Cloning of genomic DNA of rice 5-enolpyruvylshikimate 3-phosphate synthase gene and chromosomal localization of the gene

The shikimate pathway enzyme 5-enolpyruvylshikimate 3-phosphate synthase (EPSPs) is the target of nonselective herbicide glyphosate. A partial rice epsps cDNA was generated by RT-PCR with primers designed according to EST sequence in GenBank and used as probe for rice genomic library screening. In a screen of approximately 8.0×104 clones from the rice genomic library, sixteen positive clones were obtained, which strongly hybridized to the probe. One clone, E11, was selected for further analysis and the full-length 3661 bp rice epsps genomic sequence was obtained. Sequence analysis and homologous comparison revealed that epsps gene is composed of 8 exons and 7 introns. Analysis by restriction fragment length polymorphism with the probe of rice epsps cDNA fragment confirmed that rice epsps is located on chromosome 6 with an indica-japonica (ZYQ8-JX17) double-haploid (DH) population. This is the first report on the EPSP synthase from monocotyledons.     

Complete chloroplast genome sequence of Magnolia grandiflora and comparative analysis with related species

Magnolia grandiflora is an important medicinal,ornamental and horticultural plant species.The chloroplast(cp) genome of M.grandiflora was sequenced using a 454 sequencing platform and the genome structure was compared with other related species.The complete cp genome of M.grandiflora was 159623 bp in length and contained a pair of inverted repeats(IR) of 26563 bp separated by large and small single copy(LSC,SSC) regions of 87757 and 18740 bp,respectively.A total of 129 genes were successfully annotated,18 of which included introns.The identity,number and GC content of M.grandiflora cp genes were similar to those of other Magnoliaceae species genomes.Analysis revealed 218 simple sequence repeat(SSR) loci,most composed of A or T,contributing to a bias in base composition.The types and abundances of repeat units in Magnoliaceae species were relatively conserved and these loci will be useful for developing M.grandiflora cp genome vectors.In addition,results indicated that the cp genome size in Magnoliaceae species and the position of the IR border were closely related to the length of the ycf1 gene.Phylogenetic analyses based on 66 shared genes from 30 species using maximum parsimony(MP) and maximum likelihood(ML) methods provided strong support for the phylogenetic position of Magnolia.The availability of the complete cp genome sequence of M.grandiflora provides valuable information for breeding of desirable varieties,cp genetic engineering,developing useful molecular markers and phylogenetic analyses in Magnoliaceae.     

耐辐射奇球菌超氧化物歧化酶基因的克隆与序列分析

By using a 453 bp length gene fragment of superoxide dismutase(SOD)as a probe,which was firstly amplified from Deinococcus radiodurans genomic DNA by PCR with degenerate oligonucleotide primers corresponding to the conservative regions of known SODs,a putative SOD gene was identified from the database of D.radiodurans whole genome.Its 636 bp length open reading frame and 5′ and 3′ flanking sequence was determined.The conventional E.coli ribosomal and RNA polymerase binding sites were found upstream from SOD encoding region and an inverted repeat sequence downstream of the termination codon.The deduced 211 amino acid sequence of the structural gene showed a high similarity to other manganese and iron containing SODs in normally conserve regions.     

Paternal inheritance of mitochondrial DNA in the sheep (Ovine aries)

Paternal inheritance of mitochondria DNA in sheep was discovered by examination of 152 sheep from 38 hybrid families for mtDNA D-loop polymorphisms using PCR-RFLP, amplification of repeated sequence somain, and PCR-SSCP of the D-loop 5' end region of a 253 bp fragment. Our findings have provided the first evidence of paternal inheritance of mtDNA in sheep and possible mechanisms of paternal inheritance were discussed.     

Molecular mapping of split rice spikelet mutantsrs-1 and analysis of its homeotic function in rice

srs-1, a new floral organ identity gene in rice, was mapped using RAPD and RFLP markers. Firstly, the cross was made between "ZhaiYeQing 8" (ZYQ8, indica) and split rice spikelet (SRS, japonica) mutant. The ratio of wild-type individuals and mutant plants in F2 population is 3:1, which indicates that the mutant characteristics are controlled by single recessive gene, srs-1. Consequently, BSA method was adopted and 520 random 10-mer primers were used to screen polymorphic bands between two bulks. Six primers could amplify polymorphic bands, of which S465 generates the most stable RAPD patterns. Then, S465 that cosegregates in F2 population has been converted into an RFLP marker successfully. Furthermore, srs-1 gene was mapped on chromosome 3 using DH mapping population. The effect of srs-1 gene results in the mutant of split rice spikelet. The mutant has longer and softer palea/lemma than those of wild-type, and two small palea/lemma-like organs between palea and lemma. In addition, there is a flower wit     

