disease resistance

抗病性
  • 文章类型: Journal Article
    叶烫伤,由黄单胞菌引起的,是一种影响全球甘蔗的严重疾病。控制它的最实用方法之一是开发抗性甘蔗品种。确定与叶片烫伤反应相关的基因至关重要。对170个甘蔗基因型的小组在田间条件下对叶片烫伤的抗性进行了2年的评估,接下来是为期1年的温室实验。表型评估数据显示广泛的连续分布,遗传力值范围为0.58至0.84。鉴定出13种单核苷酸多态性(SNPs),与叶片抗烫伤性显着相关。其中,8个在多个环境和关联模型中保持稳定.基于RNA-seq和qRT-PCR鉴定和验证的候选基因包括两个编码NB-ARC富含亮氨酸重复(LRR)的结构域疾病抗性蛋白的基因。这些发现为甘蔗育种计划中开发标记辅助选择策略提供了基础。
    Leaf scald, caused by Xanthomonas albilineans, is a severe disease affecting sugarcane worldwide. One of the most practical ways to control it is by developing resistant sugarcane cultivars. It is essential to identify genes associated with the response to leaf scald. A panel of 170 sugarcane genotypes was evaluated for resistance to leaf scald in field conditions for 2 years, followed by a 1-year greenhouse experiment. The phenotypic evaluation data showed a wide continuous distribution, with heritability values ranging from 0.58 to 0.84. Thirteen single nucleotide polymorphisms (SNPs) were identified, significantly associated with leaf scald resistance. Among these, eight were stable across multiple environments and association models. The candidate genes identified and validated based on RNA-seq and qRT-PCR included two genes that encode NB-ARC leucine-rich repeat (LRR)-containing domain disease-resistance protein. These findings provide a basis for developing marker-assisted selection strategies in sugarcane breeding programs.
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  • 文章类型: Journal Article
    结论:使用两个完全组装的亲本基因组探索和解剖一组QTL和灰斑病抗性候选基因可能有助于加快玉米抗性育种。玉米的真菌病被称为灰叶斑病(GLS),由玉米赤孢菌和玉米赤孢菌引起,在中国是一个重大问题,南部非洲,和美国。对GLS的抗性由具有加性效应的多个基因控制,并受基因型和环境的影响。降低生产成本的最有效方法是开发抗性杂种。在这项研究中,我们利用IBMSyn10加倍单倍体(IBMSyn10DH)种群来识别与多个位置的灰叶斑病(GLS)抗性相关的数量性状基因座(QTL)。对七个不同环境的分析显示,共有58个QTL,其中49个形成了分布在染色体1、2、3、4、8和10上的12个离散簇。通过将这些发现与已发表的研究进行比较,我们在11个聚类间隔内确定了共定位的QTL或GWAS基因座。通过整合转录组数据与亲本个体之间的基因组结构变异,我们共鉴定出110个基因,这些基因在基因表达和结构改变方面均表现出显著差异.进一步的分析揭示了19个潜在的候选基因编码保守的抗性基因结构域,包括推定的富含亮氨酸的重复受体,NLP转录因子,岩藻糖基转移酶,和推定的木葡聚糖半乳糖基转移酶。我们的研究结果为玉米GLS标记抗性选择育种提供了宝贵的资源和连锁位点。
    CONCLUSIONS: The exploration and dissection of a set of QTLs and candidate genes for gray leaf spot disease resistance using two fully assembled parental genomes may help expedite maize resistance breeding. The fungal disease of maize known as gray leaf spot (GLS), caused by Cercospora zeae-maydis and Cercospora zeina, is a significant concern in China, Southern Africa, and the USA. Resistance to GLS is governed by multiple genes with an additive effect and is influenced by both genotype and environment. The most effective way to reduce the cost of production is to develop resistant hybrids. In this study, we utilized the IBM Syn 10 Doubled Haploid (IBM Syn10 DH) population to identify quantitative trait loci (QTLs) associated with resistance to gray leaf spot (GLS) in multiple locations. Analysis of seven distinct environments revealed a total of 58 QTLs, 49 of which formed 12 discrete clusters distributed across chromosomes 1, 2, 3, 4, 8 and 10. By comparing these findings with published research, we identified colocalized QTLs or GWAS loci within eleven clustering intervals. By integrating transcriptome data with genomic structural variations between parental individuals, we identified a total of 110 genes that exhibit both robust disparities in gene expression and structural alterations. Further analysis revealed 19 potential candidate genes encoding conserved resistance gene domains, including putative leucine-rich repeat receptors, NLP transcription factors, fucosyltransferases, and putative xyloglucan galactosyltransferases. Our results provide a valuable resource and linked loci for GLS marker resistance selection breeding in maize.
