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Identification and Cloning of Resistance Gene Analogues (RGAs) Encoding NBS-LRR Proteins from Gossypium arboreum L.
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作者 AZHAR Muhammad Tehseen BASHIR Aftab BRIDDON Rob W MANSOOR Shahid 《棉花学报》 CSCD 北大核心 2008年第S1期42-,共1页
Plants have developed a complicated defense mechanism during evolution to resist the harmful pathogens they encountered.The mechanism involves the interaction of the plant resistance(R)
关键词 NBS Encoding NBS-LRR Proteins from Gossypium arboreum L Identification and Cloning of resistance gene analogues LRR rgas
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Isolation of Resistance Gene Analogs from Wheat Based on Conserved Domains of Resistance Genes 被引量:1
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作者 秦跟基 陈佩度 +2 位作者 顾红雅 冯祎高 牛吉山 《Acta Botanica Sinica》 CSCD 2003年第3期340-345,共6页
Two pairs of degenerate primers were designed based on nucleotide-binding site (NBS) and serine/threonine kinase domain. PCR was performed with the primers and cDNA from the Triticum aestivum-Haynaldia villosa translo... Two pairs of degenerate primers were designed based on nucleotide-binding site (NBS) and serine/threonine kinase domain. PCR was performed with the primers and cDNA from the Triticum aestivum-Haynaldia villosa translocation line 6VS/6AL. Amplified products were cloned and sequenced. Nine clones with NBS and one with serine/threonine kinase domain were obtained. The NBS clones were classified to six groups according to their nucleotide sequence identities (90% or higher). These resistance gene analogs (RGAs) all have open reading frames (ORF), and their amino acid sequences show high similarity to Yr10 in wheat, Mla1 and Mla6 in barley, RPS2 in Arabidopsis and other resistance (R) genes with conserved motifs. They were preliminarily mapped on the chromosomes of homoeologous groups 1, 2 and 5 of common wheat by nulli-tetrasomic analysis. The 5'-end sequence of an RGA N5 was obtained by 5'-RACE PCR. It encodes six leucine zipper (LZ) and has high sequence similarity to RPS2. 展开更多
关键词 resistance gene analogs nucleotide-binding site PCR Triticum aestivum-Haynaldia villosa translocation line
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Cloning and Characterization of a Family of Disease Resistance Gene Analogs from 6VS of Haynaldia villosa
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作者 KONG Fan-jing, MA You-zhi, CHEN Xiao and XIN Zhi-yong(Institute of Crop Breeding and Cultivation , Chinese Academy of Agricultural Sciences , Beijing 100081,P. R. China Open Laboratory of Saline Lake Resources and Environment of Ministryof Land and Resources , Beijing 100037 , P.R. China) 《Agricultural Sciences in China》 CAS CSCD 2003年第8期937-942,共6页
