质谱非标记定量分析小麦抗条锈病近等基因系蛋白质变化

利用基于液相色谱串联Orbitrap质谱(Q Exactive)的非标定量(Label-free)技术,对小麦抗病单基因近等基因系Taichung29*6/Yr10和背景品种Taichung29叶片的蛋白质表达进行了比较分析。经MASCOT软件搜库,在两个样品中共同鉴定到2 257个蛋白,其中有准确定量信息的蛋白共1 549个,含量变化大于2倍的差异蛋白有102个。对102个差异表达蛋白进行了Gene Ontology(GO)功能注释和分析,发现他们多数定位于细胞基质和核糖体等细胞器,具备结合、催化等功能,主要参与代谢、细胞过程、应激等生物学进程,其中超氧化物歧化酶、甲硫氨酰氨肽酶、溶酶体-β-葡萄糖苷酶和铁蛋白等可能与小麦抗病单基因近等基因系Taichung 29*6/Yr10的抗病性有一定相关性。     

小麦抗叶锈病近等基因系TcLr41 SSH文库构建与分析

以小麦抗叶锈病近等基因系TcLr41和感病亲本Thatcher的叶片cDNA分别作为试验方和驱动方,利用抑制差减杂交技术,构建了一个包含2544个克隆的差减文库。随机提取阳性克隆质粒DNA后经PCR检测,插入片段大部分集中在200～1000bp之间,证明所构建的文库符合要求。在功能已知的基因中,推测过氧化氢酶（catalasc）基因、抗秆锈病基因（rust resistance gene）、铜蓝结合蛋白（blue copper—binding protein）基因、锌指蛋白（ring zinc finger protein）基因、胁迫反应蛋白（stress responsive protein）基因等可能是TcLr41中抗病相关差异表达基因。     

小麦抗叶锈近等基因系TcLr38抗病相关基因片段的分离

利用差异显示技术,分析小麦TcLr38受小麦叶锈菌诱导的mRNA表达丰度差异,获得了136条差异条带。对136条差异条带进行了回收、重扩增和反向Northern杂交检测,获得一条杂交信号阳性的片段,对该片段进行克隆、测序,该片段长度为425bp。在GenBank中进行Blast比对分析,与普通小麦(Triticum aestivum)同源性较高,并且与小麦抗盐cDNA序列也有较高的同源性;在GrainGenes中进行Blast比对,与小麦的远源亲本粗山羊草(Aegilops tauschii)、栽培一粒小麦(T.monococ-cum)和普通小麦具有较高同源性。利用SegMan软件进行电子克隆延长该片段,未找到与其相符的重叠群。因此确定该片段为TcLr38的cDNA片段,并初步推测该片段可能为一小麦抗病相关基因片段。     

小麦抗条锈病基因定位及分子标记研究进展

本文综述了小麦抗条锈病基因染色体定位及抗条锈病基因分子标记的研究进展,并对几种分子标记技术的应用潜力作了比较分析,特别是对ＳＳＲ、ＩＳＳＲ、ＡＦＬＰ等新型分子标记在小麦遗传育种中的应用前景作了初步探讨。     

水稻抗稻瘟病近等基因系的cDNA微阵列分析

应用cDNA微阵列对来源于中156／谷梅2号重组自交系的水稻抗稻瘟病近等基因系G205和G71的稻瘟病菌胁迫基因表达谱进行了分析,发现有3个cDNA克隆的表达仅在抗病基因系G205接种病原菌12h后受到诱导,其中两个为功能已知基因,另一个为功能未知的新基因。另有35个差异表达克隆在两个近等基因系中均检测到,其中17个克隆的表达在G205和G71均受到病原菌的诱导,另外18个克隆的表达则在G205和G71均受到病原菌原抑制。序列分析表明,这些稻瘟病菌应答基因分别与防卫反应,信号传递,逆境胁迫和光合作用及糖代谢等功能相关,为植物抗病机制提供了相关信息。另外,Northern还证实了编码富含甘氨酸蛋白基因（Glycinerich protein Grp)的表达受稻瘟病病原菌的诱导,是一个稻瘟病诱导相关基因。     

小麦拔节期盐胁迫对小麦近等基因系生理指标的影响

小麦近等基因系H8706,H8706-44,RH8706－48,RH8706－49在拔节期用0.7%NaCl进行盐胁迫,7d后耐盐性强的RH8706－49的SOD活性最高,是耐盐性差的H8706－34的SOD活性的1.875倍;且RH8706－49的MDA含量最低,比H8706－34低44.3%;ＲＨ８７０６－４９的细胞质膜透性也最低,为Ｈ８７０６－３４的５０％。     

