Molecular markers linked to Rsa resistant to soybean mosaic virus

Soybean mosaic virus (SMV) is a severe disease in worldwide soybean production. A cross was made between Kefeng No. 1 with broad spectrum resistance to SMV and Nannong 1138–2, a susceptible cultivar. The inheritance of resistance to SMV strain Sa prevailing in southern China was analyzed. Results of x² test from inoculation experiment on parents F1, F2 and F3 lines showed that the resistance to strain Sa was controlled by a single dominant gene Rsa. BSA method was adopted and 900 random 10-mer primers were used to amplify total DNA from resistant pool and susceptible pool in order to obtain polymorphic bands in two bulks. 16 primers could generate polymorphic bands, of which OPW-05 and OPAS-06 could generate the most stable RAPD patterns. RAPD markers OPW-05₆₆₀ and OPAS-06₁₈₀₀ were found to be linked to Rsa. Their order and genetic distance were OPAS-06₁₈₀₀22.2cM Rsa10.1 cM OPW-05₆₆₀. Southern blotting showed that both OPAS-06₁₈₀₀ and 0PW-05₆₆₀ were low copy DNA in genomic DNA. 0PW-05₆₆₀ has been converted into an RFLP marker successfully. Additionally, pK644H, an RFLP marker, has been identified to be linked to 0PW-05₆₆₀, and their genetic distance was 37.4 cM.     

Characterization and molecular marker screening of a rice bacteria-resistant gene Xa-min(t)

To test the resistant spectrum of the Xa-min(t) gene introgressed from Oryza minuta, thirty-four isolates of different bacterial blight pathogen, Xanthomonas oryzae pv. oryzae (Xoo), from 11 countries were used to inoculate the Xa-min(t) introgression line 78-15. Four rice cultivars, IR24, C64 (IRBB21), Nipponbare and Zhonghua 11 were used as controls. The results showed that the Xa-min(t) gene was broad-spectrum and highly resistant to diverse Xoo isolates. The methods of bulk segregant analysis (BSA), randomly amplified polymorphic DNA (RAPD) and sequence characterized amplified regions (SCAR) were used to analyze F2 individuals of the hybrid IR24×78-15 and molecular genetic markers linked to Xa-min(t) gene were identified. A total of 800 arbitrary decamer oligonucleotide primers were used for RAPD analysis. Two RAPD markers, BE05300 and BE061400, produced by primers BE05 and BE06 respectively, were closely linked to the Xa-min(t) gene. Based on the sequences of these two markers, sequence specific primers were designed and used to screen all F2 plants. One RAPD marker, BE05300, was converted into a stable SCAR marker (ScBE05300). Linkage analysis was carried out using markers ScBE05300 and BE061400 on 948 and 719 F2 individuals of the hybrid IR24×78-15. Our results indicate that the genetic distances from Xa-min(t) to ScBE05300 and BE061400 are 2.2 cM and 3.7 cM respectively on the same side. This study may facilitate the construction of the fine physical map of the Xa-min(t) gene.     

水稻苯达松敏感致死基因的RAPD标记的克隆及测序

用3S Spin DNA Agarose Gel Purification Kit试剂盒将与水稻苯达松敏感致死基因相连锁的RAPD遗传标记S20—420和S316—600回收纯化，连接于pGEM—T载体并克隆测序，得到了S20—420和S316—600的全序列，其长度分别为423bp、606bp．将两端序列设计特异PCR扩增引物可用于检测水稻苯达松敏感致死基因和标记辅助育种．     

Identification of an AFLP marker linked to the stripe rust resistance geneYr10 in wheat

AFLP analysis of near-isogenic lines of the stripe rust resistance gene Yr10 was carried out with 6 PstⅠ- primers and 10 TaqⅠ-primers with the donor parent of Yr10 gene as the check. A total of about 4200 distinguishable bands were amplified, of which 5 were stable. The genetic linkage of the 5 polymorphic DNA fragments with the target gene were tested preliminarily on a segregating F₂ population derived from a cross between the gene donor parent “Moro” and susceptible cultivar “Mingxian 169”. The DNA fragment PT0502 was found closely linked to the Yr10 gene and cloned and sequenced. Based on the sequence specific primers for PCR were designed and synthesized. Genetic linkage analysis with 195 segregating F₂ plants indicated that the genetic distance was 0.5 cM between the main product SC₂₀₀ fragment produced by PCR with the primers and the Yr10 gene. The primers can be used to detect the Yr10 gene quickly, effectively and exactly.     

Quantitative Estimates of Outcrossing Rates in a Natural Population of Caldesia grandis （Alismataceae）

Outcrossing rate in a natural population of Caldesia grandis was estimated by the dominant random amplified polymorphism DNA (RAPD) marker using 10 open-pollinated progeny arrays of 24 individuals. The multilocus outcrossing rate estimated based on all 25 RAPD loci was 0.872 ±0.033 and the single-locus outcrossing rate was 0.795 ±0.032. Multilocus estimates did not differ significantly from the single-locus estimates. The fixation index, F, in the progeny estimated from RAPD data was -0.142 ±0.000. The estimates of multilocus outcrossing rates (t_m) and single-locus outcrossing rates (t_s) obtained from MLDT clearly indicate that outcrossing is predominant in the open-pollinated C. grandis population. An empirical analysis suggests that 15 should be the minimum number of dominant marker loci necessary to achieve robust estimates of t_m.     

