Stripe Rust Partial Resistance Increases Spring Bread Wheat Yield in South‐eastern Anatolia,Turkey

Stripe rust caused by Puccinia striiformis f.sp. tritici is the most serious disease of wheat globally including south‐eastern Anatolia of Turkey, where wheat originated. In this study, 12 spring wheat genotypes were artificially inoculated and preserved in two locations, Diyarbak?r and Ad?yaman, during the 2011–2012 season to investigate loss in yield and yield components. Genotypes were evaluated at the adult plant stage using two partial resistance parameters: final disease severity and area under the disease progress curve (AUDPC). AUDPC ranged from 14.8 to 860 in Diyarbak?r, and 74 to 760 in Ad?yaman. Yield loss ranged from 0.6 to 68.5% in Diyarbak?r and 9.8 to 56.8% in Ad?yaman. Genotypes G1, G5, G7 and G8 were found to lose less yield, while higher yield loss was observed in G3, G4 (Nurkent), G5 and G9 (Karacada?‐98). The highest loss in thousand kernel weight was observed in a susceptible cultivar Karacada?‐98 in Diyarbak?r followed by 43.4 and 24.4% in Ad?yaman. Test weight loss reached 8.89% in Diyarbak?r and 20.8% in Ad?yaman. Yield loss and AUDPC had a positive significant relationship. Based on the values of AUDPC, final disease severity and yield loss, three major clusters were formed for 12 wheat genotypes. Partially resistant genotypes were found to lose less grain yield and seemed to be stronger against severe stripe rust pressure.     

Stripe Rust Resistance in Roegneria kamoji (Poaceae: Triticeae) and its Genetic Analysis

The Roegneria kamoji accession ZY 1007 was resistant to the mixed predominant races of Puccinia striiformis f.sp. tritici (Pst) in China based on field tests at adult‐plant stage. The seedling resistance evaluation of ZY 1007 showed that it was resistant to stripe rust physiological strains CYR29, CYR33 and PST‐V26, which were the predominant races of Pst in China. The female parent R. kamoji cv. Gansi No.1 (susceptible to Pst) was crossed with ZY 1007 (resistant to Pst). Parents, F₁ and F₂ populations were tested in a field inoculated with the mixed urediniospores. ZY 1007 and all the observed 11 F₁ hybrid plants were resistant, while plants of Gansi No.1 were susceptible. Among the 221 F₂ plants, 168 plants were resistant and 53 were susceptible, and the segregation of resistant and susceptible plants fits 3R:1S ratio (χ² = 0.074, P > 0.75). It confirmed that the resistance of stripe rust in ZY 1007 was controlled by a single dominant gene and temporarily designated as YrK1007.     

小偃6号抗条锈基因遗传分析及分子标记

用小麦条锈菌CY 29-m u t3、CY 28、CY 27和CY 25分别接种小偃6号、铭贤169及其F2代各株系,在常温下(15~17℃)和高温下(20~22℃)进行了小偃6号抗条锈基因的遗传分析.结果发现,在常温下,小偃6号对4个条锈菌生理小种的抗病性均由1对显性核基因控制;在高温下,其抗病性由2对或3对基因控制,但其正反交的作用方式不同,抗锈性也可能与细胞质遗传有关;筛选到与抗条锈基因连锁的RAPD标记,分别命名为OPT 17650、OPC 111000.同时,具有长穗偃麦草血缘的小麦品种小偃22对OPC 11进行了验证,明确了其在分子辅助育种中的价值.     

