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黄花柳基因组微卫星分离及多态性位点检测 总被引:1,自引:0,他引:1
以生物素标记的(CT)15和(GT)15为探针进行杂交,借助磁珠筛选出含微卫星的Sau3A I酶切片段,构建了黄花柳微卫星富集文库,获得960个阳性克隆.随机挑选360个阳性克隆进行测序,发现含有微卫星的克隆比例达45%,最后获得的44条非同源性克隆中共含有53个微卫星位点,其中(TC/AG)n,(GA/CT)n,(CA/GT)n比例最高,占74%.随机选取其中的18个微卫星位点设计引物,用5个种个体混合DNA组成模板池,检测引物种间的多态性信息,初步筛选出5对引物在柳属种间有很好的通用性.说明微卫星富集法开发SSR标记不失为一种有效的方法. 相似文献
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甜叶菊微卫星富集文库的构建与多态性标记的筛选 总被引:1,自引:0,他引:1
甜叶菊是我国一种重要特种经济作物, 其分子标记相关遗传背景研究甚少。本研究基于生物素与链霉亲和素的强亲和性原理, 用链霉亲和素顺磁颗粒捕捉人工合成的标记有生物素的寡核苷酸探针(AG)15, 间接筛选出含有甜叶菊基因组微卫星序列的DNA酶切片段, 将筛选得到的片段连接到pUC-T载体中, 构建甜叶菊微卫星序列的富集文库。挑取354个克隆进行菌落PCR检验, 从中筛选出158个阳性克隆进行测序。结果表明, 134个(84.81%)克隆中含有微卫星序列, 其中完美型85个(63.43%)、非完美型15个(11.19%)、复合型34个(25.38%)。根据微卫星序列共设计出71对微卫星引物, 其中62对能扩增出稳定的条带。利用24个甜叶菊品系对这62对引物的遗传多样性的分析表明, 有16个位点表现出多态性, 等位基因数为2~8个, 平均每个位点扩增得到4.5个等位基因, 多态性信息含量在0.3163~0.7595之间, 观测杂合度(Ho)与期望杂合度(He)的范围分别为0.2174~0.9167与0.3555~0.8076。通过聚类分析, 将甜叶菊分为大小叶两大类。本研究开发出的微卫星标记可为甜叶菊的分子遗传育种提供有效的遗传标记。 相似文献
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通过磁珠富集法筛选扁吻鱼的微卫星分子标记。利用限制性内切酶Sau3AI对扁吻鱼的基因组DNA进行酶切,并选取片段大小在250~750 bp间的片段,利用PCR技术进行全基因组扩增,采用生物素标记的(CA)8探针对微卫星片段进行富集。富集后的片段与T载体连接后利用DH5α大肠杆菌进行转化,然后以Sau3AI为引物对菌落进行PCR扩增,扩增后选片段大小符合条件的菌落挑取至测序板,进行测序。结果表明:PCR筛选共获得563个阳性克隆,其中测序192个阳性克隆后发现有53个微卫星序列;序列分析表明,完美型占67.92%,非完美型为22.64%;混合性标记占9.43%。根据测序结果设计微卫星引物24对,经PCR扩增筛选,琼脂糖凝胶电泳结果显示,其中22对引物可扩增出清晰的条带,其中具有多态性的13对。利用13对多态性引物对扁吻鱼野生群体进行扩增,PCR扩增结果显示,等位基因数为3~6,多态信息含量(PIC)为0.625 3,12个位点处于高度多态水平(PIC>0.5)。 相似文献
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基于ISSR和AFLP标记开发甜菜 SSR 引物的研究 总被引:1,自引:1,他引:0
本研究以ISSR-PCR和AFLP标记原理为基础,介绍一种新的分离甜菜基因组微卫星引物的方法。首先对甜菜基因组DNA进行酶切并连接已知序列的接头,构建基因组DNA酶切文库,同时用一个或两个ISSR引物,扩增文库中两端含微卫星序列片段并进行克隆测序,根据测序结果设计微卫星序列间的IP1引物和IP1与微卫星序列间IP2 引物;再根据侧翼序列克隆原理,采用巢式PCR进行基因组步移,扩增IP2引物下游序列,根据巢式PCR产物测序结果,设计微卫星序列另一侧的引物IP3 ,IP2和IP3即为SSR标记引物,对获得的SSR引物进行PCR验证,结果表明SSR引物产率为16%,本研究获得的SSR引物具有较高的多态性,对于后续的遗传多样性检测和遗传连锁图构建具有重要意义。 相似文献
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利用FIASCO技术进行波纹巴非蛤微卫星 总被引:1,自引:0,他引:1
为揭示波纹巴非蛤种质遗传特性、开发种质库,利用FIASCO(Fast Isolation by AFLP of Sequences Containing Repeats)技术开展了其基因组微卫星标记的分离与筛选研究。基因组DNA经限制性内切酶Mse I 酶切后与接头连接,用生物素标记的(CA)15或(AAG)7探针与其杂交,然后用磁珠富集、洗脱获得单链目的片段,经PCR扩增后形成双链,最后进行克隆转化,构建微卫星富集文库。挑选克隆用探针引物(CA)15或(AAG)7和载体引物进行PCR筛选,测序得到含有微卫星DNA的序列,根据序列设计和合成微卫星引物,进行引物适用性分析,并分析了湛江群体的遗传结构。结果表明,8对微卫星引物在湛江群体共检测到108个等位基因,每个位点等位基因数为5~19,期望杂合度为0.666~0.926,观测杂合度为0.400~0.882,4个位点(Pun4,Pun5,Pun6,Pun7)显著偏离哈迪-温伯格平衡(P<0.00625);PIC介于0.62~0.92,所有位点均属于高度多态位点(PIC>0.5)。说明FIASCO技术适合于波纹巴非蛤微卫星标记的分离与筛选,筛选得到的8个微卫星位点能用于波纹巴非蛤遗传多样性分析及野生群体与养殖群体的群体结构分析。 相似文献
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苎麻基因组微卫星的分离与鉴定 总被引:1,自引:0,他引:1
