栽培大豆与半野生大豆杂种F2九体中RFLP标记的偏分离及其形成原因…

本文研究了大豆５６个ＤＮＡ限制性片长度多态性（ＲＦＬＰ）村记在一栽培大豆／半野生大豆杂种Ｆ２群体中的分离,结果表明,２５％的ＲＦＬＰ标记表现了偏分离,偏离的方向主要趋于栽培大豆亲本,其形成原因主要是存在着配子体选择。这对研究大豆的遗传及育种选择等有着重要的指导意义。     

大豆遗传图谱的构建和分析

分子标记连锁图的构建为植物基因组的结构和功能分析提供了有力的工具。较高密度的遗传图谱在数量性状基因定位、图位克隆重要农艺性状基因等研究中发挥了巨大作用。应用栽培大豆长农４和半野生大豆新民６杂交得到的Ｆ８代重组自交系,构建了一张较高密度的遗传图谱。该图谱共有２４０个标记,其中包括２个形态标记、１００个ＲＦＬＰ标记、３３个ＳＳＲ标记、４２个ＡＦＬＰ标记、６２个ＲＡＰＤ标记和１个ＳＣＡＲ标记,分布在２２     

利用RFLP、SSR、AFLP和RAPD标记分析玉米自交系遗传多样性的比较研究

利用 ＲＦＬＰ、ＳＳＲ．ＡＦＬＰ和ＲＡＰＤ ４种分子标记方法研究了 １５个玉米（Ｚｅａ ｍａｙｓ Ｌ．）自交系的遗传多样性,同时对４种标记系统进行比较。在供试材料中筛选到具多态性的ＲＦＬＰ探针酶组合５６个,６６对ＳＳＲ引物,２０个ＲＡＰＤ引物和９个ＡＦＬＰ引物组合,分别检测到多态性带１６７、２０１、８７和１０８条。ＳＳＲ标记位点的平均多态性信息量（ＰＩＣ）最大（０．５４）,ＡＦＬＰ标记位点最小（０．３６）,但ＡＦＬＰ标记具有最高的多态性检测效率（Ａｉ,３２．２）。４种分子标记所得遗传相似系数相关性显著,比较相关系数表明 ＲＡＰＤ可靠性较低。依据 ４种分子标记结果将 １５个供试自交系划分为塘四平头、旅大红骨、兰卡斯特、瑞德和ＰＮ共５个类群,与系谱分析基本一致。认为ＳＳＲ和ＲＦＬＰ两种分子标记方法适合进行玉米种质遗传多样性的研究。     

微卫星DNA和AFLP标记在水稻分子标记连锁图上的分布

以一个栽培稻（ＯｒｙｚａｓａｔｉｖａＬ．ｓｐ．ｉｎｄｉｃａ）和野生稻（Ｏ．ｒｕｆｉｐｏｇｏｎＧｒｉｆ）杂交的Ｆ２作图群体以及由该群体构建的ＲＦＬＰ标记连锁图,分析了微卫星ＤＮＡ和ＡＦＬＰ标记的多态性、遗传行为及其在染色体上的分布。共定位了２８个微卫星ＤＮＡ标记和１７２个ＡＦＬＰ标记。２８个微卫星ＤＮＡ标记中有６个为华中农业大学作物遗传改良国家重点实验室根据数据库中序列而设计,其余２２个来自美国Ｃｏｒｎｅｌ大学已发表的结果。１７２个ＡＦＬＰ标记出自２５对引物扩增得到的２２８个多态性带的片段。这些标记分布于水稻的１２条染色体。将此２００个ＰＣＲ标记与华中农业大学作物遗传改良国家重点实验室构建的ＲＦＬＰ连锁图整合,得到一张含６１２个分子标记位点的遗传连锁图。     