In the present study, microdissection of 6VS and the cloning of the resistance gene analogs(RGA)from them were reported. The 6VS were microdissected with needle and 10 types of resistance gene analogs were obtained by... In the present study, microdissection of 6VS and the cloning of the resistance gene analogs(RGA)from them were reported. The 6VS were microdissected with needle and 10 types of resistance gene analogs were obtained by PCR with degenerate oligonucleotide primer designed according to resistance genes. They were designated as Hvrgak1-Hvrgak10, GenBank accession numbers are AF387113-AF387121, AY040671- AY040672. Identity among RGAs was about 10-50%, and identity with cloned R gene from plants was 5-20%. Southern hybridization analysis results showed 3 RGAs, Hvrgak2, Hvrgak4, and Hvr-gak5 were linked with wheat powdery mildew resistance. These RGAs may be used as direct entrance or probes for cloning the disease resistance genes. 展开更多
关键词 6VS of Haynaldia Villosa MICRODISSECTION resistance gene analogs(rga) CLONING
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An Integrated QTL Map of Fungal Disease Resistance in Soybean (Glycine max L. Merr):A Method of Meta-Analysis for Mining R Genes 被引量:5
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作者 WANG Jia-lin LIU Chun-yan +4 位作者 WANG Jing QI Zhao-ming LI Hui HU Guo-hua CHEN Qing-shan 《Agricultural Sciences in China》 CAS CSCD 2010年第2期223-232,共10页
Diseases caused by fungal pathogens account for approximately 50% of all soybean disease losses around the world. Conflicting results of fungal disease resistance QTLs from different populations often occurred. The ob... Diseases caused by fungal pathogens account for approximately 50% of all soybean disease losses around the world. Conflicting results of fungal disease resistance QTLs from different populations often occurred. The objectives of this study were to: (i) evaluate evidence for reported fungal disease resistance QTLs associations in soybean and (ii) extract relatively reliable and useful information from the "real" QTLs and mine putative genes in soybean. An integrated map of fungal disease resistance QTLs in soybean was established with soymap 2 published in 2004 as a reference map. QTLs of fungal disease resistance developed from each of separate populations in recent 10 years were integrated into a combinative map for gene cloning and marker assisted selection in soybean. 107 QTLs from different maps were integrated and projected to the reference map with the software BioMercator 2.1. A method of meta-analysis was used to narrow down the confidence interval, and 23 "real" QTLs and their corresponding markers were obtained from 12 linkage groups (LG), respectively. Two published R genes were found in these "real" QTLs intervals. Sequences in the "real" QTLs intervals were predicted by GENSCAN, and these predicted genes were annotated in Goblet. 228 resistance gene analogs (RGAs) in 12 different terms were mined. The results will lay the foundation for a bioinformatics platform combining abundant QTLs, and offer the basis for marker assisted selection and gene cloning in soybean. 展开更多
