中国野生葡萄mybA转录因子SNP特征分析

本研究以中国野生葡萄14个种为材料,对控制花色苷合成的mybA转录因子进行克隆和序列分析,获得VvmybA1和VlmybA2两个转录因子的全长基因序列,共检测到121个SNP,表现出丰富的遗传多样性。3种中性检测方法比较序列变异模式,结果表明,中国野生种葡萄VvmybA1和VlmybA2基因没有偏离中性模型,反映出基因漂移和选择性中性突变之间的平衡。不同野生种材料的mybA 基因结构存在很高的同源相似性。但是在启动子区、内含子区以及第三个外显子区存在不同程度碱基的缺失、插入和替换,而且野生种葡萄mybA基因存在一些特有序列或突变,这些突变可以作为分子标记区分不同的野生种材料。通过基因结构比对和系统进化树分析,可将野生种葡萄细分为5个类群。初步推测桦叶葡萄和变叶葡萄进化地位较为原始。     

8个山葡萄及山欧杂种葡萄品种的SSR分析

选取9对SSR引物对8个山葡萄及山欧杂种葡萄品种进行扩增,估算了扩增片段长度,结果表明,利用这9对SSR引物可以把8个山葡萄及山欧杂种葡萄品种区分。8个山葡萄及山欧杂种葡萄品种的等位基因数（Na）平均为2.8889,有效等位基因数（Ne）平均为2.2162,Shannon多样性指数（I）平均为0.8669,期望杂合度（Nei）平均为0.5217。9对引物中,UDV-067提供的信息量最大,引物VMC7bl最小。     

葡萄属种子发育的物候、萌发行为及其对冷层积的反应

以3个起源和分布中心的不同葡萄种及其杂交种作为实验材料,观察了开花、果实和种子成熟的物候,研究了成熟种子的基本特性和最初萌发率以及冷层积对成熟种子萌发的影响。结果表明,葡萄种子具有休眠特性,生理成熟时都具有分化完全的胚,在休眠解除过程中胚的形态不发生变化;美洲种休眠最深,欧亚种休眠最浅,其它种类的葡萄种子的休眠程度介于美洲种和欧亚种之间;不同种葡萄花期、果实和种子成熟过程的物候存在差异,果实成熟与种子成熟不同步,其间隔时间越短,种子休眠程度越深。冷层积60天能有效地解除东亚种、欧亚种、欧山杂种和蘡欧杂种的种子休眠,但对解除美洲种、美洲种种间杂种和欧美杂种的种子休眠效果较差。     

葡萄属种子发育的物候、萌发行为及其对冷层积的反应

以3个起源和分布中心的不同葡萄种及其杂交种作为实验材料, 观察了开花、果实和种子成熟的物候, 研究了成熟种子的基本特性和最初萌发率以及冷层积对成熟种子萌发的影响。结果表明, 葡萄种子具有休眠特性, 生理成熟时都具有分化完全的胚, 在休眠解除过程中胚的形态不发生变化; 美洲种休眠最深, 欧亚种休眠最浅, 其它种类的葡萄种子的休眠程度介于美洲种和欧亚种之间; 不同种葡萄花期、果实和种子成熟过程的物候存在差异, 果实成熟与种子成熟不同步, 其间隔时间越短, 种子休眠程度越深。冷层积60天能有效地解除东亚种、欧亚种、欧山杂种和蘡欧杂种的种子休眠, 但对解除美洲种、美洲种种间杂种和欧美杂种的种子休眠效果较差。     

8个山葡萄及山欧杂种葡萄品种的SSR分析

选取9对SSR引物对8个山葡萄及山欧杂种葡萄品种进行扩增,估算了扩增片段长度,结果表明,利用这9对SSR引物可以把8个山葡萄及山欧杂种葡萄品种区分.8个山葡萄及山欧杂种葡萄品种的等位基因数(Na)平均为2.8889,有效等位基因数(Ne)平均为2.2162,Shannon多样性指数(I)平均为0.8669,期望杂合度(Nei)平均为0.5217.9对引物中,UDV-067提供的信息量最大,引物VMC7b1最小.     

