兼抗型成株抗性小麦品系的培育、鉴定与分子检测

小麦条锈病、叶锈病和白粉病是我国小麦的重要真菌病害,培育兼抗型成株抗性品种是控制病害最为经济有效和持久安全的方法。本研究选用由成株抗性育种方法培育的21份冬小麦高代品系和96份春小麦高代品系,在多个环境下进行这3种病害的成株期抗性鉴定,并利用紧密连锁的分子标记检测了兼抗型基因Lr34/Yr18/Pm38、Lr46/Yr29/Pm39和Sr2/Yr30的分布。田间鉴定表明,21份冬小麦品系中有17份兼抗3种病害,占80.9%;96份春小麦品系中有85份兼抗3种病害,占88.5%。分子标记检测发现,21份冬小麦品系均含QPm.caas-4DL,其中7份还含QPm.caas-2BS,9份还含QPm.caas-2BL;96份春小麦品系中,18份含Lr34/Yr18/Pm38,37份含Lr46/Yr29/Pm39,29份含Sr2/Yr30。以上结果表明,分子标记与常规育种相结合,可有效培育兼抗型成株抗性品种,为我国小麦抗病育种提供了新思路。     

Race Specific Powdery Mildew Resistance in 31 Northwest European Wheat Cultivars

Race specific powdery mildew resistance in 23 winter wheat cultivars, eight spring wheat cultivars, and 14 lines/cultivars possessing known powdery mildew resistance genes, has been studied by analyzing host/pathogen interactions. The cultivars were tested as intact seedlings, and as detached primary leaf segments on water agar; both methods revealed reproducible and concordant results. The 45 cultivars/lines were divided into 24 resistance spectra according to the patterns of reaction to the powdery mildew isolates used. Of the 31 cultivars investigated, eight did not possess any of the resistance genes detected, and the remaining 23 were divided in 16 resistance spectra. The race specific resistance of nine cultivars was conferred by the single resistance genes Pm2, Pm4b, Pm5/Ml-i: or Pm6, while the race specific resistance of 14 cultivars was conferred by 2, 3, 4 or 5 genes in combination.     

小麦新品种“山农20”抗病基因的分子检测

山农20是2011年和2012年分别通过国家黄淮南、北片审定的小麦高产多抗新品种,在国家区试抗病性鉴定和生产中都表现出良好的抗黄淮麦区主要病害的特性。本研究利用与小麦抗白粉病、条锈病、叶锈病、纹枯病基因和抗赤霉病主效QTL紧密连锁的SSR、SCAR、STS等标记对该品种进行了分子检测,发现山农20含有6个抗白粉病基因(Pm12、Pm24、Pm30、Pm31、Pm35和Pm36),6个抗条锈病基因(Yr5、Yr9、Yr15、Yr24、Yr26和YrTp1),2个抗叶锈病基因(Lr21和Lr26),1个抗纹枯病基因(Ses1),但未检测到抗赤霉病主效QTL。分子检测结果部分解释了山农20的优良抗病性,也为利用分子标记辅助选择培育抗病稳产小麦新品种提供参考。     

Molecular and cytogenetic identification of new wheat-Dasypyrum breviaristatum additions conferring resistance to stem rust and powdery mildew

Two cytologically stable wheat-Dasypyrum breviarisatatum addition lines, Y93-1-6-6 and Y93-1-A6-4, were identified by integrated molecular and cytogenetic techniques. C-banding and genomic in situ hybridization (GISH) showed that Y93-1-6-6 and Y93-1-A6-4 were different wheat-D. breviaristatum additions. A total of 51 markers (primer/enzyme combinations), including 6 PCR-based Landmark Unique Gene (PLUG) markers and 45 Sequence-Tagged-Site (STS) markers, were selected from 3,774 primer/enzyme combinations to further characterize these two additions. Marker haploytpes suggested that both D. breviaristatum chromosomes in Y93-1-6-6 and Y93-1-A6-4 were rearranged. Stem rust resistance screening indicated that both additions were highly resistant to race RKQQC, whereas only Y93-1-6-6 was resistant to race TTKSK (Ug99). Powdery mildew resistance screening showed that only Y93-1-6-6 was resistant. Pedigree analysis suggested that the stem rust and powdery mildew resistance of Y93-1-6-6 was derived from D. breviaristatum, indicating that the D. breviaristatum chromosomes in Y93-1-6-6 possess a new powdery mildew resistance gene(s), and new stem rust resistance gene(s). These two additions could be used as stem rust or powdery mildew resistance sources in wheat breeding programs.     

