大豆抗豆秆黑潜蝇遗传的初步研究

为研究大豆品种抗蝇性遗传规律,利用5个品种配制了3个杂交组合,在田间利用自然虫源,对P_1、P_2、F_1、F_2和F_3的抗感反应进行鉴定。结果表明,大豆品种抗蝇性系受单个显性主基因控制;可能受某些微效多基因及环境的修饰。在大豆抗蝇性遗传中未发现细胞质遗传效应。     

小偃麦衍生品系CH7086抗白粉基因的遗传及SSR分析

CH7086是兼抗白粉病、条锈病的小麦新品系,衍牛于来自十倍体长穗偃麦草的八倍体小偃麦与普通小麦的杂种后代.温室接种鉴定结果显示,CH7086对白粉病菌系E09、E21、E26均表现为免疫,且其抗件来自长穗偃麦草.抗性遗传分析表明CH7086的白粉病抗性由1对显性基因控制,暂定名为MlCH86.应用分离群体分组法(BSA)对从CH5241×CH7086的F2中随机选取的95个单株进行微卫星标记检测,发现位于2BL、2DL上的SSR位点Xbarc159在双亲和抗、感池间有特异性,并与抗性基因MlCH86连锁,其遗传距离为10.8 cM.用中国春第2部分同源群的缺体-四体系和双端体系进行验证,进一步将MlCH86定位在2BL上.用白粉病菌系E21、E26接种鉴定表明,MlCH86的抗性反应明显不同于2BL上已命名的抗性基因Pm6、Pm33.根据抗性基因的来源、染色体位置及抗性反应,初步推断存在于CH7086的抗性基因来自长穗偃麦草,它不同于已有的抗白粉病基因,可能是一个新基因.     

抗稻瘟病水稻资源抗性基因Pita、Pib、Pi9以及Pikm的分布研究

利用抗稻瘟病水稻资源品种杂交,聚合多个抗性基因是培育持久抗稻瘟病水稻新品种的主要育种途径.利用分子标记技术对水稻抗性资源进行基因型鉴定是分子辅助聚合育种的基础.通过以亚华种业科学院稻瘟病病圃抗病水稻资源为材料,利用特异性分子标记对Pi9、Pita、Pib以及Pikm基因在水稻抗稻瘟病资源的分布进行了鉴定,初步建立了抗性基因数据库.同时对抗性基因及与抗性反应的相关性进行了探讨,结果表明以Pi9为主效基因,同时聚合Pita和Pib抗性基因能提高持久抗稻瘟病能力.     

小粒野生稻导入系对稻飞虱的抗性鉴定与分析

稻飞虱是水稻生产最严重的害虫之一。野生稻拥有丰富的抗虫基因资源,导入系是鉴定和利用野生稻有利基因的有效途径。本研究通过对371份小粒野生稻导入系进行抗褐飞虱和白背飞虱接虫鉴定,分别筛选出了11份抗、72份中抗褐飞虱的材料和7份抗、45份中抗白背飞虱的材料,其中有5份材料兼抗褐飞虱和白背飞虱,这是从小粒野生稻中鉴定出抗白背飞虱材料的首次报道。通过对2份抗性导入系材料与感虫亲本杂交构建的F1和F2群体的抗虫鉴定和分析表明:K41对褐飞虱和白背飞虱的抗性受2对显性抗虫基因通过互补作用所控制;P114对褐飞虱和白背飞虱的抗性都是由1对主效的隐性基因控制。这些结果必将有利于小粒野生稻抗稻飞虱的基因定位和育种利用。     

自然环境分离磺胺甲噁唑抗性细菌抗药性及其抗性基因分析

为了解自然环境源细菌对磺胺类抗生素的抗性特征,采用纯培养物分离技术从淮河底泥中筛选磺胺甲噁唑(SMZ)抗性细菌,测定其抗性水平,PCR扩增进一步分析其抗性基因(sul)和一类整合子(intl)。结果从该底泥样品中分离出4株SMZ抗性细菌,经鉴定分别为Arthrobacter spp.Y1、Bacillus spp.Y2、Acinetobacter spp.Y4和Bacillus spp.H。菌株对SMZ的抗性水平从低到高依次为Y4 (0.5)、Y1 (5)、H (10)和Y2 (10 mg/mL)。4个SMZ抗性菌株均携带sul1基因,但均不含sul3和sulA基因,其中菌株H同时携带sul2基因。菌株Y2和Y4含有一类整合子,但是菌株Y1和H不含该整合子。本研究有助于加深对自然环境源SMZ抗性细菌抗性特征及其潜在风险的认知。     

