春菊资源分析,研究了菊花的EST-SSR特征、标记开发及其在万寿菊上的可转移性。结果表明,菊花EST-SSR出现频率为5.35%,平均每10.64 kb存在1个SSR位点。在这些SSR位点中,共有83种重复基元,2-6核苷酸重复类型分别为10、40、14、5和14种。以14个菊花品种DNA为模板,22对菊花EST-SSR引物中14对可以扩增到清晰且稳定的PCR产物,共检出49个位点,平均每对引物可扩增出3.5条多态性片段,平均多态性信息含量(PIC)为0.751。在14对有效引物中,8对可以在待检万寿菊样品中扩增到清晰稳定的条带,可转移率为57.14%。综上所述,菊花以三核苷酸重复类型占主导,六核苷酸重复类型高于其它植物种类,菊花EST-SSR引物多态性信息含量处于较高水平。本研究可为万寿菊分子标记辅助育种奠定科学基础。 相似文献
8.
根据本实验室已获得的荔枝果皮cDNA文库EST序列,通过SSRIT在线检索,从3391条EST序列中,发现305条含有SSR,占整个文库EST的8.99%。利用SSR-ESTs序列共设计100对EST-SSR引物,其中62对在荔枝上有扩增产物,50对有扩增多态性,即具有一定的通用性。接着从96份荔枝种质中选取12个品种的基因组DNA,开展核心引物筛选,共筛选出多态性较好的EST-SSR分子标记30个;这30个EST-SSR分子标记在96份资源共扩出284条带,不同引物的扩增条带在3~18条之间,平均9.47条,其中有282条为多态性带,多态率高达99.30%,每对引物的Nei's基因多样度范围为0.186~0.396,香农信息指数范围为0.318~0.558;此外,系统聚类分析结果表明,在相似系数0.5525处,可将96份荔枝种质资源分成了8大类群,该8大类群基本与其生态类型和植物学性状特征相符。在此基础上,还对荔枝的主栽品种和特殊种质进行鉴别,结果表明,该30个EST-SSR分子标记在不同品种间可产生较清晰可辨的多态性差异,为荔枝品种以及种质资源鉴别和鉴定的分子指纹的构建奠定了良好基础。 相似文献
9.
换锦花EST-SSR标记开发及遗传多样性分析 总被引:2,自引:0,他引:2
为开发换锦花EST-SSR标记和分析其遗传多样性,本研究利用MISA软件对换锦花转录组信息进行SSR位点检测,再利用Primer3.0设计引物,经PCR扩增和非变性聚丙烯酰胺凝胶电泳检测引物的有效性和多态性,并绘制换锦花种质资源的聚类图。结果表明,共检测到9 918个SSR位点,发生频率为18.59%,分布距离为3.729 kb;SSR位点重复单元为1~3个碱基,其中,单碱基重复三碱基重复二碱基重复,分别占SSR总数的61.08%、23.22%和14.23%,四碱基及以上重复单元相对较少。共设计出9 302对SSR引物,随机选取并合成278对引物进行PCR扩增,能够清晰扩增出的引物有185对(66.55%),在石蒜属的七个种中具有多态性的有59对(31.89%),其中11对(18.64%)能够在浙江和江苏种群的30份换锦花种质资源表现出丰富的多态性。综上,本研究开发的EST-SSR标记具有丰富的多态性,在换锦花以及石蒜属植物的遗传多样性分析、杂交种鉴定及遗传图谱的构建应用中具有重要意义。 相似文献
10.
