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1.
分子标记辅助选择小麦抗白粉病兼抗赤霉病聚合体   总被引:1,自引:0,他引:1  
 Sumai 3, a wheat variety resistant to Fusarium head blight(FHB), was crossed with Neimai 9, a commercial wheat cultivar with the resistance to powdery mildew.The SCAR(sequence characterized amplified region) markers of powdery mildew resistance gene Pm21 and four SSR(simple sequence repeats)markers flanking the major FHB resistance QTL(Qfhs.ndsu-3BS) in Sumai 3 were used to detect the resistance loci by marker assisted selection(MAS) in the plants of the F2 population.Identification of resistance to both powdery mildew and FHB in field showed that 12 plants resistant to both diseases were obtained.In addition, the agronomic traits of these plants were better than those of Sumai 3, and are perhaps the excellent parental materials for wheat breeding.  相似文献   

2.
亚麻品系9801-1抗白粉病基因的RAPD标记   总被引:2,自引:0,他引:2  
 F2 populations were obtained from the cross between 9801-1 and DIANE.Bulked segregate and RAPD analyses were employed to identify molecules linked to the resistance to powdery mildew.OPP02 amplified about 792 bp polymorphic band in all individuals from 9801-1 and resistant bulk,but absent in all individuals from DIANE and susceptible bulk.By further analysis in F2 segregating population,the polymorphic band was found to be cosegregated with the resistant gene possibly.The fragment was sequenced,  相似文献   

3.
小麦-滨麦易位系M8657-1抗条锈病基因遗传分析和分子标记   总被引:3,自引:0,他引:3  
 M8657-1, one of the wheat translocation lines derived from Leymus mollis Trin. Hara, is possessed of effective resistance at all stages to Su-ll and other dominant races of Puccinia striiformis f. sp. tritici in China. Seedlings of the parents, F1, and F2 progeny derived from the cross of M8657-1 (resistant) Mingxian169 (susceptible) were inoculated with Su-ll in greenhouse to identify and map the probable new stripe rust resistance gene. The results suggested that the stripe rust resistance in M8657-1 was conferred by a pair of recessive genes. Simple sequence repeat (SSR) technique was used to detect molecular marker associated with the resistance gene:208 pairs of wheat SSR primers were used to screen the two parents, as well as resistant and susceptible bulks and then three SSR markers were selected for genotyping the F2 population. The geue, temporarily designated as YrLml, was found to be located on the chromosome 7DL and flanked by three SSR markers GDM67, WMC150 and WMC671, with the genetic distance of 5.0, 9.7 and 11.8cM, respectively.  相似文献   

4.
小麦抗白粉病基因Pm6的微卫星标记鉴定   总被引:3,自引:0,他引:3  
 Wheat powdery mildew, caused by Blumeria graminis f. sp. tritici, is a prevalent disease worldwide. Breeding and planting resistance cultivars have been proved effective and environmental friendly for control of the disease. To develop easily used PCR-based markers in marker assisted selection (MAS) for Pm6, a dominant powdery mildew resistance gene in wheat, 25 microsatellite markers on chromosome 2BL in wheat were screened between susceptible parent Yumai13 and resistance parent Timgalen carrying Pm6. F2 population derived from Yumai13 and Timgalen was further analyzed by the marker Xgwm501. The results indicated that Xgwm501 was a co-dominant marker linked to Pm6 gene at a distance of 14.8 cM. 29 Pm-carrying varieties were tested by the marker Xgwm501 and only those carrying Pm6 showed 117 bp resistance specific band. This marker is proved to have high practicability and can be used in MAS of Pm6 gene in wheat breeding programs.  相似文献   

5.
 It have proved that wheat translocation line H9020-1-6-8-3 derived from Psathyrostachys huashanica Keng is an important resistant resource to stripe rust.To confirm the existence of resistant genes,it was crossed with susceptible cultivar MingXian 169 as male and female parent,respectively.Seedlings of parents and F2 progeny were tested for resistance to selected CY29 of races of Puccinia striiformis f.sp.tritici from China.H9020-1-6-8-3 had one dominant resistant gene which temporarily named YrHs,whatever it was male or female parent.By using BSA method,two markers,Xgwm261 and Xgwm455 located on 2DL were found.The distance to YrHs were 4.3 and 5.8 cM respectively.The result could be used in molecular-assisted breeding.  相似文献   