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  • 文章类型: Journal Article
    背景:JUB1,一个含有过氧化氢诱导的转录因子的NAC结构域,在植物免疫中起着至关重要的作用。关于JUB1对小麦叶锈病的反应知之甚少。基因组学的最新发现也揭示了许多通常被认为是无功能的sORF,主张将它们纳入翻译的潜在监管参与者的必要性。然而,SORF上的甲基化是否跨越JUB1等调节基因的3UTR调节基因表达,尚不清楚。
    结果:在这项研究中,我们鉴定了小麦JUB1同源基因3UTR中两个sORF的甲基化状态,TaJUB1-L,CpG中的胞嘧啶残基,在小麦的两个近等基因系(HD2329)中,在疾病进展的不同时间点的CHH和CHG位点,在叶锈病发病过程中有无Lr24基因。这里,我们报告了在感染后24小时后,耐药等值线中3'UTR的sORF中发生的CpG二核苷酸的显着去甲基化。此外,通过RT-qPCR观察到的上调基因表达与sORF中CpG位点的去甲基化成正比。
    结论:我们的发现表明,TaJUB1-L可能是在叶锈病发病过程中提供耐受性的正调节因子,3'UTR的胞嘧啶甲基化可能充当其表达控制的开关。这些结果丰富了常规甲基化测定技术的潜在益处,用于以具有成本效益和机密的结论性方式在植物-病原体相互作用期间解开表观遗传学中未探索的谜团。
    BACKGROUND: JUB1, a NAC domain containing hydrogen peroxide-induced transcription factor, plays a critical role in plant immunity. Little is known about how JUB1 responds to leaf rust disease in wheat. Recent discoveries in genomics have also unveiled a multitude of sORFs often assumed to be non-functional, to argue for the necessity of including them as potential regulatory players of translation. However, whether methylation on sORFs spanning the 3\'UTR of regulatory genes like JUB1 modulate gene expression, remains unclear.
    RESULTS: In this study, we identified the methylation states of two sORFs in 3\'UTR of a homologous gene of JUB1 in wheat, TaJUB1-L, at cytosine residues in CpG, CHH and CHG sites at different time points of disease progression in two near-isogenic lines of wheat (HD2329), with and without Lr24 gene during leaf rust pathogenesis. Here, we report a significant demethylation of the CpG dinucleotides occurring in the sORFs of the 3\'UTR in the resistant isolines after 24 h post-infection. Also, the up-regulated gene expression observed through RT-qPCR was directly proportional to the demethylation of the CpG sites in the sORFs.
    CONCLUSIONS: Our findings indicate that TaJUB1-L might be a positive regulator in providing tolerance during leaf rust pathogenesis and cytosine methylation at 3\'UTR might act as a switch for its expression control. These results enrich the potential benefit of conventional methylation assay techniques for unraveling the unexplored enigma in epigenetics during plant-pathogen interaction in a cost-effective and confidentially conclusive manner.
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  • 文章类型: Journal Article
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  • 文章类型: Journal Article
    核苷酸结合和富含亮氨酸的重复受体(NLR)是植物中最重要和最大的一类免疫受体。Pi36基因编码一种典型的CC-NBS-LRR蛋白,该蛋白赋予对稻瘟病真菌感染的抗性。这里,我们显示Pi36的CC结构域在细胞死亡诱导中起作用。此外,自缔合是CC域介导的细胞死亡所必需的,自缔合能力与细胞死亡水平相关。此外,NB-ARC结构域可以通过分子内相互作用抑制CC结构域的活性。MHD基序中RNBS-D基序旁边的突变D440G和D503V自动激活Pi36,但P环基序中的突变K212抑制了这种自动激活,表明NB-ARC结构域的核苷酸结合对于Pi36激活是必需的。我们还发现LRR结构域是D503V-和D440G-介导的Pi36自激活所必需的。有趣的是,CC结构域中的一些突变损害了CC结构域介导的细胞死亡,而不影响D440G或D503V介导的Pi36自激活.自激活Pi36变体表现出比非活性变体更强的自缔合。一起来看,我们推测Pi36的CC域执行细胞死亡活动,而NB-ARC结构域通过分子间相互作用抑制CC介导的细胞死亡。NB-ARC域释放其对CC域的抑制,并加强Pi36的自关联以支持CC域,可能是通过核苷酸交换.