大白菜表达序列标签SSR标记分析* 总被引:18,自引:2,他引:18
对大白菜(Brassica campestris L.ssppekinensis)13007个EST序列进行拼接共得到7714个片段重叠群(contig),其中10.4%(890个)非冗余EST含有SSR标记(EST-SSR),标记间平均间隔距离为3.9kb,单、双和三核苷酸重复序列大约各占1/3左右。CDS所包含的三核苷酸重复序列最多,而且AAG/CTT重复序列的含量最高。通过同源性比较分析,获得功能已知的SSR-ESTs774个,共计含有846个SSR,其中50.2%位于5'-UTR,31.4%位于3'-UTR,18.4%位于CDS。实验选取123个SSR座位设计引物,利用芜菁花叶病毒(Turnip mosaic virus,TuMV)的高抗和高感大白菜F6代自交系材料各2份,分析EST-SSR标记多态性。结果表明,其中37个标记可进行有效扩增,但是没有表现出多态性,23个标记(18.7%)至少在1份材料中具有多态性。对这些EST-SSR标记在大白菜和其它芸薹属植物的系统发育关系分析、遗传作图和基因定位的应用进行了讨论。 相似文献
11.
核桃EST-SSR标记的开发 总被引:4,自引:1,他引:3
从GenBank数据库上公布的5025条核桃(Juglans regia)EST序列中,用SSRHunter软件搜索到485条EST序列中含有540个SSR,SSR出现频率为10.75%,SSR-ESTs检出率为9.7%。利用检出的SSR-ESTs序列设计SSR引物43对,对6个核桃样品、1个黑核桃(J. nigra)样品和1个核桃楸(J. mandshurica)样品进行了PCR扩增,其中40对引物有扩增带,占设计引物的93%,35对引物有多态性,占可扩增引物的87.5%。在有多态性的35对引物中,27对引物在核桃种内有多态性;8对引物在核桃种内无多态性,而在核桃、核桃楸和黑核桃种间有多态性。应用UPGMA方法对检测样品进行聚类分析,结果与传统分类一致。 相似文献
12.
Genetic variation present in wild and cultivated barley populations was investigated using two sources of microsatellite also
known as simple sequence repeat (SSR) markers. EST-SSRs are derived from expressed sequences and genomic SSRs are isolated
from genomic DNA. Genomic SSR markers detected a higher level of polymorphism than those derived from ESTs. Polymorphism information
content was higher in genomic SSRs than EST-derived SSRs. This study showed that the EST-SSR markers developed in cultivated
barley are polymorphic in wild and cultivated varieties and produced high quality markers. Ten of these functional markers
were polymorphic across the accessions studied. EST markers indicated clearer separation between wild and cultivated barley
than genomic SSRs. The EST-SSRs are a valuable source of new polymorphic markers and should be highly applicable to barley
genetic resources, providing a direct estimate of functional biodiversity. 相似文献
13.
Lihua Yao Xiaoyan Zheng Danying Cai Yuan Gao Kun Wang Yufen Cao Yuanwen Teng 《Genetic Resources and Crop Evolution》2010,57(6):841-851
A total of 8117 suitable SSR-contaning ESTs were acquired by screening from a Malus EST database, among which dinudeotide SSRs were the most abundant repeat motif, within which, CT/TC followed by AG/GA were
predominant. Based on the suitable sequences, we developed 147 SSR primer pairs, of which 94 pairs gave amplifications within
the expected size range while 65 pairs were found to be polymorphic after a preliminary test. Eighteen primer pairs selected
randomly were further used to assess genetic relationship among 20 Malus species or cultivars. As a result, these primers displayed high level of polymorphism with a mean of 6.94 alleles per locus
and UPGMA cluster analysis grouped twenty Malus accessions into five groups at the similarity level of 0.6800 that were largely congruent to the traditional taxonomy. Subsequently,
all of the 94 primer pairs were tested on four accessions of Pyrus to evaluate the transferability of the markers, and 40 of 72 functional SSRs produced polymorphic amplicons from which 8
SSR loci selected randomly were employed to analyze genetic diversity and relationship among a collection of Pyrus. The 8 primer pairs produced expected bands with the similar size in apples with an average of 7.375 alleles per locus. The
observed heterozygosity of different loci ranged from 0.29 (MES96) to 0.83 (MES138), with a mean of 0.55 which is lower than 0.63 reported in genome-derived SSR marker analysis in Pyrus. The UPGMA dendrogram was similar to the previous results obtained by using RAPD and AFLP markers. Our results showed that
these EST-SSR markers displayed reliable amplification and considerable polymorphism in both Malus and Pyrus, and will contribute to the knowledge of genetic study of Malus and genetically closed genera. 相似文献
14.
