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首页> 外文期刊>American journal of enology & viticulture >Resistance Gene Analogs From Vitis Cinerea, Vitis Rupestris,and Vitis Hybrid Horizon
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Resistance Gene Analogs From Vitis Cinerea, Vitis Rupestris,and Vitis Hybrid Horizon

机译:葡萄,葡萄树和葡萄杂交视野的抗性基因类似物

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摘要

Resistance gene analogs (RGAs) characterized by the presence of nucleotide-binding sites (NBS) were cloned from Vitis cinerea, V. rupestris, and V. hybrid Horizon. Two degenerate PCR primer pairs were designed from conserved regions of NBS motifs within known resistance (R) genes and used for PCR amplification of putative RGAs. A total of 122 putative RGA sequences were cloned from all three genotypes by P-loop/GLPLAL-1 primers. Based on nucleic acid sequence-identity of 90% or greater, RGA clones were subdivided into eight, four, and seven groups for V. cinerea, V. rupestris, and Horizon, respectively. All of these clones showed similarity of nucleotide sequences to other known R genes or NBS-type nucleotide sequences, and seven clones showed high similarity. Thirty sequences were cloned from V. cinerea by P-loop/Rev loop and subdivided into four sequence groups, none of which were similar to nucleotide sequences of other R genes. Nineteen representative RGA clones were classified into 13 TIR- (Drosophila Toll and mammalian biterleukin-1 Receptors) NBS-leucine rich repeat (LRR)-like genes and six non-TIR-NBS-LRR-like genes based primarily on nucleotide sequences of kinase-2 motifs and phylogenetic analysis with known TIR or non-TIR proteins. Twenty-three sequence tagged site (STS) and three cleaved amplified polymorphic sequence (CAPS) markers developed from RGAs were checked for segregation among 179 seedlings from Horizon x Illinois (Ill.) 547-1, and 18 showed goodness-of-fit using a chi-square test. Marker stkVaOll correlated with segregation for downy mildew resistance in this population. These STS markers are currently being investigated for their potential in molecular breeding for disease resistance.
机译:从灰葡萄,葡萄红斑病菌和杂交杂种地平线中克隆了以核苷酸结合位点(NBS)为特征的抗性基因类似物(RGA)。从已知抗性(R)基因中NBS基序的保守区域设计了两个简并PCR引物对,并用于PCR推定的RGA。通过P-loop / GLPLAL-1引物,从所有三种基因型中共克隆了122个推定的RGA序列。基于90%或更高的核酸序列同一性,将RGA克隆分别分为灰葡萄孢,小菜蛾和地平线的8个,4个和7个组。所有这些克隆均显示出与其他已知的R基因或NBS型核苷酸序列相似的核苷酸序列,而七个克隆均显示出高度相似性。通过P-loop / Rev loop从灰葡萄中克隆了30个序列,并细分为四个序列组,它们均与其他R基因的核苷酸序列相似。主要根据激酶的核苷酸序列,将19个代表性RGA克隆分为13个TIR-(果蝇Toll和哺乳动物biterleukin-1受体)NBS-亮氨酸富集重复(LRR)样基因和6个非TIR-NBS-LRR样基因。 -2基序和已知TIR或非TIR蛋白的系统发育分析。检查了由RGA产生的23个序列标签位点(STS)和3个裂解的扩增多态序列(CAPS)标记在Horizo​​n x Illinois(IL。)547-1的179株幼苗中的分离情况,其中18株表现出拟合优度卡方检验。标记stkVaOll与该人群中霜霉病抗性的隔离相关。目前正在研究这些STS标记在抗病分子育种中的潜力。

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