南方玉米锈病抗病基因的定位及不同遗传背景对基因标记的比较分析

玉米自交系齐319高抗南方玉米锈病。利用SSR标记技术和BSA分析对齐319抗南方玉米锈病基因进行了标记分析,结果表明SSR标记phi041和phi118与齐319抗南方锈病基因连锁,其遗传距离分别为7.69cM和8.55cM。因此南方玉米锈病抗病基因定位于玉米10号染色体短臂上。本研究进行的抗病基因标记,选择使用了两个杂交组合的3个分离群体,标记结果显示同一杂交组合的不同分离群体其标记结果是一致的,而不同组分分离群体的标记结果有显著差异,这可能与基因的遗传背景相关。因此,在进行基因标记分析时,选择合适的分离群体是至关重要的。     

玉米抗南方锈病基因的QTL定位

为发掘新的抗南方锈病基因资源,本研究以感病自交系黄早四为母本、抗病自交系W456为父本,构建F2群体并开展抗病基因定位研究。采用人工接种鉴定的方法对两个亲本、F1、F2群体及对照材料进行表型鉴定和遗传分析。利用均匀覆盖10条染色体的200个SSR标记,分析240个F2单株的基因型并构建含有200个SSR位点的遗传连锁图,连锁图总长度3331 cM,标记间平均距离16.6 cM。使用QTL IciMapping V4.1软件中的完备区间作图法对抗病QTL进行分析,共检测到6个控制南方锈病的QTL:qSCR3、qSCR7、qSCR8-1、qSCR8-2、qSCR9和qSCR10,邻近标记分别为umc2105和umc1729、umc1066和bnlg2271、umc1904和umc1984、umc1984和bnlg1651、umc1957和bnlg1401、umc2034和umc1291,分别位于3、7、8、9和10号染色体上,其中8号染色体上有两个位点,标记区间长度在5～19 cM之间。单个QTL的表型贡献率在2.61%～24.19%之间,可以解释表型总变异的62.3%,其中3个QTL贡献率大于10%,位于10号染色体上的qSCR10贡献率最大,可解释表型变异的24.19%。通过对目标区间标记加密,将该位点的定位区间进一步缩小到2.51 cM内,与两侧标记的距离分别是2.15 cM和0.36 cM。初步定位得到10号染色体上存在抗南方锈病的主效QTL,可为抗病品种的培育提供参考。     

两个玉米矮花叶病显性互补抗病基因的发现和定位

玉米矮花叶病是世界普通发生危害严重的玉米病毒病害之一,迄今为止,只有少数几个抗病基因被发现并定位,优良自交系四一是鉴定出定的玉米筹花叶病新抗源,它表现为全生育抗性,通过连续两年的经典遗传学研究发现,四一的成株期抗性表现为一种新的抗病遗传模式,该抗性是由两个显性互补抗病基因控制,87对微卫星标记分析进一步证实了以上推论,并把两个抗病基因分别定位在第三和第六染色体上,第三染色体上的抗病基因与微卫星标记phi029相距14.5cM,第六染色体上的抗病基因与微卫星标记phil26相距7.2cM.     

玉米P25自交系抗锈病基因的遗传分析及SSR分子标记定位

以玉米南方型锈病免疫自交系P2 5和感病自交系F3 4 9及F1、F2 、B1和B2 为材料 ,采用主基因 多基因混合遗传模型研究了P2 5的抗病遗传规律。结果表明 :自交系P2 5的抗病基因为一主基因 ,表现为加性效应 ,没有检测出多基因 ,其在F2 、B1和B2 群体的遗传率分别为 81 88%、38 14 %和 5 5 1%。利用SSR分子标记技术 ,以组合P2 5×F3 4 9的F2 :3 家系作为构图群体 ,构建了玉米SSR遗传连锁图谱 ,并将玉米抗南方型锈病基因定位于 10号染色体上 ,与phi0 5 9标记的遗传距离为 5 8cM。     

齐319携带的南方玉米锈病抗性基因的遗传初析

我国选育的优良玉米自交系齐319高抗南方玉米锈病。通过用病原菌接种齐319分别与5个不同感病自交系的杂交,回交4个世代的P1,P2,F1,F2,BC1F110个分离群体和抗病感病参数的调查结果表明：F1整齐一致,表现抗病;F2和BC1F1抗感分离,经x^2－检验分别符合3：1和1：1的分离比例。据此,齐319携带的南方玉米锈病抗性基因是由显性单基因所控制。     