两系杂交小麦恢复系MR168抗条锈病基因遗传分析及分子标记定位

小麦条锈病是影响杂交小麦普及推广的重要因素。文章利用基因推导法和SSR分子标记技术,研究了温光型两系杂交小麦恢复系MR168的抗条锈性遗传规律及其控制基因染色体位置。结果表明,MR168对CY29、CY31、CY32、CY33等条锈菌生理小种表现高抗至免疫;对SY95-71/MR168杂交组合的正反交F1、BC1、F2和F3群体分单株接种鉴定显示,MR168对CY32号小种的抗性受1对显性核基因控制,该抗病基因来源于春小麦品种辽春10号。利用集群分离分析法(Bulked segregant analysis,BSA)和简单重复序列(Simple sequence repeat,SSR)分子标记分析抗病亲本MR168、感病亲本SY95-71及183个F2代单株,发现了与MR168抗条锈病基因连锁的5个微卫星标记Xgwm273、Xgwm18、Xbarc187、Xwmc269、Xwmc406,并将该基因初步定位在1BS着丝粒附近,暂命名为YrMR168;构建了包含YrMR168的SSR标记遗传图谱,距离YrMR168最近的两个微卫星位点是Xgwm18和Xbarc187,遗传距离分别为1.9 cM和2.4 cM,这两个微卫星标记可用于杂交小麦抗条锈病分子标记辅助育种。     

一粒小麦抗白粉病和条锈病基因的分析

一粒小麦是普通小麦抗性改良的宝贵资源.本研究对24份一粒小麦分别进行了白粉病和条锈病混合菌种苗期接种鉴定,进一步分别用一套白粉病菌菌株(15个)对2份乌拉尔图小麦和条锈病菌小种(21个)对1份栽培一粒小麦进行接种鉴定,其中乌拉尔图小麦UR206能抵抗所有供试白粉菌菌株,UR204除对白粉菌菌株E11感病外,对其余菌株表现抗性;栽培一粒小麦MO205对不同条锈菌小种表现出不同的抗性反应,研究表明乌拉尔图小麦UR206、UR204和栽培一粒小麦MO205分别含有与已知抗白粉病和抗条锈病基因不同的新基因.对乌拉尔图小麦UR204、UR206和栽培一粒小麦MO205分别进行抗白粉和条锈病基因的遗传分析,结果表明乌拉尔图小麦UR204和UR206分别含有一对显性抗白粉病基因,栽培一粒小麦MO205含有两对独立遗传的显性抗条锈病基因.     

小麦抗条锈病基因YrCN19的诊断检测和遗传分析

用小麦条锈病抗性基因YrCN19的诊断标记Xgwm410对19个小麦品种或品系进行PCR筛选,其中川农19、新抗5号、爱民5号和爱民6号扩增出与条锈病抗性基因YrCN19共分离的特征片断,其大小为391个碱基,而在其他的小麦品种或品系中未能检测到该片断。系谱分析和抗性鉴定结果表明川农19、新抗5号、爱民5号和爱民6号含有小麦条锈病基因YrCN19。抗性遗传分析发现小麦条锈病抗性在川农19,新抗5号和爱民5号中的遗传符合单个显性基因的遗传规律(3抗:1感);杂交组合烟辐188/爱民6号的抗性遗传也符合单个显性基因的遗传规律,而另外一些杂交组合(如R25/爱民6号,鲁955159/爱民6号和苏3110/爱民6号)中的抗性分离则符合两对基因互补的遗传规律(9抗:7感)。本研究揭示了小麦条锈病抗性基因YrCN19在不同遗传背景和杂交组合的抗性表达和分离有差异,从而加速YrCN19在小麦抗条锈育种中的开发与利用。     

大豆Harosoy近等基因系低聚糖及其组分含量的变异分析

以高效液相色谱技术检测在北京和内蒙古种植的供试材料Harosoy近等基因系的低聚糖及其组分含量,考查Harosoy近等基因系的低聚糖含量的变异和不同地点材料的低聚糖及其组分含量相互间的相关性,低聚糖及其组分含量分别与蛋白质、脂肪含量间的相关性。研究结果表明,内蒙古种植材料低聚糖含量的平均值均高于北京种植的材料,说明内蒙古的条件有利于大豆的低聚糖形成和贮存。北京和内蒙古的材料蔗糖含量分布范围分别是3.3%~6.5%、3.9%~6.9%,棉籽糖分布范围分别是0.6%~1.4%、0.7%~1.1%,水苏糖分布范围分别是2.7%~3.7%、2.8%~3.8%,大豆低聚糖分布范围分别是6.9%~10.9%、7.8%~11.3%。同时发现,两地种植材料的低聚糖含量间和蔗糖含量间均具有显著负相关性,蔗糖含量间r=-0.7810,低聚糖含量间r=-0.7355;低聚糖及其组分含量与蛋白质、脂肪含量间均无相关性(P0.05)。还发现了低聚糖及其组分含量在两地稳定表达的材料共10个。     

