水稻端粒相关序列的克隆及鉴定

端粒不仅包括简单的端粒重复序列 ,也包括较复杂的端粒相关序列 .参照拟南芥菜的端粒重复序列 (TTTAGGG) _n,设计了 2个引物 :(TTTAGGG) ₃ 和 (CCC TAAA) ₃ CCC .利用单引物采取 2种方法在水稻中进行PCR圹增 ,得到了 8个片段 .然后用Bal31酶解和RFLP图谱定位的方法检测了它们的亚端粒特性 .用此方法鉴定了 6个端粒相关序列 ,分别定位于水稻第 5 ,6 ,7,9号染色体 .     

一个含端粒序列的水稻BAC克隆的分析和定位

对一个含 (TTTAGGG) _n 同源序列的水稻BAC克隆 (BAC2 )进行了分析 ,揭示出水稻近端区DNA的组成 .BAC2的插入片段中除含有大量的以串联形式存在的称之为TA35 2序列的卫星DNA外 ,还含有TTTAGGG或其变体组成的简单重复 .荧光原位杂交 (FISH)将含 (TTTAGGG) _n 序列的 0 .8kbPstⅠ片段定位在至少 5对染色体的端粒区 .通过对BAC2中低拷贝序列的RFLP分析 ,BAC2被定位在水稻第 6号染色体端部 .这些结果说明水稻的端粒序列可能也是TTTAGGG或其变体构成的简单重复 ,而与其相连的卫星DNATA35 2则属于端粒相关序列 .     

在植物粗线期染色体和DNA纤维上的荧光原位杂交技术

介绍了两种荧光原位杂交技术的详细实验步骤。第一种技术是在减数分裂粗线期染色体上的荧光原位杂交,包括从花粉母细胞中制备粗线期染色体和在这种染色体上定位ＤＮＡ序列,其分辨率水平能够达到１００ｋｂ。第二种技术是从植物细胞核中制备ＤＮＡ纤维,并在上面进行原位杂交,能够直接分析ＤＮＡ序列的分子排列关系,其分辨率水平能达到几个ｋｂ。为了说明这两种原位杂交技术在研究基因组和染色体结构、构建高分辨率的ＤＮＡ物理图谱上的能力,将展示用该技术直接分析番茄染色体端粒重复序列和端粒联接重复序列的染色体定位和ＤＮＡ分子排列。     

端粒保护蛋白

端粒保护蛋白（pmtection of telomere 1,PoT1）是存在于人和裂殖酵母的端粒相关蛋白,特异性地与端粒单链DNA相结合。人POT1基因位于7号染色体上,由22个外显子组成,其中4个外显子属于跳跃外显子,可形成5个剪接变异体。POT1的功能在于维持端粒的稳定,通过TRF1．TIN2．PIP1-POT通路调节端粒长度。     

筛选和定位含水稻端粒相关序列的BAC克隆

根据水稻的端粒重复序列 ,设计了 2个引物 :(TTTAGGG) ₃ 和 (CCC TAAA) ₃ CCC ,利用单引物在水稻总DNA中进行PCR扩增 ,分别得到Tas1和Tas2 .这 2个片段在定位亲本间均无多态性 .Tas1的原位杂交表明该序列位于 2对染色体端部 .以Tas1为探针在所构建的水稻基因组BAC文库中筛选到 1个克隆 ,South ern杂交证明此克隆也包含序列Tas2 ,取该克隆中的单拷贝序列利用ZYQ/JX1 7DH群体将其定位在第 6号染色体的端部 .并对Tas1和Tas2在此克隆中的排列进行了初步研究     

上位性和QTL×环境互作对水稻(Oryza sativa L.)抽穗期的影响

水稻抽穗期是重要的农艺性状之一,对水稻品种的地理分布和适应性起到关键性作用。适宜的抽穗期是获得高产的前提。因此确定水稻抽穗期的遗传基础在育种计划中具有重要的意义。本研究用一套来源于亲本IR64/Azucena的双单倍体（DH）群体在两个种植季节的试验资料,用基于混合线性模型的复合区间作图方法,对水稻抽穗期QTL的加性、上位性及其与环境互作效应进行了研究。结果表明共有14个QTL影响水稻抽穗期,它们分布在除第5和第9条染色体外的10条染色体上,有8个位点携带单位点效应,5对位点携带双位点互作效应,2个单位点和1对双位点存在与环境的互作,所有效应值介于1.179～2.549天之间,相应的贡献率为1.04%～4.84%。基于所估算的QTL效应值,本研究预测了两个亲本和两个极端型品系的遗传效应值,并讨论了影响遗传效应值与实际观测值偏差的可能原因,以及研究群体所具有的遗传潜力。对水稻抽穗期QTL的定位结果与前人研究基本一致,并进一步证实了上位性和QE互作效应是水稻抽穗期的重要遗传基础。     

