Identification of eight Berberis species from the Yunnan-Guizhou plateau as aecial hosts for Puccinia striiformis f.sp.tritici,the wheat stripe rust pathogen

Puccinia striiformis Westend.f.sp.tritici Erikss.(Pst)infects wheat and causes stripe rust.The rust is heteroecious with wheat as the primary uredinial and telial host and barberry(Berberis spp.)as the alternate pycnial and aecial host.More than 40 Berberis species have been identified as alternate hosts for Pst,and most of these are Chinese Berberis species.However,little is known about Berberis species or their geographic distributions in the Yunnan-Guizhou plateau in southwestern China.The Yunnan-Guizhou plateau is considered to be an important and relatively independent region for the evolution of the wheat stripe rust pathogen in China because the entire disease cycle can be completed within the region.In this study,we conducted a survey of barberry plants in the Yunnan-Guizhou plateau and identified the eight Pst-susceptible Berberis species under controlled conditions,including B.julianae,B.tsienii,B.veitchii,B.wilsonae,B.wilsonae var.guhtzunica,B.franchetiana,B.lepidifolia and B.pruinosa.These species are reported here for the first time to serve as alternate hosts for the wheat stripe rust pathogen under controlled conditions.

Yr5-virulent races of Puccinia striiformis f.sp.tritici possess relative parasitic fitness higher than current main predominant races and potential risk

Wheat stripe rust,caused by Puccinia striiformis f.sp.tritici(Pst),is one of the most destructive fungal diseases of wheat,and seriously threatens safe production of the crop worldwide.In China,new races historically appeared and rapidly developed to be predominant races and have resulted in ineffectiveness and replacement of wheat resistance cultivars as well as massive reduction in yield.In the present study,the relative parasitic fitness of the two newlyemerged Yr5-virulent races(TSA-6 and TSA-9)were compared with those of four currently predominant Chinese races(CYR31,CYR32,CYR33,and CYR34)based on evaluation on 10 Chinese wheat cultivars.As a result,there were significant differences in the relative parasitic fitness parameters among overall tested races based on multiple comparison(LSD)analysis(P<0.05).The principal component analysis(PCA)of overall parasitic fitness parameters indicated that the sporulation ability,infection and spore survivability,expansion capacity,and potential pathogenicity were the most important parasitic fitness attributes of the tested races.Based on the establishment of extracted three principal components and a comprehensive factor score mathematical models,evaluations of the parasitic fitness attributes of tested races showed that the level of relative parasitic fitness of the tested six races was:CYR32(1.15)>TSA-9(0.95)>TSA-6(0.92)>CYR34(0.29)>CYR31(–1.54)>CYR33(–1.77).The results indicated that two Yr5-virulent races TSA-9 and TSA-6 possessed relative parasitic fitness higher than races CYR34,CYR31,and CYR33,but lower than race CYR32,and have potential risks in developing to be predominant races.Therefore,continual monitoring of both Yr5-virulent races,and their variants is needed.The use of wheat cultivars(lines)with Yr5 resistance gene singly in wheat breeding is essential for being avoided,and is suggested to combine with other effective stripe rust resistance genes.

High-throughput RNA sequencing reveals differences between the transcriptomes of the five spore forms of Puccinia striiformis f.sp.tritici,the wheat stripe rust pathogen

The devastating wheat stripe(yellow)rust pathogen,Puccinia striiformis f.sp.tritici(Pst),is a macrocyclic and heteroe-cious fungus.Pst produces urediniospores and teliospores on its primary host,wheat,and pycniospores and aeciospores are produced on its alternate hosts,barberry(Berberis spp.)or mahonia(Mahonia spp.).Basidiospores are developed from teliospores and infect alternate hosts.These five spore forms play distinct roles in Pst infection,disease development,and fungal survival,etc.However,the specific genes and mechanisms underlying these functional differences are largely unknown.In this study,we performed,for the first time in rust fungi,the deep RNA sequencing to examine the transcriptomic shift among all five Pst spore forms.Among a total of 29,591 identified transcripts,951 were specifically expressed in basidiospores,whereas 920,761,266,and 110 were specific for teliospores,pycniospores,aeciospores,and urediniospores,respectively.Additionally,transcriptomes of sexual spores,namely pycniospores and basidiospores,showed significant differences from those of asexual spores(urediniospores,teliospores,and aeciospores),and transcriptomes of urediniospores and aeciospores were more similar to each other than to the three other spore forms.Especially,the basidiospores and pycniospores which infected the berberis shows wide differences in the cell wall degrading-enzymes and mating and pheromone response genes.Besides,we also found that there are 6234 differential expressed genes between the urediniospores and pycniospores,while only have 3 genes have alternative splicing enents,suggesting that differential genes expression may make more contribution than AS.This comprehensive transcriptome profiling can substantially improve our understanding of the developmental biology of the wheat stripe rust fungus.

