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Isolation and sequence analysis of wheat NBS-LRR type disease resistance gene analogs using degenerate PCR primers

机译:简并PCR引物对小麦NBS-LRR型抗病基因的分离和序列分析

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Isolation of disease resistance gene analogs (RGAs) using the conserved motifs of the resistance genes has attracted considerable attention since it was first reported more than a decade ago. In this study, RGAs are isolated using homology-based PCR to target the nucleotide binding site (NBS) conserved regions from hexaploid wheat varieties and a few accessions of wild types. Based on sequence similarity analysis, 83 of the sequenced clones were clustered as groups. Of these RGAs, 40 were in the NBS-LLR class, containing kinase-1a (GGVGKTT or GGVGKTA), kinase-2 (KRFLIVLDDXW), kinase-3a (GSXIVVITTR or GCXVLATTR), and the GLPL motif of the NBS-spanning region. Among these, 15 contained possible intron regions, similar to Avena sativa O2 NBS-LLR type disease resistance gene (AF078874), and one to Rpm1 of rice and Yr10 and Lr10 of wheat. To our knowledge, this is the first observation of an intronic site within the P-loop domain of wheat RGAs. We detected an unspecified motif (VMVCVS) between the kinase-1a and kinase-2 domains within our clones. Additionally, one of the clones showed replacement with the kinase-3a motif with an undefined sequence.
机译:自从十多年前首次报道使用抗病基因的保守基元分离抗病基因类似物(RGA)以来,就引起了相当大的关注。在这项研究中,使用基于同源性的PCR分离RGA,以靶向六倍体小麦品种和少数野生型材料的核苷酸结合位点(NBS)保守区域。根据序列相似性分析,将83个测序克隆作为一组进行聚类。在这些RGA中,有40个属于NBS-LLR类,包含激酶1a(GGVGKTT或GGVGKTA),激酶2(KRFLIVLDDXW),激酶3a(GSXIVVITTR或GCXVLATTR)和NBS跨区的GLPL基序。其中15个含有可能的内含子区域,类似于Avena sativa O2 NBS-LLR型抗病基因(AF078874),水稻的Rpm1和小麦的Yr10和Lr10之一。据我们所知,这是小麦RGAs P-环域内一个内含子位点的首次观察。我们在克隆中的激酶-1a和激酶2域之间检测到未指定的基序(VMVCVS)。另外,其中一个克隆显示被具有不确定序列的激酶-3a基序替代。

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