共查询到20条相似文献,搜索用时 15 毫秒
1.
柑橘CAPS 标记和AS-PCR 引物的开发 总被引:1,自引:0,他引:1
以从GenBank中下载的93 955条甜橙[Citrus sinensis(L.)Osbeck]EST序列为源序列,利用QualitySNP软件包从中挖掘出1 521个单核苷酸多态性(single nucleotide polymorphism,SNP)候选位点。进一步利用酶切位点查找软件WatCut进行分析,发现其中125个SNP为酶切扩增多态性序列(cleaved amplified polymorphic sequences,CAPS)位点。随机挑选40个CAPS候选位点设计引物,对12个含多种类型的柑橘品种进行分型,以此验证各标记的有效性。同时,还挑选了25个经生物信息学预测可导致其编码蛋白氨基酸序列改变的SNP位点,分别设计出一组等位基因特异PCR(allele specific PCR,AS-PCR)引物,以6个不同类型柑橘品种的DNA为模板进行PCR扩增,扩增产物采用琼脂糖凝胶电泳进行检测,筛选多态性引物。结果显示,40个CAPS候选位点中有26个位点具有酶切扩增多态性,且分型结果稳定,可作为CAPS标记。此外,还筛选获得15组在不同柑橘品种间检测到多态性的AS-PCR引物,重复性好,可有效用于柑橘品种的SNP分型。 相似文献
2.
甘蓝显性雄性不育基因的延长随机引物扩增DNA(ERPAD)标记 总被引:10,自引:2,他引:8
获得了一个与甘蓝显性雄性不育基因连锁的延长随机引物扩增DNA(ExtendedRandomPrimerAmplifiedDNA,ERPAD)标记EPT11900。EPT11900是在与甘蓝显性雄性不育基因连锁的RAPD标记OT11900的基础上,通过逐步筛选3’端延长的随机引物的方法转化而成的稳定性和特异性都得到增强的新标记。这种标记的稳定性和特异性接近SCAR标记,但不需要克隆和测序。该方法首先根据OPT11的序列合成3’端添加A、T、C、G4种碱基的4个引物,组成10个引物对。以不育池为模板筛选出OT11C+OT11G为唯一能够扩增长度与OT11900相同的一个片段的引物对。在此引物对基础上,又添加4种碱基得到8个新的引物,相互组合成16个引物对。进一步以不育池为模板筛选出OT11CT+OT11GA,在严格条件下,它可特异扩增长度与OT11900相同的一个片段EPT11900。通过分离群体分析证实这一片段与OT11900处于同一位点。 相似文献
3.
4.
通过HRM技术筛查与梨矮生性状决定位点PcDw紧密连锁的SNP标记 总被引:1,自引:0,他引:1
在果树的基因组中存在大量的SNP(single nucleotide polymorphism)位点,筛查与目标性状紧密连锁的SNP标记,对目标基因的精细定位具有重要意义。以‘矮生梨’(Pyrus communis L.‘Aishengli’)与‘茌梨’(Pyrus bretschneideri Rehd.‘Chili’)的F1杂交分离群体共215个单株为试材,参考苹果基因组的序列设计26对适合HRM分析的引物,依据分离群体分组分析(bulked segregant analysis,BSA)原理,通过高通量熔解曲线(high resolution melting,HRM)分析,筛选到两个与决定梨矮生性状的PcDw基因连锁的标记CNqau012和CNqau039,二者与目标位点的连锁距离分别是13.3 cM和2.3 cM。对CNqau012和CNqau039的扩增子测序分析表明,在矮生型与普通型中都存在一处单核苷酸变化(分别是G/A和C/T)。这些标记的获得对PcDw基因的精细定位及克隆具有重要意义。 相似文献
5.
中华猕猴桃矮型性状EST-SSR连锁标记的筛选 总被引:3,自引:0,他引:3
以中华猕猴桃(Actinidia chinensis Planch)矮型种质‘赣猕5号’为母本,普通型中华猕猴桃‘奉雄2号’为父本构建F1群体,采用优越而高效的基于表达序列标签(Expressed Sequence Tags,EST)的简单序列重复(Simple Sequence Repeats,SSR)标记技术,结合群体分离分析法(Bulked Segregant Analysis,BSA)在荧光DNA测序仪(ABI3130)上进行了‘赣猕5号’矮型性状连锁的EST-SSR分子标记研究。结果表明,通过本实验室开发并设计的85对EST-SSR荧光引物的扩增筛选,其中引物EST-Ad042在亲本及其矮型与普通型DNA 池之间扩增出一条285 bp 的多态性片段,经对其F1代分离群体部分矮型与普通型单株的随机验证,该片段稳定出现,在矮型植株中表现为有带,在普通型植株中表现为无带。遗传连锁分析表明,该标记与矮型基因之间的连锁距离为8.8 cM。EST-SSR荧光引物能够有效地筛选到中华猕猴桃的特异标记,可以作为鉴别矮型与普通型植株的标记引物。 相似文献
6.