Molecular Detection of Stripe Rust Resistance Gene(s) in 115 Wheat Cultivars (lines) from the Yellow and Huai River Valley Wheat Region

Stripe rust (yellow rust), caused by Puccinia striiformis f.sp. tritici (Pst), is a serious disease of wheat worldwide, including China. Growing resistant cultivars is the most cost‐effective and environmentally friendly approach to control the disease. To assess the stripe rust resistance in commercial wheat cultivars and advanced lines in the Yellow and Huai River Valley Wheat Region, 115 wheat cultivars (lines) collected from 13 provinces in this region were evaluated with the most prevalent Chinese Pst races CYR32, CYR33 and the new race V26 at seedling stage. In addition, these wheat entries were inoculated with the mixed races of CYR32 and CYR33 at the adult‐plant stage in the field. The results indicated that 53 (46.1%) cultivars (lines) had all‐stage resistance to all the three races, and 16 (13.9%) cultivars (lines) showed adult‐plant resistance. The possible stripe rust resistance genes in these entries were postulated by the closely linked markers of all‐stage resistance genes Yr5, Yr9, Yr10, Yr15 and Yr26 and adult‐plant resistance gene Yr18. Molecular analysis indicated that resistance genes Yr5, Yr9, Yr10, Yr18 and Yr26 were found in 5 (4.3%), 38 (33.0%), 1 (0.9%), 2 (1.7%) and 8 (7.0%) entries, respectively. No entry was found to carry the Yr15 gene. In future breeding programs, Yr5, Yr15 and Yr18 should be used to pyramid with other effective genes to develop wheat cultivars with high‐level and durable resistance to stripe rust, whereas Yr9, Yr10 and Yr26 should not be used or used in a limited way due to the virulent races present in China.     

Genetic and Molecular Mapping of Stripe Rust Resistance Genes in Wheat Cultivar Zhongliang 12

Stripe rust, caused by Puccinia striiformis f.sp. tritici (Pst), is one of the most widespread and destructive diseases of wheat worldwide. Resistance breeding is constantly pursued for decades to tackle the variations of prevalent Pst races. Zhongliang 12 has strong resistance to abiotic stresses, wide adaptability, higher resistance to stripe rust and excellent biological characteristics. To identify the resistance gene(s) against stripe rust, Zhongliang 12 was crossed with stripe rust susceptible genotype Mingxian 169, and F₁, F₂, F_2 : 3 and BC₁ progenies were tested with Chinese Pst race CYR30 and CYR31 in seedling stage in greenhouse. Zhongliang 12 possessed different dominant genes for resistance to each race. Linkage maps were constructed with four simple sequence repeats (SSRs) markers, Xwmc695, Xcfd20, Xbarc121 and Xbarc49, for the gene on wheat chromosome 7AL conferring resistance to CYR30 (temporarily designated as Yrzhong12‐1) with genetic distance ranging from 3.1 to 10.8 cM and four SSR markers, Xpsp3003, Xcfd2129, Xwmc673 and Xwmc51, for the gene on wheat chromosome 1AL conferring resistance to CYR31 (temporarily designated as Yrzhong12‐2) with genetic distance ranging from 3.9 cM to 9.3 cM. The molecular markers closely linked to each gene should be useful in marker‐assisted selection in breeding programmes for against stripe rust.     

Genetic Analysis and Molecular Mapping of a Stripe Rust Resistance Gene in Chinese Wheat Differential Guinong 22

Stripe rust, caused by Puccinia striiformis f.sp. tritici (Pst), is one of the most damaging diseases of wheat worldwide, especially in China. Growing resistant cultivars is the most effective approach to control the disease, but few effective resistance genes are available. Guinong 22, one of the wheat cultivars used for differentiated Chinese race of the pathogen, has unknown resistance gene(s) to stripe rust. Genetic analysis, molecular mapping and allelic analysis were used in this study to determine the inheritance and chromosomal location of the gene(s) in Guinong 22 with the most prevalent Pst race CYR33. Genetic analysis indicated that a single recessive gene yrGn22 confers the resistance to CYR33. A total of 450 simple sequence repeat (SSR) primer pairs and 31 pairs of sequence‐tagged site (STS) or conserved primers were selected to screen the resistant bulk and susceptible bulk as well as the parents. Seven polymorphic SSR markers and two STS markers were then used to genotype 113 F₂ individual plants. Linkage analysis indicated that all nine markers were linked to yrGn22, with genetic distances ranging from 2.2 to 11.1 cM. Based on the chromosomal locations of the linked markers, yrGn22 was located on wheat chromosome 1B near the centromere. The pedigree, common markers, chromosome location, resistance and allelism tests indicated that yrGn22 is either linked to Yr26 or possibly the same gene.     