利用小麦微卫星标记定位一个来自野生二粒小麦的抗白粉病基因

培育抗病品种是控制小麦白粉病危害最经济有效而又安全的手段.寻找和创造新抗源是抗病育种的基础工作,是解决抗源单一化问题的有效途径.来自以色列的野生二粒小麦G-305-M对北京地区小麦白粉菌流行小种15号表现免疫,用G-305-M与小麦品种781杂交并用京411回交(G-305-M/781//京411*3),成功地将G-305-M的抗白粉病基因转入普通小麦中.遗传分析表明转入小麦中的抗病性苗期表达受一对显性基因控制,该基因暂定名为MlG.用96对小麦微卫星引物对一个167株的抗性分离家系进行了SSR分析,发现引物WMS570扩增产物在抗感个体间存在多态性.经分离群体验证,抗病基因MlG与小麦染色体6AL上的微卫星位点Xgwm570连锁,遗传距离为14.9±3.0cM,据此将MlG定位于6AL.根据系谱和基因位点分析,推断MlG基因是不同于已知抗白粉病基因的一个新基因.     

几个四倍体小麦-山羊草双二倍体及其部分亲本的抗小麦白粉病基因分析

用离体叶段接种方法鉴定了11个四倍体小麦一山羊草双二倍体、波斯小麦PS5、硬粒小麦DR147、5份山羊草、杂交高代材料Am9／莱州953*^2F5和(DR147／Ael4)／／莱州953*^2F4对20个具有不同毒力白粉菌株的抗谱。通过与含有已知抗病基因品种或品系的反应模式比较,推测Am9／莱州953*^2F5含有Pm4b,波斯小麦PS5含有Pm4b与一个未知抗病基因组合;(DR147／Ael4)／／莱州953*^2F4和硬粒小麦DR147含有Pm4a和一个未知抗病基因组合;尾状山羊草Ael4和小伞山羊草Y39抗所有白粉菌株,由于迄今还没有在尾状山羊草和小伞山羊草中鉴定出抗白粉病基因,推测这2份山羊草含有新的抗白粉病基因。除Am9外,在其它双二倍体中波斯小麦或硬粒小麦的抗性部分受到抑制。山羊草的抗性部分或完全量到抑制。     

小麦背景中来自华山新麦草的抗条锈病基因的遗传学分析和分子标记

H9020—17—5是一个通过杂交和回交选育的普通小麦—华山新麦草易位系,接种鉴定表明其对条锈病具有优良抗性。遗传学分析证明易位系H9020—17—5的抗条锈性是由单基因控制的显性性状,抗性基因来自于华山新麦草,暂定名为YrHua。为了标记这个来自华山新麦草的抗条锈病基因,利用H9020—17—5与感病小麦品种铭贤169杂交,建立了F2分离群体。应用81对AFLP引物对119个经条锈菌生理小种CY30接种鉴定的F2单株进行了分析,结果得到两个与YrHua基因连锁的AFLP标记PM14(301)和PM42(249),遗传距离分别为5．4cM和2．7cM,并分别位于目标基因的两侧。将标记片段克隆、测序后,根据序列信息和酶切位点多态性设计特异性引物,将AFLP标记PM14(301)转换成了简单的PCR标记。研究结果为标记辅助育种提供了分子选择工具,同时也为进一步精细定位和图位克隆YrHua基因奠定了基础。     

水稻抗衰老IPT基因与抗白叶枯病基因Xa23的聚合研究

以转抑制衰老有关的异戊烯基转移酶(IPT)基因株系GC-1、携带抗白叶枯病基因Xa23的“CBB23”和抗稻瘟病水稻品种“合系15号”为供体．采用分子标记辅助选择与生物学鉴定相结合的方法,将IPT基因与Xa23及抗稻瘟病基因进行聚合。在3个复交组合中获得了17株聚合IPT基因与Xa23基因的植株,用这些植株与两系杂交稻亲本9311、E32、培矮64S及W9834S进行杂交和回交,经PCR分子检测和抗白叶枯病、抗稻瘟病鉴定和细胞分裂素含量的测定,最终在4个BC,回交组合“(9311／／／合系15／CBB23／／GC-1)X9311”、“(E32／／／合系15／CBB23／／GC-1)XE32”、“(培矮64S／／／合系15／CBB23／／GC-1)X培矮64S”和“(GC-1／CBB23／／W9834S／合系15)XW9834S”中获得了17株携带IPT基因与Xa23基因的BC1F1植株,这些植株对来自北方稻区21个稻瘟病菌系全部表现为抗。携带IPT基因的抗病植株再与杂交稻亲本进行回交．在2个BC2回交组合“[(9311／／／合系15／CBB23／／GC-1)X9311]X9311’’和“[(E32／／／合系15／CBB23／／GC-1)XE32]XE32”中获得了7株携带IPT基因与Xa23基因的植株,这些植株再经过1—2代回交和自交,即可用于杂交稻育种。     