利用RFLP,SSR,AFLP和RAPD标记分析玉米自效系遗传多样性的比较研究

利用ＲＦＬＰ、ＳＳＲ、ＡＦＬＰ和ＲＡＰＤ４种分子标记方法研究了１５个玉米（Ｚｅａ ｍａｙｓ Ｌ．）自交系的遗传多样性,同时对４种标记系统进行比较。在供试材料中筛选到具多态性的ＲＦＬＰ探针酶组合５６个,６７６对ＳＳＲ引物,２０个ＲＡＰＤ引物和９个ＡＦＬＰ引物组合,分别检测到多态性带１６７、２０１、８７和１０８条。ＳＳＲ标记位点的平均多态性检测效率（Ａｉ,３２．２）。４种分子标记所得遗传相似自交系划分     

利用RAPD技术进行植物性状标记及辅助选择

近等基因系、混合分离群体法是ＲＡＰＤ 标记的主要策略。目前,ＲＡＰＤ标记广泛用于抗线虫、抗病、雄性不育等辅助选择的研究中,取得了可喜的成绩。由于遗传距离的不同,使ＲＡＰＤ 标记具有基因型的差异。寻找无重组的ＲＡＰＤ 标记或将ＲＡＰＤ标记转化为ＲＦＬＰ标记,可以解决这一问题。随着连锁程度的降低选择效率也随着降低。相斥相的ＲＡＰＤ标注可提高选择效率将ＲＡＰＤ标记转化为ＳＣＡＲｓ、ＡＰＳＰｓ 标记,可以解决ＲＡＰＤ 标记稳定性差的问题。来源于ＲＡＰＤ 标记的ＳＣＡＲｓ 标记将在辅助选择中发挥巨大的作用。     

扩增片段长度多态性(AFLP)——一种新的分子标记技术

ＡＦＬＰ（扩增性片段长度多态性）是一种新的ＤＮＡ分子标记。与ＲＦＬＰ、ＲＡＰＤ相比,ＡＦＬＰ具有在一次试验中可同时观察到大量的限制性片段的优点。本文阐述了ＡＦＬＰ的原理和方法,综述了ＡＦＬＰ目前在植物遗传育种研究中的应用进展,并对ＡＦＬＰ技术在植物遗传育种中的应用前景提出了初步设想。     

糖单孢菌16S rDNA的PCR-RFLP分析

ＰＣＲ－ＲＦＬＰ分析适用于种和种间水平的多相分类研究。文章对ＰＣＲ－ＲＦＬＰ方法应用于糖单孢菌属分类有具体方法进行了探讨;报道了一组适于糖单孢菌属ＰＣＲ－ＰＦＬＰ分析的限制性内切酶,并用这组酶对６株糖单孢菌属分离株进行了研究,进一步探讨了实验菌株在该属的分类地位。同时指出了ＰＣＲ－ＲＦＬＰ方法应用中应注意的问题。     

一个新的水稻迟熟性基因的遗传分析和分子标记定位

中籼迟熟水稻品系８９８７含未知的长生育期基因,在杂交水稻育种中有重要的利用价值,应用该品系与４个不同生态类型的水稻品种杂交,对其Ｆ１和Ｆ２群体进行生育期调查和遗传分析,确认８９８７的长生育期受１对隐性主效基因控制。以（８９８７Ｘ地谷）Ｆ２群体为基础,应用ＲＦＬＰ和微卫星标记结合群分法,发现第７染色体的ＲＦＬＰ标记Ｃ２１３与该基因连锁;进一步应用Ｆ２分离群体将该基因定位于第７染色体上,暂定名为ｌｆ－３。此基因的发现和定位将有助于分子标记辅助选择和杂交水稻的改良。     

植物种群研究中的分子标记及其应用

综述了植物种群分子生态研究中各种标记法及其应用,包括等位酶、ＡＦＬＰ、ＲＡＰＤ、ＳＳＲ及ＲＦＬＰ等方法,并根据所涉及的有关研究论述及研究工作总结比较了各种方法应用在植物种群学研究中的利弊,强调应依不同的研究目的采用不同的分子标记方法,各种标记方法对解决不同的问题在质和量上是不同的。     