The TaFIM1 gene mediates wheat resistance against Puccinia striiformis f. sp. tritici and responds to abiotic stress

Fimbrin, a regulator of actin cytoskeletal dynamics that participates in numerous physiological and biochemical processes, controls multiple developmental processes in a variety of tissues and cell types. However, the role of fimbrin in pathogen defense of wheat and the mechanisms have not been well studied. Here, we investigated that the expression of TaFIM1 gene of wheat was significantly induced in response to avirulent race of Puccinia striiformis f. sp. tritici(Pst) and silencing of TaFIM1 by virus-induced gene silencing method. The results show that silencing of TaFIM1 resulted in a reduction of resistance against the stripe rust indicated by both phenotypes and a histological examination of Pst growth. Additionally, the expression level of Ta FIM1 gene was up-regulated under abiotic stresses. These findings suggest that Ta FIM1 functions as a positive regulator of pathogen resistance of wheat plants and response to abiotic stress. Our work may show new light on understanding the roles of fimbrin in wheat.

Effects of Different Cultivation Patterns of Wheat on Population Structure of Puccinia striiformis West.f. sp. tritici

The paper was to study the effects of different cultivation patterns( mix cultivation and monocultivation) of wheat on population structure of Puccinia striiformis West. f. sp. tritici in the fields. Five race-specific-markers( CY32,CY31,CY29,CY23 and Shuiyuan pathotype) were used to survey 113 infected samples collected from two cultivation patterns. The results indicated that frequency of race-specific-markers under monocultivation was higher than that under mix cultivation; the dominant race-specific-markers were CY32 and CY29 under monocultivation,and the frequency of detection were 81. 5% and 78. 5%,respectively. The dominant race-specific-markers were CY29 and Shuiyuan pathotype under mix cultivation,and the frequency of detection are 41. 7% and 18. 8%,respectively.Several race-specific-markers were detected in single infected leaf,and 41. 7% of infected single leaf were detected with more than two race-specific-markers,58. 3% of infected single leaf were detected with one race-specific-marker under mix cultivation pattern,while there were 75. 0% infected leaves with more than two race-specific-markers and 25. 0% infected single leaf detected with one race-specific-marker under monocultivation pattern. The results indicated that mix cultivation pattern of wheat can reduce races on single leaf,affect the distribution of races in infected leaves,and suppress the occurrence frequency of dominant races of P. striiformis in the fields significantly,subsequently reduced severity and prevalence of the disease.

Association Analysis of SP-SNPs and Avirulence Genes in Puccinia striiformis f. sp. tritici, the Wheat Stripe Rust Pathogen

Puccinia striiformis f. sp. tritici (Pst) is one of the pathogenic fungi on wheat, caused stripe rust that is a great threat for wheat production all over the world. Intensive efforts have been made to study genetics of wheat resistance to this disease, but few on avirulence of the pathogen due mainly to the nature of obligate biotrophism and the lack of systems for studying its genetics and molecular manipulations. To overcome these limitations, a natural Pst population comprising 352 isolates representative of a diverse virulence spectrum was genotyped using 97 secreted protein-single nucleotide polymorphism (SP-SNP) markers to identify candidate avirulence genes using association analysis. Among avirulence genes corresponding to 19 resistance genes, significantly associated SP-SNP markers were detected for avirulence genes AvYr1, AvYr2, AvYr6, AvYr7, AvYr8, AvYr44, AvYrExp2, AvYrSP, and AvYrTye. These results indicate that association analysis can be used to identify markers for avirulence genes. This study has laid the foundation for developing more SP-SNPs for mapping avirulence genes using segregating populations that can be generated through sexual reproduction on alternate hosts of the pathogen.

