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Gene expression analysis in Musa acuminata during compatible interactions with Meloidogyne incognita

机译:与南方根结线虫相容性互作期间尖锐草中的基因表达分析

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摘要

>Background and Aims Endoparasitic root-knot nematodes (RKNs) (Meloidogyne spp.) cause considerable losses in banana (Musa spp.), with Meloidogyne incognita a predominant species in Cavendish sub-group bananas. This study investigates the root transcriptome in Musa acuminata genotypes 4297-06 (AA) and Cavendish Grande Naine (CAV; AAA) during early compatible interactions with M. incognita. >Methods Roots were analysed by brightfield light microscopy over a 35 d period to examine nematode penetration and morphological cell transformation. RNA samples were extracted 3, 7 and 10 days after inoculation (DAI) with nematode J2 juveniles, and cDNA libraries were sequenced using lllumina HiSeq technology. Sequences were mapped to the M. acuminata ssp. malaccensis var. Pahang genome sequence, differentially expressed genes (DEGs) identified and transcript representation determined by gene set enrichment and pathway mapping. >Key Results Microscopic analysis revealed a life cycle of M. incognita completing in 24 d in CAV and 27 d in 4279-06. Comparable numbers of DEGs were up- and downregulated in each genotype, with potential involvement of many in early host defence responses involving reactive oxygen species and jasmonate/ethylene signalling. DEGs revealed concomitant auxin metabolism and cell wall modification processes likely to be involved in giant cell formation. Notable transcripts related to host defence included those coding for leucine-rich repeat receptor-like serine/threonine-protein kinases, peroxidases, thaumatin-like pathogenesis-related proteins, and DREB, ERF, MYB, NAC and WRKY transcription factors. Transcripts related to giant cell development included indole acetic acid-amido synthetase GH3.8 genes, involved in auxin metabolism, as well as genes encoding expansins and hydrolases, involved in cell wall modification. >Conclusions Expression analysis in M. acuminata during compatible interactions with RKNs provides insights into genes modulated during infection and giant cell formation. Increased understanding of both defence responses to limit parasitism during compatible interactions and effector-targeted host genes in this complex interaction will facilitate the development of genetic improvement measures for RKNs.
机译:>背景和目的内寄生根结线虫(RKNs)(Meloidogyne spp。)在香蕉(Musa spp。)中造成相当大的损失,其中Meloidogyne incognita是卡文迪许亚组香蕉中的主要物种。这项研究调查了与M. incognita的早期相容性相互作用期间,Mus acuminata基因型4297-06(AA)和Cavendish Grande Naine(CAV; AAA)的根转录组。 >方法在35 d的时间内通过明场光学显微镜对根进行了分析,以检查线虫的穿透和形态细胞的转化。线虫J2幼虫接种(DAI)后3、7和10天提取RNA样品,并使用lllumina HiSeq技术对cDNA文库进行测序。序列被映射到M. acuminata ssp。马六甲变种彭亨(Pahang)基因组序列,鉴定的差异表达基因(DEGs)和通过基因集富集和途径作图确定的转录本代表。 >主要结果显微镜分析显示,隐孢子虫的生命周期在CAV中24天内完成,在4279-06中27天内完成。在每种基因型中,可比较数量的DEGs上调和下调,许多潜在参与早期宿主防御反应,包括活性氧和茉莉酸/乙烯信号传导。 DEGs揭示了可能伴随着巨细胞形成的生长素代谢和细胞壁修饰过程。与宿主防御相关的显着转录本包括编码富含亮氨酸的重复受体样丝氨酸/苏氨酸蛋白激酶,过氧化物酶,索马甜蛋白样致病相关蛋白,DREB,ERF,MYB,NAC和WRKY转录因子的转录本。与巨细胞发育有关的转录物包括涉及植物生长素代谢的吲哚乙酸-酰胺基合成酶GH3.8基因,以及涉及细胞壁修饰的编码扩展蛋白和水解酶的基因。 >结论在与RKNs兼容相互作用过程中的尖锐湿疣中的表达分析提供了对感染和巨细胞形成过程中调节的基因的见解。在这种复杂的相互作用中,增加对限制相互作用中限制寄生虫的防御反应的认识以及这种复杂相互作用中以效应子为靶标的宿主基因,将有助于RKNs遗传改良措施的发展。

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