大豆分子标记在RIL群体中的偏分离分析

利用栽培大豆与半野生大豆杂交得到的Ｆ８代重组自交系,对２３８个分子标记的偏分离现象进行了分析。结果表明,２９．４％的位点出现偏分离,并且有偏向母本“长农４号”的趋势。     

Selective Embryo Abortion Hypothesis Revisited - A Molecular Approach

Abstract: Many plant species abort a large fraction of their embryos. It has often been suggested that embryos of genotypes that would perform worse later in life are preferentially aborted. Such selective embryo abortion would lead to investment of resources only in the offspring with the highest potential fitness. Many studies have shown that otherwise viable embryos are aborted. However, only few manipulative studies have indeed shown a correlation between the level of abortion and offspring quality and these studies have been challenged for their experimental design. Molecular techniques open new opportunities to study selective embryo abortion. Non-random abortion at the level of molecular markers can be observed as a deviation from Mendelian segregation: over- or under-representation of markers in the offspring. Subsequently, the over- or under-represented markers can be related to offspring quality later in life. We reviewed the literature on the genetic maps of intraspecific crosses of wild plant species and the selection of cultivated species. The level of non-Mendelian segregation we found in these maps is high. On average, 11.5 % of the tested markers in the genetic maps of wild species and 14.6 % in the cultivated ones, show a departure from Mendelian segregation. From six studies, providing sufficient data, it was calculated that in 68 % of loci segregating in non-Mendelian fashion post-fertilization selection is involved. We propose that the deviation from Mendelian segregation can be partly explained by selective embryo abortion. We describe an experimental design that allows for attributing selective embryo abortion to the non-Mendelian segregation that is found in a genetic map.     

Segregation patterns of isozyme loci and microsatellite markers show the diploidy of African yam Dioscorea rotundata (2n=40)

The cultivated yam species Dioscorea rotundata (2n=40) has been considered by most authors as a tetraploid species with a basic chromosome number of ten. In this paper, we analysed the segregation of two isozyme loci and six microsatellite markers in the progeny of a self-fertilised monoecious plant. For the eight markers, segregation patterns could be explained by only two genetic models: diploidy or tetraploidy with two null alleles. Given the nature of studied markers, the most parsimonious hypothesis was that the parental plant was diploid. These results, data from a diversity survey and results of other authors led to the conclusion that D. rotundata is a diploid species.     

Diversity,genetic mapping,and signatures of domestication in the carrot (Daucus carota L.) genome,as revealed by Diversity Arrays Technology (DArT) markers

Carrot is one of the most economically important vegetables worldwide, but genetic and genomic resources supporting carrot breeding remain limited. We developed a Diversity Arrays Technology (DArT) platform for wild and cultivated carrot and used it to investigate genetic diversity and to develop a saturated genetic linkage map of carrot. We analyzed a set of 900 DArT markers in a collection of plant materials comprising 94 cultivated and 65 wild carrot accessions. The accessions were attributed to three separate groups: wild, Eastern cultivated and Western cultivated. Twenty-seven markers showing signatures for selection were identified. They showed a directional shift in frequency from the wild to the cultivated, likely reflecting diversifying selection imposed in the course of domestication. A genetic linkage map constructed using 188 F2 plants comprised 431 markers with an average distance of 1.1 cM, divided into nine linkage groups. Using previously anchored single nucleotide polymorphisms, the linkage groups were physically attributed to the nine carrot chromosomes. A cluster of markers mapping to chromosome 8 showed significant segregation distortion. Two of the 27 DArT markers with signatures for selection were segregating in the mapping population and were localized on chromosomes 2 and 6. Chromosome 2 was previously shown to carry the Vrn1 gene governing the biennial growth habit essential for cultivated carrot. The results reported here provide background for further research on the history of carrot domestication and identify genomic regions potentially important for modern carrot breeding.     