籼稻品种窄叶青8号抗稻瘟病基因分析

籼稻品种窄叶青８号是我国北方稻区水稻育种上重要的稻瘟病抗源之一。本文利用我国北方稻区的代表菌系中１０－８－１４和日本的代表菌系研５４－０４,对窄叶青８号与感病品种京系１７号和丽江新团黑谷的杂交Ｆ１Ｆ２、ＤＨ和Ｂ１Ｆ１群体进行抗病性鉴定,根据抗病性的分离,确认窄叶青８号的抗性由１对显性主效基因,即朱立煌等报道的Ｐｉ－ｚｈ基因控制。利用系研５４－０４接种窄叶青８号与９个具有已知抗病基因的鉴别品种杂交的Ｆ２群体,各群体都表现二基因的独立遗传,证明Ｐｉ－ｚｈ基因与Ｐｉ－ｉ、Ｐｉ－ｋｍ、Ｐｉ－ｚ、Ｐｉ－ｔａ、Ｐｉ－ｔａｚ、Ｐｉ－ｚｔ、Ｐｉ－ｋｐ、Ｐｉ－ｂ和Ｐｉ－ｔ等９个已知抗病基因间存在非等位关系,是新的抗稻瘟病基因。     

High-resolution genetic mapping of rice bacterial blight resistance gene Xa23

Bacterial blight (BB) caused by Xanthomonas oryzae pv. oryzae (Xoo) is the most devastating bacterial disease of rice (Oryza sativa L.), a staple food crop that feeds half of the world’s population. In management of this disease, the most economical and effective approach is cultivating resistant varieties. Due to rapid change of pathogenicity in the pathogen, it is necessary to identify and characterize more host resistance genes for breeding new resistant varieties. We have previously identified the BB resistance (R) gene Xa23 that confers the broadest resistance to Xoo strains isolated from different rice-growing regions and preliminarily mapped the gene within a 1.7 cm region on the long arm of rice chromosome 11. Here, we report fine genetic mapping and in silico analysis of putative candidate genes of Xa23. Based on F₂ mapping populations derived from crosses between Xa23-containing rice line CBB23 and susceptible varieties JG30 or IR24, six new STS markers Lj36, Lj46, Lj138, Lj74, A83B4, and Lj13 were developed. Linkage analysis revealed that the new markers were co-segregated with or closely linked to the Xa23 locus. Consequently, the Xa23 gene was mapped within a 0.4 cm region between markers Lj138 and A83B4, in which the co-segregating marker Lj74 was identified. The corresponding physical distance between Lj138 and A83B4 on Nipponbare genome is 49.8 kb. Six Xa23 candidate genes have been annotated, including four candidate genes encoding hypothetical proteins and the other two encoding a putative ADP-ribosylation factor protein and a putative PPR protein. These results will facilitate marker-assisted selection of Xa23 in rice breeding and molecular cloning of this valuable R gene.     

Identification of Quantitative Trait Loci for Bacterial Blight Resistance Derived from Oryza meyeriana and Agronomic Traits in Recombinant Inbred Lines of Oryza sativa

Bacterial blight (BB) is one of the major diseases that affect rice productivity. In previous studies, BB resistance was transferred to cultivated rice Oryza sativa from wild rice Oryza meyeriana using asymmetric somatic hybridization. One of the resistant hybrid progenies (Y73) has also been shown to possess novel resistance gene(s) different from any of those previously associated with BB resistance. We have mapped quantitative trait loci (QTLs) for BB resistance in a recombinant inbred line (RIL) population derived from a cross between Y73 and a BB‐susceptible cv. IR24. Five QTLs were detected where Y73 alleles contributed to increased BB resistance. Three minor QTLs were identified on chromosomes 3, 10 and 11, and two major QTLs on chromosomes 1 and 5, respectively. QTL on chromosome 5, designated qBBR5, had the strongest effect on BB resistance, explaining approximately 37% of the phenotypic variance. Using the same RIL population, we also mapped QTLs for agronomic traits including plant height (PH), heading date (HD), plant yield (PYD) and PYD component traits. A total of 21 QTLs were identified, of which four were detected for PH, six for HD, three for panicle number per plant (PNPP), one for spikelets per panicle (SPP), six for 1000‐grain weight (TGW) and one for PYD. qPH1 (a QTL for PH) was found in the same interval as qBBR1 for BB resistance, and qHD11 for HD and qBBR11 for BB resistance also shared a similar interval. Additionally, BB resistance was significantly correlated with PH or HD in the RIL population. This suggests that the resistance genes may have pleiotropic effects on, or close linkage to, genes controlling PH or HD. These results will help deduce the resistance mechanisms of the novel resistance gene(s) and provide the basis for cloning them and using them in marker‐assisted breeding.     