以苎麻[Boehmeria nivea (L.) Gaud.]栽培品种芦竹青为材料,经MseⅠ酶切并与相应接头连接,然后与生物素标记的探针(CT)15杂交,再用链亲和素包被磁珠(Dynabeads M-280)捕捉杂交产物,以21碱基接头寡核苷酸为引物经PCR扩增获得了双链目的片段,回收300~1 000 bp DNA片段,然后克隆到pMD18-T载体上,转化至DH5α中,这样就构建了苎麻富含(GA)n微卫星的部分基因组文库。随机挑取36个克隆,以锚定简单重复序列为引物对其进行PCR筛选。测序分析了22个阳性克隆,每个克隆都含有微卫星DNA,阳性克隆率为61.1%,微卫星种类以与探针互补的(GA/CT)n为主,占83.3%,同时还存在(TG/AC)n和三碱基、六碱基为单元构成的苎麻微卫星,如(GAC)n、(ACG)n、(TCT)n、(TCG)n、(GAA)n、(CCGACG) n、(GAGAAA)n等。最后以18个微卫星位点设计了18对苎麻微卫星特异引物。GA/CT重复单元的长度从7到40范围内变化,平均为19.2,显示了它们将产生良好多态性,为一种强有力的遗传标记。苎麻微卫星DNA标记可广泛应用于苎麻基因型鉴定,基因和QTL分析,分子标记辅助育种,系谱分析等。 相似文献
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应用Dynal磁珠-生物素标记的微卫星探针(AC)8,(AG)8和(ATG)12与地黄基因组DNA酶切片段杂交,捕获含有微卫星序列的DNA片段,连接到pMD 18-T栽体上,转入感受态细胞Trans 5 α,构建地黄富集微卫星文库.利用M13F和M13R载体序列引物筛选文库,对插入片段长度为400~ 800 bp的克隆进行测序.共获得96条序列,48条(50%)含有微卫星位点,其中完美型占66%,非完美型22%,混合型12%.微卫星重复基元中,二核苷酸(AG)n和三核苷酸(CAT)n最为常见. 相似文献
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采用Dynal磁珠富集法构建了香椿微卫星富集文库,通过测序结果对文库的特性进行了分析。实验使用改良CTAB法提取香椿基因组DNA,用(AC)8、(AG)8和(ATG)123种带有生物素标记的探针与香椿基因组DNA的酶切片段进行杂交,将磁珠捕获的含有微卫星序列的DNA片段插入p MD 18-T载体,并转入感受态细胞Trans 5α构建克隆,经筛选后得到含356个克隆的香椿基因组微卫星富集文库。从富集文库中挑选插入片段长度为400~800 bp的128个克隆进行测序,其中含有SSR的序列77条,得率达60.16%,其中完美型占82.69%,非完美型8.65%,混合型8.65%。上述结果为SSR位点的进一步开发奠定了基础。 相似文献
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亚麻木质素合成途径中关键酶基因片段的克隆与序列分析 总被引:2,自引:0,他引:2
亚麻是一种重要的韧皮纤维作物, 木质素对亚麻纤维的性能和品质具有较大影响。以亚麻(Linum usitatissimum L.)茎秆表皮细胞的mRNA为模板, 利用木质素合成途径中关键酶基因的同源基因保守序列设计简并引物, 通过RT-PCR扩增, 电泳获得13个特异带。分别将这些DNA片段连接到T载体后转化大肠杆菌, 从重组质粒转化菌分别挑取5~8个单菌落测定插入片段序列, 得到关键酶基因新的片段序列8个。生物信息学分析结果表明, 这些新片段分别属于3个基因家族。其中, 2个CCoAOMT基因片段(GenBank登录号为EF214740, EF214741), 3个4CL基因片段(GenBank登录号为EF214737, EF214738, EF214739), 3个F5H基因片段(GenBank登录号为EF214745, EF214746, EF214747), 推测亚麻中这几个木质素代谢关键调控酶基因存在多基因家族。新获得的基因片段序列为进一步克隆全序列和了解调控亚麻木质素的生物合成奠定了基础。 相似文献
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为了解鸡白痢沙门氏菌与鸡伤寒沙门氏菌的基因组差别,筛选鸡白痢沙门氏菌特有的序列,利用SSH对鸡白痢沙门氏菌C79-13(实验方)与鸡伤寒沙门氏菌Sg9(驱动方)基因组进行了比较。选择四碱基内切酶Rsa I将C79-13与Sg9基因组DNA酶切,酶切的C79-13基因组DNA分成两份,分别与接头1和接头2R连接,然后进行两轮杂交和两轮PCR ,得到消减混合物, 将其与PCR?2.1克隆载体连接,转化感受态E.coli DH5α建立消减文库。结果共获得400个阳性克隆;筛选240个克隆制备质粒进行PCR检测,均扩增出100~2000 bp大小的片段。差异DNA消减文库的构建为进一步筛选、克隆鸡白痢沙门氏菌特异的未知新基因、建立分子鉴别新体系奠定了基础。 相似文献
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Summary Generation of Simple Sequence Repeat (SSR) DNA markers was based on the construction of genomic DNA library of avocado (Persea americana M.). The library was screened with the four dinucleotide probes (AG), (AT), (GC) and (CA). Positive clones were sequenced to validate the presence of simple sequence repeats (SSR) and to generate polymerase chain reaction (PCR) primers based on the sequences flanking the simple sequence repeat. Twenty six different pairs of primers which yield a PCR product in the initial screening were synthesized. The SSR A1E11 was found to have eleven alleles while A3F8 has eight alleles. The SSRs in avocado were found to be inherited in a Mendelian fashion.Contribution from the Agricultural Research Organization, The Volcani Center, Bet-Dagan, Israel. No. 1335-E, 1994 series. 相似文献