RFLP mapping of major and minor genes for important agronomic characters in rice

A molecular genetic map with 233 RFLP markers which covered about 2070 cM of rice genome was constructed based on a doubled haploid (DH) population derived from anther culture of a cross between an indica variety Gui630 and a japonica variety 02428. Quantitative trait loci (QTLs) for agronomic characters such as number of panides, heading date, plant height, number of spikelets, number of grains, fertility and 1 000-grain weight were analyzed using interval mapping approach. 8 major genes and 29 minor genes were identified associating with these traits. The results also indicated that great phenotypic difference between parents was profitable in detection of major genes.     

Construction of a full bacterial artificial chromosome （BAC） library of Oryza sativa genome

We have constructed a full BAC library for the superior early indica variety of Oryza sativa,Guang Lu Ai 4.The MAX Efficiency DH10B with increased stability of inserts was used as BAC host cells.The potent pBelo BACII with double selection markers was used as cloning vector.The cloning efficiency we have reached was as high as 98%,and the transformation efficiency was raised up to 10^6 transformants/μg of large fragment DNA.The BAC recombinant transformants were picked at random and analyzed for the size of inserts,which turned out to be of 120 kb in length on average.We have obtained more than 20,000 such BAC clones.According to conventional probability equation,they covered the entire rice genome of 420,000 kb in length.The entire length of inserts of the library obtained has the 5-to 6-fold coverage of the genome.To our knowledge,this is the first reported full BAC library for a complex genome.     

水稻胞质核糖体蛋白基因OsRPS7的克隆与序列分析

以已公布的黑麦胞质核糖体蛋白基因ScRPS7的cDNA序列为信息探针,在中国华大水稻基因组数据库中搜索与之高度同源的基因组重叠群。采用计算机拼接和RT-PCR方法克隆了水稻胞质核糖体蛋白基因的全长cDNA序列,命名为OsRPS7。该cDNA序列全长919bp,编码192个氨基酸;其与黑麦、拟南芥和芸薹的S7核糖体蛋白的氨基酸一致率分别为88%、72%和72%。对OsRPS7 的基因组结构和基因的功能进行了分析和预测。Abstract：Using the cDNA of rye cytoplasmic ribosomal protein ScRPS7 as a query probe, a highly homologous rice genomic contig was obtained from Huada rice genome database. The full-length cDNA sequence of rice cytoplasmic ribosomal protein S7 was assembled by informatics based on the contig. Furthermore, with the two primers designed according to this assembled cDNA, the full-length cDNA of rice ribosomal protein was cloned by RT-PCR and named as OsRPS7. The cDNA was 919bp in length and contained a complete Open Reading Frame (ORF) of 576bp, encoding a protein of 192 amino acid residues. The deduced amino acids of OsRPS7 showed 88%、72% and 72% identity with those from Secale cereale、Arabidopsis thaliana and Brassica oleracea, respectively. The genome structure of OsRPS7 was analyzed, and its function was predicted in this paper.     

Cloning and Sequence Analysis of Genome from the Inner Mongolia Strain of the Endogenous Betaretroviruses （enJSRV）

In order to amplify the complete genome of enJSRV from the strain of Inner Mongolia （enJSRV-NM）, we used enJSRV-specific and JSRV-specific DNA probes in dot blot hybridization. Seven pairs of primers were designed based on Genbank sequences. Seven fragments were obtained by PCR and were cloned into the PMD19-T vectors. The recombinant plasmids were sequenced and analyzed. The results showed that the genome was 7 942 bp in length and contained four overlapping open reading frames corresponding to the gag, pro, pol and env genes as well as an additional open reading frame （orf-x） that overlaps the 3＇ end of the pol gene. The nucleotide acid sequences of the enJSRV-NM loci were compared with the sequences of South Africa enJS56A1 strain （Accession No.AF153615） and USA JSRV21 strain （Accession No. AF105220）. The nucleotide acid identities were 99.2% and 92.3% respectively. Two zinc fingers were found in the NC region in the predicted amino acid sequence. However, the YXXM motif, which is a reliable molecular marker for the infectious exogenous virus, was not found in the TM region. It was found that the enJSRV-NM region was 90%-98% identical at the amino acid level to its exogenous infectious counterparts in most of the retroviral genome. This is the first nucleotide sequence of enJSRV reported in P.R China. The resource work has provided a wide range of information useful not only for expression genomics and annotation of genomic DNA sequence, but also for further research on the clinical diagnosis of OPA.     