应用Bulked-DNA寻找白菜型油菜核雄性不育基因的RAPD标记

采用随机扩增多态ＤＮＡ（ＲＡＰＤ）标记方法从白菜型油菜核不育两用系中筛选出了一个与白菜型 油菜育性基因连锁的ＲＡＰＤ标记。该ＤＮＡ片段大小约０．７２ｋｂ,与育性基因之间的遗传连锁距离为６．０８ｃＭ,ＬＯＤ值为９．１０。     

白菜型油菜核育性相关基因片段的克隆与序列分析

通过ＲＡＰＤ标记,所获得的与育性基因紧密连锁的基因片段进行克隆与序列分析,结果表明,该育性基因片段为与油菜小孢子发育早期ＢＰ４调控基因５８％同源,并含有一ＭＡＰＤＳ盒高度同源的保邓列。Ｓｏｕｔｈｅｒｎ杂交结果表明该基因为单拷贝基因。     

ISSR 和 RAPD PCR技术对东北地区主推玉米品种的鉴别

运用现代分子生物学简单重复区间序列扩增多态性（ISSR）和随机扩增片段多态性DNA（RAPD）两种分子标记技术， 对吉林省主推6个玉米杂交种及其父本、 母本共计18份基因图谱进行鉴别. 以ISSR为主要检测方法、 RAPD为验证方法，分别从30条ISSR引物中选出4条、 从30条RAPD引物中筛选出2条扩增效果明显、 特异性高的引物. 结果表明， 运用ISSR和RAPD-PCR技术提高了玉米品种鉴定和纯度鉴定的准确性.     

高粱抗丝黑穗病基因的分子标记RAPD分析

丝黑穗病是影响我国高粱生产发展的主要病害之一,在高粱产区每年都有发生,发病率有时高达70 %,给生产造成很大损失,而选育抗病品种是最为有效的抗病策略.分别以高粱2381恢复系(抗病)、矮四恢复系(感病)的叶片为试材,采用CTAB法提取高粱基因组DNA,并应用RAPD筛选技术对高粱基因进行分子标记.在最佳的RAPD反应体系中共筛选了100个RAPD随机引物,筛选出来27个适宜引物,获得了稳定的RAPD扩增结果及多态性较好的DNA谱带.其中有6个引物对DNA扩增产生了差异谱带.     

Molecular mapping of a novel yellow rust resistance gene of wheat using microsatellite markers

Identification and genetic analysis of yellow rust resistance have suggested that wheat line R55 carries single dominant gene conferring yellow rust resistance. The bulked segregant analysis (BSA) for an F₂ population using microsatellite marker technique has indicated that the yellow rust resistance gene is located on the short arm of chromosome 1B, tightly linked to the microsatellite markers WMS11-193 bp and WMS18-184 bp, the linkage distance between the markers and the gene is 1.9 cM. This gene has been formally namedYr26. It is inferred from the pedigree, resistance and gene locus analysis that theYr26 has been transferred fromTriticum turgidum L. and is different from the other known yellow rust resistance genes.     

内蒙古3个绒山羊品种RAPD的初步研究

利用随机扩增多态DNA（RAPD）技术,研究了内蒙古地区3个绒山羊品种的DNA多态性,由此推导它们之间的遗传距离和系统发育关系。在所使用的12种随机引物中,有8种随机引物扩增出多态谱带,共检测到32个RAPD标记,其中有21个发生变异。用Nei的片段公享度公式计算了品种间的遗传距离,用UPGMA聚类法构建了系统发育树。结果表明：内蒙古白绒山羊的3个类群彼此亲缘关系较近,分化不明显;内蒙古白绒山羊与罕山白绒山羊聚为一个大类,辽宁绒山羊和乌珠穆沁白绒山羊聚为一个大类,说明内蒙古白绒山羊与罕山白绒山羊有较近的亲缘关系,乌珠穆沁白绒山羊与辽宁绒山羊的亲缘关系较近。     

Fine mapping of the rice bacterial blight resistance gene Xa-4 and its co-segregation marker

An F₂ population developed from theXa-4 near isogenic lines, IR24 and IRBB4, was used for fine mapping of the rice bacterial blight resistance gene,Xa-4. Some restriction fragment length polymorphism (RFLP) markers on the high-density map constructed by Harushima et al. and the amplified DNA fragments homologous to the conserved domains of plant disease resistance (R) genes were used to construct the genetic linkage map around the geneXa-4 by scoring susceptible individuals in the population.Xa-4 was mapped between the RFLP marker G181 and the polymerase chain reaction (PCR) marker M55. The R gene homologous fragment marker RS13 was found co-segregating withXa-4 by analyzing all the plants in the population. This result opened an approach to map-based cloning of this gene, and marker RS13 can be applied to molecular marker-assisted selection ofXa-4 in rice breeding programs.     