葡萄果实成熟期花色苷与白藜芦醇合成相关基因的表达

以酿酒葡萄‘赤霞珠’为试材,采用pH示差法和高效液相色谱(HPLC)法分别测定葡萄成熟期果皮花色苷和白藜芦醇含量,用实时荧光定量PCR检测两者合成途径中相关基因的表达量,分析花色苷含量和白藜芦醇含量与其相关基因表达的关系,以揭示结构基因与调控基因的调控机制,为筛选富含花色苷和白藜芦醇的酿酒葡萄提供理论依据。结果显示:(1)葡萄果皮花色苷含量在花后112d达到最高值(0.77mg/g),反式白藜芦醇含量在花后126d达到最高值(30.87μg/g)。(2)花色苷和白藜芦醇合成途径中,CHSs、CHI、STS、UFGT、MybA1、MybA2基因的表达量除花后98d下调外,其余时间均呈上调表达,而Myb5a则始终呈上调表达。(3)相关分析表明,STS基因表达量与CHS1、CHS2基因表达量呈极显著和显著正相关关系,MybA1、MybA2基因表达量与CHSs、CHI、STS、UFGT基因的表达量呈极显著正相关关系;Myb5a基因表达量与CHS3基因表达量呈极显著正相关关系。研究表明,部分结构基因的表达与花色苷和白藜芦醇的变化不同步,MybA1和MybA2可能调控花色苷合成途径中多个结构基因的表达,花色苷与白藜芦醇的关系并不固定,而是处在动态变化中。     

葡萄品种资源果刷性状及果粒褐化调查与分析

为认识葡萄品种资源果刷特征以及果刷脱落后对果粒的影响,本研究对126个葡萄品种成熟期的果刷性状以及74个品种果洞褐化情况进行分析,研究结果表明,果刷特性在品种之间存在一定差异。果刷可分为完整和不完整两类,果刷拔出后粘连果肉情况不同,欧亚种果刷与果肉粘连程度高于欧美杂种(V. vinifera L.×V. labrusca L.);欧亚种葡萄果刷耐拉力与果刷长度、果刷粗度之间均呈极显著正相关;欧美杂种葡萄果刷耐拉力与果刷长度之间相关性不显著,与果刷粗度之间呈极显著正相关;欧亚种与欧美杂种葡萄果刷耐拉力之间存在显著性差异,且欧亚种耐拉力明显大于欧美杂种葡萄品种耐拉力;果肉褐化速度和褐化程度在品种间差异大,且成熟度愈高褐化程度愈轻。不同品种果洞褐化速度不一致,果洞的大小不同对果实造成损伤程度有异,在一定程度上影响采后果实的耐贮性,通过对果刷性状的研究,以期为葡萄种质资源评价以及新品种的育种工作提供一定的理论依据。     

栽培稻杂种不育性的遗传研究——Ⅲ.不同类型品种F_1花粉不育性的等位基因分化

以台中65等基因F_1不育系为遗传测验种,测定了栽培稻(O.sativa)45个品种在3个F_1不育基因座的基因型和等位基因的分化度。在S-E3基因座上,除Dular带有S_i/S_i基因型外,其余被测品种均带有S_i/S_i基因型。在S-E2和S-E5基因座上,籼型品种带有高频率的S_i基因,而粳型品种带有高频率的S_i基因。S_i和S_i均具有不同的分化度。籼型品种携带的S_i基因和粳型品种携带的S_i基因具有较高的分化度。中间型品种和广亲和品种的等位基因分化在S-E2基因座上与粳型品种相似,而在S-E5基因座上与籼型品种相似。此外,分析了各类型品种相互杂交F_1杂种在S-E2和S-E5基因座的杂合率、杂合度和杂合性。与籼/粳杂种相比,中间型品种(包括广亲和品种)与籼型和粳型品种杂交,F_1杂种均具有较低的平均杂合性,从而表现出较高的亲和性。因此,无论是杂种不育性还是杂种亲和性均由花粉不育基因控制。花粉不育基因也称为特异亲和基因。     

不同种源的葡萄种子休眠及其解除的研究

为探讨葡萄种子休眠与解除的规律, 我们选择起源于东亚、北美–中美、欧洲–中亚3个分布中心的不同种类及其杂种的20个品种, 研究了它们成熟种子的外部形态与萌发行为, 种子的休眠特性与休眠解除的方法, 并模拟四季温度的交替变化研究了环境温度对种子休眠的影响。结果表明, 不同起源的各类葡萄种子的休眠类型均为生理休眠, 但其休眠程度不同, 休眠解除方式也存在差异。其中欧亚种和东亚种的种子休眠较浅, 美洲种种子休眠较深; 杂交种比亲本所属类别的种子休眠程度浅。对于欧亚种、东亚种及其杂交种(欧山杂种)而言, 5ºC冷层积和变温层积(即20ºC (14 h) /10ºC (10 h)和30ºC (14 h) /20ºC (10 h))2个月能够有效地或部分解除它们的种子休眠; 但对美洲种和欧美杂种而言, 仅5ºC冷层积且层积时间需要延长至6个月才能解除其休眠, 变温层积和25ºC暖层积都不能解除休眠。四季温度的交替变化模拟实验进一步证明了不同起源的葡萄种子的休眠程度不同。这些休眠特性及其解除方式反映了不同起源葡萄种类的环境适应性。本文研究结果为葡萄资源的引种和育种提供了参考数据。     