Early molecular diagnosis and detection of Puccinia striiformis f. sp. tritici in China

Aims: Wheat stripe (yellow) rust, caused by Puccinia striiformis f. sp. tritici (Pst), is the most important foliar disease on wheat in China. Early molecular diagnosis and detection of stripe rust will provide a useful aid to the accurate forecast and seasonal control of this destructive disease. Our objective was to develop PCR assays for the rapid identification and detection of P. striiformis. Methods and Results: The genomic DNA of P. striiformis and P. triticina were amplified by a pair of primers derived from conserved β‐tubulin gene sequence. A 235‐bp specific DNA fragment of P. striiformis was isolated and purified. Based on its sequence, another two primer sets were designed successfully to obtain new sequence‐characterized amplified region (SCAR) markers of P. striiformis, which could be amplified in all test isolates of P. striiformis, whereas no DNA fragment was obtained in other nontarget wheat pathogens. The detection limit of the primer set YR (f)/YR (r1) was 2·20 pg μl^?1. The new SCAR markers of P. striiformis can also be detected in Pst‐infected wheat leaves postinoculated for 2 days. Conclusions: Our assays are significantly faster than the conventional methods used in the identification of P. striiformis. Significance and Impact of the Study: Development of a simple, high‐throughput assay kit for the rapid diagnosis and detection of wheat stripe rust would be anticipated in a further study.     

中国小麦条锈菌转主寄主小檗的鉴定

用萌发的小麦条锈菌冬孢子接种采自陕西省境内的陕西小檗、少齿小檗和长穗小檗,3种小檗均产生了性孢子器和锈孢子器。用人工接种小麦条锈菌冬孢子在陕西小檗上产生的锈孢子器接种小麦铭贤169产生了典型的条锈菌夏孢子堆症状。特异性PCR和DNA序列分析表明,人工接种产生于小檗上的锈孢子、接种锈孢子于小麦上产生的夏孢子堆与小麦条锈菌DNA的ITS区序列完全一致。更为重要的是,用采自田间受锈菌侵染的小檗叶片产生的锈孢子接种小麦铭贤169,经培养在小麦铭贤169叶片上产生了典型的条锈病症状。从而证实,在自然条件下,在中国,小檗不仅可作为小麦条锈菌的转主寄主,而且小麦条锈菌可在小檗上完成其有性繁殖过程。这一发现对进一步揭示我国小麦条锈菌高度的群体遗传多样性与毒性变异机理、完善小麦条锈病的防治策略具有十分重要的理论和实际意义。     

Virulence variation of Puccinia striiformis Westend. f. sp. tritici in Pakistan

Yellow rust populations of Pakistan were characterised for their virulence pathotypes/races and pathogenetic variation using seedling evaluation of differential genotypes under glasshouse conditions in Murree (6000 feet above sea level). Differential genotypes comprised a world set, an European set, near isogenic lines and the universally susceptible bread wheat cultivar “Morocco”. Over the two-year study a total of 18 race groups were identified. Out of these 18 race groups, several (68E0, 64E0, 66E0, 70E0, 6E0, 71E0, 6E0, 2E0, 67E0, and 68E16) were found previously. The new race group 70E32 found probably evolved because of mutation from the previously existing 70E16. Virulence frequencies of yellow rust (Yr) resistance genes were also determined on near isogenic lines. The highest virulence frequencies (%) were found for Yr7 (88%), Yr9 (57%), Yr18 (70%), and Yr24 (69%). Virulence frequencies were low for Yr 1 (4%), Yr5 (7%), Yr10 (10%) and Yr15 (4%). Our studies indicated that virulence existed for almost all yr genes, necessitating regular monitoring of the yellow rust populations and intensifying efforts to identify new sources of resistance to this pathogen.     

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.     