Characterisation and origin of rust and powdery mildew resistance genes in VPM1 wheat

Summary The expression of rust resistances conferred by closely linked genes derived from VPM1 varied with environmental conditions and with genetic backgrounds. Under low light and low temperature conditions seedlings carrying Yr17 showed susceptible responses. Stem rust and leaf rust resistance genes Sr38 and Lr37 tended to confer more resistance at 17±2° C than at normal temperatures above > 20° C. These studies supported the hypothesis that Yr17, Lr37 and Sr38 were derived from Aegilops ventricosa, whereas Pm4b was probably derived from T. persicum. Studies on certain addition lines and parental stocks indicated that wheat cytoplasm may enhance the expression of Sr38.     

Cytogenetical studies in wheat iv. Chromosome location and linkage studies involving thePM2 locus for powdery mildew resistance

Summary The genePm2 conditioning resistance to powdery mildew in the cultivar Ulka was located on chromosome 5D by monosomic analysis. It showed genetic segregation independent of geneLr3 conditioning resistance to leaf rust on the same chromosome. Results of telocentric mapping demonstrated thatLr1 was on the long arm of 5D whereasPm2 was very close to the centromere on this arm or, more likely, on the opposite arm. Evidence from chimaeric sectoring favoured the latter alternative.     

Variation of characters in near-isogenic lines of wheat with added genes for leaf rust resistance

Summary Using the cultivar Arina as the recurrent parent, six backcrosses were made with two donor lines carrying the leaf rust resistance genes Lr1 and Lr9, respectively. Selection for leaf rust resistance occurred at the seedling stage in the greenhouse; the first plants transferred to the field were BC₆F₄s. Frequency distribution of the 332 Lr1/7 × Arina and the 335 Lr9/7 × Arina lines showed continuous variation for yellow rust resistance and heading date in these leaf rust near-isogenic lines (NILs). Similar results were also obtained for plant height, for resistance to powdery mildew and glume blotch, as well as for baking quality characters in another set of more advanced NILs. The available information on the behaviour of one of the parents of cultivar Arina led to the conclusion that the expressed yellow rust resistance is quantitative and might possibly be durable.     

Evidence of allelism between genes Pm8 and Pm17 and chromosomal location of powdery mildew and leaf rust resistance genes in the common wheat cultivar'Amigo'

TIBL-1RS wheat-rye translocation cultivars utilized in wheat programmes worldwide carry powdery mildew resistance gene Pm8. Cultivar‘Amigo’possesses resistance gene Pm17 on its TIAL-1RS translocated chromosome. To be able to use Pm17efficiently in breeding programmes, this gene was transferred to a TIBL-1RS translocation in line Helami-105, and allelism between Pm8 and Pm17was studied. The progenies of the hybrids in the F₂ generation and F₃ families provided evidence that the two genes are allelic. Genetic studies using monosomic analyses confirmed that in cultivar‘Amigo', Pm17 and leaf rust resistance gene Lr24 are located on a translocated chromosome involving 1 A and 1B, respectively.     

Transfer of disease resistance genes from Triticum araraticum to common wheat

The wild tetraploid wheat species Tr$$ (Zhuk) Zhuk Var. araratieum is a source of pest resistance genes for T$$ aesti$$ L. Our objectives were to describe the breeding behaviour of T.arartuititm when backcrossed to common wheat and transfer resistance to leaf rust (caused by Pu$$) and powdery mildew (caused by Blumeria $$wheat. Crosses were made between five wheat genotypes and $$ accessions. Fertifity and chromosome numbers of BC$$_; plants were determined. Resistance to leaf rust was transferred toBC₂ -derived families from 10 different T’ararati$$an accessions. Leaf rust resistance genes in nine T. araratieum accessions can be assigned to at least four loci. Leaf rust resistance transferred from three accessions was inherited in the hexaploid derivatives as a single. $$ gene in each case. Resistance to powdery mildew was also detected in the T. araratie$$ backcross derivatives. Fertile hexaploid derivatives expressing T’araratieum-derived resistance genes can be recovered after two backcrosses to wheat cultivars.     