水稻双单倍体群体的分子标记图示基因型分析

利用窄叶青８号（籼稻）／京系１７（粳稻）花培产生的双单倍体群体建立了一个包含１６０个分子标记的遗传连锁图,在此基础上利用ＨＹＰＥＲＧＥＮＥ软件建立了５２个ＤＨ系的图示基因型,并对ＤＨ系的亲本基因组比率和染色体的交换重组频率进行了比较分析。结果表明本实验所用的ＤＨ群体没有显著偏离正态分布,籼粳稻杂交后代中植株的籼粳表现与同工酶、形态指数和基因组比率的分析结果一致,此外还发现ＤＨ群体中出现了大量的交换罕见染色体。利用图示基因型分析发现株高和分子标记ＲＺ９７８和ＲＧ４Ａ相关,生育期和ＲＲＫ０８－１、ＲＧ４７７和ＲＧ５１１相关。本文还就图示基因型分析技术在ＤＨ群体的遗传分析和选择育种中的应用进行了讨论．     

水稻纹枯病抗性QTL分析

对灿稻窄叶青8号（ZYQ8）和粳稻京系17（JX17）以及由它们构建的加倍单倍体（DH）群体,分别在杭州和海南岛,采用注射器接种法进行纹枯病抗性鉴定,并使用该群体的分子链锁图谱进行数量性状座位（QTL）分析。共检测到4个抗纹枯病的QTL（qSBR-2、qSBR-3、qSBR-7和qSBR-11）,分别位于第2、第3、第7和第11染色体。其中qSBR-2、qSBR-3、qSBR-7的抗性基因由抗病亲本ZYQ8贡献,而qSBR-11的抗性基因来自感病亲本JX17。qSBR-2、qSBR-3、qSBR-7在杭州和海南岛都能检测到,而qSBR-11只在杭州检测到。在杭州的实验中,纹枯病病级与秆长和抽穗期呈显著负相关;在控制秆长和抽穗期的QTL中,控制秆长的qCL-3与qSBR-3位于同一染色体区域,其余QTL与抗纹枯病的QTL之间无连锁关系。     

水稻柱头外露率的QTL分析

利用高柱头外露率的籼稻窄叶青8号(ZYQ8)和极低外露率的粳稻京系17(JX17)以及由它们构建的加倍单倍体(DH)群体,在海南对各DH株系的柱头外露率进行调查,并使用该群体的分子连锁图谱进行数量性状座位(QTL)分析。共检测到2个控制水稻柱头外露率的QTL(qPES-2,qPES-3),分别位于第2、第3染色体;并发现控制柱头单边外露率的QTL与柱头外露率完全一致,而控制柱头双边外露率的QTL在第2染色体上检测到;其增效基因均来源于ZYQ8。同时定位的控制穗粒数的QTL位于第6染色体和第8染色体上,与柱头外露率之间没有连锁关系。     

籼粳杂种双单倍体的配子选择

对典型的灿与粳稻杂种,窄叶青８号／京系１７Ｆ１花药进行培养获得的１３２个双单倍体的形态特性、同工酶与ＲＦＬＰ标记的分离与重组进行了考察分析,研究是否存在配子选择问题。结果表明：（１）对４个重要数量性状和６个涉及籼、粳特征的形态指数进行考察所获数据均为连续分布,并呈正态曲线;（２）用８种同工酶对５２个ＤＨ系分析结果表明,只有２种同工酶显著偏离期望的１：１比率,而灿与粳的总基因型比率相近;（３）应用１６７个ＲＦＬＰ标记对１３２个ＤＨ系进行的分析发现,有３６％标记发生偏分离,但偏籼与偏粳的比率相近,两个亲本基因组在ＤＨ群体中所占比率相同（各５０％）,各种基因组成呈正态分布。综上所述,本研究虽观察到一些轻微偏分离现象,但籼粳基因基本上随机分离与重组,等位基因总频率未偏离１：１比率。     