黄瓜抗炭疽病相关基因AFLP标记的SCAR转换 总被引:2,自引:0,他引:2
将黄瓜抗炭疽病相关基因的一个共显性AFLP标记成功地转换成了简单实用的SCAR标记。对AFLP标记片段进行序列测定,根据序列特点设计了特异的SCAR引物,引物长18~21 bp。PCR结果表明,引物对(1)可以扩增出131 bp和125 bp两条带,引物对(2)可以扩增出178 bp和172 bp两条带,分别为抗炭疽病的特征带和感炭疽病的特征带。将该两个标记命名为SCEM131/125和SCEM178/172,两对引物在F2单株和抗感病材料验证中符合率高达97.27%,可以用于黄瓜炭疽病的分子鉴定。 相似文献
7.
8.
CAO Kai-yuan FU Yong-shui XU Lin YUAN Guang-qing HUANG Xiao-rong DAI Shu-qin TANG Yong-ping 《园艺学报》2003,19(10):1349-1352
AIM:To amplify from leader peptide region and obtain human monoclonal anti-D variable region gene with high specificity and affinity, and analyze the nucleotide and deduced amino acid sequences.METHODS:The total RNA was extracted from an Epstein-Barr-virus-transformed cell line secreting monoclonal anti- (rhesus D) antibody. The leader region primers containing a ribosome recognition site were designed. By using PCR method, the cDNA of human anti-(rhesus D) antibody (IgM κ) variable region gene was amplified. Cloning and subsequent sequence analysis of the variable region gene was performed. The deduced amino acid sequence was also compared and analyzed with previously published sequences.RESULTS:A band of approximate 440 and 410 base pairs were amplified using heavy chain primers and light chain primers, respectively. Sequence analysis indicated that the deduced amino acid sequence was in agreement with the characterization of the amino acid present in the human Ig variable region. CONCLUSION:The cloning and sequencing of a human anti- (Rhesus D) antibody variable region cDNA will make benefits for production of recombinant anti-(Rhesus D) antibody and prevention of Rh haemolytic disease in newborns. 相似文献
9.
对小白菜品种进行游离小孢子培养,得到9株再生植株,其中2株为单倍体,7株为二倍体,二倍体自然加倍率为77.7 %。为
避免材料间差异,取单倍体和二倍体再生植株各2株,提取单株DNA,分别构建单倍体和二倍体DNA混合池。利用甲基化敏感性限制性
内切酶-PCR法,结合SRAP分子标记技术,对2个DNA混合池进行筛选,共筛选768对引物,只有在未酶切的单倍体和二倍体DNA池中SRAP
引物扩增无差异,而酶切后有差异的条带,才认为是单倍体和二倍体甲基化差异。试验共获得8对含有多态性的引物,试验结果证明
小白菜小孢子培养获得的再生植株的倍性与基因组DNA甲基化有关。 相似文献
10.
利用SSR技术鉴定西瓜甜瓜种子纯度 总被引:1,自引:0,他引:1
利用SSR分子标记技术对西瓜‘W1806’与甜瓜‘M1805’各3个批次及其亲本间的多态性进行引物筛选和种子的纯度鉴定。结果表明,在28对西瓜的SSR引物中,有5对引物在西瓜‘W1806’的F1代与亲本之间有很好的多态性。其中BVWS00839引物特异性好,条带清晰,父母本条带间隔明显,即作为3个批次的西瓜纯度鉴定的引物,其鉴定纯度分别为99.47%、98.96%和97.92%;在18对甜瓜的SSR引物中,只有1对CMBR052引物在F1代扩出的条带为典型的双亲互补型条带,故用该引物对甜瓜进行纯度鉴定,其纯度分别为97.90%、96.80%和97.40%。与田间鉴定结果的吻合率都在98%以上。这2个材料的吻合率说明SSR分子标记技术对西瓜和甜瓜纯度鉴定结果都是可靠的。 相似文献
11.