6.
 Using resistant and susceptible cultivars as controls, the resistant evaluation to Pseudoperonospora cubensis was carried out in 12 introgression lines from wide cross between cucumber(Cucumis sativus L.) and sour cucumber(Cucumis hystrix Chakr.). Three enzyme activities including POD, SOD and PAL were analyzed before and 7 d after inoculation, and the POD isozyme was detected by polyacrylamide electrophoresis. The inoculation results showed that, of the 12 accessions, 3 were identified as high resistant, 5 were moderately resistant and 4 were moderately susceptible to downy mildew. The enzyme activities of POD, SOD and PAL were greatly increased in resistant accessions after inoculation. PAL enzyme activities showed close correlation with disease rating before or after inoculation, which implicated that PAL enzyme activity might be used to estimate the resistance to downy mildew. POD isozyme electrophoresis showed that the number and intensity for the bands of resistant lines were significantly increased more than those of susceptible lines after inoculation.  相似文献   

7.
2008年我国部分麦区小麦白粉病菌群体对温度的敏感性   总被引:1,自引:1,他引:0  
 The sensitivity of 113 isolates of wheat powdery mildew (Blumeria graminis f. sp. tritici) sampled from 6 provinces or cities in 2008 to temperature was tested by detached leaf segment method with setting up 5 different temperatures indoor. The results showed the mean ET50 (which represents the temperature that is required to obtain 50% of the maximum effect) of all isolates tested was 23.02℃. ET50 values of 17.70% isolates were more than 24℃. The highest and the lowest ET50 of isolates were 25.22℃ and 19.42℃, respectively. There were a certain differences for isolates sensitivity to temperature among different provinces or cites. It was also found that when temperature increased during 22-26℃, the latent period of isolates prolonged, and the latent period of different isolates was different at the same temperature, too. These results will provide a reference for the oversummering division of wheat powdery mildew, as well as the effect of climate to the disease.  相似文献   

8.
基于小麦白粉病菌rDNA ITS序列的PCR分子检测   总被引:6,自引:0,他引:6  
 Wheat powdery mildew(Blumeria graminis f.sp.tritici) is the one of main wheat diseases in China.Based on the internal transcribed spacer(ITS) sequences of ribosome of B.graminis f.sp.tritici,three molecular primer pairs(F1/R,F2/R and F3/R) were designed to detect the fungal pathogen of wheat powdery mildew.The species specificity of these primers was confirmed.F1/R was demonstrated a higher sensitivity than the other two primer pairs,and could detect as low as 1 pg DNA of B.graminis f.sp.tritici.Furthermore,F1/R primer pair was used to detect the pathogen DNA extracted from wheat leaves showing chlorosis and typical symptoms of powdery mildew caused by artificial inoculation with B.graminis f.sp.tritici.The preliminary results demonstrated the usefulness of this primer pair and its potential applications in efficient detection of wheat powdery mildew pathogen from leaves with latent infections at early growth stages of wheat.  相似文献   

9.
油茶苗圃炭疽病菌抗药性研究   总被引:1,自引:0,他引:1  
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10.
结球甘蓝抗TuMV基因的RAPD和SCAR标记研究   总被引:4,自引:0,他引:4  
 One hundred and forty-four F2 individuals from a cross combination between 1047 (susceptible) and A21 (resistant) were analyzed for the presence of random amplified polymorphic DNA (RAPD) markers linked to Turnip mosaic virus (TuMV) resistant gene in cabbage by using bulked segregant analysis (BSA).Two polymorphic markers were screened out of 200 random primers.These two RAPD fragments were linked to the resistant gene at 7.7 cM and 8.38 cM respectively and converted to SCAR markers successfully.  相似文献   