两个不同葡萄种对高湿弱光气候的表现

在高湿弱光条件下 ,对欧亚种葡萄无核白鸡心、京玉、汤姆逊无核、火红无核、深红无核、红地球、里查马特和美人指与欧美杂交种葡萄巨峰、藤稔、醉金香和金星无核进行了研究。与欧美杂交种比较 ,欧亚种葡萄普遍表现徒长 ,花芽形成困难 ,产量低下。高湿弱光使大部分欧亚种葡萄 PS 光化学效率 Fv/ Fm、光化学猝灭系数 q P、最大荧光 Fm和 PS 非环式电子流的量子效率 PS 下降 ,而初始荧光 Fo与非光化学猝灭系数 q N上升 ,净光合作用与初始荧光 Fo、最大荧光 Fm、PS 光化学效率 Fv/Fm、PS 非环式电子流的量子效率 PS 、光化学猝灭系数 q P和荧光非化学猝灭系数 q N之间存在着显著或极显著的相关性(r=- 0 .782 1* ,r=0 .9384 * * ,r=0 .8176 * ,r=0 .90 11* * ,r=0 .880 1* * ,r=- 0 .86 2 5 * * ) ,表明光合结构受到一定的破坏。大部分欧亚种葡萄叶片叶绿素 a与叶绿素 b显著或极显著低于欧美杂交种葡萄 ,表明吸收光的能力较差 ;部分欧亚种葡萄叶片叶绿素 a/ b与欧美杂交种无明显差异 ,表明利用散射光的能力较强 ;叶绿素 a/ b与乙醇酸氧化酶活性存在着显著的负相关 (r=- 0 .780 0 * ) ,叶绿素 a/ b高的品种光呼吸也高。大部分欧亚种葡萄乙醇酸氧化酶活性低于欧美杂交种 ,乙醇酸氧化酶活性与产量和净光合速     

Genetic structure and differentiation in cultivated grape,Vitis vinifera L

222 cultivated (Vitis vinifera) and 22 wild (V. vinifera ssp. sylvestris) grape accessions were analysed for genetic diversity and differentiation at eight microsatellite loci. A total of 94 alleles were detected, with extensive polymorphism among the accessions. Multivariate relationships among accessions revealed 16 genetic groups structured into three clusters, supporting the classical eco-geographic grouping of grape cultivars: occidentalis, pontica and orientalis. French cultivars appeared to be distinct and showed close affinity to the wild progenitor, ssp. sylvestris from south-western France (Pyrenees) and Tunisia, probably reflecting the origin and domestication history of many of the old wine cultivars from France. There was appreciable level of differentiation between table and wine grape cultivars, and the Muscat types were somewhat distinct within the wine grapes. Contingency chi2 analysis indicated significant heterogeneity in allele frequencies among groups at all loci. The observed heterozygosities for different groups ranged from 0.625 to 0.9 with an overall average of 0.771. Genetic relationships among groups suggested hierarchical differentiation within cultivated grape. The gene diversity analysis indicated narrow divergence among groups and that most variation was found within groups (approximately 85%). Partitioning of diversity suggested that the remaining variation is somewhat structured hierarchically at different levels of differentiation. The overall organization of genetic diversity suggests that the germplasm of cultivated grape represents a single complex gene pool and that its structure is determined by strong artificial selection and a vegetative mode of reproduction.     

Genetic Diversity in Wild Grapes Native to China Based on Randomly Amplified Polymorphic DNA (RAPD) Analysis

The use of the RAPD technique was investigated on a set of 73 genotypes of 18 wild grape species native to China, and one interspecific hybrid, seven Vitis vinifera L. cultivars, one rootstock cultivar and one strain of V. riparia L. Genetic diversity among these grapes was investigated based on RAPD analysis. The screening of 280 decamer oligonucleotides allowed the selection of 20 primers used for the analysis. A total of 191 RAPD markers were produced from the 20 selected primers. Relationships among the 83 clones or accessions based on their genetic distances were clustered using unweighted pair-group method arithmetic average (UPGMA) analysis in a dendrogram. Twenty-two clusters which fortunately adapted to 22 grape species level were clearly resolved on the dendrogram. The 18 wild grape species native to China were grouped into ten subclusters. The largest distance was found between V. riparia L., V. vinifera L., interspecific hybrid ( V. vinifera L.× V. larbrusca L.) and the wild grapes native to China. Among the wild grapes native to China, the largest distance was found between V. hancockii Hance and the other wild species. V. qinlingensis P.C.He was the second. Large genetic variation occurred among the different flower-type clones in one species.     