3个小麦条锈菌鉴别寄主的抗性遗传分析

根据对鉴别寄主的毒性谱,选用小麦条锈病菌生理小种2E16单孢菌系为接种病菌,鉴定了小麦务锈病菌鉴别寄主Chinese166、HeinesⅦ和Vilmorin23的抗性基因构成及其遗传特征。通过对3个鉴别寄主与感病品种铭贤169杂交,分别在苗期鉴定了亲代、F1、F2、BC1及正反交后代对小种2E16的抗性反应。结果表明：供试品种Chinese166对生理小种2E16的抗性由二对显性基因,即显性基因Yr1和另一对显性基因独立或重叠控制;HeinesⅦ对生理小种2E16的抗性由一对显性基因Yr2和一对隐性基因控制;Vilmorin23对生理小种2E16的抗性则由显性基因Yr3和一对隐性基因控制。     

Distribution, Frequency and Variation of Stripe Rust Resistance Loci Yr10, Lr34/Yr18 and Yr36 in Chinese Wheat Cultivars

Wheat stripe rust is a devastating disease in many regions of the world. In wheat, 49 resistance genes for stripe rust have been officially documented, but only three genes are cloned, including the race-specific resistance Yr10 candidate gene (Yr10_CG) and slow-rusting genes Lr34/Yr18 (hereafter designated as Yr18) and Yr36. In this study, we developed gene-specific markers for these genes and used them to screen a collection of 659 wheat accessions, including 485 Chinese cultivars. Thirteen percent and eleven percent of the tested Chinese cultivars were positive for the markers for Yr10_CG and Yr18_RH (the resistant haplotype of Yr18), respectively, but none were positive for the Yr36 marker. Since there is a limited use of the Yr10 gene in Chinese wheat, the relatively high frequency of wheat varieties with the Yr10_CG marker suggests that the identity of the Yr10 gene is unknown. With regards to the Yr18 gene, 29% of the tested cultivars that are used in the Middle and Lower Yangtze Valleys' winter wheat zone were positive for Yr18_RH markers. A non-functional allele of Yr18_RH was identified in ‘Mingxian 169’, a commonly used susceptible check for studying stripe rust. The data presented here will provide useful information for marker-assisted selection for wheat stripe rust resistance.     

Histopathology of Leaf Rust Infection and Development in Wheat Genotypes containing Lr12 and Lr13

Evidence exists that certain genes for resistance to leaf rust in wheat, e.g. Lr13 and Lr34 , may interact with other genes to condition higher levels of resistance than that conferred by each gene individually. In this study, the hypothesis that Lr12 and Lr13 , both genes for adult plant resistance to Puccinia recondita Roberge ex. Desmaz f. sp. tritici Eriks. and Henn., interact to confer an improved level of resistance, was investigated using fluorescence and phase-contrast microscopy. Flag leaf segments of monogenic and digenic Thatcher lines, sampled 64 and 240 h post-inoculation, were stained with Uvitex 2B and screened, using fluorescence microscopy, for development of infection structures or host response. To study cell wall appositions, specimens were stained with trypan blue and a solution of picric acid in methyl salicylate. Aborted penetration, consisting of nonpenetrating appressoria and aborted substomatal vesicles, showed that inhibition of fungal growth in wheat lines containing Lr12 and/or Lr13 was activated, to a certain degree, before haustoria were formed. At 240 h after inoculation colony size indicated that fungal colonies in the Lr gene combination lines were generally smaller than in the parents, but not necessarily smaller than those in a line with Lr13 only. Host cell necrosis was more frequently associated with infection sites, specifically of pathotype UVPrt2, in the combination lines than in the parents. The morphology of cell wall appositions varied considerably from a narrow, luminous zone slightly wider in the centre, to a thick central part opposite the haustorium mother cell, sharply decreasing towards both ends. Histological assessments could, however, not conclusively prove pronounced resistance enhancement or unconventional resistance mechanisms due to combining the genes Lr12 and Lr13 .     