An improved method for RNA extraction from urediniospores of and wheat leaves infected by an obligate fungal pathogen, Puccinia striiformis f. sp. tritici

Stripe rust, caused by Puccinia striiformis f. sp. tritici, is an important wheat disease in China, seriously threatening wheat production. Understanding the winter survival of the fungus is a key for predicting the spring epidemics of the disease, which determines the crop loss. Estimation of P. striiformis f. sp. tritici winter survival requires processing a large number of samples for sensitive detection of the pathogen in wheat leaf tissue using real-time quantitative reverse transcription PCR （qRT-PCR）. A bottleneck for the analysis is the acquisition of a good yield of high quality RNA suitable for qRT-PCR to distinguish dead and alive fungal hyphae inside leaves. Although several methods have been described in the literatures and commercial kits are available for RNA extraction, these methods are mostly too complicated, expensive and inefficient. Thus, we modified three previously reported RNA extraction methods with common and low-cost reagents （LiCI, SDS and NaCI） to solve the problems and selected the best to obtain high quality and quantity RNA for use in qRT-PCR. In the three improved methods, the NaCI method was proven to be the best for extracting RNAfrom urediniospores of and wheat leaves infected by P. striiformis f. sp. tritici, although the modified LiCI and SDS methods also increased yield of RNA compared to the previous methods. The improved NaCI method has the following advantages： 1） Complete transfer of urediniospores of P. striiformis f. sp. tritici from the mortar and pestle can ensure the initial amount of RNA for the qRT-PCR analysis; 2） the use of low-cost NaCI to replace more expensive Trizol can reduce the cost; 3） the yield and quality of RNA can be increased; 4） the improved method is more suitable for a large number and high quantity of samples from fields. Using the improved NaCI method, the amount of RNA was increased three times from urediniospores of P. striiformis f. sp. tritici compared from the extraction kit. Approximately, 10.11 IJg total RNA of high quality was obtained from 100 mg of infected leaves, which was 8.8, 6.5, 3.4 and 2.1 folds of the amounts obtained from the previous LiCI, SDS, NaCI and traditional Trizol methods, respectively. The method could be used to study the overwintering rates of R striiformis f. sp. tritici over a large region of wheat production for predicting epidemic levels by determining pathogen survival levels after winter. The method can alsobe used in any studies which need a large number of high quality RNA samples.

A FIASCO-Based Approach for Detection and Diagnosis of Puccinia graminis f.sp.tritici in China

Stem or black rust of wheat, caused by the fungus Puccinia graminis Pers. f. sp. tritici Eriks.＆E. Henn. （Pgt）, has historically caused severe losses to wheat （Triticum aestivum L.） production worldwide. In the Fujian and Guangdong provinces of China, six moderate-to-severe epidemics of wheat stem rust have occurred, which caused destructive losses of wheat between 1949 and 1966, although these were brought under control by integrated management. A rapid and reliable detection of the pathogen will contribute to the accurate forecast and seasonal control of this disease. The objective of this study was to develop a diagnostic molecular marker generated from simple sequence repeats （SSR） for the early rapid identiifcation of P. graminis. The genomic DNA of P. graminis, Puccinia striiformis, Puccinia triticina and seven other species was ampliifed by a pair of SSR primers generated by the FIASCO （fast isolation by AFLP sequences containing repeats） enrichment protocol. The primer set Pgtw （f）/Pgtw （r） generated a polymorphic pattern displaying a 330-bp DNA fragment speciifc for P. graminis whereas no DNA fragment was obtained from other non-target wheat fungal pathogens. The detection limit of the primer was 1 ng DNA in a 25-mL PCR reaction. The SSR markers of P. graminis can also be used to detect the presence of latent hyphae in Pgt-infected wheat leaves as early as 30 h post-inoculation. A rapid approach to distinguish P. graminis from similar pathogenic fungi would be anticipated in further study.

Characterization of wheat monogenic lines with known Sr genes and wheat cultivars for resistance to three new races of Puccinia graminis f. sp. tritici in China