Molecular markers for the identification of resistance genes and marker-assisted selection in breeding wheat for leaf rust resistance

The resistance genes Lr9, Lr24, Lr25, Lr29, Lr35 and Lr37, which were not previously utilised in Hungary, have been incorporated into four Martonvásár winter wheat cultivars using marker-assisted selection with PCR-based markers. In the course of a backcross programme, the genes were transferred into Martonvásár wheat varieties and various BC generations were produced. Work aimed at pyramiding resistance genes is currently underway in Martonvásár, and plants containing the gene combinations Lr9 + Lr24, Lr9 + Lr25 and Lr9 + Lr29 are now available. From the BC₂F₄ generation of the ‘Mv Emma’*3/’R.L.6010’ combination (‘R.L.6010’ is the donor of the Lr9 gene) 287 lines were tested for leaf rust resistance in an artificially inoculated nursery. A co-dominant primer combination was designed to identify both resistant and susceptible offsprings. The results of resistance tests and molecular marker detection agreed in most cases. Designated leaf rust resistance genes were identified with molecular markers in wheat varieties and breeding lines. The Lr26 and Lr34 resistance genes occur frequently in the Martonvásár gene pool, and the presence of the Lr37 gene has also been detected in a number of Hungarian genotypes.     

Genetic linkage of the Yr1 and Pm4 genes for stripe rust and powdery mildew resistances in wheat

Summary Genes Yr1 for resistance to stripe rust and Pm4a for resistance to powdery mildew showed linkage of 2.0±0.6 cM. Close repulsion linkage probably accounts for the absence in European wheats of genes Yr1 and Pm4b in combination.     

兼抗全蚀病和白粉病小麦新种质的创制与鉴定

TaLTP5是从小麦中分离到的一个脂质转移蛋白编码基因。利用基因枪介导法将TaLTP5表达载体pA25-TaLTP5转入抗白粉病的小麦品种扬麦18 (含抗白粉病基因Pm21)中, 旨在选育兼抗全蚀病和白粉病的小麦新种质。对转基因小麦T₀~T₃代植株中引入TaLTP5基因进行分子检测和抗病性鉴定。PCR检测、Southern杂交分析结果表明, 外源TaLTP5基因已转入、整合到3个转基因小麦株系的基因组中, 并能稳定遗传; 荧光定量RT-PCR的分析以及全蚀病菌的接种与鉴定结果表明, 与受体小麦扬麦18相比, 这3个转基因小麦株系中TaLTP5表达量显著提高, 其对全蚀病的抗性也明显增强。对3个转基因株系的Pm21分子标记和白粉病抗性鉴定表明, 外源TaLTP5基因的导入没有影响受体小麦对白粉病抗性, 说明这些转基因株系为兼抗全蚀病和白粉病小麦新种质。     

Molecular mapping and detection of the yellow rust resistance gene Yr26 in wheat transferred from Triticum turgidum L. using microsatellite markers

