基于nSSR和cpDNA序列的城步峒茶群体遗传多样性和结构研究

采用简单重复序列标记(nSSR)与叶绿体DNA序列(cpDNA)分析技术,对城步峒茶群体进行了遗传多样性、遗传结构和遗传分化等研究。结果表明,15对nSSR引物在参试81份资源中共获得142个等位位点,平均每对引物9.47个,城步峒茶群体的观测杂合度(Ho)、期望杂合度(He)和Nei期望杂合度(Nei)分别为0.49、0.62和0.62,具有较高的遗传多样性。Structure分析将79份峒茶资源分成3个类群,但各类群的遗传背景较为复杂,没有明显的群体结构。F检验表明,城步峒茶群体的近交系数F_IS为正值(F_IS=0.177 5),群体间的遗传分化系数F_ST较小(F_ST=0.034 5),分化程度较低,基因流Nm较高(Nm=7.01)。3对cpDNA引物分别获得了473 bp(rbcL)、704 bp(matK)和320 bp(psbH-trnA)的片段序列,变异位点占总位点的比例分别为0.42%、0.71%和1.25%。将3个序列依次拼接,共产生了9个单倍型,单倍型数由多到少的居群依次为TXZ(6)、DZC(4)、DPS(4)、TYS(3)、HJZ(2),群体的单倍型多样性(Hd)和核苷酸多样性(π)分别为0.732和0.001 39。9个单倍型中,单倍型H1和H5处于进化网络图的中心节点上,并且包含资源数量最多,属于比较原始的单倍型。同时,nSSR和cpDNA的AMOVA分析结果基本一致,居群内的变异百分比分别达到96.69%和80.54%,城步峒茶的遗传变异主要存在于居群内。     

Attaining inter-subgeneric hybrids in fragrant azalea breeding and the inheritance of organelle DNA

Inter-subgeneric hybrids were successfully obtained in reciprocal cross combinations between evergreen azaleas (Rhododendron nakaharae and its hybrids) and fragrant deciduous azaleas (R. arborescens and R. viscosum) for the purpose of fragrant evergreen azalea breeding. Nuclear and organelle DNA of these hybrids was investigated using PCR-RFLP markers. Viable hybrid seedlings have nuclear ribosomal DNA (nrDNA) inherited biparentally, mitochondrial DNA (mtDNA) from the seed parent, and chloroplast DNA (cpDNA) from the deciduous azalea, regardless of cross combination. These results suggest that the chloroplast genome from deciduous azaleas and the nuclear genome from evergreen azaleas are compatible in viable hybrid progenies.     

Assessment of the Genetic Relationship and Diversity of Mango and Its Relatives by cplSSR Marker

Chloroplast inter-simple sequence repeat markers in mango were developed and used to analyze the genetic relationship and diversity of mango and its relatives. Thirty-six mango cultivars （Mangifera indica L.） and its relative species collected from the fruit germplasm collection in the Guangxi Academy of Agricultural Sciences, China, were examined by ISSR-PCR with chloroplast DNA （cpDNA）. Eight better primers for chloroplast DNA that provided reproducible, polymorphic DNA amplification patterns were screened from 50 ISSR primers and used for UPGMA analysis. According to the band patterns with 8 primers for chloroplast DNA, all cultivars tested were distinguished from each other and these showed ample genetic diversity; the average percentage of polymorphism was 77.2%. The 36 samples could be clustered into four groups by UPGMA analysis at the coefficient 0.74. The results indicated that the cplSSR marker was a new powerful tool for the identification of mango cultivars or its relative species, and their genetic relationship analysis and diversity evaluation.     

基于叶绿体DNA PCR-RFLP分析柿及其近缘种亲缘关系

 应用5对叶绿体DNA（cpDNA）特异引物对柿及其近缘的8个种共32个基因型的cpDNA进行PCR扩增。采用7种限制性内切酶对其扩增产物酶切位点变异分析表明,在供试柿属植物中存在丰富的种间多态性,但供试22个柿种内基因型未检测到变异位点。应用NTSYS中UPGMA法聚类和主坐标分析表明：柿与金枣柿最近缘,其次分别是油柿、云南野毛柿、浙江柿和君迁子,而与美洲柿和乌柿相距较远。野柿（浙江）为柿的变种,聚类结果也表明野柿（浙江）与柿有一定差异。     

桑树TrnL-trnF基因间隔区序列的特点及分析

设计桑树TrnL trnF基因间隔区序列的特异引物 ,扩增并分析了桑属育 71 1和桑莲 2个品种的TrnL trnF基因间隔区序列 ,其长度分别为 4 14bp和 4 17bp ,且富含A/T。该序列有 4 2 1个分析性状 ,具有 17个变异位点。在这些变异中主要以碱基的插入和缺失 (主要是插入 /缺失dA)为进化形式 ,其余的发生了少数置换。除这些变异位点以外的核苷酸序列完全相同 ,说明两者有高度同源性 ,与桑科、菊科和蔷薇科的TrnL trnF基因间隔区序列有一定同源性。用Clustalx软件对 2 1份材料的TrnL trnF基因间隔区序列进行聚类分析 ,建立了系统进化发育树     

