SRAP分子标记分析西瓜遗传多态性

目的:探讨西瓜遗传多样性和遗传基础。方法:采用SRAP分子标记对西瓜品种D1、D2、D3、H1、H2、H3、M1、M2、M3、m1、m2、m3的多态性进行了分析。结果:每对引物组合产生13~25对比较清晰的扩增带.8对引物组合共产生131条扩增带。平均每对引物组合产生16.375条。8对引物组合共产生多态性带37条,每对引物组合产生3~7条,平均4.625条。每对引物组合产生的多态性带的比例为16.666%~38.464%,平均为28.675%。另外,对银染过程进行了优化。结论:SRAP标记多态性还是较高的,可以适于分析西瓜等遗传差异小的作物。     

甜瓜抗白粉病基因SRAP分子标记筛选

以感白粉病甜瓜A120和抗白粉病甜瓜A119为亲本构建F2代分离群体,采用BSA和SRAP相结合的方法筛选与甜瓜抗白粉病基因相连锁的分子标记.结果显示,294条SRAP引物中有6条引物在抗病与感病池间表现出多态性;对8个高抗和8个高感单株进行扩增,引物me46em51和me3em6分别在高感单株中扩增出210 bp和205 bp的多态性条带,而高抗单株无此扩增带,与抗病、感病池结果一致.采用JoinMap3.0软件进行连锁分析,两标记与抗白粉病基因的连锁距离分别为18.2 cM和23.4 cM,初步推测本实验中甜瓜白粉病抗性为隐性多基因控制.     

大豆种质资源SRAP分子标记中的引物筛选

以113个大豆栽培品种和20个野生品种为材料,从288对引物组合中筛选出12对多态性丰富、条带清晰、可重复性好的SRAP引物组合。用筛选出的12对引物组合对大豆品种进行PCR扩增,获得了带型丰富和清晰可辨的DNA的PAGE指纹图谱;共扩增出251条谱带,其中多态性条带220条,多态性谱带比率为87.6%,平均每个引物扩增出18.3条谱带。结果显示,所筛选出的12对引物组合可以有效的应用于大豆种质资源的SRAP分析。     

相关序列扩增多态性(SRAP)标记及其应用研究进展

SRAP是一项基于PCR技术的分子标记技术,利用其独特的引物设计对基因组的开放阅读框(ORFs)进行特异扩增,利用个体以及物种的内含子、启动子和间隔序列的不同,产生基于内含子和外显子的SRAP多态性。阐述了SRAP的原理和流程,详细论述了SRAP标记目前在植物遗传多样性、作物品种鉴定、遗传图谱构建等方面的研究进展及应用前景。     

基于SRAP分子标记的冰草遗传连锁图谱构建

构建高密度遗传连锁图谱是冰草抗性、品质、产量等重要性状QTL精细定位及标记辅助育种研究的基础。该试验以四倍体杂交冰草F2群体的202个分离单株及其亲本为材料,利用SRAP分子标记技术和Join Map 4.0作图软件对冰草的遗传连锁图谱进行了构建。结果表明:(1)共筛选出22对多态性好、标记位点清晰稳定的SRAP适宜引物,对冰草杂种F2分离单株的基因组DNA进行PCR扩增,共获得510个SRAP多态性标记位点,其比率占88.2%。(2)偏分离分析表明,偏分离标记比率仅为14.12%,符合遗传作图的要求。(3)成功构建了冰草的SRAP分子标记遗传连锁图谱,该图谱有14个连锁群、510个标记,连锁群间长度范围86.4～179.0cM,覆盖基因组总长度1 912.9cM,标记间平均间距3.75cM,为高密度遗传图谱。     

烟草主要栽培类型的SRAP标记研究

利用SRAP分子标记从700对引物中筛选到普通烟草栽培种内(Nicotiana tabacum L.)两条晾烟(马里兰烟、白肋烟)类型的特征标记带、一条晒烟(香料烟和名优晒烟)类型的特征标记带,一条烤烟与晾烟特征标记带。这些标记不但可以直接转化成SCAR标记,而且可通过分离群体的遗传分析用于烟草类型间遗传转化的特征带,也可进一步用于测序发掘新基因。在分子水平上为研究普通烟草种内不同栽培类型间的遗传差异和类型划分奠定了可行性实验基础。     