一种含有端粒重复序列非编码RNA的发现及最新研究进展

端粒是染色体末端的特化结构,由简单呈串联线性排列的核酸重复序列及相关蛋白质组成。其核酸序列具有高度的保守性,均富含GC。在人类为TTAGGG的高度重复序列具有维持基因组完整性的作用。端粒功能异常会导致染色体失去稳定性,促进肿瘤的发生和发展。以往认为端粒附近区域不具有转录活性,但最近在Science杂志上Azzalin等首次报道了该区域可以转录一种非编码RNA,即端粒RNA(telomeric RNA)。该分子具有特殊的UUAGGG重复序列,在调控端粒长度和端粒酶活性上具有重要作用,在发育、衰老和肿瘤发生发展等研究中已成为热点。该文将对近期有关端粒RNA的研究进展予以综述。     

老幼龄扬子鳄端粒相对长度的差异性分析

端粒（Telomere）是线性真核细胞染色体末端的一种结构,由高度重复的DNA序列和结合蛋白所构成。在脊椎动物中,端粒通常为富含TG简单重复序列（TFAGGG）,其生物学功能是完成染色体末端复制,使DNA免受不恰当的修复以及防止端一端融合和核酸外切酶的降解（Dreesen et al．,2007）。     

端粒保护蛋白TRF2的研究进展

端粒是染色体末端的核蛋白结构。染色体末端重复的端粒DNA可以规避不适当的DNA损伤反应(DNA damage response, DDR)的激活,维持染色体的稳定性,端粒的缺失会引起染色体融合并导致细胞的衰老及死亡。端粒特异性蛋白复合物Shelterin在保护端粒完整性方面具有重要作用。在这个复合体中,端粒结合因子2 (telomeric-repeat binding factor 2, TRF2)在维持端粒稳定、防止端粒染色体末端融合以及端粒染色体复制过程中发挥关键作用。该文综述了TRF2介导的保护染色体末端的多方面的机制。     

基于CSSL的水稻抽穗期QTL定位及遗传分析

抽穗期是水稻（Oryza sativa）品种的重要农艺性状之一,适宜的抽穗期是获得理想产量的前提。鉴定和定位水稻抽穗期基因/QTL,分析其遗传效应对改良水稻抽穗期至关重要。以籼稻品种9311（Oryzasativa ssp.indica‘Yangdao 6’）为受体,粳稻品种日本晴（Oryza sativa ssp.japonica‘Nipponbare’）为供体构建的94个染色体片段置换系群体为材料,以P≤0.01为阈值,对置换片段上的抽穗期QTL进行了鉴定。采用代换作图法共定位了4个控制水稻抽穗期的QTL,分别位于第3、第4、第5和第8染色体;QTL的加性效应值变化范围为–6.4––2.7,加性效应百分率变化范围为–6.4%––2.7%;qHD-3和qHD-8加性效应值较大,表现主效基因特征。为了进一步定位qHD-3和qHD-8,在目标区域加密16对SSR引物,qHD-3和qHD-8分别被界定在第3染色体RM3166–RM16206之间及第8染色体RM4085–RM8271之间,其遗传距离分别为13.9cM和6.4cM。研究结果为利用分子标记辅助选择改良水稻抽穗期奠定了基础。     

Clustering of C2-H2 zinc finger motif sequences within telomeric and fragile site regions of human chromosomes.

Ninety-three phage clones identified by hybridization with a C2-H2 zinc finger sequence probe have been grouped into 23 genetic loci. Partial sequencing verified that each locus belonged to the zinc finger family. Oligonucleotide primer pairs were developed from these sequences to serve as STS markers for these loci. One or more clones from each locus was mapped onto human metaphase chromosomes by fluorescence in situ hybridization. Several loci map to identical chromosomal regions, indicating the possible presence of multigene clusters. Zinc finger loci were found to reside predominantly either in telomeric regions or in chromosomal bands known to exhibit chromosome fragility. Chromosome 19 carries a disproportionate fraction (10 of 23) of the mapped zinc finger loci.     