Xiao-Ping Jia Yun-Su Shi Yan-Cun Song Guo-Ying Wang Tian-Yu Wang Yu Li 《Genetic Resources and Crop Evolution》2007,54(2):233-236
The development of EST-SSR in foxtail millet (Setaria italica) for polymorphism and transferability study was reported here. From 1213 EST sequences, 30 SSRs were obtained and primers
were designed for 26 SSRs. Among them, four pairs of SSR primers amplified polymorphic products in 12 foxtail millet cultivars
and one accession of Setaria viridis, a wild relative of foxtail millet, with 10 alleles detected for the four loci and 2.5 alleles per locus. In addition, ten
SSR markers could be transferred to other nine Gramineae species. The putative functions of 11 ESTs containing polymorphic
and transferable SSRs were also identified. 相似文献
15.
用鲤鱼EST-SSRs分子标记分析长江黑龙江鲤种群结构 总被引:4,自引:0,他引:4
从鲤鱼ESTs的数据库(10691个)中进行微卫星序列筛选,共发现微卫星序列127个,占整个ESTs数据库的1.19%,另外从本研究室构建的鲤鱼脑组织cDNA文库中筛选到微卫星序列20个。根据筛选得到的微卫星序列设计引物68对,合成引物40对,其中27对引物能够获得预期的目的片段,20对引物在所检测的群体内及群体间表现出多态性。用此20个多态性标记分析了长江鲤和黑龙江鲤的群体遗传结构,结果表明:长江鲤和黑龙江鲤在多数位点表现出较高的遗传多样性,20个位点的平均有效等位基因数分别为3.9135、3.4820;平均观察杂合度为0.6067、0.5667;平均期望杂合度为0.6737、0.6194;平均多态信息含量为0.6308、0.5714。长江鲤的遗传结构好于黑龙江鲤,两个群体的Hardy-Weinberg偏离指数较小,群体基本保持平衡,群体结构较合理;其中HLJE1、HLJE10位点在长江鲤和黑龙江鲤的扩增结果相差较大,长江鲤的多态性明显高于黑龙江鲤,位点多态信息含量相差一倍以上,可用于群体的鉴别。 相似文献
16.
Nahla V. Bassil B. Gilmore J. M. Oliphant K. E. Hummer J. A. Henning 《Genetic Resources and Crop Evolution》2008,55(7):959-969
Eight genic SSR loci were evaluated for genetic diversity assessment and genotype identification in Humulus lupulus L. from Europe and North America. Genetic diversity, as measured by three diversity indices, was significantly lower in European
cultivars than in North American wild accessions. Neighbor Joining cluster analysis separated the hop genotypes into European
and North American groups. These eight SSRs were useful in uniquely identifying each accession with the exception of two sets
of European landraces and a pair of Japanese cultivars, ‘Shinshuwase’ and ‘Kirin II’. An accession from Manitoba grouped with
the European (EU) cluster reflecting the group’s genetic similarity to older Manitoba germplasm used to develop ‘Brewer's
Gold’ and the gene pool arising from this cultivar. Cultivars grouped closely with one of their immediate parents. ‘Perle’
grouped with its parent ‘Northern Brewer and ‘Willamette’ grouped with its parent ‘Fuggle H’. Wild American accessions were
divided into two subgroups: a North Central group containing mostly H. lupulus var. lupuloides and a Southwestern group containing H. lupulus var. neomexicanus accessions. These eight SSRs will be valuable for genotype identification in European and wild American germplasm and may
potentially prove useful for marker-assisted selection in hop. PCR products from four previously reported primer pairs that
amplify the same intronic SSR regions as do the genic SSRs in this study were compared in eight common cultivars. Different
primer pairs generated robust markers at the chs2 and chi loci. However, only the HLC-004B and HLC-006 primer pairs amplified successfully at the chs3 and chs4 loci.
Electronic supplementary material The online version of this article (doi:) contains supplementary material, which is available to authorized users. 相似文献