11.
小麦抗白粉病基因Pm21 的抑制基因   总被引:1,自引:0,他引:1  
 小麦-簇毛麦6VS. 6AL 易位染色体含有抗白粉病基因Pm21,在我国的小麦育种中被广泛应用。近年来,一些含有Pm21 基因的小麦品种(系)开始感染白粉病。为探索含Pm21 的品种(系)感染白粉病的原因,本研究在6VS. 6AL 易位系与小麦品系(种)R14 和川农12 的杂交后代中利用分子标记CINAU17-1086 和CINAU18-723 辅助选择的遗传背景相对简单的F7 和F8 近等基因系为材料,研究了小麦抗白粉病基因Pm21 的抗病性表达。结果发现,在3 个含有6VS. 6AL 易位染色体的感病F6 植株繁殖的F7 近等基因系中发生了白粉病抗性的分离,分离比率符合13 感病︰ 3 抗病的理论值。在随机选取的F7 感病小麦单株所繁殖的F8 近等基因系中,有7 / 13 的株系一致地重感白粉病,有6 / 13 的株系发生了抗白粉病的分离,其中2 / 13 的株系分离比符合3 感病︰ 1 抗病、4 / 13 的株系分离比符合13 感病︰ 3 抗病的分离模式。这一结果指出,小麦株系中的抗白粉病基因Pm21 的抗性表达受小麦基因组中的一对显性抑制基因所控制,该基因来源于小麦品种(系)川农12或R14,建议命名为SuPm21。本研究指出,在把外源基因引入小麦的研究中,有利的外源基因与不含抑制基因的受体遗传资源同等重要。  相似文献   

12.
[目的]对3份小麦农家品种‘矮秆芒麦’、‘红头麦’和‘大红头’进行苗期抗性的遗传分析,研究它们的抗白粉病遗传特点,为其在抗病育种中的有效利用提供依据.[方法]将这3份小麦农家品种分别与感病品种‘铭贤169’正、反杂交,获得了F1和F2代.利用白粉菌E09菌株,分别对这3份农家品种、感病亲本‘铭贤169’以及各自的F1和F2代植株进行抗性鉴定.调查统计的数据经卡方测验分析其符合度.[结果]这3份农家品种对白粉菌E09菌株的抗性均由1对隐性核基因控制.[结论]3份农家品种对石家庄本地区的混合白粉病菌表现出良好的抗性,并且对E09的抗性均由1对隐性基因控制.可以进一步对它们进行分子标记及定位研究,为其作为抗源在小麦抗白粉病育种中的应用奠定基础.  相似文献   

13.
小麦抗白粉病基因Pm13Pm4累加体的分子标记辅助选择   总被引:8,自引:0,他引:8  
 利用Pm4的STS-PCR标记及Pm13的SCAR标记,检测含Pm4b的YW243与含Pm13抗性基因品系杂交的F3代的抗感单株,初步筛选到累加了Pm4bPm13两个抗性基因的植株R1、R4;并分别对R1和R4自交后代(F4代)的15个抗病单株进行跟踪检测,得到13株累加体,而另外2株仅具Pm4b基因。本研究说明分子标记是检测抗病基因累加体、辅助育种的有效手段。  相似文献   

14.
为明确海南省苦瓜白粉病的病原菌、生理小种及苦瓜对白粉病的抗性遗传规律,结合形态学鉴定和分子鉴定解析白粉病菌及生理小种种类,通过显微镜观察白粉病菌侵染过程,并应用主基因+多基因混合遗传模型分析法探讨苦瓜对白粉病的主要抗性遗传规律。结果表明:采集自海南省6个市(县)的苦瓜白粉病病原菌均为单囊壳白粉菌Sphaerotheca fuliginea,属生理小种2F,该菌在侵染苦瓜叶片时有4个关键时期:接种后4 h为分生孢子萌发高峰期,8 h为附着孢形成高峰期,16~24 h为次生菌丝形成高峰期,5 d为分生孢子梗形成高峰期。将其接种于苦瓜抗、感品系,对白粉病的抗性符合2对加性-显性-上位性主基因+加性-显性多基因模型,主基因和多基因共同控制苦瓜对白粉病的抗性,其中以主基因遗传为主,且会受到环境变异的影响。根据苦瓜抗性遗传规律,F2代主基因遗传率最高,受环境影响最小,在苦瓜的白粉病抗性育种中,以早期世代F2代作为有效选择世代。研究表明白粉病菌侵染叶片的前2 d是白粉病防治的最佳时期,所以在白粉病易发的物候期,可将防治时间提前1~2 d。  相似文献   