条形柄锈菌小麦专化型葡萄糖-6-磷酸脱氢酶基因PsG6PDH1的表达特征及功能分析

葡萄糖-6-磷酸脱氢酶是磷酸戊糖途径中的关键限速酶。基于已测序的条形柄锈菌小麦专化型基因组序列,利用RT-PCR方法克隆了该病菌葡萄糖-6-磷酸脱氢酶PsG6PDH1的全长cDNA序列（1 497bp）,编码498个氨基酸的蛋白。编码蛋白含有葡萄糖-6-磷酸脱氢酶的保守功能域。系统进化分析发现,PsG6PDH1与禾柄锈菌小麦专化型的G6PDH聚为一簇。qRT-PCR分析表明,PsG6PDH1在病菌侵染早期的表达明显上调,其中侵染24h时表达量最高,为对照夏孢子的30倍。将PsG6PDH1导入酿酒酵母G6PDH缺失突变体中成功表达,并表现出较强的葡萄糖-6-磷酸脱氢酶活性,明显酵母增强了菌株对过氧化氢的耐受性。由此推测,PsG6PDH1可能参与了条形柄锈菌小麦专化型在侵染寄主时抵御寄主的氧化胁迫反应。研究结果为进一步研究该病菌基础代谢及侵染机理奠定一定的理论基础。     

小麦条锈菌PsNCS1基因的克隆及转录表达特征

摘要：【目的】克隆小麦条锈菌神经钙离子感应蛋白基因PsNCS1,分析其在病菌不同发育时期的表达水平。【方法】利用文库筛选和RT-PCR技术克隆PsNCS1的cDNA序列,采用生物信息学技术预测分析该基因编码蛋白的保守结构域及基本特性,构建系统发育树;运用实时荧光定量RT-PCR技术分析PsNCS1在病菌不同生长发育时期的表达水平。【结果】PsNCS1全长cDNA为1007 bp（GenBank登录号GU134621）,开放阅读框为573 bp,编码190个氨基酸,分子量为22.17 kDa, 等电点为4.     

四川省小麦条锈菌群体遗传多样性的SSR分析

利用TP-M13-SSR自动荧光检测技术,对四川省小麦条锈菌群体遗传多样性水平进行了分析。研究结果表明,四川省小麦条锈菌群体遗传多样性比较丰富,地区之间存在明显的差异,川西北和四川盆地的种群遗传多样性相对较高,而四川西南部和四川东南部的种群遗传多样性较低。四川小麦条锈菌群体存在一定的遗传分化,地区间的遗传变异仅占14.92%,群体间的遗传变异占总变异的23.06%,群体内遗传变异占60.02%,遗传变异主要存在于群体内部。基因流和共享基因型从分子水平证实了四川小麦条锈菌在地区间的传播,且川西北和四川盆地之间的菌源交流最为广泛。     

Race analysis of Puccinia striiformis f.sp. tritici in Iran

The wheat stripe (yellow) rust is one of the most important diseases in Iran. In this study, 41 races out of 104 isolates in greenhouse were determined from 2008 to 2010. Races 6E6A+, 6E10A+ and 6E0A+ were more common. Races 0E0A+ was less aggressive than races 166E158A+ and 134E158A+ with virulence on 11 known genes. Virulence on plant/s with gene/s Yr1, Yr2, Yr4, Yr6, Yr7, Yr8, Yr9, Yr10, Yr25, Yr27, YrSU, YrSD, YrND, Yr3, Yr2+, Yr6+, Yr9+, Yr7+, YrCV and YrA was detected. The majority of isolates with high frequency (more than 70%) showed virulence on plant/s with Yr2, Yr7, Yr9 and YrA genes. No virulence was detected on plant/s with Yr3, Yr5 and YrSP. In greenhouse test, frequency of virulence to wheat genotypes with Yr1, Yr4, Yr10, YrCV (32+) and YrSD gene was less than 7%. Frequency of virulence to other wheat genotypes was between 8 and 100%.     

Alterations in some oxidative parameters in susceptible and resistant wheat plants infected with Puccinia recondita f.sp. tritici

We studied the systemic effects after infection of susceptible and resistant (expressing HSR) wheat plants with leaf rust (Puccinia recondita f.sp. tritici) on the amount of hydrogen peroxide and activity of some ROS scavenging enzymes. Measurements were performed 7 and 21 days after inoculation. In susceptible cultivar (Sadovo 1), an inhibition of activity of catatase and GST was found. By contrast, in resistant cultivar (Kristal), the infection caused an activation of these enzymes. Moreover, it was established that cv. Kristal plants possess constitutive higher levels of hydrogen peroxide, as well as higher superoxide dismutase activity.