温室条件下条形柄锈菌体细胞重组的分子确证

为了获得温室条件下条形柄锈菌发生体细胞重组而导致毒性变异的直接证据,本研究选取7个美国条形柄锈菌小麦专化型菌系和2个美国条形柄锈菌大麦专化型菌系按照夏孢子颜色和专化型与毒性差异组成9对菌系组合,对于室内混合接种产生的子代菌系用具有不同抗性的小麦或大麦品种进行筛选,采用毒性分析及SSR分子标记技术对条形柄锈菌体细胞重组现象进行了研究。对获取的413个单孢子代菌系进行的毒性分析结果显示,有84个单孢子代菌系的毒性谱表现与亲本菌系不同,初步证明体细胞重组过程的存在。SSR标记分析结果显示,11对SSR引物中有6对引物在5对菌系组合的28个毒性谱不同的单孢子代菌系中,检测发现3个单孢菌系的扩增条带与其亲本菌系不同,且表现为亲本菌系扩增条带的重组,为体细胞重组菌系。这一结果从分子水平上证明了条形柄锈菌在室内接种条件下可以通过体细胞重组产生新小种而导致毒性变异。     

TaADF4, an actin‐depolymerizing factor from wheat,is required for resistance to the stripe rust pathogen Puccinia striiformis f. sp. tritici

Actin filament assembly in plants is a dynamic process, requiring the activity of more than 75 actin‐binding proteins. Central to the regulation of filament assembly and stability is the activity of a conserved family of actin‐depolymerizing factors (ADFs), whose primarily function is to regulate the severing and depolymerization of actin filaments. In recent years, the activity of ADF proteins has been linked to a variety of cellular processes, including those associated with response to stress. Herein, a wheat ADF gene, TaADF4, was identified and characterized. TaADF4 encodes a 139‐amino‐acid protein containing five F‐actin‐binding sites and two G‐actin‐binding sites, and interacts with wheat (Triticum aestivum) Actin1 (TaACT1), in planta. Following treatment of wheat, separately, with jasmonic acid, abscisic acid or with the avirulent race, CYR23, of the stripe rust pathogen Puccinia striiformis f. sp. tritici, we observed a rapid induction in accumulation of TaADF4 mRNA. Interestingly, accumulation of TaADF4 mRNA was diminished in response to inoculation with a virulent race, CYR31. Silencing of TaADF4 resulted in enhanced susceptibility to CYR23, demonstrating a role for TaADF4 in defense signaling. Using a pharmacological‐based approach, coupled with an analysis of host response to pathogen infection, we observed that treatment of plants with the actin‐modifying agent latrunculin B enhanced resistance to CYR23, including increased production of reactive oxygen species and enhancement of localized hypersensitive cell death. Taken together, these data support the hypothesis that TaADF4 positively modulates plant immunity in wheat via the modulation of actin cytoskeletal organization.     

Microscopic Observation on the Development of Puccinia striiformis in the Spike and Stem of Wheat

The majority of germ tubes of the pathotype CYR32 of Puccinia striiformis f.sp. tritici formed on the surface of spike organs of the susceptible wheat cv. Suwon 11 penetrated through the stomatal pore, only a few germ tubes formed small appressoria over the stomata. In the lemma, palea and glume, the stripe rust fungus spread between the parenchyma cells close to the inner epidermal layer, but the fungus did not develop between the thick‐walled cells near the outer epidermal layer of these organs. In the awn and stem, spread of the stripe rust was confined to the intercellular spaces of the chlorophyll parenchyma, beneath the invaded stomatal pore of the epidermis and the urediniospores to be released disrupted the epidermis. In the caryopsis, the spread of hyphae was restricted to the intercellular spaces of the pericarp cells.     

一氧化氮在寡糖素诱导的小麦对条锈菌系统获得抗性中的时序性

研究了寡糖素在诱导感病小麦品种辉县红系统抗条锈性中的作用,同时利用ESR测定了系统获得抗性（SAR）中一氧化氮(NO)的时间进程,结果表明寡糖素可以诱导辉县红对条锈菌毒性小种CY29-1的系统抗性,此系统抗性与内源NO信号启动的时间及强度有关.     