Clustering of C2---H2 zinc finger motif sequences within telomeric and fragile site regions of human chromosomes

Ninety-three phage clones identified by hybridization with a C₂---H₂ zinc finger sequence probe have been grouped into 23 genetic loci. Partial sequencing verified that each locus belonged to the zinc finger family. Oligonucleotide primer pairs were developed from these sequences to serve as STS markers for these loci. One or more clones from each locus was mapped onto human metaphase chromosomes by fluorescence in situ hybridization. Several loci map to identical chromosomal regions, indicating the possible presence of multigene clusters. Zinc finger loci were found to reside predom nantly either in telomeric regions or in chromosomal bands known to exhibit chromosome fragility. Chromosome 19 carries a disproportionate fraction (10 of 23) of the mapped zinc finger loci.     

Genetic mapping of hypervariable minisatellite sequences in rice (Oryza sativa L.)

Minisatellites, or DNA fingerprinting sequences, have been utilized in animal linkage studies for several years but have not been used as markers for plant genome mapping. In animal genome mapping they have resulted in limited success because they are evenly dispersed in some species but are often clustered near telomeric regions, as observed on human chromosomes. The purpose of the present study was to generate DNA fingerprints utilizing several rice-derived minisatellites containing different core sequences and numbers of repeat units, followed by assessing their potential for use as genetic markers when mapped to a rice recombinant inbred line (RIL) population. Sites of segregating minisatellite loci were mapped onto 11 of the 12 rice RIL linkage maps. The implications for the use of rice minisatellite core sequences as genetic markers on linkage maps in rice are discussed. Received: 1 March 1999 / Accepted: 22 June 1999     

A mapped set of DNA markers for human chromosome 17

We have developed and mapped by genetic linkage a primary set of markers for chromosome 17. The map consists of 21 loci derived from 27 probe/enzyme systems, including eight highly informative markers at loci containing a variable number of tandemly repeated DNA sequences (VNTRs). The map is continuous from the telomeric region of the short arm to the telomeric region of the long arm, covering estimated genetic distances of 218 cM in males and 279 cM in females. The average heterozygosity among all 21 loci in the population sample analyzed is 58%; 77% heterozygosity was observed among the eight VNTR markers that were highly informative. This map will make it possible to detect by linkage the location of genetic defects associated with chromosome 17 and will also provide anchor points for a high-resolution map of this chromosome.     

A genetic linkage map of 41 restriction fragment length polymorphism markers for human chromosome 3.

A genetic linkage map for human chromosome 3 has been constructed using 41 polymorphic DNA markers genotyped in 40 CEPH reference families. The map spans a genetic distance of 261 cM in males and 413 cM in females; the ratio of these distances (approximately 1.6 in favor of female meioses) was fairly constant across the map. Frequency of recombination was relatively uniform throughout much of the chromosome, except that in both telomeric regions recombination was more frequent than the physical distances would predict. The genetic map was basically in agreement with physical localization of 24 loci that were mapped by fluorescent in situ hybridization. This map can be used for linkage studies for genetic diseases, and it will serve as a step toward a high-resolution map for human chromosome 3.     

水稻日本晴与广陆矮4号杂交F2群体SSR标记偏分离原因探析

以全基因组测序已经完成的材料粳稻日本晴和完成了第4染色体全序列测序的籼稻广陆矮4号的杂交F2作为构图群体,共90个单株,构建了一张含148个微卫星标记的水稻分子遗传图谱。该F2群体显著偏分离非常高,发现有49个分子标记表现偏分离（P〈0．05）,占总标记数的33．11％,这些偏分离标记中有36个偏向广陆4号,13个偏向杂合体,没有偏向日本晴的偏分离标记。讨论了配子体基因和孢子体基因导致偏分离的原因,通过已经定位的配子体基因和杂种不育基因分布在偏分离集中的区域来进一步说明配子体基因和杂种不育基因确实是导致偏分离形成的原因,而且还通过未定位的标记分析了偏分离的原因。     

A high-density cytogenetic map of the Aegilops tauschii genome incorporating retrotransposons and defense-related genes: insights into cereal chromosome structure and function