关键词 SOYBEAN fungal disease QTL META-ANALYSIS resistance gene analogs
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Isolation and Characterization of NBS-LRR Class Resistance Homologous Gene from Wheat 被引量:3
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作者 ZHANG Nan WANG Shen WANG Hai-yan LIU Da-qun 《Agricultural Sciences in China》 CAS CSCD 2011年第8期1151-1158,共8页
One resistance gene analog fragment named RGA-CIN14 was isolated from TcLr19 wheat,which contains kinase-2,kinase-3a,and the GLPL motif of the NBS-spanning region,using degenerated primers according to the nucleotide ... One resistance gene analog fragment named RGA-CIN14 was isolated from TcLr19 wheat,which contains kinase-2,kinase-3a,and the GLPL motif of the NBS-spanning region,using degenerated primers according to the nucleotide binding site (NBS) conserved domain.Based on the RGA-CIN14,a full-length cDNA,CIN14,which was 2 987 bp encoding 880 amino acids,was obtained by using the method of the rapid amplification cDNA ends (RACE).Bioinformatics analysis showed that the deduced amino acids of CIN14 protein consisted of a NB-ARC conserved domain and many leucine-rich repeats (LRR) domains.The phylogenetic tree analysis indicated a considerable identity of the protein encoded by CIN14 with that of wheat leaf rust resistance gene Lr1,but a lower similarity with Lr21.The expression profile of the CIN14 gene detected by semi-quantitative RT-PCR showed that the CIN14 gene was not induced by Puccinia triticina and it was a constitutive gene with low abundance in the wheat leaf tissue.The resistance homology sequence was successfully obtained,which provides the shortcut for cloning of the resistance gene in TcLr19 wheat. 展开更多
关键词 wheat leaf rust resistance gene NBS-LRR resistance gene analogs (rgas) rapid amplification cDNA end (RACE) RT-PCR
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Development and mapping of SSR markers linked to resistance-gene homologue clusters in common bean
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作者 Luz Nayibe Garzon Matthew Wohlgemuth Blair 《The Crop Journal》 SCIE CAS 2014年第4期183-194,共12页