利用SNP分析软件从辣椒(Capsicum annuum L.)251 068条Unigenes中筛选出18 159个SNP,其中有1 781个SNP位点被匹配在1 291个注释基因上,基因功能分类和代谢途径分析表明,其中有853个基因参与初生代谢(28.7%)、细胞代谢(17.3%)、生物合成过程(15.7%),另有125个(9.7%)基因序列参与新陈代谢途径,53条(4.1%)序列参与次生代谢产物合成途径,31条(2.4%)序列参与植物激素合成途径。 EST-SNP序列中4 172条(22.9%)满足设计CAPS引物条件,为了验证EST-SNP正确性,并选取了15对CAPS引物对5份辣椒材料进行扩增,结果发现有8对(53.3%)引物表现出多态性。表明筛选出这些EST-SNP标记可作为辣椒基因分型、图谱构建等的候选分子标记。 相似文献
12.
13.
苹果柱型基因Co的一个AFLP 标记的SCAR转换 总被引:15,自引:4,他引:15
将苹果柱型基因的一个AFLP 标记成功地转换成了简单实用的SCAR 标记。首先对AFLP 标记片段进行序列测定, 然后根据序列特点设计了两对特异引物CoA1/ CoA2 和CoA1/ CoA3 , 每条引物长20 bp。PCR 结果表明CoA1/ CoA2 可以扩增出216 bp 和148 bp 两条带, 其中216 bp 的为柱型性状的特征带; CoA1/CoA3 可以扩增出273 bp 和205 bp 的两条带, 其中273 bp 的为柱型性状的特征带。两对引物在杂交后代中扩增出的特征带与柱型性状的分离重组率都很低(CoA1/ CoA2 为6. 3 % ±2. 5 %; CoA1/ CoA3 为7. 3 % ±2. 6 %) , 所以它们都可以作为该SCAR 标记的特异引物所用。 相似文献
14.
本试验旨在开发一种新的设计共显性SNP标记的方法,以提高SNP标记检验的效率,并将其成功应用于番茄抗黄化曲叶病毒基因Ty-1的SNP标记开发中,提高了种质资源鉴定和育种分离世代材料筛选的效率。通过对抗病基因Ty-1和等位感病基因ty-1的cDNA序列进行比对,挑选了两个稳定扩增的多元非同义突变位点,分别用来设计Ty-1和ty-1的SNP标记NL3和NL2,将两个标记进行混合得到双重SNP标记NL2-3。通过用NL2-3检验已知的抗病和感病番茄材料,验证了其多态性和稳定性。并用NL2-3对抗感病材料的F3代杂交分离群体和普通自交系进行了Ty-1的筛选,并经过田间观察进一步验证了该标记的可靠性。此方法开发得到的双重SNP标记只需要进行一次PCR反应和一次凝胶电泳就可以区分纯合抗、杂合抗、纯合感3种基因型,提高了育种选择的效率。 相似文献
15.
基于EST信息的百合SSR标记的建立 总被引:19,自引:6,他引:13
依据已知的百合EST(expressed sequence tags)序列信息,开发新的SSR(simple sequence repeats)标记,在NCBI的EST数据库1 688 EST中检索到98条含有101个SSR的序列, SSR的检出率为5.98%,其中三核苷酸重复类型占主导地位,出现频率为2.84%。EST-SSR的重复基元共搜索到47种,其中三核苷酸重复基元类型最为丰富,大约占重复基元类型总数的一半。利用部分EST-SSRs序列共设计23对SSR引物, 以铁炮百合‘Snow Queen' DNA为模板,对引物进行筛选,其中18对引物有扩增产物,占所设计引物总数的78.26%;进一步用这些引物在5个杂种系列13个百合品种进行多态性测试,显示多态性的引物占可扩增引物的66.7%。本研究结果证明了基于百合EST信息建立SSR标记是一种有效而又可行的方法。 相似文献
16.
Li-Wang Liu Li-Ping Zhao Yi-Qin Gong Ming-Xia Wang Li-Ming Chen Jin-Lan Yang Yan Wang Fan-Min Yu Long-Zhi Wang 《Scientia Horticulturae》2008
Three molecular marker systems, RAPD (random amplified polymorphic DNA), ISSR (inter-simple sequence repeat) and SRAP (sequence-related amplified polymorphism), were employed for identification and genetic diversity analysis of 35 elite late-bolting radish cultivars. Detected by 35 RAPD primers, 22 ISSR primers and 17 SRAP primer combinations, the proportions of polymorphic bands were 85.44%, 85.2% and 85.41%, respectively, and the mean genetic similarity coefficients between pairs of genotypes were 0.781, 0.787 and 0.764, respectively. Each of the three molecular marker systems can identify all the cultivars. Five sets of three-RAPD primers, 3 sets of three-ISSR primers and 16 sets of three-SRAP primer combinations were able to distinguish all the cultivars. A linear relationship was observed between Resolving power (Rp) of a primer and its ability to distinguish genotypes. The 35 cultivars were clustered into three major groups based on the RAPD, ISSR and marker combination data with UPGMA, which are in high accordance with their own origins and main characteristics. The results demonstrated that these three marker systems could be useful for identification and genetic diversity analysis of radish cultivars. 相似文献
17.