Aegilops tauschii (Coss.) Schmal. (2n = 2x = 14, DD) (syn. A. squarrosa L.; Triticum tauschii) is well known as the D-genome donor of bread wheat (T. aestivum, 2n = 6x = 42, AABBDD). Because of conserved synteny, a high-density map of the A. tauschii genome will be useful for breeding and genetics within the tribe Triticeae which besides bread wheat also includes barley and rye. We have placed 249 new loci onto a high-density integrated cytological and genetic map of A. tauschii for a total of 732 loci making it one of the most extensive maps produced to date for the Triticeae species. Of the mapped loci, 160 are defense-related genes. The retrotransposon marker system recently developed for cultivated barley (Hordeum vulgare L.) was successfully applied to A. tauschii with the placement of 80 retrotransposon loci onto the map. A total of 50 microsatellite and ISSR loci were also added. Most of the retrotransposon loci, resistance (R), and defense-response (DR) genes are organized into clusters: retrotransposon clusters in the pericentromeric regions, R and DR gene clusters in distal/telomeric regions. Markers are non-randomly distributed with low density in the pericentromeric regions and marker clusters in the distal regions. A significant correlation between the physical density of markers (number of markers mapped to the chromosome segment/physical length of the same segment in microm) and recombination rate (genetic length of a chromosome segment/physical length of the same segment in microm) was demonstrated. Discrete regions of negative or positive interference (an excess or deficiency of crossovers in adjacent intervals relative to the expected rates on the assumption of no interference) was observed in most of the chromosomes. Surprisingly, pericentromeric regions showed negative interference. Islands with negative, positive and/or no interference were present in interstitial and distal regions. Most of the positive interference was restricted to the long arms. The model of chromosome structure and function in cereals with large genomes that emerges from these studies is discussed.     

An interspersed repeated sequence specific for human subtelomeric regions.

A family of DNA loci (DNF28) from the pseudoautosomal region of the human sex chromosomes is characterized by a repeated element (STIR: subtelomeric interspersed repeat) which detects homologous sequences in the telomeric regions of human autosomes by in situ hybridization. Several STIR elements from both the pseudoautosomal region and terminal parts of autosomes were cloned and sequenced. A conserved 350 bp sequence and some characteristic structural differences between the autosomal and pseudoautosomal STIRs were observed. Screening of the DNA sequence databases with a consensus sequence revealed the presence of STIRs in several human loci localized in the terminal parts of different chromosomes. We mapped single copy probes flanking the cloned autosomal STIRs to the subtelomeric parts of six different chromosomes by in situ hybridization and genetic linkage analysis. The linkage data show a greatly increased recombination frequency in the subtelomeric regions of the chromosomes, especially in male meiosis. The STIR elements, specifically located in subtelomeric regions, could play a role in the peculiar recombination properties of these chromosomal regions, e.g. by promoting initiation of pairing at meiosis.     

Analysis of Segregation Distortion of Molecular Markers in F2 Population of Rice

A genetic linkage map comprising 148 SSR markers loci was constructed using an F₂ population consisting of 90 lines derived from a sub-specific cross between a japonica variety Nipponbare and an indica variety Guangluai-4. The F₂ population showed high significantly distorted segregations. Among these SSR markers, 49 markers (33.11%) showed the genetics distortion(P<0.05). Of them, 36 markers deviated toward male parent indica GuangLuAi-4 and 13 markers toward heterozygote, but none toward the female parent Nipponbare. It was found that the segregation distortion might be caused by gametophyte and zygote. Since most gametophyte loci and sterility loci were mapped in segregation distortion regions, it indicated that the segregation distortion may be caused by these gametophyte loci and sterility loci. Finally, this research also analyzed the skewed segregation of some markers, which had not been mapped on chromosome.     

A genetic linkage map for coho salmon (Oncorhynchus kisutch)

Construction of genetic linkage maps is an important first step for a variety of genomic applications, such as selective breeding in aquaculture, comparative studies of chromosomal evolution and identification of loci that have played key roles in the evolution of a species. Here we present a sex-specific linkage map for coho salmon. The map was constructed using 148 AFLP markers, 133 microsatellite loci and the phenotypic locus SEX . Twenty-four linkage groups spanning 287.4 cM were mapped in males, and 33 linkage groups spanning 429.7 cM were mapped in females. Several male linkage groups corresponded to two female linkage groups. The combination of linkage groups across both sexes appeared to characterize regions of 26 chromosomes. Two homeologous chromosomes were identified based on information from duplicated loci. Homologies between the coho and rainbow trout maps were examined. Eighty-six loci were found to form common linkage relationships between the two maps; these relationships provided evidence for whole-arm fissions, fusions and conservation of chromosomal regions in the evolution of these two species.