Qtl Analysis of Transgressive Segregation in an Interspecific Tomato Cross

Two accessions, representing the species Lycopersicon esculentum (cultivated tomato) and Lycopersicon pennellii (a wild relative), were evaluated for 11 quantitative traits and found to be significantly different for 10 of the traits. Transgressive segregation was observed for eight of the traits in a large interspecific F(2) population. When restriction fragment length polymorphism markers were used as probes for the quantitative trait loci (QTL) underlying the traits, 74 significant QTL (LOD > 2) were detected. Thirty-six percent of those QTL had alleles with effects opposite to those predicted by the parental phenotypes. These QTL were directly related to the appearance of transgressive individuals in the F(2) for those traits which showed transgressive segregration. However, the same types of QTL (with allelic effects opposite to those predicted by the parents) were also observed for traits that did not display transgressive segregation in the F(2). One such trait was dry weight accumulation. When two overdominant QTL (detected in the F(2)) for this trait were backcrossed into the L. esculentum genetic background, transgressive individuals were recovered and their occurrence was associated with the two QTL demonstrating the potential for transgressive segregation for all characters and implicating overdominance as a second cause of transgressive segregation. Epistasis was not implicated in transgressive segregation in either the F(2) or backcross generations. Results from this research not only reveal the basis of wide-cross transgressive segregation, but demonstrate that molecular markers can be used to identify QTL (from wild species) responsible for transgressive phenotypes and to selectively transfer them into crop species. This strategy might be used to improve many traits of economic importance including those for which wild species appear phenotypically inferior to their cultivated counterparts.     

Evidence for tetrasomic inheritance in a tetraploid Solanum commersonii (+) S. tuberosum somatic hybrid through the use of molecular markers

In order to assess the potential for interspecific recombination between the cultivated Solanum tuberosum (tbr) and the sexually isolated wild species Solanum commersonii (cmm), genetic analysis of a F₂ progeny obtained by selfing one tetraploid cmm (+) tbr somatic hybrid was performed through molecular markers. For this purpose, the extent of disomic and/or tetrasomic inheritance of species-specific RAPD and AFLP markers was determined by following their segregation in a 90-genotype progeny, and testing all the possible segregation ratios in a selfed tetraploid progeny. The RAPD analysis performed using 16 primers revealed that the cmm-specific RAPDs were mainly (93.7%) duplex markers and were equally distributed between loci with a disomic (46.7%) and tetrasomic (53.3%) inheritance. The AFLP analysis led to the identification of 272 (58%) informative AFLPs, which were either cmm- or tbr-specific markers. About 63% of cmm-specific AFLPs were duplex loci, most of which (92.6%) were inherited as tetrasomic loci. As regards the tbr-specific AFLPs, the percentage of simplex loci (52.9%) was higher than that of duplex loci (32.6%), and among the latter most (88.5%) were inherited as tetrasomic loci. Overall, 130 duplex markers were found, of which 53.1% were cmm-specific and 46.9% were tbr-specific. Out of 130 markers, 18 (13.8%) were inherited as disomic, and 112 (86.2%) as tetrasomic, loci. This implies that the majority of duplex markers were located on chromosomes which at meiosis tend to randomly pair as bivalents or to form tetravalents. The total number of simplex loci was 119, and most of them (82.3%) were tbr-specific loci. In some cases the observed segregation ratios even allowed us to clearly determine whether a random chromosome or chromatid segregation was detected. This was the case of three cmm-specific RAPDs, 19 cmm- and 25 tbr-specific AFLPs, which fit a 20.8:1 or 2.5:1 ratio, both cases for which a clear random chromatid segregation can be assumed, since they represent the limit of segregation expected when the distance between the locus and the centromere always leads to a cross-over event. The percentage of ascertained crossing-over events was around 37% out of the tetrasomically inherited loci clearly identified (128 loci), a value indicating that the flow of genes from the sexually isolated S. commersonii to the cultivated potato is possible, for at least a large proportion of genes. Received: 23 July 2001 / Accepted: 9 August 2001     

Production of inbred progenies of diploid potatoes using an S-locus inhibitor (Sli) gene, and their characterization.