    Nucleotide-binding and leucine-rich repeat receptors (NLRs) are the most important and largest class of immune receptors in plants. The Pi36 gene encodes a canonical CC-NBS-LRR protein that confers resistance to rice blast fungal infections. Here, we show that the CC domain of Pi36 plays a role in cell death induction. Furthermore, self-association is required for the CC domain-mediated cell death, and the self-association ability is correlated with the cell death level. In addition, the NB-ARC domain may suppress the activity of the CC domain through intramolecular interaction. The mutations D440G next to the RNBS-D motif and D503V in the MHD motif autoactivated Pi36, but the mutation K212 in the P-loop motif inhibited this autoactivation, indicating that nucleotide binding of the NB-ARC domain is essential for Pi36 activation. We also found that the LRR domain is required for D503V- and D440G-mediated Pi36 autoactivation. Interestingly, several mutations in the CC domain compromised the CC domain-mediated cell death without affecting the D440G- or D503V-mediated Pi36 autoactivation. The autoactivate Pi36 variants exhibited stronger self-associations than the inactive variants. Taken together, we speculated that the CC domain of Pi36 executes cell death activities, whereas the NB-ARC domain suppressed CC-mediated cell death via intermolecular interaction. The NB-ARC domain releases its suppression of the CC domain and strengthens the self-association of Pi36 to support the CC domain, possibly through nucleotide exchange.
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  • 文章类型: Journal Article
    泛素化在响应各种环境压力的蛋白质合成的翻译后阶段调节信号通路中起着至关重要的作用。已经发现E3泛素连接酶通过赋予待降解的蛋白质特异性来最终控制各种细胞内活性。进行这项研究是为了确认U盒E3型泛素连接酶(PUB)基因对水稻(OryzasativaL.)生物胁迫的生物学和遗传功能。设计了OsPUB9基因特异性sgRNA,并通过农杆菌介导的转化开发了转化体。使用愈伤组织进行深度测序以确认T0植物的突变类型,并进行总共三个步骤以选择没有T-DNA插入的无效个体。在OsPUB9基因编辑的情况下,基因编辑产生了一个bp的插入,并且证实了通过插入胸腺嘧啶来创建早期终止密码子和多个开放阅读框(ORF)位点。据推测,泛素化功能也随着U-boxE3泛素连接酶蛋白质结构的变化而变化。用细菌性叶枯病接种OsPUB9基因编辑的无效品系,并最终证实具有与Jinbaek相似的抗性表型,一种抗细菌性枯萎病的品种。因此,假设来自OsPUB9基因的氨基酸序列发生了很大变化,导致与生物学机制相关的原始蛋白质功能丧失。全面来说,已证实,当OsPUB9基因的特定位点发生突变时,对细菌性叶枯病胁迫的抗性增强。
    Ubiquitination plays a crucial role in regulating signal pathways during the post-translation stage of protein synthesis in response to various environmental stresses. E3 ubiquitin ligase has been discovered to ultimately control various intracellular activities by imparting specificity to proteins to be degraded. This study was conducted to confirm biological and genetic functions of the U-box type E3 ubiquitin ligase (PUB) gene against biotic stress in rice (Oryza sativa L.). OsPUB9 gene-specific sgRNA were designed and transformants were developed through Agrobacterium-mediated transformation. Deep sequencing using callus was performed to confirm the mutation type of T0 plants, and a total of three steps were performed to select null individuals without T-DNA insertion. In the case of the OsPUB9 gene-edited line, a one bp insertion was generated by gene editing, and it was confirmed that early stop codon and multiple open reading frame (ORF) sites were created by inserting thymine. It is presumed that ubiquitination function also changed according to the change in protein structure of U-box E3 ubiquitin ligase. The OsPUB9 gene-edited null lines were inoculated with bacterial leaf blight, and finally confirmed to have a resistance phenotype similar to Jinbaek, a bacterial blight-resistant cultivar. Therefore, it is assumed that the amino acid sequence derived from the OsPUB9 gene is greatly changed, resulting in a loss of the original protein functions related to biological mechanisms. Comprehensively, it was confirmed that resistance to bacterial leaf blight stress was enhanced when a mutation occurred at a specific site of the OsPUB9 gene.