福建省梨地方品种的遗传多样性研究

利用叶绿体DNA非编码区序列acc D-psa I和17对SSR引物对原产于福建省的49个梨地方品种的遗传多样性进行分析,旨在为育种利用提供参考。获得49份福建地方品种的acc D-psa I序列,并检测到4个多态性位点,包含5个叶绿体单倍型(Hap1~Hap5),其中核苷酸多态性(Pi)为0.00139,单倍型多样性(Hd)为0.660。TCS网络图显示Hap5是最古老的单倍型,其仅在两个样品中检测到。17个SSR位点共检测到211个等位基因位点,有效等位基因数(A)为5~23个,平均值为12.41;观察杂合度(Ho)和期望杂合度(He)的平均值分别为0.5802和0.7549;17个SSR位点的Shannon’s信息指数(I)值为0.5830~2.7683,平均值为1.8661,表现出较高的遗传多样性。基于Nei和Li的遗传距离的邻接法(Neighbor-Joining,NJ)将49份样品聚为9个组,其中大部分聚类结果与单倍型类型表现的亲缘关系较为一致。叶绿体单倍型和SSR多态性位点信息证实福建地方品种具有较为丰富的遗传多样性。     

用改进的高盐低pH法分离和纯化棉花叶绿体及叶绿体DNA

报道了用改进的高盐低ｐＨ法分离和纯化棉花叶绿体及叶绿体ＤＮＡ的实验过程，即先在高盐（离子强度）介质下，通过ｐＨ值变换，多次洗涤的方法去除叶绿体表面的静电附着杂质，得到纯净的叶绿体；然后氯仿抽提纯化ＤＮＡ；最后采用界面针挑法得到高纯度的ｃｐＤＮＡ。实验过程中针对棉花的特点，采用ＰＶＰ排除棉酚和丹宁的干扰，用ＤＩＥＣＡ抑制酚氧化酶活性，并对实验细节作了较大改进。得到的ＤＮＡ可满足酶切、ＰＣＲ等分子生物学分析。     

Indica-japonica differentiation in Chinese rice landraces

Summary Ninety Chinese rice landraces were examined with special reference to the indica-japonica differentiation in terms of traditional criteria, isozyme analysis and PCR analysis of the chloroplast DNA (cpDNA). Cultivars were separated into indica and japonica defined by a discriminant function (Z) based on key characters, as well as by isozyme genotypes. Most indica landraces had chloroplast DNAs with a deletion at the Pst-12 fragment, while most japonica landraces had cpDNAs without the deletion. Two traditionally recognized varietal groups in China, keng and hsien, corresponded largely to the respective japonica and indica revealed in our study. The results obtained in this study showed good agreement for classification of indica and japonica types by the three methods: discriminant analysis by Z value, isozyme analysis, and PCR analysis for cpDNA.     

RFLP characterization of Indian Musa germplasm for clonal identification and classification

Summary Nineteen single-copy clones isolated from a PstI genomic library (cv. Maiden Plantain), and eight Vigna chloroplast DNA clones were used to probe total genomic DNA digests of 57 genotypes of Musa from India. The 19 genomic clones detected a total of 107 polymorphisms among the 57 genotypes. Principal coordinates and phenetic analyses of these data placed cultivars and species into distinct groups that were in general agreement with a previously published RAPD-based classification of these same plant materials. The 107 polymorphisms were sufficient to differentiate each clone from every other clone. Heterologous Vigna chloroplast DNA probes were used to characterize the cytoplasm of Musa cultivars and species. PCO analysis of these RFLPs were detected both within and between the generally recognized genome groups, indicating multiple hybridization pathways in the origin of hybrid clones. Data presented demonstrate that RFLPs are sufficiently abundant to classify Musa germplasm and that genetic relationships among Musa cultivars, based upon RFLP data, are in general agreement with relationships determined by analysis of morphology and RAPDs.     

Chloroplast DNA variation in cultivated and wild Prunus avium L: a comparative study

Chloroplast DNA variation in 96 Prunus avium L. cultivars was assessed and compared with the results of a previous study of cpDNA diversity in 23 wild populations of the species. The polymerase chain reaction‐restriction fragment length polymorphism method was used in these studies. Approximately 9% of the chloroplast genome was analyzed, using five universal primer pairs and three restriction enzymes. Ten polymorphic fragments were common to both the wild and sweet cherry; eight polymorphic fragments were found only in the wild cherry. In the cultivars, all mutations were small (5‐30 bp) indels. In the wild populations, a point mutation was also detected in addition to indels. The mutational combinations revealed three haplotypes in the cultivars, which are the main haplotypes in the wild cherry populations. Chloroplast DNA diversity in wild cherry is higher (16 haplotypes) than in sweet cherry cultivars (three haplotypes). The probable wild origin of the sweet cherry cultivars in the maternal line, on the basis of haplotypic similarity, was discussed.