Identification and fine mapping of a new bacterial blight resistance gene,Xa43(t), in Zhangpu wild rice (Oryza rufipogon)

• Bacterial blight (BB) is currently considered one of the most serious rice diseases and is caused by Xanthomonas oryzae pv. oryzae (Xoo). Numerous studies have shown that breeding resistant rice varieties is one of the most effective methods to prevent BB, and it is important to identify and isolate more BB resistance (R) genes from different rice resources.
• Using a map-based approach, we identified a new QTL/gene, Xa43(t), from ZhangPu wild rice, which was highly resistant to the BB isolate PX099. We performed bulked segregant analysis combined with candidate gene prediction to identify the candidate gene.
• The Xa43(t) gene was narrowed down to a 29-kb region containing four putative genes. More importantly, the candidate gene Xa43(t) did not affect the main agronomic traits of rice. We also identified a widely applicable molecular marker, namely Inde1-18, which co-segregates with the Xa43(t) gene.
• The Xa43(t) gene is a new broad-spectrum BB resistance gene without identified alleles and has good application prospects for rice disease resistance breeding.

     

云南野生稻中的抗白叶枯病基因Xa21的鉴定

水稻白叶枯病是水稻生产上的主要细菌病害之一。从野生稻中发掘优异的水稻白叶枯病抗性材料,可以拓宽栽培稻抗白叶枯病遗传基础。经过温室接菌鉴定和PCR标记分析,对云南野生稻进行Xa21基因的检测鉴定。温室接菌鉴定表明,云南野生稻对广谱致病小种PX099及云南强致病菌Y8具有较好的抗性能力,特别是疣粒野生稻对致病菌株达到免疫程度;PCR标记分析表明,云南野生稻不含有Xa21基因,但含有与Xa21基因某些区域同源的片段。本研究结果为寻找新的抗源材料及快速发掘利用云南野生稻中的抗白叶枯病基因提供理论依据。     

MQ2: visualizing multi-trait mapped QTL results

Bacterial blight (BB) of rice (Oryza sativa L.) caused by Xanthomonas oryzae pv. oryzae (Xoo) is a destructive disease in rice worldwide. Xa3, a gene conferring resistance to BB at the booting stage of the rice plant, has been characterized previously using map-based cloning. We cloned and sequenced the Xa3/xa3 gene in the Korean cultivars Hwayeong, Ilmi, and Goun and conferred resistance or susceptibility to BB. We detected polymorphisms, and polymerase chain reaction-based functional markers were developed based on the single nucleotide polymorphism from the Xa3 and xa3 nucleotide sequence. Susceptible or resistant individuals from an F2 population developed from a cross between Milyang 244 and Ilmi, near-isogenic lines carrying BB resistance genes, were screened with functional markers. The BB3-RF and BB3-RR primers consistently amplified a resistance-specific fragment of 255 bp only in resistant plants, whereas the BB3-SF and BB3-SR primers were specific to susceptible plants. Genotyping results were co-segregated with phenotype by conducting the BB resistance test with the K₃ race. These markers could be effective for marker-assisted selection of the Xa3 gene in rice breeding programs.     

水稻抗白叶枯病基因Xa-4的PCR标记研究

根据与水稻抗白叶枯病基因Ｘａ－４紧密连锁的分子标记Ｍ５５的序列设计引物,通过对国际水稻研究所育成的抗白叶枯病近等基因系和基因累加系的叶片ＤＮＡ、半粒种子提取物及Ｘａ－４基因的杂合体ＤＮＡ的ＰＣＲ特异扩增,初步建立了Ｘａ－４的ＰＣＲ标记体系。进而用该标记体系对我国籼型杂交水稻常用的亲本材料进行分析,揭示出了Ｘａ－４在这些材料中的分布情况。