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  • 文章类型: Journal Article
    菌核病菌(Ss)是最具破坏性的真菌病原体之一。在包括油菜在内的多种经济重要作物中造成巨大的产量损失。植物对Ss的抗性与由多个次要基因控制的定量抗病性(QDR)有关。涉及QDR至Ss的基因的全基因组鉴定尚未进行。在这项研究中,我们整合了几种检测方法,包括全基因组关联研究(GWAS),多组学共定位,和机器学习预测来识别,在全基因组范围内,涉及油菜QDR到Ss的基因。采用GWAS和多组学共定位,我们确定了与油菜对Ss的抗性相关的七个抗性相关基因座(RALs)。此外,我们开发了一种机器学习算法,并将其命名为综合多组学分析和目标基因预测机器学习(iMAP),它整合了多组学数据,以快速预测广泛染色体区域内的疾病抗性相关基因。通过基于识别RAL的iMAP,我们揭示了与SsQDR相关的多个钙信号基因。对变异的选择性扫描和单倍型的群体水平分析证实了进化过程中预测的钙信号基因的阳性选择。总的来说,这项研究开发了一种集成了多组数据和机器学习方法的算法,为预测与特定性状相关的靶基因提供了强有力的工具。此外,为进一步了解钙信号基因在SsQDR中的作用和机制奠定了基础。
    Sclerotinia sclerotiorum (Ss) is one of the most devastating fungal pathogens, causing huge yield loss in multiple economically important crops including oilseed rape. Plant resistance to Ss pertains to quantitative disease resistance (QDR) controlled by multiple minor genes. Genome-wide identification of genes involved in QDR to Ss is yet to be conducted. In this study, we integrated several assays including genome-wide association study (GWAS), multi-omics co-localization, and machine learning prediction to identify, on a genome-wide scale, genes involved in the oilseed rape QDR to Ss. Employing GWAS and multi-omics co-localization, we identified seven resistance-associated loci (RALs) associated with oilseed rape resistance to Ss. Furthermore, we developed a machine learning algorithm and named it Integrative Multi-Omics Analysis and Machine Learning for Target Gene Prediction (iMAP), which integrates multi-omics data to rapidly predict disease resistance-related genes within a broad chromosomal region. Through iMAP based on the identified RALs, we revealed multiple calcium signaling genes related to the QDR to Ss. Population-level analysis of selective sweeps and haplotypes of variants confirmed the positive selection of the predicted calcium signaling genes during evolution. Overall, this study has developed an algorithm that integrates multi-omics data and machine learning methods, providing a powerful tool for predicting target genes associated with specific traits. Furthermore, it makes a basis for further understanding the role and mechanisms of calcium signaling genes in the QDR to Ss.
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  • 文章类型: Journal Article
    作为丝裂原活化蛋白激酶(MAPK)级联反应的重要成员,MAPK在植物对生物和非生物胁迫的防御反应中起着重要作用;然而,大多数MAPK家族成员对青枯菌和热应激(HS)的参与仍然知之甚少。在本研究中,从辣椒基因组中鉴定出CaMAPK1,并分析了其对青枯病和HS的功能。CaMAPK1的转录积累和其天然启动子的活性均显着诱导了青枯菌接种。HS,和外源激素的应用,包括SA,MeJA,和ABA。CaMAPK1的瞬时表达表明,CaMAPK1可以靶向遍及烟草的整个细胞,并引发辣椒叶片的萎黄和超敏反应样细胞死亡。伴随着H2O2的积累,以及激素和H2O2相关标记基因的上调。CaMAPK1的敲低部分通过下调激素和H2O2相关基因的表达而增强了对青枯菌的易感性,并可能通过减弱CaHSFA2和CaHSP70-1转录本而损害了辣椒的耐热性。一起来看,我们的结果表明,CaMAPK1受SA调节,JA,和ABA信号传导,并协调辣椒对青枯菌感染和HS的反应。
    As an important member of mitogen-activated protein kinase (MAPK) cascades, MAPKs play an important role in plant defense response against biotic and abiotic stresses; however, the involvement of the majority of the MAPK family members against Ralstonia solanacearum and heat stress (HS) remains poorly understood. In the present study, CaMAPK1 was identified from the genome of pepper and its function against R. solanacearum and HS was analyzed. The transcript accumulations of CaMAPK1 and the activities of its native promoter were both significantly induced by R. solanacearum inoculation, HS, and the application of exogenous hormones, including SA, MeJA, and ABA. Transient expression of CaMAPK1 showed that CaMAPK1 can be targeted throughout the whole cells in Nicotiana benthamiana and triggered chlorosis and hypersensitive response-like cell death in pepper leaves, accompanied by the accumulation of H2O2, and the up-regulations of hormones- and H2O2-associated marker genes. The knock-down of CaMAPK1 enhanced the susceptibility to R. solanacearum partially by down-regulating the expression of hormones- and H2O2-related genes and impairing the thermotolerance of pepper probably by attenuating CaHSFA2 and CaHSP70-1 transcripts. Taken together, our results revealed that CaMAPK1 is regulated by SA, JA, and ABA signaling and coordinates responses to R. solanacearum infection and HS in pepper.