The RLK protein TaCRK10 activates wheat high-temperature seedling-plant resistance to stripe rust through interacting with TaH2A.1

Plants sense various pathogens and activate immunity responses through receptor-like kinases (RLKs). Cysteine-rich receptor-like kinases (CRKs) are involved in massive transduction pathways upon perception of a pathogen. However, the roles of CRKs in response to stripe rust are unclear. In the present study, we identified a CRK gene (designated TaCRK10) from wheat variety Xiaoyan 6 (XY6) that harbors high-temperature seedling-plant (HTSP) resistance to stripe rust caused by fungal pathogen Puccinia striiformis f. sp. tritici (Pst). The expression level of TaCRK10 was induced by Pst inoculation and high temperature treatment. Knockdown of TaCRK10 by virus-induced gene silencing resulted in attenuated wheat HTSP resistance to Pst, whereas there is no effect on Pst development and host responses under normal temperatures. Notably, overexpression of TaCRK10 in susceptible variety Fielder provided resistance only under normal temperatures at 14 days with reactive oxygen species accumulation and defense-related gene expression of the salicylic acid pathway. Moreover, TaCRK10 physically interacted with and phosphorylated a histone variant TaH2A.1, which belongs to the H2A.W group. Silencing of TaH2A.1 suppressed wheat resistance to Pst, indicating that TaH2A.1 plays a positive role in wheat resistance to Pst. Thus, TaCRK10 serves as an important sensor of Pst infection and high temperatures, and it activates wheat resistance to Pst through regulating nuclear processes. This knowledge helps elucidate the molecular mechanism of wheat HTSP resistance to Pst and promotes efforts in developing wheat varieties with resistance to stripe rust.     

SRAP Technique Efficiently Generates Polymorphisms in Puccinia striiformis Isolates

Wheat stripe rust, caused by the fungal pathogen Puccinia striiformis f.sp. tritici (PST), is a major disease of wheat in temperate‐cold climates. The identification of new markers would ease the procedure for evaluating the ongoing pathogen evolution. Twelve single pustule isolates were generated from samples of PST obtained in UK during 1987–2001. They were evaluated for their pathogenic behaviour on a set of differential cultivars and were analysed by sequence‐related amplified polymorphisms (SRAP) technique, to identify polymorphisms useful to evaluate variability among isolates. This is the first report of the application of SRAP technique to Uredinales order.     

人工合成小麦CI184条锈病成株抗性基因的鉴定及分子标记定位

以硬粒小麦-粗山羊草人工合成小麦CI184、感病品种‘铭贤169’及其杂交组合的正反交F1以及CI184/‘铭贤169’F2、F2:3家系为材料,鉴定其条锈病抗性,对CI184条锈病抗性进行遗传分析;采用SSR分子标记技术和集群分离分析法进行多态性筛选,以F3抗病鉴定数据为依据,对CI184中条锈病抗性基因进行分子标记定位。结果显示:(1)CI184在苗期抗性鉴定中,对30种小麦条锈菌生理小种表现抗性,但对中国四川新出现的条锈菌生理小种V26表现苗期感病;在田间成株抗性接种鉴定中,CI184对中国流行的小麦条锈菌生理小种条中32、条中33、水源4、水源5、水源7和V26等表现出成株抗性。(2)CI184中条锈病抗性由隐性基因位点控制。(3)仅检测到一个控制条锈病抗性的QTL位点,位于1B染色体上Xgwm18和Xwmc626之间,暂时命名为Qyr.zz_1B,在四川和北京2个环境中可分别解释CI184中13.36%和18.07%的成株抗性贡献率。(4)Qyr.zz_1B位点的3个SSR标记和Yr15的1个SSR标记可以区分该位点与1B染色体上的其他抗条锈病基因,如Yr15、Yr24和Yr26/YrCH42。表明Qyr.zz_1B位点在小麦条锈病的抗病育种中具有潜在的应用价值。     

Competition Alters Temporal Dynamics of Sporulation in the Wheat Stem Rust Fungus