Wheat stem rust, caused by Puccinia graminis f. sp. tritici(Pgt), is a potentially devastating fungal disease of wheat worldwide. The present study was to evaluate the resistance of 42 wheat monogenic lines with known stem rust resistance(Sr) genes and 69 wheat cultivars to three new Pgt races(34C0MRGQM, 34C3MKGQM, and 34C6MTGSM)identified from aeciospores at the seedling and adult-plant stages. The phenotyping results revealed that monogenic lines harboring resistance genes Sr9e, Sr17, Sr21, Sr22, Sr26, Sr30, Sr31, Sr33, Sr35, Sr36, Sr37, Sr38, Sr47, SrTmp,and SrTt3 were effectively resistant to all three Pgt races at the seedling and adult-plant stages. In contrast, monogenic lines containing Sr5, Sr6, Sr7b, Sr9a, Sr9d, Sr9f, Sr9g, Sr9b, Sr16, Sr24, Sr28, and Sr39 were highly susceptible to these races at both seedling and adult-plant stages. The other lines with Sr8a, Sr10, Sr11, Sr13, Sr14, Sr15, Sr18, Sr20,Sr19, Sr23, Sr25, Sr27, Sr29, Sr32, and Sr34, displayed variable levels of resistance to one or two of the tested races.Seedling infection types(ITs) and adult-plant infection responses(IRs) indicated that 41(59.4%) of the wheat cultivars showed high resistance to all the three races. Molecular marker analysis showed that four wheat culitvars likely carried Sr2, 20 wheat culitvars likely carried Sr31, 9 wheat culitvars likely carried Sr38, and none of the cultivars carried Sr24,Sr25, and Sr26. Our results provide a scientific basis for rational utilization of the tested Sr genes and wheat cultivars against these novel Pgt races.

Population Diversity of Puccinia graminis is Sustained Through Sexual Cycle on Alternate Hosts

A high degree of virulence diversity has been maintained in the population of Puccinia graminis f. sp. tritici （Pgt） in northwestern United States. Although Berberis vulgaris is present in the region and Pgt has been isolated from aecial infections on B. vulgaris, the population is too diverse to be explained by the limited presence of B. vulgaris alone. Since 2008, we have isolated P. graminis from aecial infections on fruits of Mahonia repens and Mahonia aquifolium from northwestern United States. These two native woody shrub species, widely distributed in western North America, were once classified as resistant to P. graminis based on artificial inoculations. By isolating P. graminis from aecia, we established that M. repens and M. aquifolium along with B. vulgaris （albeit infrequent） serve as the alternate hosts ofP. graminis in the region. The isolates of P. graminis from Mahonia of North America had diverse virulence patterns and most of the isolates could be differentiated on Morocco, Line E, Chinese Spring, Little Club, LMPG-6, Rusty, and other genotypes that are considered to be universally susceptible to most Pgt isolates. This discovery explained the persistence of virulence diversity of Pgt observed in isolates derived from uredinia on cereal crops in the region. In addition to cereal crops, uredinial stage of the P. graminis population is sustained by wild grasses, especially Elymus glaucus, a native grass sharing the same habitat with the rusted Mahonia spp. Although virulence to some important stem rust resistance genes was observed in some isolates derived from Mahonia of North America when tested against single stem rust resistance gene stocks, the overall virulence is very limited in these isolates. This is likely a result of limited selection pressure on the rust population. In contrast to northwestern United Sates, the Pgt population in east of the Rocky Mountains of North America has declined steadily with a single race, QFCSC, being predominant in the last decade. This decline is likely due to a combination of factors, of which a lack of sexual recombination in the region is perhaps the most important one.

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 flg22or nonpathogenic bacteria.Overexpression of Hasp98 in wheat(Triticum aestivum)suppressed avirulent Pst-triggered immunity,leading to decreased H2O2accumulation and promoting P.striiformis infection,whereas stable silencing of Hasp98 impaired P.striiformis pathogenicity.Hasp98 interacts with the wheat mitogenactivated 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 Hasp98inhibits 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.

A small knottin-like peptide negatively regulates in wheat to stripe rust resistance during early infection of wheat

Although Blufensins(Bln)have important functions in the response of plants to biotic stress the precise functioning of Bln in wheat remains largely unknown.Here we isolated a Bln gene(TaBln4)from Suwon 11 infected by Puccinia striiformis f.sp.tritici(Pst).Expression of TaBln4 increased in host plants at the early stage of infection with a virulent Pst race(CYR31)but was unchanged in response to infection by an avirulent race(CYR23).Transcription levels of TaBln4 were also regulated by hormone and abiotic stresses.Expression of TaBln4 in tobacco leaves suppressed Bax-induced programmed cell death.Knockdown of TaBln4 by virus-induced gene silencing inhibited colonization of race CYR31 by increasing the accumulation of H2O2 and formation of hypersensitive responses(HR).Transient overexpression of TaBln4 by a transient overexpression system(BSMV-VOX)increased the susceptibility of wheat to CYR31.Results from bimolecular fluorescence complementation and pull-down assays demonstrated that TaBLN4 interacted with calmodulin.Taken together,our results suggest that TaBln4 negatively regulates resistance in wheat to Pst in a reactive oxygen species(ROS)-and HR-dependent manner.