玉米种质资源抗南方锈病鉴定

玉米南方锈病已成为近几年我国夏玉米生产区间歇性暴发流行的病害,对玉米生产构成严重威胁,病害流行年份可造成10%以上的产量损失。目前,已确认的抗病自交系非常有限,而抗病育种急需不同抗性控制背景的自交系。为发掘和丰富可利用的南方锈病抗源,于2008～2012年,在广西南宁采用田间人工接种方法对1589份玉米种质资源进行抗南方锈病鉴定。通过高病害压力和连续多年的鉴定,从1589份玉米种质中鉴定出高抗（HR）材料26份,占鉴定总数的1.64%;抗病（R）材料137份,占鉴定总数的8.62%;中抗（MR）水平的材料382份,占鉴定总数的24.04%;感病（S）材料489份,占鉴定总数的30.77%;高感（HS）材料555份,占鉴定总数的34.93%。总体上抗南方锈病种质较少,引进种质中抗病类型材料的比例略高。经重复鉴定,筛选出赤556等18份自交系、老来秕等3份地方品种、A69等4份来自津巴布韦的材料、引自CIMMYT的Dr11表现稳定高抗南方锈病,为今后我国玉米抗南方锈病育种提供了新的抗性资源。     

玉米抗南方锈病种质资源初步鉴定及遗传多样性分析

南方锈病是玉米生产上的重要病害。2013-2015年在广西南宁和北京昌平对903份玉米种质资源进行了抗南方锈病的初步鉴定与评价,并利用SSR标记对筛选出的部分抗性材料进行了遗传多样性分析。结果表明,在903份种质中,8份自交系在广西南宁和北京昌平均对南方锈病表现高抗(HR),占总鉴定种质的0.9%;29份材料表现为抗病(R),占比3.2%,包括27份自交系和2份农家种;中抗种质(MR)100份,占比11.1%;感病(S)和高感(HS)种质分别为181和585份,占鉴定材料的20.0%和64.8%。由此可见,玉米资源中高抗南方锈病的种质较为匮乏,在不同地点均表现高抗的材料是难得的抗源。不同地理来源的玉米种质对南方锈病的抗性水平存在较大差异,其中抗性资源较为丰富的是源自内蒙古和山西的种质。42对多态性SSR引物在50份抗锈病材料中,共扩增出141个条带,多态性条带139个,多态位点百分率(PPB)为98.58%。平均等位基因数(Na)1.98,平均有效等位基因数(Ne)1.59,平均Nei's基因多样性(H)0.34,平均多态性信息含量(PIC)0.78,平均Shannon's信息指数(I)0.51;通过UPGMA聚类分析,50份抗病材料被划分为2个类群,其中,第Ⅰ类群又可划分为5个亚类,表现出较高的遗传多样性,为抗病育种中抗源的选择和利用提供参考信息。     

一个新的抗玉米矮花叶病基因位点的微卫星标记

通过混合遗传模型P1、P2、B1、B2、F1、F2 6世代联合分析发现, 玉米(Zea mays L.)自交系黄早四对玉米矮花叶病B株系的抗性是由一对主基因和多基因共同控制,从而鉴别出一对主效基因的存在;利用位于第六染色体上的27对微卫星标记,对黄早四×Mo17的 F2群体进一步分析,筛选出两个与主效抗病基因(mdm1(t))紧密连锁的微卫星标记phi077和 bnlg391,它们在分子图谱上的顺序为phi077-mdm1(t)-bnlg391,两个区间的遗传距离分别是4.74 centiMorgan (cM)和6.72 cM.     