To investigate the effects of competition on the timing of pathogen reproduction, urediniospores of two strains of Puccinia graminis f.sp. tritici (SR22 and SR41) were inoculated onto leaves of wheat seedlings singly and in 1 : 1 mixture at three inoculum densities. On randomly sampled leaves, uredinia were counted 9 days after inoculation and urediniospores were collected and quantified every other day from the seventh to the 29th day after inoculation. Increases in inoculum density resulted in progressively smaller increases in uredinial numbers. However, total urediniospore production per leaf was not significantly affected by inoculum, and hence uredinial, density over a range of approximately 10-300 uredinia on the leaf. Total urediniospore production per uredinium generally decreased with increasing inoculum or uredinial density. At high densities, sporulation per uredinium peaked earlier in the sporulation period, had a less distinct peak, and dropped off earlier than for the lower densities. Logistic model fits to cumulative sporulation curves over time revealed that strain SR41 had a greater epidemic rate parameter (r) than SR22 at low and intermediate inoculum or uredinial densities, while SR22 had a higher r-value than SR41 at high density. Both strains also exhibited greater r-values in the presence of the other strain than when alone. Results suggest that strains may have different ecological strategies in their timing of reproduction, and that both intra- and interstrain competition can have complex effects on the temporal dynamics of sporulation in pathogen strains.     

小麦抗条锈病近等基因系感染条锈病后丁布含量变化

选用2套遗传背景不同的抗条锈病近等基因系作为供试寄主材料,研究了不同抗条锈病近等基因系丁布的含量及其在感病过程中丁布含量的动态变化.结果表明,在未受病菌侵染情况下,2套分别含有Yr2、Yr9和YrSpP基因的近等基因系（抗病系）与其轮回亲本Taichung 29、铭贤169(感病系)间丁布含量没有显著差异（P＞0.05）.接种条锈病菌后,感病系在病菌侵染初期丁布含量下降,而抗病系在病菌侵染初期丁布含量迅速大幅度上升.感染条锈病最终导致感病植株丁布含量比未接种的植株明显减少, 感病系的减少幅度明显高于抗病系.在整个病程中,抗病系丁布的含量始终高于感病系,表明接种条件下小麦植株体内丁布含量变化与小麦抗条锈近等基因系的抗性有关.     

Isolation of twelve microsatellite loci,using an enrichment protocol,in the phytopathogenic fungus Puccinia striiformis f.sp. tritici

We report the characterization of 12 microsatellite markers in the biotrophic fungus Puccinia striiformis f.sp. tritici, responsible for yellow rust on wheat. An enrichment protocol was used to isolate microsatellite loci, and polymorphism was explored with 96 isolates from natural populations collected from several French and Chinese locations. Eight primers (67%) showed cross‐amplification when tested with eight isolates of P. triticina.     

The Puccinia striiformis effector Hasp98 facilitates pathogenicity by blocking the kinase activity of wheat TaMAPK4

The obligate biotrophic fungus Puccinia striiformis f. sp. tritici (Pst) employs virulence effectors to disturb host immunity and causes devastating stripe rust disease. However, our understanding of how Pst effectors regulate host defense responses remains limited. In this study, we determined that the Pst effector Hasp98, which is highly expressed in Pst haustoria, inhibits plant immune responses triggered by flg22 or nonpathogenic bacteria. Overexpression of Hasp98 in wheat (Triticum aestivum) suppressed avirulent Pst-triggered immunity, leading to decreased H₂O₂ accumulation and promoting P. striiformis infection, whereas stable silencing of Hasp98 impaired P. striiformis pathogenicity. Hasp98 interacts with the wheat mitogen-activated protein kinase TaMAPK4, a positive regulator of plant resistance to stripe rust. The conserved TEY motif of TaMAPK4 is important for its kinase activity, which is required for the resistance function. We demonstrate that Hasp98 inhibits the kinase activity of TaMAPK4 and that the stable silencing of TaMAPK4 compromises wheat resistance against P. striiformis. These results suggest that Hasp98 acts as a virulence effector to interfere with the MAPK signaling pathway in wheat, thereby promoting P. striiformis infection.