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紫云英SSR分子标记的开发及在品种鉴别中的应用 总被引:2,自引:0,他引:2
利用生物素标记的(AG)15、(CT)15、(AC)15、(GT)15探针及链霉素亲和磁珠,从紫云英的基因组中富集微卫星(SSR)序列。在用富集片段构建插入文库的950个转化子中,经PCR检测及测序共得到127个SSR序列,微卫星序列的富集效率达15.8%。除去重复或无效的序列,得到33个序列用于引物设计。对征集的9个紫云英品种进行多态性分析,有6对引物扩增出明显且稳定的多态性位点18个。在紫云英的品种水平上,这些SSR位点产生的多态率为50%~100%,有效等位基因数为1.19~1.64,Nei氏遗传多样性为0.13~0.38,Shannon多态信息指数为0.22~0.56;利用这6对引物可将参试品种完全区分开,证明这些SSR位点可用于紫云英品种的指纹鉴别。根据SSR位点的相似性系数,将 9个紫云英品种主要聚成两个类群, 与传统按生育期的紫云英品种划分结果无必然的联系。 相似文献
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Development of simple sequence repeat (SSR) markers in Eucalyptus from amplified inter-simple sequence repeats (ISSR) 总被引:6,自引:0,他引:6
M. A. Van Der Nest E. T. Steenkamp B. D. Wingfield M. J. Wingfield 《Plant Breeding》2000,119(5):433-436
Eucalyptus spp. are widely used in exotic plantations. Since many of these trees are derived from vegetative propagation, the routine identification of clones has become increasingly important. The most widely used molecular based method for fingerprinting these clones is by random amplified polymorphic DNAs (RAPDs). Although this technique is useful, its results are not very repeatable, especially between laboratories. The aim of this study was to develop microsatellite markers that are highly repeatable, and to investigate their value in Eucalyptus fingerprinting. Typically, this process involves the expensive procedure of constructing an enriched genomic library. However, we used an intersimple sequence repeat (ISSR) polymerase chain reaction (PCR)‐based enrichment technique for microsatellite‐rich regions. With this relatively inexpensive method, microsatellite‐rich regions were amplified directly from genomic DNA, after which PCR products were cloned and sequenced. From these microsatellite‐rich sequences, primer sets were constructed to amplify mono‐, di‐, tri‐, hexa‐and nona‐nucleotide repeats. These markers were all inherited in a Mendelian fashion in the progeny of a test cross between two Eucalyptus grandis trees. The primer sets developed were also able to amplify the corresponding microsatellite loci from five different Eucalyptus spp., namely E. grandis, E. nitens, E. globulus, E. camaldulensis and E. urophylla. 相似文献
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Zhengjun Xia Hiroko Sato Satoshi Watanabe Shiji Kawasaki Kyuya Harada 《Euphytica》2005,141(1-2):129-137