Common bean is an important but often a disease-susceptible legume crop of temperate,subtropical and tropical regions worldwide. The crop is affected by bacterial, fungal and viral pathogens. The strategy of resistanc... Common bean is an important but often a disease-susceptible legume crop of temperate,subtropical and tropical regions worldwide. The crop is affected by bacterial, fungal and viral pathogens. The strategy of resistance-gene homologue(RGH) cloning has proven to be an efficient tool for identifying markers and R(resistance) genes associated with resistances to diseases. Microsatellite or SSR markers can be identified by physical association with RGH clones on large-insert DNA clones such as bacterial artificial chromosomes(BACs). Our objectives in this work were to identify RGH-SSR in a BAC library from the Andean genotype G19833 and to test and map any polymorphic markers to identify associations with known positions of disease resistance genes. We developed a set of specific probes designed for clades of common bean RGH genes and then identified positive BAC clones and developed microsatellites from BACs having SSR loci in their end sequences. A total of 629 new RGH-SSRs were identified and named BMr(bean microsatellite RGH-associated markers). A subset of these markers was screened for detecting polymorphism in the genetic mapping population DOR364 × G19833. A genetic map was constructed with a total of 264 markers,among which were 80 RGH loci anchored to single-copy RFLP and SSR markers. Clusters of RGH-SSRs were observed on most of the linkage groups of common bean and in positions associated with R-genes and QTL. The use of these new markers to select for disease resistance is discussed. 展开更多
关键词 Bacterial artificial chromosome(BAC) clone end sequences(BES) Simple sequence repeats(SSRs) Plant disease resistance(R) genes Nucleotide binding site targeted sequencing resistance gene analogs
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Transgenic Rice Plants Harboring Genomic DNA from Zizania latifolia Confer Bacterial Blight Resistance 被引量:1
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作者 SHEN Wei-wei SONG Cheng-li +3 位作者 CHEN Jie FuYaping WU Jian-li JIANG Shao-mei 《Rice science》 SCIE 2011年第1期17-22,共6页
Based on the sequence of a resistance gene analog FZ14 derived from Zizania latifolia (Griseb.), a pair of specific PCR primers FZ14P1/FZ14P2was designed to isolate candidate disease resistance gene. The pooled-PCR ... Based on the sequence of a resistance gene analog FZ14 derived from Zizania latifolia (Griseb.), a pair of specific PCR primers FZ14P1/FZ14P2was designed to isolate candidate disease resistance gene. The pooled-PCR approach was adopted using the primer pair to screen a genomic transformation-competent artificial chromosome (TAC) library derived from Z. latifolia. A positive TAC clone (ZR1) was obtained and confirmed by sequence analysis. The results indicated that ZR1 consisted of conserved motifs similar to P-loop (kinase la), kinase 2, kinase 3a and GLPL (Gly-Leu-Pro-Leu), suggesting that it could be a portion of NBS-LRR type of resistance gene. Using Agrobacterium-mediated transformation of Nipponbare mature embryo, a total of 48 independent transgenic To plants were obtained. Among them, 36 plants were highly resistant to the virulent bacterial blight strain PXO71. The results indicate that ZR1 contains at least one functional bacterial blight resistance gene. 展开更多