玉米抗甘蔗花叶病毒分子标记开发

由甘蔗花叶病毒引起的玉米矮花叶病是我国黄淮海地区玉米生产的重要病害,开发抗矮花叶病基因分子标记是开展抗病分子标记辅助育种的基础。本文基于玉米6.00-6.01区域的“一致性抗甘蔗花叶病毒QTL区间”寻找抗病基因的功能保守域,依据序列多态性开发出抗病分子标记InDel-130和InDel-110,在已知抗性的102份玉米自交系中进行验证。通过分析标记抗病带型和感病带型中的抗病和感病自交系数目,卡平方测验表明标记InDel-130在供试自交系中与抗病性的表现独立无关,而标记InDel-110与甘蔗花叶病毒抗性高度相关,为共显性标记,可用于玉米抗甘蔗花叶病毒种质筛选和分子标记辅助育种。     

一个新的抗玉米矮花叶病基因位点的微卫星标记

通过混合遗传模型P1、P2 、B1、B2 、F1、F2 6世代联合分析发现 ,玉米 (ZeamaysL .)自交系黄早四对玉米矮花叶病B株系的抗性是由一对主基因和多基因共同控制 ,从而鉴别出一对主效基因的存在 ;利用位于第六染色体上的 2 7对微卫星标记 ,对黄早四×Mo17的F2 群体进一步分析 ,筛选出两个与主效抗病基因 (mdm1(t) )紧密连锁的微卫星标记phi0 77和bnlg391,它们在分子图谱上的顺序为phi0 77 mdm1(t) bnlg391,两个区间的遗传距离分别是 4.74centiMorgan (cM)和 6 .72cM。     

Mapping of HtNB, a gene conferring non-lesion resistance before heading to Exserohilum turcicum (Pass.), in a maize inbred line derived from the Indonesian variety Bramadi

The gene HtNB confers non-lesion resistance to the fungal pathogen Exserohilum turcicum in maize. To map this gene, we developed two F(2) populations, P111 (resistant line) x HuangZao 4 (susceptible line) and P111 x B73 (susceptible). HtNB was located on chromosome 8.07 bin, flanked by MAC216826-4 and umc2218 at distances of 3.3 and 3.4 cM, respectively. HtNB appears to be a new gene responsible for resistance to northern corn leaf blight. Functions of the genes in the region between umc1384 and umc2218 were predicted. In addition, several genes were found to be related to disease resistance, such as the genes encoding Ser/Thr protein kinase and protein-like leaf senescence.     

Mapping of stripe rust resistance gene in an <Emphasis Type="Italic">Aegilops caudata</Emphasis> introgression line in wheat and its genetic association with leaf rust resistance

A pair of stripe rust and leaf rust resistance genes was introgressed from Aegilops caudata, a nonprogenitor diploid species with the CC genome, to cultivated wheat. Inheritance and genetic mapping of stripe rust resistance gene in backcross-recombinant inbred line (BC-RIL) population derived from the cross of a wheat–Ae. caudata introgression line (IL) T291-2(pau16060) with wheat cv. PBW343 is reported here. Segregation of BC-RILs for stripe rust resistance depicted a single major gene conditioning adult plant resistance (APR) with stripe rust reaction varying from TR-20MS in resistant RILs signifying the presence of some minor genes as well. Genetic association with leaf rust resistance revealed that two genes are located at a recombination distance of 13%. IL T291-2 had earlier been reported to carry introgressions on wheat chromosomes 2D, 3D, 4D, 5D, 6D and 7D. Genetic mapping indicated the introgression of stripe rust resistance gene on wheat chromosome 5DS in the region carrying leaf rust resistance gene LrAc, but as an independent introgression. Simple sequence repeat (SSR) and sequence-tagged site (STS) markers designed from the survey sequence data of 5DS enriched the target region harbouring stripe and leaf rust resistance genes. Stripe rust resistance locus, temporarily designated as YrAc, mapped at the distal most end of 5DS linked with a group of four colocated SSRs and two resistance gene analogue (RGA)-STS markers at a distance of 5.3 cM. LrAc mapped at a distance of 9.0 cM from the YrAc and at 2.8 cM from RGA-STS marker Ta5DS_2737450, YrAc and LrAc appear to be the candidate genes for marker-assisted enrichment of the wheat gene pool for rust resistance.     