We have constructed a soybean (Glycine max (L.) Merrill) bacterial artificial chromosome (BAC) library from green leaf protoplasts of the cultivar, Misuzudaizu. The library contains 53,760 clones with an average insert size of 116 kb. About 2.9% chloroplast DNA origin was revealed by PCR and colony hybridization. Apart from 2.8% clones having no insert, this library represents 5.2 genome equivalents. With this genome coverage, the probability of having any DNA sequence represented in the library is higher than 99.5%. Three-dimensional pools of the BAC library in combination with the use of a high efficiency genome scanning (HEGS) electrophoresis facilitate rapid and efficient PCR-based screening. An average of five positive clones were identified after screening the BAC library with SSR and STS markers. BAC-end walking was performed for three SSR associated BACs. This library will provide a good resource for positional cloning of agronomically and biologically important QTL genes that Misuzudaizu possesses. 相似文献
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黏类小麦细胞质雄性不育系mtDNA消减文库的构建 总被引:1,自引:0,他引:1
本研究利用抑制性消减杂交技术,构建了黏类小麦细胞质雄性不育线粒体DNA的消减文库。分别提取相同细胞质背景下的不育和可育等基因系线粒体基因组DNA(mtDNA),用RsaⅠ酶切成大小不等的片段,并各自与不同的接头连接,连续经过两次消减杂交和两次PCR扩增,将PCR产物与克隆载体连接,转化为大肠杆菌感受态细胞DH5α,经蓝白斑筛选后,再用PCR方法插入片段筛选出阳性重组质粒,构建差异DNA消减文库。在构建的不育mtDNA文库中,将SSH文库的全部扩增产物与SSH文库中的单条扩增条带分别进行胶回收和克隆转化,分别挑取54个和6个阳性克隆进行测序分析和相关功能初步比对。结果表明,不育mtDNA的SSH文库差减杂交效率较高,质量较好;回收单条扩增条带分别进行克隆测序的结果准确率较高;对测序序列进行BLASTx比对及功能注释分析发现,约90%的序列来源于线粒体基因nad1和nad5的非编码区。 相似文献
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Development and variability analysis of microsatellite markers in peach 总被引:25,自引:0,他引:25
A genomic DNA library enriched with AG/CT repeats has been developed from the peach cultivar ‘Merrill O'Henry’. The enrichment method was efficient, with 61% of the clones obtained carrying a microsatellite sequence and a yield of one polymorphic microsatellite every 2.17 sequenced clones. From 35 microsatellites detected, 24 were polymorphic in a set of 25 cultivars including 14 peaches and 11 nectarines. A total of 82 alleles were found with the polymorphic microsatellites, with an average of a 37% of observed heterozygosity. Microsatellites with a high number of repeats were generally those having the largest number of alleles. All cultivars except two (‘Spring Lady’ and ‘Queencrest’) could be individually distinguished with the markers used. Just three selected microsatellites were enough for the discrimination of 24 out of the 25 possible genotypes. Cluster analysis grouped all nectarines in a single cluster. Peaches, with 75 of the 82 alleles found, were more variable than nectarines, with only 64. Microsatellites appear to be powerful and suitable markers for application in peach genetics and breeding. 相似文献