基于InDel标记的大白菜育种材料分子身份证构建 总被引:1,自引:0,他引:1
以105份大白菜育种材料为试材,精选20对均匀分布于大白菜基因组、且只能检测出2个等位基因的共显性InDel标记引物进行分子标记检测,构建分子身份证。结果表明:20对引物中有16对引物在所有材料中均扩增出单一条带,另外各有2对引物在部分材料中存在缺失和加倍现象。将所有标记引物按其所处染色体编号由小(A01)到大(A10)排列,同一染色体上的标记则按照物理位置从小到大排列,按顺序对标记赋值,构建了105份大白菜材料的分子身份证。所筛选的20对引物对未知新种质的身份证构建具有通用性和兼容性,表明InDel标记技术可以作为大白菜鉴定和分子身份证构建的有效技术手段。 相似文献
18.
采用生物信息学方法通过比较ESTs数据和基因组数据开发了猕猴桃的双亲遗传单拷贝的EPIC标记以用于猕猴桃属植物系统发育研究。通过比较中华猕猴桃(Actinidia chinensis)和美味猕猴桃(A. deliciosa)的ESTs数据和葡萄(Vitis vinifera)基因组数据,以一致性85%为标准共检测到129个EPIC标记,并从中设计96对引物。其中21对EPIC引物在中华猕猴桃和美味猕猴桃两个商业化栽培品种中呈现稳定扩增,核酸多态性(Pi)为0.003 ~ 0.069,变异位点为0.7% ~ 14.8%,简约性信息位点为0 ~ 9.4%。用其中的EPIC-1标记重建中华猕猴桃、美味猕猴桃、毛花猕猴桃(A. eriantha)、绵毛猕猴桃(A. fulvicoma var. lanata)和金花猕猴桃(A. chrysantha)的系统发育关系,显示其跨种间扩增的实用性并获得分辨率较高的系统发育树。本研究中开发的EPIC标记可以作为通用引物用于猕猴桃属植物系统发育分析。 相似文献
19.
Twenty-one rootstock accessions were analyzed with seven grape microsatellite (SSR) primers and seven AFLP primer combinations. SSR primers detected 56 alleles across 21 genotypes and primer heterozygosity varied from 0.617 to 0.856. Similarly 252 AFLP bands were obtained with seven primer pairs. The average similarity index for different rootstocks was relatively low and ranged from 0.068 to 0.36 for AFLP data and from 0.13 to 0.36 for SSR data. A combination of three SSR primers was sufficient to distinguish 21 rootstocks. In cluster analysis majority of rootstocks belonging to same species grouped together. Although the dendrograms obtained with two marker systems were not identical, rootstocks belonging to same species or having common parents were grouped together in both the dendrograms. 相似文献
20.
C. Johnson T. A. Cullis M. A. Cullis 《The Journal of Horticultural Science and Biotechnology》2013,88(6):591-594
SummarySimple sequence repeats (SSRs; microsatellites) are currently the favoured type of molecular marker for identifying plant germplasm. However, identifying polymorphic SSRs and then using them to distinguish closely-related varieties can be time-consuming. Polymorphic markers originating from particularly labile regions of the genome are likely to be easier to develop and also have the potential to identify markers that have higher polymorphic information contents. Genomic regions that vary in somaclonal “off-types” are a possible source of such labile regions of the genome. Thirty-seven primer pairs, developed from sequences that differed between normal and mantled somaclonal mutant oil palm (Elaeis guineensis Jacq.) plants, were used in polymerase chain reactions to screen DNA from 18 varieties of date palm (Phoenix dactylifera L.). From the resulting polymorphisms, three primer pairs were selected which, when used in combination, could identify each of the date palm varieties, unambiguously. The polymorphic bands were isolated, sequenced, and new internal primers were designed. However, all of the amplifications using these new primers yielded only monomorphic bands, indicating that the variation among these date palm varieties lay mainly at or near the original primer sites, and that the internal sequences were conserved. 相似文献