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鹰嘴豆中参与识别的关键抗性基因类似物的测定

Determination of the Key Resistance Gene Analogs Involved in Recognition in Chickpea.

作者信息

Zhou Ziwei, Bar Ido, Sambasivam Prabhakaran Thanjavur, Ford Rebecca

机构信息

Environmental Futures Research Institute, School of Environment and Science, Griffith University, Nathan, QLD, Australia.

出版信息

Front Plant Sci. 2019 May 17;10:644. doi: 10.3389/fpls.2019.00644. eCollection 2019.

Abstract

Chickpea ( L.) is an important cool season food legume, however, its production is severely constrained by the foliar disease Ascochyta blight caused by the fungus (syn. ). Several disease management options have been developed to control the pathogen, including breeding for host plant resistance. However, the pathogen population is evolving to produce more aggressive isolates. For host resistance to be effective, the plant must quickly recognize the pathogen and instigate initial defense mechanisms, optimally at the point of contact. Given that the most resistant host genotypes display rapid pathogen recognition and response, the approach taken was to assess the type, speed and pattern of recognition via Resistance Gene Analog (RGA) transcription among resistant and susceptible cultivated chickpea varieties. RGAs are key factors in the recognition of plant pathogens and the signaling of inducible defenses. In this study, a suite of RGA loci were chosen for further investigation from both published literature and from newly mined homologous sequences within the National Center for Biotechnology Information (NCBI) database. Following their validation in the chickpea genome, 10 target RGAs were selected for differential expression analysis in response to infection. This was performed in a set of four chickpea varieties including two resistant cultivars (ICC3996 and PBA Seamer), one moderately resistant cultivar (PBA HatTrick) and one susceptible cultivar (Kyabra). Gene expression at each RGA locus was assessed via qPCR at 2, 6, and 24 h after inoculation with a previously characterized highly aggressive isolate. As a result, all loci were differentially transcribed in response to pathogen infection in at least one genotype and at least one time point after inoculation. Among these, the differential expression of four RGAs was significant and consistently increased in the most resistant genotype ICC3996 immediately following inoculation, when spore germination began and ahead of penetration into the plant's epidermal tissues. Further analyses indicated that the differentially transcribed RGAs function through ADP-binding within the pathogen recognition pathway. These represent clear targets for future functional validation and potential for selective resistance breeding for introgression into elite cultivars.

摘要

鹰嘴豆(L.)是一种重要的冷季食用豆类,然而,其产量受到由真菌(同义词)引起的叶部病害Ascochyta枯萎病的严重制约。已经开发了几种病害管理方法来控制病原体,包括培育寄主植物抗性。然而,病原体群体正在进化以产生更具侵袭性的分离株。为了使寄主抗性有效,植物必须快速识别病原体并启动初始防御机制,最好是在接触点。鉴于最抗病的寄主基因型表现出快速的病原体识别和反应,所采用的方法是通过抗性基因类似物(RGA)转录来评估抗性和感病栽培鹰嘴豆品种之间识别的类型、速度和模式。RGA是识别植物病原体和诱导防御信号传导的关键因素。在本研究中,从已发表的文献以及美国国立生物技术信息中心(NCBI)数据库中新挖掘的同源序列中选择了一组RGA基因座进行进一步研究。在鹰嘴豆基因组中验证后,选择了10个目标RGA进行响应感染的差异表达分析。这在一组四个鹰嘴豆品种中进行,包括两个抗病品种(ICC3996和PBA Seamer)、一个中度抗病品种(PBA HatTrick)和一个感病品种(Kyabra)。在用先前鉴定的高侵袭性分离株接种后2、6和24小时,通过qPCR评估每个RGA基因座的基因表达。结果,所有基因座在接种后至少一种基因型和至少一个时间点对病原体感染有差异转录。其中,四个RGA的差异表达显著,并且在最抗病的基因型ICC3996中,接种后孢子萌发开始且在穿透植物表皮组织之前,差异表达立即持续增加。进一步的分析表明,差异转录的RGA通过病原体识别途径内的ADP结合发挥作用。这些是未来功能验证的明确目标,也是将选择性抗性育种渗入优良品种的潜力所在。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ef38/6546118/4e87efab1484/fpls-10-00644-g001.jpg

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