15.
燕麦种质资源抗白粉病鉴定及利用评价   总被引:1,自引:0,他引:1  
采用田间自然感病的方法,于2009-2011年在甘肃省天水市甘谷县对128份燕麦品种进行了由白粉菌(Blumeria graminis f.sp.avenae)引起的燕麦白粉病田间抗性鉴定和评价,该地区属于白粉菌病害常发区。结果表明,所有供试材料均程度不同地感染燕麦白粉病,无免疫材料,2份材料‘MF9715’、‘4607’表现高抗;8份材料‘QO245-7’、‘白燕2号’、‘VAO-1’、‘709’、‘4663’、‘4641’、‘4628’和‘青永久307’表现中抗;其余118份材料表现中感、高感和极度感病。说明抗燕麦白粉病的材料严重匮乏,可利用的抗性种质资源相对更少。筛选出的高抗和中抗材料对燕麦白粉病有较好抗性,是今后可利用的抗性种质资源。  相似文献   

16.
抗白粉病胡麻种质资源田间鉴定与筛选   总被引:2,自引:0,他引:2  
白粉病目前已成为影响胡麻产量和质量最常见的病害之一, 种植抗病品种是防控病害最经济环保的有效措施, 然而抗病亲本材料的缺乏已成为制约抗病品种选育的关键因素。为筛选出抗白粉病胡麻材料, 本研究在田间自然感病的条件下, 采用病情指数法对300份国内外胡麻种质资源材料进行了抗白粉病鉴定和评价。结果表明, 所有供试材料均程度不同地感染胡麻白粉病, 无免疫材料, 仅有5份材料为中抗; 其余295份均为感病材料, 其中8份材料中感, 52份材料感病, 235份材料高度感病。本研究可为抗白粉病胡麻品种的培育及相关抗病基因的发掘提供参考。  相似文献   

17.
 小麦(Triticum aestivumL.)品系‘兰考90(6)’在2AL染色体臂上携带1个隐性抗白粉病基因,暂命名为PmLK906。以‘中国春’/‘兰考90(6)21-12’杂交F3代纯合株系构建的抗、感cDNA池为探针进行小麦基因芯片杂交,结果表明与粗山羊草(Aegilops tauschii)csAtPR5类似的基因在抗病池中的表达量比感病池中约高24.2倍。随后,从‘兰考90(6)21-12’中成功克隆了一个2 125 bp的全长csAtPR5-类似基因cDNA序列,暂命名为TaAetPR5(GenBank登录号:EU082094)。TaAet-PR5与csAtPR5的cDNA序列有93%的相同。TaAetPR5编码1个由657个氨基酸组成的多肽,与csAtPR5有88%的相同。蛋白推导分析表明TaAetPR5的分子量为74.5 kDa,pI 6.82,可能是一个可溶性的球蛋白,存在于细胞核中的可能性是95%。接种小麦白粉病菌(Blumeria graminisf.sp.tritici)后12至72 h,‘兰考90(6)21-12’幼苗叶片中的TaAetPR5基因转录水平不断提高。感白粉病的‘中国春’中没有检测到TaAetPR5基因。  相似文献   

18.
Shi AN  Leath S  Murphy JP 《Phytopathology》1998,88(2):144-147
ABSTRACT A major gene for resistance to wheat powdery mildew (Blumeria graminis f. sp. tritici = Erysiphe graminis f. sp. tritici) has been successfully transferred into hexaploid common wheat (Triticum aestivum, 2n = 6x = 42, AABBDD) from wild einkorn wheat (Triticum monococcum subsp. aegilopoides, 2n = 2x = 14, AA). NC96BGTA5 is a germ plasm line with the pedigree Saluda x 3/PI427662. The response patterns for powdery mildew resistance in NC96BGTA5 were tested with 30 differential isolates of B. graminis f. sp. tritici, and the line was resistant to all tested isolates. The analyses of P(1), P(2), F(1), F(2), and BC(1)F(1) populations derived from NC96BGTA5 revealed two genes for wheat powdery mildew resistance in the NC96BGTA5 line. One gene, Pm3a, was from its recurrent parent Saluda, and the second was a new gene introgressed from wild einkorn wheat. The gene was determined to be different from Pm1 to Pm21 by gene-for-gene and pedigree analyses. The new gene was identified as linked to the Pm3a gene based on the F(2) and BC(1)F(1) populations derived from a cross between NC96BGTA5 and a susceptible cultivar NK-Coker 68-15, and the data indicated that the gene was located on chromosome 1A. It is proposed that this new gene be designated Pm25 for wheat powdery mildew resistance in NC96BGTA5. Three random amplified polymorphic DNA markers, OPX06(1050), OPAG04(950), and OPAI14(600), were found to be linked to this new gene.  相似文献   

19.
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