Yellow rust (stripe rust), caused by Puccinia striiformis Westend f. sp. tritici, is one of the most devastating diseases of wheat throughout the world. Wheat-Haynaldia villosa 6AL.6VS translocation lines R43, R55, R64 and R77, derived from the cross of three species, carry resistance to both yellow rust and powdery mildew. An F₂ population was established by crossing R55 with the susceptible cultivar Yumai 18. The yellow rust resistance in R55 was controlled by a single dominant gene, which segregated independently of the powdery mildew resistance gene Pm21 located in the chromosome 6VS segment, indicating that the yellow rust resistance gene and Pm21 are unlikely to be carried by the same alien segment. This yellow rust resistance gene was considered to beYr26, originally thought to be also located in chromosome arm 6VS. Bulked Segregation Analysis and microsatellite primer screens of the population F₂ of Yumai 18 × R55 identified three chromosome 1B microsatellite locus markers, Xgwm11, Xgwm18 and Xgwm413, closely linked to Yr26. Yr26 was placed 1.9 cM distal of Xgwm11/Xgwml8, which in turn were 3.2 cM from Xgwm413. The respective LOD values were 21 and 36.5. Therefore, Yr26 was located in the short arm of chromosome 1B. The origin and distribution of Yr26 was investigated by pedigree, inheritance of resistance and molecular marker analysis. The results indicated that Yr26 came from Triticum turgidum L. Three other 6AL.6VS translocation lines, R43, R64 and R77, also carried Yr26. These PCR-based microsatellite markers were shown to be very effective for the detection of the Yr26 gene in segregating populations and therefore can be applied in wheat breeding. This revised version was published online in July 2006 with corrections to the Cover Date.     

Identification and chromosomal locations of novel genes for resistance to powdery mildew and stripe rust in a wheat line 101-3

Wheat powdery mildew and stripe rust, caused by Blumeria graminis f.sp.tritici (syn. Erysiphe graminis f.sp.tritici) and Puccinia striiformis Westend., respectively, are two important fungal diseases of wheat in many regions in the world that cause significant annual yield losses. In the present study, a dominant powdery mildew and a dominant stripe rust resistance gene in wheat line 101-3 which derived from the progenies of the wide cross between common wheat and Dasypyrum villosum Candary L., was located on chromosome 6B and 1B, respectively, by monosomic analyses. The two genes are different from known resistance genes on chromosome 6B for powdery mildew and 1B for stripe rusts, suggesting that the two genes might be novel resistance genes for powdery mildew and stripe rust, respectively. It is uncertain whether the two genes are allelic or lined with other resistance genes located on chromosome 6B for powdery mildew and 1B for stripe rust. Further allelism tests are necessary to determine the relationships between the resistance gene and other genes located on chromosome 6B for powdery mildew and 1B for stripe rust through molecular markers.     

小麦多基因聚合体YW243的改良与利用

YW243是兼抗白粉、黄矮、三锈5种病害的普通小麦新种质。将其与农艺性状优良的丰产品种进行回交转育，选育出丰产、抗病的小麦新品系CB031、CB032、CB034和CB035。对这些新品系与YW243及回交亲本的抗性、品质、丰产性进行鉴定、比较分析，并用分子标记解析它们抗病性的遗传基础及其决定品质的高分子量麦谷蛋白亚基组成。结果表明，CB031是抗白粉病高产小麦新品系，至少含抗白粉病基因Pm2+6和高分子量麦谷蛋白亚基1, 7+9, 2+12；CB032和 CB034均为白粉病、条锈病免疫的小麦新品系，CB032至少含抗白粉病基因Pm2+Pm4+Pm21、抗条锈病基因YrX 4个基因和高分子量麦谷蛋白亚基7+9, 2+12；CB034至少含Pm21基因和高分子量麦谷蛋白亚基7+9, 5+10；CB035为免疫白粉病的优质小麦新品系，至少含Pm2+6+Pm21基因和高分子量麦谷蛋白亚基7+8, 2+12。CB031、CB032、CB034和CB035的穗粒性状、千粒重和秆高等农艺性状均较YW243有所改善。YW243是一个优良性状易于遗传、不良性状易于改造的育种亲本，有良好的应用前景。     

Resistance to leaf rust in cultivars of bread wheat and durum wheat grown in Spain

A set of bread wheat and durum wheat cultivars adapted to Spanish conditions was tested for resistance against leaf rust caused by different pathotypes of Puccinia triticina in field trials and in growth chamber studies. Lower levels of resistance were found in durum wheat than in bread wheat. The most frequent Lr genes found in bread wheat were Lr1, Lr10, Lr13, Lr20, Lr26 and Lr28. In durum wheat, additional resistance genes that differed from the known Lr genes were identified. The level of partial resistance to leaf rust was in general low, although significant levels were identified in some bread wheat and durum wheat cultivars.     