关键词 Zizania latifolia transformation-competent artificial chromosome library resistance-gene analog Oryza sativa bacterial blight resistance gene transfer
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云南抗白叶枯病稻种的RGA初析 被引量:9
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作者 姬广海 张世光 +2 位作者 魏兰芳 崔汝强 徐绍忠 《作物学报》 CAS CSCD 北大核心 2004年第10期969-974,共6页
根据水稻抗白叶枯病Xa2 1基因的富含亮氨酸重复区域 (LRR)和番茄抗细菌性斑点病 (Pseudomonassyringaepv tomato)的Pto基因编码蛋白质激酶的DNA序列 ,设计 2对引物用于扩增抗水稻白叶枯病品种中的抗病基因同源序列。经聚丙烯酰胺凝胶电... 根据水稻抗白叶枯病Xa2 1基因的富含亮氨酸重复区域 (LRR)和番茄抗细菌性斑点病 (Pseudomonassyringaepv tomato)的Pto基因编码蛋白质激酶的DNA序列 ,设计 2对引物用于扩增抗水稻白叶枯病品种中的抗病基因同源序列。经聚丙烯酰胺凝胶电泳和聚类分析 ,结果表明供试抗病品种间具有丰富的RGA多态性 ,用同一引物测定的属于同一簇的品种显示相似的抗性和抗谱。从XLRRfor/XLRRrev引物的聚类图中可知 ,在遗传距离为 0 2 5时 ,测试的 4 7个抗白叶枯病水稻品种可分为 9个簇。其中 3、4、7组为主要组群 ,第 3组包括 2 3个水稻品种 ,在遗传距离为 0 2时 ,可进一步分为 5个亚群。RGA分析结果为水稻抗病育种选择亲本和利用品种布局进行白叶枯病生态控制提供了依据。 展开更多
关键词 水稻 白叶枯病抗性 抗病基因同源序列 rga指纹
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大豆品种RGA分析与疫霉根腐病抗性鉴定 被引量:9
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作者 孙石 赵晋铭 +5 位作者 武晓玲 郭娜 王源超 唐卿华 盖钧镒 邢邯 《作物学报》 CAS CSCD 北大核心 2008年第10期1704-1711,共8页
采用7个具有不同毒性基因的大豆疫霉菌株,对黄淮地区48个优良大豆种质资源进行了苗期接种鉴定,筛选出一批具有不同抗性的优异抗源,说明黄淮地区蕴藏着丰富的大豆抗病资源。以相似系数0.682聚类,48个大豆品种可以分成8类。同时,根据抗病... 采用7个具有不同毒性基因的大豆疫霉菌株,对黄淮地区48个优良大豆种质资源进行了苗期接种鉴定,筛选出一批具有不同抗性的优异抗源,说明黄淮地区蕴藏着丰富的大豆抗病资源。以相似系数0.682聚类,48个大豆品种可以分成8类。同时,根据抗病基因在保守区域序列同源性的原理,利用RGA-PCR方法对48个品种的遗传多样性进行分析,从48个大豆品种的抗病基因同源序列中共扩增出53条谱带,各品种之间谱带较清晰且呈现明显的多态性,以相似系数0.746聚类,48个大豆品种可以分成7类。尽管抗性表型和RGA聚类的类与类之间没有一一对应关系,但抗谱广的品种,能较好地聚在一类,如丰收黄、科丰36、即墨油豆等。因此,综合利用抗性表型和RGA分析可以为大豆疫霉根腐病抗性基因鉴定、品种的培育和合理布局提供一定的理论依据。 展开更多
关键词 大豆 抗病基因同源序列分析 多态性 抗性鉴定
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水稻品种RGA分析与抗瘟性鉴定 被引量:4
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作者 李晔 范静华 +1 位作者 何月秋 朱有勇 《江西农业大学学报》 CAS CSCD 北大核心 2007年第1期11-15,共5页
根据抗病基因在保守区域序列同源的原理,利用RGA方法对云南省主要栽培品种和地方资源品种的遗传多样性进行了分析。从22个水稻品种的抗病基因同源序列中,共扩增出155条谱带,各品种之间谱带较清晰呈现明显的多态性,聚类分析结果可以明显... 根据抗病基因在保守区域序列同源的原理,利用RGA方法对云南省主要栽培品种和地方资源品种的遗传多样性进行了分析。从22个水稻品种的抗病基因同源序列中,共扩增出155条谱带,各品种之间谱带较清晰呈现明显的多态性,聚类分析结果可以明显将品种的抗感水平分开,也与温室人工接种试验结果相似。因此,利用RGA分析可以为水稻品种抗瘟性鉴定提供一定的理论依据。 展开更多
关键词 水稻 抗病基因同源序列分析 多态性 抗性鉴定
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小麦抗病基因同源序列(RGAs)的克隆与分析(英文) 被引量:9
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作者 刘松青 何莎 +3 位作者 蒋芳 韦先超 周翰林 涂睿 《中国农学通报》 CSCD 2007年第3期83-88,共6页
RGA(抗性基因同源序列)法是克隆植物抗性基因的一种经济有效的方法,成为近年来的研究热点。本实验综合分析了拟南芥,西红柿,水稻,烟草等植物已克隆的抗性基因,并以这些抗性基因的NBS(核酸结合位点),LRR(富含亮氨酸重复),STK(丝氨酸/苏... RGA(抗性基因同源序列)法是克隆植物抗性基因的一种经济有效的方法,成为近年来的研究热点。本实验综合分析了拟南芥,西红柿,水稻,烟草等植物已克隆的抗性基因,并以这些抗性基因的NBS(核酸结合位点),LRR(富含亮氨酸重复),STK(丝氨酸/苏氨酸激酶)保守结构域设计并合成了几十对RGA引物,对小麦抗条锈病材料进行PCR扩增,获得以Xal-NBS为引物的R88RGA片段,经克隆和序列比对分析,发现该片段与逆境条件下植物抗病信号传导相关,与蛋白激酶同源性达到96%。此项研究对抗病机理的研究和基因的发掘有重要的指导意义。 展开更多