Genetic mapping of adult plant leaf rust resistance genes Lr48 and Lr49 in common wheat

Hypersensitive adult plant resistance genes Lr48 and Lr49 were named based on their genetic independence of the known adult plant resistance genes. This study was planned to determine genomic locations of these genes. Recombinant inbred line populations derived from crosses involving CSP44 and VL404, sources of Lr48 and Lr49, respectively, and the susceptible parent WL711, were used to determine the genomic locations of these genes. Bulked segregant analyses were performed using multiplex-ready PCR technology. Lr48 in genotype CSP44 was mapped on chromosome arm 2BS flanked by marker loci Xgwm429b (6.1 cM) and Xbarc7 (7.3 cM) distally and proximally, respectively. Leaf rust resistance gene Lr13, carried by the alternate parent WL711, was proximal to Lr48 and was flanked by Xksm58 (5.1 cM) and Xstm773-2 (8.7 cM). Lr49 was flanked by Xbarc163 (8.1 cM) and Xwmc349 (10.1 cM) on chromosome arm 4BL. The likely presence of the durable leaf rust resistance gene Lr34 in both CSP44 and VL404 was confirmed using the tightly linked marker csLV34. Near-isogenic lines for Lr48 and Lr49 were developed in cultivar Lal Bahadur. Genotypes combining Lr13 and/or Lr34 with Lr48 or Lr49 were identified as potential donor sources for cultivar development programs.     

Molecular tagging of a rust resistance gene in cultivated groundnut (Arachis hypogaea L.) introgressed from Arachis cardenasii

Rust is a serious and the most prevalent groundnut disease in tropical and subtropical growing regions of the world. A total of 164 recombinant inbred lines derived from resistant (VG 9514) and susceptible (TAG 24) cultivated groundnut parents were screened for rust resistance in five environments. Subsequent genotyping of these lines with 109 simple sequence repeat (SSR) markers generated a genetic linkage map with 24 linkage groups. The total length of the linkage map was 882.9 cM with an average of 9.0 cM between neighbouring markers. The markers pPGPseq4A05 and gi56931710 flanked the rust resistance gene at map distances of 4.7 cM and 4.3 cM, respectively, in linkage group 2. The significant association of these two markers with the rust reaction was also confirmed by discriminant analysis. The informative SSR markers classified rust-resistant and susceptible groups with 99.97% correctness. The SSR markers pPGPseq4A05 and gi56931710 were able to identify all the susceptible genotypes from a set of 20 cultivated genotypes differing in rust reaction. Tagging of the rust resistance locus with linked SSR markers will be useful in selecting the rust resistant genotypes from segregating populations and in introgressing the rust resistance genes from diploid wild species.     

Restriction fragment length polymorphisms linked to genes for resistance to crown rust (Puccinia coronata) in near-isogenic lines of hexaploid oat (Avena sativa).

Crown rust, perhaps the most important fungal disease of oat, is caused by Puccinia coronata. An examination of near-isogenic lines (NILs) of hexaploid oat (Avena sativa) was conducted to identify markers linked to genes for resistance to crown rust. These lines were created such that a unique resistance gene is present in each of the two recurrent parent backgrounds. The six NILs of the current study, X434-II, X466-I, and Y345 (recurrent parent C237-89) and D486, D494, and D526 (recurrent parent Lang), thus provide a pair of lines to study each of three resistance genes. Restriction fragment length polymorphisms and resistance loci were mapped using BC1F2 populations. Three markers were found linked to a locus for resistance to crown rust race 203, the closest at 1.9 cM in line D494 and 3.8 cM in line X466-I. In lines D526 and Y345 a marker was placed 1.0 and 1.9 cM, respectively, from the locus conferring resistance to crown rust race 345, and in D486 and X434-II a marker mapped at 8.0 and 10.2 cM from the locus for resistance to rust race 264B.     

Molecular tagging and genetic mapping of the disease resistance gene<Emphasis Type="Italic"> RppQ</Emphasis> to southern corn rust