SRAP分子标记在园林植物遗传育种中的应用

相关序列扩增多态性(sequence-related amplified polymorphism,SRAP)分子标记作为一种新型的分子标记技术,以其多态性高、稳定性高、重复性好、操作简便、效率高及成本低等优点,已经在园林植物中广泛应用.简单介绍SRAP标记的原理和特点,综述其目前在遗传多样性评析、亲缘关系分析、遗传图谱构建、种质资源鉴定及基因克隆与基因定位等方面的研究进展,并对该标记在园林植物的遗传育种的应用前景进行了展望.     

甘蓝Ogura胞质雄性不育基因的SRAP标记

本研究以甘蓝Oguar胞质雄性不育系CMS451及其保持系为材料,优化甘蓝SRAP体系,并用SRAP标记分析了Oguar胞质不育基因。结果表明:总反应体积为25μL,含有Mg Cl2,2.5 mmol/L;primer,0.2μmol/L;DNA,45ng;NTPs,0.4 mmol/Ld;1.5 U Taq DNA聚合酶,2.5μL10×buffer,其余用dd H2O填充;这个体系适合甘蓝的SRAP标记。利用92对SRAP组合引物和优化的SRAP体系,发现Me6Em8扩增出稳定的特异条带,特其大小在250-500bp之间,对其进行单株验证,用Jionmap ver3.0分析计算出此条带与不育基因的遗传距离为22.548c M。     

五味子果色相关的SRAP标记鉴定

[目的]寻找与五味子果实颜色相关的分子标记为辅助育种提供技术支持。[方法]利用SRAP技术对五味子不同果实颜色(白果、黄果与红果)的DNA多态性进行分析。[结果]共筛选引物对120个组合,获得2个与果实颜色基因有关的特异条带ME1-EM15-129bp、ME3-EM12-420bp,其中ME3-EM12-420bp成功转化成SCAR标记。[结论]2个标记可对五味子不同果实颜色进行分子鉴定,结果稳定可重复性高。     

Diversity and relationships among Turkish okra germplasm by SRAP and phenotypic marker polymorphism

Germplasm characterization is essential and molecular markers provide valuable information for breeding programs. Sequence-related amplified polymorphism (SRAP) and phenotypic markers were studied to determine diversity and relationships among 23 okra (Abelmoschus esculentus (L) Moench) genotypes. The 39 combinations of forward and reverse SRAP primers were used to evaluate the 21 Turkish and two randomly selected USA genotypes as outgroups, and produced 97 scorable markers, of which 50% was polymorphic for all 23 genotypes. Seventeen out of the 23 genotypes (74%) were distinguished from each other with mean similarity of 0.93. As to phenotypic markers, 33 heritable traits were evaluated in field with ten replications, 28 of them (85%) were found to be polymorphic. The UPGMA (unweighted-pair group method arithmetic average) dendrogram based on the 33 phenotypic markers distinguished all genotypes, but failed to detect any geographic association of okra genotypes, being consistent with previous study. It can be concluded that SRAP markers are useful for studying diversity and relationships among okra germplasm, and have potential in marker-aided selection, linkage mapping, and evolutionary studies.     

北极狐GHR基因cDNA的克隆及序列分析

本文根据狗(AF133835)的GHR基因cDNA编码全序列设计了三对引物,利用RT-PCR方法克隆出北极狐GHR基因编码区全长cDNA序列(GenBank accession No.EU304325)。结果表明,北极狐GHR的ORF为1917bp,编码638个氨基酸的前体蛋白,由18个氨基酸的信号肽和620个氨基酸的成熟肽组成。通过同源性比较发现北极狐与狗的同源性最高,达到98%。另外,利用邻接法(NJ法)构建的分子系统进化树聚类结果表明,北极狐与狗先聚为一类,该聚类结果与传统的物种进化关系基本一致。另外,通过氨基酸对位序列比较发现,北极狐GHR在氨基酸序列上存在明显的特异性,如45和451位分别为A和E,而其它物种均分别为T(大鼠为K)和A(牛羊为V,鼠为T)。     