与葡萄抗霜霉病基因紧密连锁的分子遗传标记

以种间杂交组合88-110［83-4-96（毛葡萄,抗霜霉病）×粉红玫瑰（欧洲葡萄,感霜霉病）］的F     

Isolation and characterization of new polymorphic simple sequence repeat loci in grape (Vitis vinifera L.).

Four new simple sequence repeat (SSR) loci (designated VVMD5, VVMD6, VVMD7, and VVMD8) were characterized in grape and analyzed by silver staining in 77 cultivars of Vitis vinifera. Amplification products ranged in size from 141 to 263 base pairs (bp). The number of alleles observed per locus ranged from 5 to 11 and the number of diploid genotypes per locus ranged from 13 to 27. At each locus at least 75% of the cultivars were heterozygous. Alleles differing in length by only 1 bp could be distinguished by silver staining, and size estimates were within 1 or 2 bp, depending on the locus, of those obtained by fluorescence detection at previously reported loci. Allele frequencies were generally similar in wine grapes and table grapes, with some exceptions. Some alleles were found only in one of the two groups of cultivars. All 77 cultivars were distinguished by the four loci with the exception of four wine grapes considered to be somatic variants of the same cultivar, 'Pinot noir', 'Pinot gris', 'Pinot blanc', and 'Meunier'; two table grapes that are known to be synonymous, 'Keshmesh' and 'Thompson Seedless'; and three table grapes, 'Dattier', 'Rhazaki Arhanon', and 'Markandi', the first two of which have been suggested to be synonymous. Although the high polymorphism at grape SSR loci suggests that very few loci would theoretically be needed to separate all cultivars, the economic and legal significance of grape variety identification requires the increased resolution that can be provided by a larger number of loci. The ease with which SSR markers and data can be shared internationally should encourage their broad use, which will in turn increase the power of these markers for both identification and genetic analysis of grape. Key words : grape, Vitis, microsatellite, simple sequence repeat, DNA typing, identification.     

Anthocyanin Profiles in Grape Berry Skins of Different Species of Wine Grapes in Shanxi,China

To understand the anthocyanin characteristics of wine grape varieties, the anthocyanin composition and content of 31 wine grape varieties were analyzed to explore the use of anthocyanins as chemical fingerprints to distinguish varieties. Results showed that a total of 21 anthocyanins were detected in the skins, including cyanidin, delphinidin, petunidin, peonidin and malvidin 3-monoglucosides (or 3,5-diglucosides) along with the corresponding acetyl and p-coumaroyl derivatives. The highest and lowest total amount of anthocyanins were detected in ‘Ruby Cabernet’ and ‘Muscat Rouge’, respectively. In the 21 Vitis vinifera grapes, there were 3~11 monoglucoside anthocyanins detected, however, there were 4 to 9 monoglucoside anthocyanins and 1~7 diglucoside anthocyanins detected in the 10 other species of grapes. Except for ‘Zhesexiang’ ‘Seibel Noir’, ‘44-6-7-1’ and ‘Beibinghong’, the contents of diglucoside anthocyanins in the other six varieties accounted for more than 52% of the total anthocyanins. Except for ‘Zhesexiang’, ‘Muscat Rouge’ and ‘Beibinghong’, the content of methylated anthocyanins accounted for more than 75% of total anthocyanins. There were significant differences in the anthocyanin types and contents in the skins among V. vinifera and other grapes. The results of the principal component analysis and the cluster classification of 31 grape varieties (lines) were nearly consistent, which suggested that anthocyanins can be used as chemical fingerprints to distinguish wine grape varieties.     

Chloroplast phylogenomics of the New World grape species (Vitis,Vitaceae)

Vitis L. (the grape genus) is the economically most important fruit crop, as the source of grapes and wine. Phylogenetic relationships within the genus have been highly controversial. Herein, we employ sequence data from whole plastomes to attempt to enhance Vitis phylogenetic resolution. The results support the New World Vitis subgenus Vitis as monophyletic. Within the clade, V. californica is sister to the remaining New World Vitis subgenus Vitis. Furthermore, within subgenus Vitis, a Eurasian clade is robustly supported and is sister to the New World clade. The clade of Vitis vinifera ssp. vinifera and V. vinifera ssp. sylvestris is sister to the core Asian clade of Vitis. Several widespread species in North America are found to be non‐monophyletic in the plastome tree, for example, the broadly defined Vitis cinerea and V. aestivalis each needs to be split into several species. The non‐monophyly of some species may also be due to common occurrences of hybridizations in North American Vitis. The classification of North American Vitis by Munson into nine series is discussed based on the phylogenetic results. Analyses of divergence times and lineage diversification support a rapid radiation of Vitis in North America beginning in the Neogene.