Southern corn rust (SCR), Puccinia polysora Underw, is a destructive disease in maize (Zea mays L.). Inbred line Qi319 is highly resistant to SCR. Results from the inoculation test and genetic analysis of SCR in five F₂ populations and five BC₁F₁ populations derived from resistant parent Qi319 clearly indicate that the resistance to SCR in Qi319 is controlled by a single dominant resistant gene, which was named RppQ. Simple sequence repeat (SSR) analysis was carried out in an F₂ population derived from the cross Qi319×340. Twenty SSR primer pairs evenly distributed on chromosome10 were screened at first. Out of them, two primer pairs, phi118 and phi 041, showed linkage with SCR resistance. Based on this result, eight new SSR primer pairs surrounding the region of primers phi118 and phi 041 were selected and further tested regarding their linkage relation with RppQ. Results indicated that SSR markers umc1,318 and umc 2,018 were linked to RppQ with a genetic distance of 4.76 and 14.59 cM, respectively. On the other side of RppQ, beyond SSR markers phi 041 and phi118, another SSR marker umc1,293 was linked to RppQ with a genetic distance of 3.78 cM. Because the five linkage SSR markers (phi118, phi 041, umc1,318, umc 2,018 and umc1,293) are all located on chromosome 10, the RppQ gene should also be located on chromosome 10. In order to fine map the RppQ gene, AFLP (amplified fragment length polymorphism) analysis was carried out. A total 54 AFLP primer combinations were analyzed; one AFLP marker, AF1, from the amplification products of primer combination E-AGC/M-CAA, showed linkage with the RppQ gene in a genetic distance of 3.34 cM. Finally the RppQ gene was mapped on the short arm of chromosome 10 between SSR markers phi 041 and AFLP marker AF1 with a genetic distance of 2.45 and 3.34 cM respectively.Communicated by H. F. Linskens     

Molecular mapping of genes for opposite leafing in maize using simple-sequence repeat markers

Maize with opposite phyllotaxy (OP) and also initiating ears in opposite pairs is an aberrant mutant and also precious material for maize breeding and plant evolution studies. Mapping and identifying the markers closely linked to genes for the OP trait are essential for cloning the gene and marker-assisted selection in breeding. We established H14D, a near-isogenic line of the OP trait with H53 genetic background. We found that the OP trait is regulated by two independent dominant genes with mutually complementary relations, named Opp-1 and Opp-2. Screening of seven simple-sequence repeat (SSR) markers among the 105 pairs of SSR primers showed polymorphism between the inbred lines H14D and H53. The polymorphic SSR markers were then used to determine linkage with the trait in an F(2) population with 441 progeny, suggesting that SSR marker umc2094 in the Bin2.01 region is linked with Opp-1 at 6.7 cM, and bnlg1831 in Bin2.06 is linked with Opp-2 at 6.1 cM. Further investigation showed that bnlg1092 and umc1028 are linked to Opp-1 and Opp-2 genes, with genetic distances of 12.2 and 1.9 cM. It was also found that the four SSR markers flank the two OP genes, respectively. These results will be useful for marker-assisted selection breeding of OP maize and will also strengthen the basis for cloning of the opposite leafing gene.     

Genetic analyses and mapping of a new thermo-sensitive genic male sterile gene in maize

The present study describes a novel thermo-sensitive genic male sterile (TGMS) line, Qiong68ms. To analyse the mode of fertility inheritance and tag the TGMS gene, a set of F₂, BC₁ and F_2:3 populations derived from a cross between Qiong68ms and K12 were evaluated for a period of 2 years. Classical genetic analyses and QTL mapping using the mean restoration percentage of the F_2:3 populations revealed that the fertility of Qiong68ms was likely to be governed by a single recessive gene, which was named tms3; the tms3 gene was mapped to a location between SSR markers umc2129 and umc1041, at a distance of 3.7 cM form umc2129 and 1.5 cM form umc1041. The molecular markers tightly linked with tms3 gene will aid in the transfer of the TGMS gene to various background inbred lines using the MAS method.     

Identification of Transposable Element Markers for a Rust (Puccinia arachidis Speg.) Resistance Gene in Cultivated Peanut

Peanut rust (Puccinia arachidis Speg.) affects pod yield and quality up to an extent of 10–50%. Efforts have been made on transferring the rust resistance gene to cultivated peanut species through interspecific hybridization. But, in most of the cases, it failed due to linkage drag of undesirable plant and pod features. Identification of tightly linked molecular markers will help to identify the desirable recombinants more efficiently. A recombinant inbred line population comprising 164 lines was developed from a cross between a rust‐resistant parent VG 9514 and a rust susceptible parent TAG 24. Using a modified bulk segregant analysis, 243 transposable element (TE) primer pairs were screened for putative linkage with rust resistance. Of the 243, 40 TE primer pairs were found polymorphic between parents and two transposable element markers, and TE 360 and TE 498 were found associated with rust resistance gene. Based on genetic mapping, TE 360 was found linked to the rust resistance gene at 4.5 cM distance. Identification of such markers could be applied for marker‐assisted selection of rust resistance plants in peanut.