基于SRAP标记的墨西哥落羽杉优良单株的遗传多样性分析

采用SRAP标记方法,分析了原产地及种植地不同的18个墨西哥落羽杉(Taxodium mucronatum Tenore)优良单株的遗传多样性,并根据遗传相似系数、采用UPGMA法对它们的遗传关系进行了聚类分析.结果显示:用7对引物组合从18个单株的总DNA中共扩增出87条带,其中多态性条带71条,多态性条带百分率为81.6％.按照原产地和种植地可将18个单株分为4组,它们的总体Nei's基因多样性指数、Shannon信息指数和基因分化系数分别为0.229、0.355和0.479 9,而基因流仅为0.542,说明各组间的基因交流较少.18个单株间的遗传相似系数为0.632 2～0.919 5,平均值为0.753 9.聚类分析结果显示:18个单株可分为3组,其中18号和14号单株分别单独成组,其余16个单株聚为1组.后者可进一步分为8个亚组:1号、7号、12号和15号单株各自单独成亚组;2号、3号、5号、9号、11号和13号单株聚为1个亚组;4号和6号单株、8号和17号单株、10号和16号单株分别聚为3个亚组.研究结果表明:18个优良单株间存在丰富的遗传变异,但它们的遗传关系与原产地及种植地明显不相关.     

SRAP技术研究烟粉虱遗传多样性

采用AFLP、SRAP2种标记方法分别对2个烟粉虱Bemisia tabaci Gennadius种群(一品红、甘蓝)的多态性进行分析。结果表明,(1)2种方法平均每对引物组合产生的条带数分别为29.4和21.8。(2)AFLP法每对引物组合产生10～23条多态性带,平均17.20条,多态性带的比例平均为57.93%。SRAP法每对引物组合产生5～18条多态性带,平均13.3条,多态性带的比例平均为60.59%。(3)前者的基因多样性范围为0.1503～0.2838,平均为0.2297;后者的基因多样性范围为0.0977～0.2911,平均为0.2332。证明利用SRAP技术和AFLP技术研究烟粉虱的遗传多样性是有效的。     

Effect of Sub-Polar Gyre, North Atlantic Oscillation and ambient temperature on size and abundance in the Icelandic Arctic fox

Animals are exposed to environmental factors that influence their life history and body size. Here we used the Arctic fox ( Vulpes lagopus ) as an indicator of the complex links between largescale environmental variables that influence both marine and tundra trophic dynamics to demonstrate how they affect the fox's body size and abundance. The Arctic fox inhabits throughout Iceland, where it preys mainly on birds. We studied the effects of the Sub-Polar Gyre (SPG), winter and summer North Atlantic Oscillation (NAO), mean annual winter and summer temperature, and geographic sector (eastern and western Iceland, which differ in their ecology) on variations in mandible size (6345 specimens) and body mass (2732 specimens) as well as abundance on the Arctic fox in Iceland. We found that (a) SPG index negatively affected male mandible length as well as body mass of both sexes. SPG was also negatively related to fox abundance. (b) Summer NAO had a negative effect on Arctic foxes, that is, cold summers were correlated with shorter mandibles and lower body mass. (c) Winter NAO had a significant negative effect (although weaker than that of summer NAO) on female mandible length, but not on body mass. (d) Summer temperature had a positive effect on female mandible length, but no effect on body mass. However, winter temperature had no effect on either the mandible or body mass. (e) Foxes in the eastern sector had shorter mandibles and were of lighter mass than those in the western sector. We suggest that climate conditions during the growth period of the young affected their final size both directly, by influencing energy metabolism for maintenance, but mainly through their effects on food availability. As far as we are aware, this is the first report that the SPG has an effect on vertebrates, let alone terrestrial ones.     