关键词 抗病基因同源序列(rgas) 克隆 小麦
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RGA法克隆候选抗病基因的研究进展 被引量:15
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作者 徐兵强 杜中军 黄俊生 《分子植物育种》 CAS CSCD 2004年第3期421-428,共8页
RGA法是克隆植物抗病基因的一条新途径,也是近年来分子生物学领域的一个研究热点并受到植物病理学家广泛地关注。其作用原理是根据已克隆植物抗病基因的保守结构域设计简并引物,扩增获得RGAs,然后分析RGAs与抗病基因的关系,确定候选抗... RGA法是克隆植物抗病基因的一条新途径,也是近年来分子生物学领域的一个研究热点并受到植物病理学家广泛地关注。其作用原理是根据已克隆植物抗病基因的保守结构域设计简并引物,扩增获得RGAs,然后分析RGAs与抗病基因的关系,确定候选抗病基因并从而获得新的抗病基因。研究还发现,已克隆的RGAs与R基因紧密连锁。最近获得的RGAs主要是根据NBS-LRR和STK两种保守结构域而得到的。前者在植物基因组中广泛存在,而后者在植物信号传导中具有重要作用。为此,本文主要对上述两种保守结构域的结构特点和所获得的RGAs特点以及RGA法的应用前景进行了综述,以期让人们对RGA法有更进一步的认识。 展开更多
关键词 rga法克隆 抗病基因 分子生物学 作用原理 植物
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利用RGA-PCR方法进行水稻抗瘟基因分子标记 被引量:7
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作者 陈夕军 周益军 +2 位作者 徐敬友 范永坚 童蕴慧 《扬州大学学报(农业与生命科学版)》 CAS CSCD 2004年第3期55-58,69,共5页
用28对RGA引物对LTH近等基因系品种进行PCR扩增,其中11对引物扩增出特异性条带。将扩增到的33个特异性片段回收并进行重扩增,有11个片段产生单一条带。选择2个片段HS-1和HS-19进行探针标记。经Southern杂交发现,探针HS-1在含有Pi-ta2抗... 用28对RGA引物对LTH近等基因系品种进行PCR扩增,其中11对引物扩增出特异性条带。将扩增到的33个特异性片段回收并进行重扩增,有11个片段产生单一条带。选择2个片段HS-1和HS-19进行探针标记。经Southern杂交发现,探针HS-1在含有Pi-ta2抗瘟基因品种F-128-1、NO4中有特异杂交信号,表明该片段可能与抗瘟基因Pi-ta2连锁或是其一部分。对特异性片段HS-1进行克隆、测序,全长为478bp,与Mago等从水稻中克隆的一个抗病基因同源序列RGA29有95%同源性。 展开更多
关键词 水稻 抗瘟基因 抗病基因同源序列 分子标记 近等基因系
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黄瓜RGA基因的半定量RT-PCR表达分析 被引量:6
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作者 丁国华 许春梅 +2 位作者 于虹 周秀艳 秦智伟 《西北植物学报》 CAS CSCD 北大核心 2010年第4期659-664,共6页
以黄瓜(Cucumis sativusL.)抗霜霉病品种东农129为材料,利用RT-PCR半定量法研究了接种霜霉病菌(Pseudoperonospora cubensisRostow)、喷施水杨酸(SA)和氯化钙(CaCl2)等不同处理对黄瓜抗病基因类似序列(RGA)表达的影响.结果表明:CsRGA1和... 以黄瓜(Cucumis sativusL.)抗霜霉病品种东农129为材料,利用RT-PCR半定量法研究了接种霜霉病菌(Pseudoperonospora cubensisRostow)、喷施水杨酸(SA)和氯化钙(CaCl2)等不同处理对黄瓜抗病基因类似序列(RGA)表达的影响.结果表明:CsRGA1和CsRGA5基因的表达受霜霉病菌的侵染而启动或加强,外施SA和CaCl2都能够增强其表达;CsRGA4和CsRGA8属于组成型表达基因,其表达可能与霜霉病菌的侵染无关;CsRGA2的表达与外施SA和CaCl2缺乏密切关联. 展开更多
关键词 黄瓜 抗病基因类似序列 半定量RT-PCR 表达分析
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烟草表达抗病基因同源物(RGA)的鉴定及RGA-SSR标记的开发 被引量:7
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作者 袁清华 谢锐鸿 +4 位作者 张振臣 马柱文 李集勤 李淑玲 陈俊标 《作物学报》 CAS CSCD 北大核心 2014年第2期240-252,共13页
烟草是研究植物与病原菌互作的理想材料。鉴定烟草抗病基因及其同源物对揭示抗病机制具有重要意义。近年来公共数据库不断增长的EST序列为烟草表达RGA的鉴定提供丰富的数据。本研究通过拼接GenBank收录的412325条烟草EST序列,获得14960... 烟草是研究植物与病原菌互作的理想材料。鉴定烟草抗病基因及其同源物对揭示抗病机制具有重要意义。近年来公共数据库不断增长的EST序列为烟草表达RGA的鉴定提供丰富的数据。本研究通过拼接GenBank收录的412325条烟草EST序列,获得149606条Uni.EST序列。随后利用已克隆的112个植物R基因蛋白序列对其扫描,检测出1113个NtRGA,其中有273、546、53、102和30个分别包含NBS-LRR、LRR.PK、LRR、PK和Mlo结构域,另有109个未检测到结构域。通过序列比对将1071个NtRGA定位于Ⅳ.benthamiana基因组712个位点上。经搜索,从72个NtRGA中检测出78个SSR,根据其侧翼序列设计64对引物。54对成功从烟草基因组DNA中扩增出清晰条带,9对在24个普通烟草品种间检测出多态性,检出等位基因数2~4个,平均2.56个;41对在6个烟草种间检测出多态性,检出等位基因数2~4个,平均2.61个。 展开更多