To develop inbred lines from self-incompatible, cultivated diploid potatoes, an S-locus inhibitor (Sli) gene derived from a self-compatible variant of a wild potato species, Solanum chacoense, was incorporated into various cultivated diploid potatoes. The progeny was selfed twice by the action of the Sli gene to obtain 74 S2 inbred clones belonging to 8 families. More than 40% of them were either non-flowering or pollen sterile. Among the pollen fertile clones, self-compatible clones occurred with a much lower frequency (20.9%) than expected (83.3%). The result demonstrated that self-compatibility was introduced and expressed in the gene pool of cultivated diploid potatoes by an action of the Sli gene, although serious inbreeding depression associated with selfing occurred. The genotypes of S2 inbreds were surveyed using 46 S. chacoense-specific RFLP (restriction fragment length polymorphism) markers covering the whole potato genome. More than half of the markers (67.4%) showed distorted segregation. Particularly, all markers on chromosome 12 were overrepresented in the S2 inbreds. This confirms our earlier finding that the Sli gene locates on chromosome 12 and the alleles linked with this gene are preferentially transmitted because of its essential requirement for selfing.     

Construction of an RFLP linkage map for cultivated sunflower

 An RFLP linkage map was constructed for cultivated sunflower Helianthus annuus L., based on 271 loci detected by 232 cDNA probes. Ninety-three F₂ plants of a cross between inbred lines RHA 271 and HA 234 were used as the mapping population. These genetic markers plus a fertility restoration gene, Rf ₁, defined 20 linkage groups, covering 1164 cM of the sunflower genome. Of the 71 loci 202 had codominant genotypic segregation, with the rest showing dominant segregation. Thirty-two of the 232 probes gave multiple locus segregation. There were 39 clusters of tightly linked markers with 0 cM distance among loci. This map has an average marker-to-marker distance of 4.6 cM, with 11 markerless regions exceeding 20 cM. Received: 17 June 1997 / Accepted: 19 June 1997     

Linkage mapping of Hsa-1<Superscript>Og</Superscript>, a resistance gene of African rice to the cyst nematode, <Emphasis Type="Italic">Heterodera sacchari</Emphasis>

Inheritance of resistance to cyst nematode (Heterodera sacchari) in Oryza sativa was investigated by inoculation tests with isolate 244 from Congo in segregating populations derived from hybridisation between O. sativa and its African sister cultivated species, O. glaberrima. We found that the resistance was controlled by one major gene, Hsa-1(Og), with codominance of susceptible and resistant alleles. To map Hsa-1(Og) on the rice genome, we pooled the data obtained from segregation of the resistance trait and microsatellite markers in three kinds of progeny: BC(1)F(3), BC(1)F(4), and pseudo-F(2) populations. Hsa-1(Og) was unambiguously located between Cornell University's RM206 and RM254 markers on chromosome 11. Two additional microsatellite markers derived from Monsanto publicly available sequences were found to be tightly linked to the Hsa-1(Og) gene. It is possible that numerous plant resistances to a pathogen in fact exhibit a codominant inheritance, possibly explaining misleading conclusions in several reports on resistance segregation.     

大豆遗传图谱的构建和分析

利用大豆栽培品种科丰1号和南农1138－2杂交得到的重组近交系NJRIKY,通过RFLP,SSR,RAPD和AFLP4种分子标记的遗传连锁分析,构建了包含24个连锁群,由792个遗传标记组成的大豆较高密度连锁图谱,该图谱覆盖2320．7cM,平均图距2．9cM,SSR标记的多态性较高,在基因组中的位置相对稳定,可以作为锚定标记,有利于连锁群的归并和不同图谱的比较整合;而AFLP标记对于增加图谱密度效率较高,但其容易出现聚集现象,从而造成连锁群上有很大的空隙（gap),另外,在连锁群中有21．7％的分子标记出现偏分离,该图谱为基因定位,比较基因组学和重要农艺性状的QTL定位等研究打下了基础。