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NLR 注释工具可用于注释细胞内免疫受体库。

The NLR-Annotator Tool Enables Annotation of the Intracellular Immune Receptor Repertoire.

机构信息

John Innes Centre, Norwich Research Park, Norwich, NR4 7UH, United Kingdom.

Sainsbury Laboratory, Norwich Research Park, Norwich, NR4 7UH, United Kingdom.

出版信息

Plant Physiol. 2020 Jun;183(2):468-482. doi: 10.1104/pp.19.01273. Epub 2020 Mar 17.

Abstract

Disease resistance genes encoding nucleotide-binding and leucine-rich repeat (NLR) intracellular immune receptor proteins detect pathogens by the presence of pathogen effectors. Plant genomes typically contain hundreds of NLR-encoding genes. The availability of the hexaploid wheat () cultivar Chinese Spring reference genome allows a detailed study of its NLR complement. However, low expression and high intrafamily sequence homology hinder their accurate annotation. Here, we developed NLR-Annotator, a software tool for in silico NLR identification independent of transcript support. Although developed for wheat, we demonstrate the universal applicability of NLR-Annotator across diverse plant taxa. We applied our tool to wheat and combined it with a transcript-validated subset of genes from the reference gene annotation to characterize the structure, phylogeny, and expression profile of the gene family. We detected 3,400 full-length NLR loci, of which 1,560 were confirmed as expressed genes with intact open reading frames. NLRs with integrated domains mostly group in specific subclades. Members of another subclade predominantly locate in close physical proximity to NLRs carrying integrated domains, suggesting a paired helper function. Most (88%) display low basal expression (in the lower 10 percentile of transcripts). In young leaves subjected to biotic stress, we found up-regulation of 266 of the To illustrate the utility of our tool for the positional cloning of resistance genes, we estimated the number of genes within the intervals of mapped rust resistance genes. Our study will support the identification of functional resistance genes in wheat to accelerate the breeding and engineering of disease-resistant varieties.

摘要

抗病基因编码核苷酸结合和富含亮氨酸重复(NLR)细胞内免疫受体蛋白通过病原体效应物的存在来检测病原体。植物基因组通常包含数百个 NLR 编码基因。六倍体小麦()栽培品种春小麦参考基因组的可用性允许对其 NLR 成分进行详细研究。然而,低表达和高家族内序列同源性阻碍了它们的准确注释。在这里,我们开发了 NLR-Annotator,这是一种用于在没有转录支持的情况下进行 NLR 鉴定的计算工具。尽管是为小麦开发的,但我们证明了 NLR-Annotator 在跨多种植物类群中的普遍适用性。我们将我们的工具应用于小麦,并将其与参考基因注释中经转录验证的基因子集相结合,以表征基因家族的结构、系统发育和表达谱。我们检测到 3400 个全长 NLR 基因座,其中 1560 个被确认为具有完整开放阅读框的表达基因。具有整合结构域的 NLR 大多分组在特定的亚群中。另一个亚群的成员主要位于与携带整合结构域的 NLR 紧密物理接近的位置,这表明它们具有配对辅助功能。大多数(88%)显示低基础表达(在转录本的较低 10%位)。在受到生物胁迫的幼叶中,我们发现 266 个 NLR 被上调。为了说明我们的工具在定位克隆抗病基因方面的实用性,我们估计了 mapped rust 抗病基因区间内的基因数量。我们的研究将支持在小麦中鉴定功能抗病基因,以加速抗病品种的培育和工程改造。

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