关键词 烟草 表达序列标签 抗病基因同源物 SSR
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小麦抗叶锈病基因Lr35的RGA分析 被引量:7
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作者 高倩 王海燕 +2 位作者 刘大群 李星 杨文香 《华北农学报》 CSCD 北大核心 2008年第6期50-53,共4页
根据已知植物抗病基因的NBS,LRR等保守结构域设计引物,对小麦全套抗叶锈病近等基因系材料进行RGA分析。引物对Pto-kin1IN/XLRR-INV1从近等基因系TcLr35中扩增获得一条747 bp的特异性片段。序列分析表明,该片段与小麦基因片段Triticum ur... 根据已知植物抗病基因的NBS,LRR等保守结构域设计引物,对小麦全套抗叶锈病近等基因系材料进行RGA分析。引物对Pto-kin1IN/XLRR-INV1从近等基因系TcLr35中扩增获得一条747 bp的特异性片段。序列分析表明,该片段与小麦基因片段Triticum urartu clone BAC 210J24,Triticum monococcum DV92的BAC克隆231A16等具有较高同源性,为Lr35的克隆奠定了基础。 展开更多
关键词 小麦叶锈病 抗病基因 LR35 抗病基因类似序列
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辣椒抗疫病相关基因的RGA-STS标记的开发 被引量:3
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作者 王博 左星 +2 位作者 李永新 巩振辉 李大伟 《西北农业学报》 CAS CSCD 北大核心 2010年第10期124-127,共4页
利用西北农林科技大学园艺学院辣椒课题组克隆的辣椒抗疫病相关的全长基因RGA1(GenBank登录号:GQ386945)设计一对引物,上游引物为BY32,下游引物为RBQC-R。以对辣椒疫病高抗的品种CM334和感病品种EC为试材,利用PCR技术分析辣椒抗疫病的Se... 利用西北农林科技大学园艺学院辣椒课题组克隆的辣椒抗疫病相关的全长基因RGA1(GenBank登录号:GQ386945)设计一对引物,上游引物为BY32,下游引物为RBQC-R。以对辣椒疫病高抗的品种CM334和感病品种EC为试材,利用PCR技术分析辣椒抗疫病的Sequence Tagged Sites(STS)标记。结果表明,在高抗品种CM334中得到700 bp大小的STS700标记,而在感病品种EC中未扩增出相应大小的片段。在多个不同抗疫病辣椒品种中验证说明,STS700标记鉴定辣椒疫病抗性可靠、稳定。 展开更多
关键词 辣椒疫病 分子标记 rga-STS
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小麦抗白粉病基因Pm4b的RGA分析 被引量:3
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作者 胡楠 伊艳杰 +2 位作者 刘红彦 柴春月 刘新涛 《安徽农业科学》 CAS 北大核心 2007年第21期6379-6380,6430,共3页
为克隆抗性基因和发展Pm4b的特异分子标记奠定基础。利用10对RGA引物,对小麦抗白粉病基因的一些载体品种(系)进行扩增,将引物对R11F/R11R从Pm4b基因的载体品种VPM中扩增出的稳定多态性条带回收、克隆、测序,获得与小麦Pm4b基因的相关抗... 为克隆抗性基因和发展Pm4b的特异分子标记奠定基础。利用10对RGA引物,对小麦抗白粉病基因的一些载体品种(系)进行扩增,将引物对R11F/R11R从Pm4b基因的载体品种VPM中扩增出的稳定多态性条带回收、克隆、测序,获得与小麦Pm4b基因的相关抗病基因的同源片段,并对不同的小麦Pm基因载体品系作了检测分析。该稳定多态性条带全长1 321 bp。序列分析表明这个片段属于RGA类序列。用该标记检测小麦不同Pm基因载体品种(系),发现该多态性片段仅出现在Pm4b基因载体品种中。该研究可为分离抗性基因和发展Pm4b的特异分子标记奠定基础。 展开更多
关键词 小麦 白粉病 抗病基因 rga标记 序列分析
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小麦NBS类抗病相关基因片段RGA-A的初步研究 被引量:1
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作者 张立荣 齐爱勇 +1 位作者 杨文香 刘大群 《中国农学通报》 CSCD 北大核心 2011年第9期81-84,共4页
利用同源序列法分离小麦抗病相关基因同源序列。根据已经克隆的抗病基因保守结构NBS区设计引物,采用RT-PCR方法对小麦抗叶锈病近等基因系材料TcLr24进行扩增。获得了一条525bp条带RGA-A,通过BLASTp比较,序列中含有典型的NBS保守结构域,... 利用同源序列法分离小麦抗病相关基因同源序列。根据已经克隆的抗病基因保守结构NBS区设计引物,采用RT-PCR方法对小麦抗叶锈病近等基因系材料TcLr24进行扩增。获得了一条525bp条带RGA-A,通过BLASTp比较,序列中含有典型的NBS保守结构域,与很多已知植物抗病基因的功能相应区域一致,编码的蛋白与大麦中抗性蛋白亲缘关系较近。半定量RT-PCR分析表明,RGA-A受叶锈菌诱导表达,表明该基因在小麦叶片中与抗叶锈性相关。该NBS类抗病基因相关片段的获得为研究小麦抗病基因奠定了基础。 展开更多
关键词 小麦抗叶锈病基因 抗病基因类似物(rga) 同源基因
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RGA法标记植物抗病基因的研究进展 被引量:5
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作者 张荣 陈欧 王振英 《天津农业科学》 CAS 2009年第1期10-12,共3页
简述了植物抗病基因的结构特点,介绍了利用RGA法克隆的抗病基因同源序列及其应用,对RGA法的应用前景进行了展望。
关键词 rga 抗病基因 结构域
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