苗期水稻根部性状的QTL定位

耐旱是水稻抗逆研究中最重要的性状之一。利用水稻籼粳品种窄叶青8号（ZYQ8）和京系17（JX17）及其通过杂交F1代花药培养获得的127个单株组成的双单倍体分离群体（double haploid,DH)为材料,在营养液中培养10天后,对影响抗旱能力的根部几个主要性状进行了分析,发现最大根长（Maximum root Length,MRL)、根干重（Dry Root Weight,DRW)和根茎干重比（Root/Shoot Ratio of Dry Weight,RSR)3个性状在群体中变异较大,利用该群体建立的水稻分子遗传图谱,对上述3个水稻性状进行数量性状座位（Quantitative Trait Locus,QTL)的分析定位,结果表明,2／1／2个QTLs的亲本JX17等位基因分别控制着最大根长、根干重和茎士重比的表达,对表型变异的解释率分别为16．4％、17．0％、16．4％、10．4％和19．9％;2／1个QTLs的亲本ZYQ8等位基因分别控制着最大根长和根茎干重比的增加,表表型变异的解释率分别为19．6％、13．0％和13．2％。检测到的8个QTLs分别位地水稻的染色体2、3、4、5、6、9和10上。与其他已发表的定位结果比较表现,在3个性状的总共8个QTLs中,各有1个性状的1个QTL（控制最大根长的L169－CT106A,控制根干重的G45－G1314A和控制根茎干重比的G62－G144）与早先报道的结果相吻合。     

用双单倍体群体构建水稻的分子连锁图

本研究以窄叶青８号（籼稻）×京系１７（粳稻）的Ｆ１花培株系──ＤＨ群体为基础建立了１个水稻的ＲＦＬＰ连锁框架图,该图含ＲＦＬＰ标记、同功酶标记等共１０８个位点,标记间的平均间距为８．６ｃＭ。该图谱与已发表的用其他群体构建的图谱有很高的可比性。利用该框架图定位了２个未知位点的同功酶标记基因和１个籼稻亲本的抗稻瘟病基因。研究表明,目前的群体可进一步扩大成为一个永久性的作图群体,并应用于水稻基因定位和基因组研究     

Construction of Rice DNA Finger Print by SRFA

ＲＡＰＤ用于生物鉴定具有快速、简便、经济等优点。但是,由于该法所用引物通常为９～１０个寡聚核苷酸,与ＰＣＲ使用特异引物相比,其Ｔｍ值相对较低,扩增反应易受外界条件影响,重复性较差。ＳＲＦＡ技术采用设计有限制内切酶位点的人工合成接头与引物互补,弥补了ＲＡＰＤ法的上述不足。Ｆｉｇ．１为ＳＲＦＡ的技术路线。为提高连接效率,在同一试管内,用ＰｓｔＩ酶解基因组ＤＮＡ,并与人工接头连结,制备ＳＲＦＡ扩增的模板。合成与接头序列相应的引物。对南方５个野生稻品种和籼、粳稻各一个栽培品种进行ＳＲＦＡ扩增。Ｆｉｇ．２表示：每种材料均能获得约１０条以上的扩增条带。条带的大小在４００２０００ｂｐ之间。栽培稻品种中出现多态性片段：用引物１可得一条（１．３ｋｂ）片段,用引物２可得２条（１．１ｋｂ、０．７ｋｂ）片段。与ＦＡＰＤ法相比,ＳＲＦＡ法增加２０％的多态性。栽培稻与野生稻之间在多态性上没有差异,说明两者亲缘关系非常接近。五种野生稻的图谱可分为两类：江西、湖南、广西的与籼稻相近,广东、云南的与粳稻相近。当然,这还有待其它方面的研究来验证。接头的设计要求避免自身连结,与目的片段连结后不能再被ＰｓｔＩ切开。引物包括不变序列和选择序列两部     

SRFA法构建水稻DNA指纹图谱

水稻基因组DNA用PstⅠ酶切同时与人工接头连接后,使用选择性引物进行PCR扩增,琼脂糖凝胶电泳检测所构建的水稻DNA指纹图谱。结果表明在JX17和ZYQ8间以及5种野生稻间均存在DNA多态性片段。     

转Xa21基因水稻中T-DNA整合的遗传定位

利用转抗白叶枯病基因Xa21的水稻材料,通过TAIL－PCR方法扩增T－DNA整合的侧翼序列。从中筛选属于水稻基因组DNA的T－DNA整合的侧翼序列作为探针,将外源基因整合位点定位到窄叶青／京系17DH群体构建的水稻分子连锁图谱上。共获得属于水稻基因组DNA的T－DNA侧翼序列22个,其中的19个序列在定位群体的两个亲本之间显示RFLP多态性,分别定位在水稻基因组的第3,4,5,7,9,10,11和12染色体上。带有转基因Xa21的T－DNA整合的定位为研究外源基因在不同染色体位点的位置效应和稳定遗传打下基础。