Polymorphism of prion protein gene in Arctic fox (<Emphasis Type="Italic">Vulpes lagopus</Emphasis>)

Prion diseases are fatal neurodegenerative disorders of humans and certain other mammals. Prion protein gene (Prnp) is associated with susceptibility and species barrier to prion diseases. No natural and experimental prion diseases have been documented to date in Arctic fox. In the present study, coding region of Prnp from 135 Arctic foxes were cloned and screened for polymorphisms. Our results indicated that the Arctic fox Prnp open reading frame (ORF) contains 771 nucleotides encoding 257 amino acids. Four single nucleotide polymorphisms (SNPs) (G312C, A337G, C541T, and A723G) were identified. SNPs G312C and A723G produced silent mutations, but SNPs A337G and C541T resulted in a M–V change at codon 113 and R–C at codon 181, respectively. The Arctic fox Prnp amino acid sequence was similar to that of the dog (XM 542906). In short, this study provides preliminary information about genotypes of Prnp in Arctic fox.     

番茄耐低温相关基因的SRAP标记筛选

以番茄耐低温和不耐低温基因组DNA为材料进行SRAP分析,共筛选了225对SRAP引物,其中27对引物在两池之间表现差异,经测序只有Me2Em5扩增出与番茄耐低温相关的差异性片段,大小约为273bp,该片段仅在耐低温植株中稳定扩增。经Blast分析比对,该片段与已报道的PEG和低温诱导后在沙冬青幼苗中表达基因的cDNA片段同源。根据差异片段序列设计特异引物,将M2E5—273标记成功转化为更稳定的SCAR标记。     

棉花遗传多样性SCoT和SRAP标记的研究及比较分析

利用SCoT和SRAP两种分子标记技术对30份彩色棉与白色棉种质资源,进行遗传多样性研究。用29对SRAP引物组合和26个SCoT引物分别对供试棉花的基因组DNA进行扩增。SCoT引物共扩增出163条带,多态性比率为61.96%,遗传相似系数GS值变化范围为0.5405～0.9972。SRAP引物组合共扩增条带1067条,多态性比率仅为14.1%,遗传相似系数GS值变化范围为0.5415～0.9109。两种标记系统得到了相似但并不完全相同的聚类图,2种标记方法间存在显著相关性(r=0.5518,P<0.05)。结果表明,SRAP与SCoT标记均适用于棉花种质的遗传多样性分析,且SCoT的标记指数MI高于SRAP标记,为SCoT这种新兴的标记技术在棉花育种中的应用提供了重要的依据。     

草鱼种质相关SRAP及SCAR的分子标记

采用相关序列扩增多态性(Sequence-realted Amplified Polymorphism, SRAP)技术分析野生草鱼和家养草鱼,筛选与草鱼种质退化相关的分子遗传标记.共进行88对引物组合的检测, 产生标记数目共计905个.依据标记在群体中出现的频率和变化规律,共筛选出2 1个可能与种质相关的特异性标记,对这些特异性标记进行测序并将测序结果进行BLAST分析 .发现测得片段中有8个片段在GenBank中找到同源性较高的序列,而其他片段与数据库中序列的相似性较低.根据序列信息分别设计了3对引物.用这3对引物分别对草鱼三个群体进行 PCR扩增,分别产生了SCAR1(308 bp)、SCAR2(66 bp)、SCAR3(114 bp)3个扩增带.采用大样本对这3个标记进行验证,发现其中SCAR1在家养群体中呈现阳性,在野生群体中为阴性,可区分出这两种群体.以SCAR3为引物在174条家养群体中得到目的片段,在26个家养群体没有扩增出条带,分布频率为87%;在100个野生群体中有6个个体检测到该条带,分布频率为6%.以SCAR2为引物在野生群体中完全扩增出目的条带,淡水中心群体中有7条扩增到条带,前洲群体中没有扩增出条带,标记在家养种群中的分布频率为96.50%.因此SCAR1可作为草鱼家养群体的一个重要的分子遗传特征指标,为进一步进行分子标记辅助育种奠定了基础 [动物学报 54(3):475-481,2008].