12个小麦品种(系)白粉病抗性的遗传分析

利用17个不同来源和毒力的白粉菌菌株对12个小麦品种(系)进行苗期抗性鉴定和抗病性遗传分析,同时利用Pm2和Pm8基因的特异分子标记检测了相应基因。供试的12个品种至少能够抗11个白粉菌菌株。用E09、E20和Bg2菌株接种F₂群体,抗感植株分离比例和适合性测验证明这12个品种对不同白粉菌菌株的抗性均受1对显性基因控制。抗谱分析和基因紧密连锁分子标记(Xcfd81)分析表明良星66很可能含有Pm2或其等位基因。ω-黑麦碱基因(1RS染色体)和Glu-B1基因(1BS染色体)特异分子标记分析结果证明,山农20和郑麦9962含有T1BL·1RS易位染色体,即可能携带Pm8基因。由于Pm8基因对大多数菌株表现感病,所以这2个品种除Pm8外,还具有其他抗病基因。偃展4110与天民668对参试菌株的反应型表现一致,其他材料对不同菌株的反应型表现不同。     

Genes for resistance to wheat powdery mildew in derivatives of Triticum timopheevi and T. carthlicum

Summary The winter wheat line TP 114 derived from CI 12633, a Triticum timopheevi derivative, has two unlinked dominant genes conditioning resistance to the powdery mildew fungus (Erysiphe graminis f. sp. tritici). One of the genes is identical to gene Pm2 (Ml _u ). The other gene differs from the eleven Pm and/or Ml designated genes; a temporary designation, Ml _f ,is proposed for this gene. Gene Ml _f is closely associated with a gene conditioning resistance to the stem rust fungus (Puccinia graminis f. sp. tritici), probably gene Sr9c.The winter wheat line TP 229 derived from Triticum carthlicum has one dominant mildew resistance gene identical to gene Ml _e in Weihenstephaner M 1.     

Identification of a microsatellite marker associated with Pm3 resistance alleles to powdery mildew in wheat

The Pm3 resistance locus, located on chromosome 1A in wheat, confers race‐specific resistance to the obligate biotrophic fungus Blumeria graminis (DC) E.O. Speer f. sp. tritici, the causal agent of powdery mildew. Several Pm3 alleles are still effective in controlling the disease in Europe. A genetic map was constructed to map the Pm3g allele in the recombinant inbred line progeny from the cross ‘RE9001’ (susceptible) בCourtot’ (resistant). Two microsatellite markers were closely mapped to Pm3g. The PSP2999 marker, which cosegregates with this allele, was shown to detect the presence of the Pm3g resistance allele in other cultivars. A collection of 56 wheat cultivars or advanced lines carrying one Pm3 allele was used to assess the allele‐specific amplification of the PSP2999 marker. The same amplification pattern was obtained for lines with Pm3a, Pm3b, Pm3e, Pm3f and Pm3g alleles. Twenty genotypes carrying Pm3d showed a specific amplification pattern. This marker allowed the detection of the Pm3d allele in highly resistant lines whose resistance gene combinations were unknown. It was concluded that PSP2999 is a useful marker to detect Pm3 alleles in parents and to manage them in breeding programmes.     

Molecular genetics of race non-specific rust resistance in wheat

Over 150 resistance genes that confer resistance to either leaf rust, stripe rust or stem rust have been catalogued in wheat or introgressed into wheat from related species. A few of these genes from the ‘slow-rusting’ adult plant resistance (APR) class confer partial resistance in a race non-specific manner to one or multiple rust diseases. The recent cloning of two of these genes, Lr34/Yr18, a dual APR for leaf rust and stripe rust, and Yr36, a stripe rust APR gene, showed that they differ from other classes of plant resistance genes. Currently, seven Lr34/Yr18 haplotypes have been identified from sequencing the encoding ATP Binding Cassette transporter gene from diverse wheat germplasm of which one haplotype is commonly associated with the resistance phenotype. The paucity of well characterised APR genes, particularly for stem rust, calls for a focused effort in developing critical genetic stocks to delineate quantitative trait loci, construct specific BAC libraries for targeted APR genes to facilitate robust marker development for breeding applications, and the eventual cloning of the encoding genes.