甜菜抗根腐病基因ISSR分子标记的初步研究

以感病×抗病的甜菜种间杂交组合KWS9419×ZD204的F1代17个单株及ZD自交一代16个单株为试材,采用BSA法和ISSR技术,通过对155个随机引物的筛选,获得了一个与甜菜抗根腐病基因连锁的ISSR标记OPP0760,可以用作抗根腐病基因的分子辅助选择的依据。     

籼型光敏核不育水稻的RAPD分析

以籼型光敏核不育水稻８９０２ｓ及其可育近等基因系材料８９０２的核ＤＮＡ为模板，进行ＲＡＰＤ分析，从检测过的１５个引物中发现引物ＯＰＡ－０４在可育品系和不育品系中扩增出１个１０００ｂｐ的差异带，并初步认为此差异与育性相关     

Molecular verification of the integration ofTripsacum dactyloides DNA into wheat genome through wide hybridization

RAPD and RFLP analyses of double haploid lines which derived from hybridization between hexaploid wheat (Triticum aestivum L. 2n=42) and eastern gamagrass (Tripsacum dactyloides L. 2n=4x=72) are reported. Two of the 340 Operon primers have been screened, which stably amplified 处留情 (male parent) specific bands in the double haploid lines. These results confirm the fact that Tripsacum dactyloides DNA has been integrated into wheat genome by sexual hybridization at molecular level. This idea has been further testified by RFLP analysis. Application and potentials of transferring Tripsacum dactyloides DNA into wheat genome by sexual hybridization in wheat breeding are discussed.     

RAPD-PCR稳定性的探索

 以滇牡丹(Paeonia delevayi)为实验材料,分别测试了Mg²⁺、模板DNA、聚合酶、引物等反应成分对产物的影响,以期探索RAPD-PCR体系中各成分对产物的影响,以及各成分之间相互作用的规律,为利用RAPD进行生物学研究的人们提供一些参考.     

Fine mapping of the red plant gene R1 in upland cotton(Gossypium hirsutum)

Sub 16 is a substitution line with G. hirsutum cv. TM-1 genetic background except that the 16th chromosome (Chr. 16) is replaced by the corresponding homozygous chromosome of G. barbadense cv. 3-79, and T586 is a G. hirsutum multiple gene marker line with 8 dominant mutation genes. The R ₁ gene for anthocyanin pigmentation was tagged in Chr. 16 in T586. The objective of this research was to screen SSR markers tightly linked with R ₁ by using the F₂ segregating population containing 1259 plants derived from the cross of Sub 16 and T586 and the backbone genetic linkage map from G. hirsutum×G. barbadense BC₁ newly updated by our laboratory. Genetic analysis suggested that the segregation ratio of red plants in the F₂ population fit Mendelian 1:2:1 inheritance, confirming that the red plant trait was controlled by an incomplete dominance gene. Preliminary mapping of R ₁ was conducted using 237 randomLy selected F₂ individuals and JoinMap v3.0 software. Then, a fine map of R1 was constructed using the F₂ segregating population containing 1259 plants, and R ₁ was located between NAU4956 and NAU6752, with only 0.49 cM to the nearest maker loci (NAU6752). These results provided a foundation for map-based cloning of R ₁ and further development of cotton cultivars with red fibers by transgenic technology. Supported by National Natural Science Foundation of China (Grant No. 30730067) and Programme of Introducing Talents of Discipline to Universities (Grant No. B08025)     

小麦雌性不育基因的微卫星标记定位

以普通小麦新601×雌性不育小麦XND126的F2群体作为育性调查以及基因标记群体.通过对育性基因的分析,确定在此组合中雌性不育基因由1对主效基因控制;结合混合分组分析法(Bulk Segregant Analysis,BSA),首次对小麦雌性不育基因进行了SSR分子标记,通过对一千对微卫星引物的筛选,确定微卫星引物cfd36标记与主效基因连锁,遗传距离为20.2cM.     

Morphological and molecular characterization of two G. somalense monosomic alien addition lines （MAALs）

Two G. somalense monosomic alien addition lines were identified from the derived backcross progenies of allohexaploid between G. hirsutum and G. somalense through cytological and morphological observation. Furthermore, the alien addition chromosome was identified and distinguishedby RAPD analysis. A total of 160 RAPD primers were usedfor PCR amplification. Primer SBSG11 could produce a specific molecular marker (600 bp) for monosomic alien addition line Ⅰ (MAAL Ⅰ ). Primer SBSC03 could produce aspecific molecular marker (700 bp) for monosomic alien ad-dition line Ⅱ (MAAL Ⅱ). SBSE07 and SBSE08 could re-spectively produce common molecular marker for mono-somic alien addition lines Ⅰ and Ⅱ. G. somalense alienaddition lines could be important for cotton improvement.