RAPD技术和聚类分析在小麦条锈病菌生理小种研究中的应用

试用４５个随机引物对我国小麦条锈病菌的６个生理小种（ＣＹＲ１７，ＳＵ１１，ＣＹＲ２３，ＣＹＲ２８，ＣＹＲ２９和ＣＹＲ３０）进行了ＲＡＰＤ分析，其中１０个适宜引物具有鉴别作用，共扩增出８９条ＲＡＰＤ图带，多态性为７３％。自ＣＹＲ２３、ＣＹＲ２８和ＣＹＲ２９三个生理小种中扩增出了特征性ＲＡＰＤ图带。根据ＲＡＰＤ分析结果，将这一结果与６个小种对不同小麦品种苗期和成株期致病性的聚类分析作了比较。可将供试小种分为两组，第一组包括ＣＹＲ１７、ＳＵ１１和ＣＹＲ２３，其中前两者的相似性最大；ＣＹＲ２８和ＣＹＲ２９也较相近，属于第二组；新小种ＣＹＲ３０与其它小种的相关性尚待进一步研究。

2017年我国小麦条锈病流行特点及重发原因分析

2017年小麦条锈病在我国黄淮海麦区大范围流行,表现出汉水流域及黄淮南部见病时间早、扩散速度快、黄淮海麦区流行范围广等特点。本文在系统总结2017年全国小麦条锈病流行特点的基础上,分析认为极端暖冬气候、春季多雨适温气候条件和主产麦区缺乏抗性品种等因素是导致2017年我国小麦条锈病大流行的主要原因。

80份国外春小麦种质资源抗条锈性评价

【目的】小麦条锈病是由小麦条锈菌(Puccinia striiformis f.sp.tritici,Pst)引起的世界范围内小麦重要病害之一,培育和种植抗病品种是控制该病害的最有效策略。评价80份国外春小麦种质资源对中国当前小麦条锈菌流行小种的抗条锈性,为中国小麦抗条锈病育种提供依据和抗源。【方法】应用中国流行小麦条锈菌生理小种CYR29、CYR31、CYR32、CYR33以及致病类型PST-HY8和PST-V26对80份国外小麦种质资源进行苗期温室抗病性鉴定,以铭贤169和Av S为感病对照品种;并于2013年和2014年分别在陕西省杨凌和甘肃省天水进行田间成株期抗病性鉴定。根据苗期和田间成株期的抗病性鉴定结果对其进行抗病类型分类和评价。【结果】80份小麦种质资源的抗病类型可分为3类。第1类为全生育期抗病类型,有8份。其中PI660067、PI660119和PI660122在苗期和田间成株期均表现较高水平的抗病性。其余5个品系PI660056、PI607839、PI591045、TA5602和PI660064在苗期则对个别小种表现感病,并且在不同年份和不同测试地点成株期也表现感病。第2类为成株抗病类型,有28份。其苗期对所有测试小种均表现感病,有23份在田间成株期均表现抗病。但PI660075、PI660083、PI660085、PI660097和PI660107在不同年份和不同测试地点成株期表现感病。第3类为兼具成株期和对部分中国小种失去抗性的全生育期抗病类型,有44份,其苗期至少对一个测试小种表现抗病。有37份在田间成株期均表现抗病。但PI660065、PI660076、PI660079、PI660080、PI660095、PI660096和PI610750在不同年份和不同测试地点成株期表现感病。【结论】80份国外小麦种质资源中大部分对中国小麦条锈菌流行小种表现优良的抗病性。这些种质资源可作为抗源在今后抗病育种中加以利用,将丰富中国小麦抗条锈病基因的多样性。可能由于不同年份田间流行小种不同,造成一些成株抗病品系在不同年份和不同测试地点表现感病,由此推测成株抗病性可能也具有小种专化性。

不同小麦抗条锈基因及小麦品种在四川的有效性

将以Avocet为背景的27份抗小麦条锈病近等基因系、131个抗性基因型较明确的小麦抗源品种和59份四川小麦生产品种和抗源以及和感病对照铭贤169分行种在位于四川省雅安市草坝(N:29°57′09.6,″E:103°07′11.9,″海拔525.1 m)、梓潼县豢龙(N:31°44′07.0,″E:105°10′48.5,″海拔484.1 m)和剑阁县武连(N:31°52′21.5,″E:105°16′23.5,″海拔:481 m)的病圃中,含Yr5、Yr10、Yr15、Yr26的近等基因系、审定品种川麦43、川麦46、川麦47、川农18、川农23、绵麦39、绵麦41、绵麦42、杏麦2号、和内麦8号、区试材料C1、C5、30375和SW 18155、抗源M ega(含Yr3,4)和Hybrid 46(含Yr3 b,Yr4 b,H46)、93-1-22v-2、CP93-10-1-1-1、SMT-35、SMT-47、贵农22、贵农22-1和贵州蓝麦+MO连续两年在各病圃中表现抗病。216份品种或材料两年在雅安、剑阁和梓潼的鉴定结果中,有27个品种或材料同年在梓潼或剑阁表现感病而在雅安表现抗病,5个品种同年在梓潼或剑阁表现抗病而在雅安表现感病,紧邻阿坝州和陇南越夏菌源的剑阁、梓潼的条锈病菌毒性强于紧邻甘孜州越夏菌源的雅安。

源于硬粒小麦-节节麦人工合成种的小麦新品种川麦38抗条锈性及遗传分析

利用硬粒小麦-节节麦人工合成种与四川小麦杂交、回交,育成高抗条锈小麦新品种川麦38(99-607)。为明确川麦38抗条锈性状的遗传规律,将川麦38与绵阳26、绵阳335、SY95-71、川育12等5个高感条锈小麦品种杂交,获得杂种F1、F2群体;利用条中32对抗×感杂种F1、F2群体接种鉴定抗性分析表明,川麦38对条锈病新小种的抗性受一对显性基因控制。将川麦38与含Yr13的德国小麦8661及源于硬粒小麦-节节麦人工合成种的3个抗病新品种(川麦42、川3736、复小穗小麦)杂交,分析川麦38与4个抗病品种的抗性基因等位性,结果发现抗×抗F2群体中均分离出一定比例的感病单株,表明川麦38与德国小麦(Yr13)、川麦42、川3736、复小穗小麦等的抗锈基因不等位,为不同的抗性基因。

小麦条锈菌条中32号生理小种SCAR检测标记的建立

【目的】建立具有应用价值的小麦条锈菌条中32生理小种的SCAR检测标记。【方法】用100条随机引物对我国目前主要流行的12个小麦条锈菌生理小种进行RAPD筛选,寻找特异性片断,并对其进行克隆、测序,将该特异性片段转化成条中32号小种的SCAR专化型标记。设计并合成SCAR特异性引物,对不同来源的条中32号进行SCAR检测。【结果】引物S1271从条中32号生理小种中扩增出长度为320 bp的特异片段,该片段可作为条中32号的SCAR标记。从不同来源的条中32号生理小种中扩增出了筛选到的SCAR标记。【结论】成功建立了条中32专化SCAR标记。

小麦条锈病菌avrYr10/24/26/ch42突变体的毒性研究

自2005年起在四川省郫县病圃连续播种1．5hm^2抗病品种川麦42作为小麦条锈病菌新毒性突变捕获圃，周围感病品种上接种四川各地采集的小麦条锈病菌样品，2005—2008年川麦42反应型为0—2级。2009年川麦42乳熟后期突然普遍发病，反应型为3^-，将发病叶片分离的条锈病菌毒性突变体接种全国小麦条锈病菌生理小种鉴别寄主、含有已知抗条锈基因的小麦品种、近等基因系及四川小麦生产品种后，发现新毒性突变体对在目前在四川仍表现抗病的贵农22、川麦42、含有Yr10的近等基因系NILS12、Moro、含有Yr24的NILS16、以及合有Yr26的NILS17均具有毒性，新毒性突变体因而被命名为avrYr10／24／26／ch42；avrYr10／24／26／ch42突变体对含抗条锈基因Yr9的洛夫林13等不具毒性。avrYr10／24／26／ch42突变体的AFLP分析表明，其遗传相似度在0．94以上，因此可能来自于同一克隆。avrYr10／24／26／ch42突变体能够侵染39个四川小麦新品种中除资麦一号外的38个品种，能够引起四川大面积生产上83．26％田块种植的小麦发病。以上结果表明，建立捕获圃可以提前获得小麦条锈病菌新毒性突变，指导抗性品种选育和布局。