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  • 文章类型: Journal Article
    背景:南方根结线虫是一种重要的植物寄生线虫,给农业经济造成了巨大的损失。光是植物和病原生物的重要生计因子,充足的光线促进根结线虫感染,但潜在的机制仍不清楚。
    结果:表达水平和遗传分析表明,感光基因PHY,哭泣,和PHOT对线虫感染有负面影响。有趣的是,延长的下叶5(HY5),参与光信号调节的下游基因,与光感受器介导的根结线虫抗性负调控有关。ChIP和酵母单杂交测定法支持HY5通过直接结合参与根结线虫抗性的SWEET负调节因子来参与植物到根结线虫的反应。
    结论:本研究阐明了光信号通路在植物对线虫的抗性中的重要作用,为RKN抗性研究提供了新的视角。
    BACKGROUND: Meloidogyne incognita is one of the most important plant-parasitic nematodes and causes tremendous losses to the agricultural economy. Light is an important living factor for plants and pathogenic organisms, and sufficient light promotes root-knot nematode infection, but the underlying mechanism is still unclear.
    RESULTS: Expression level and genetic analyses revealed that the photoreceptor genes PHY, CRY, and PHOT have a negative impact on nematode infection. Interestingly, ELONGATED HYPOCOTYL5 (HY5), a downstream gene involved in the regulation of light signaling, is associated with photoreceptor-mediated negative regulation of root-knot nematode resistance. ChIP and yeast one-hybrid assays supported that HY5 participates in plant-to-root-knot nematode responses by directly binding to the SWEET negative regulatory factors involved in root-knot nematode resistance.
    CONCLUSIONS: This study elucidates the important role of light signaling pathways in plant resistance to nematodes, providing a new perspective for RKN resistance research.
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  • 文章类型: Journal Article
    弧菌病是水生动物常见的最严重的疾病之一,因此,在生物中形成稳定的遗传抗性性状已在水产养殖中获得最高优先级。然而,这种抗性性状发展的潜在机制大多难以捉摸。在这项研究中,经过四代人工选择,我们构建了太平洋白虾凡纳滨对虾的抗弧菌病和易感家族。微生物组测序表明,虾可以成功地发展出针对弧菌感染的定植抗性性状。该性状的特征是微生物群落结构,具有单一益生菌物种(即希瓦氏菌藻类)的特定富集,尤其是,它的形成是可遗传的,可能通过宿主表观遗传重塑来记忆。不管感染状况如何,通过完全甲基化的破坏,一组基因在抗性家族中被特异性激活。具体来说,与乳酸脱氢酶(LDH)和铁稳态相关的基因的低甲基化和高表达可能为S.藻类的定殖提供丰富的特定碳(乳酸)和离子来源,这直接导致虾中弧菌负荷的减少。乳酸盐喂养增加了虾的存活率,而LDH基因的敲除降低了对虾被弧菌病原体感染时的存活率。此外,用甲基转移酶抑制剂5-氮杂胞苷处理虾导致LDH和一些蛋白质加工基因上调,藻类的显著富集,同时减少虾中的弧菌。我们的结果表明,定植抗性可以被宿主记忆为表观遗传信息,在抗弧菌病方面发挥了关键作用。这项研究的发现将有助于疾病控制和选择具有高抗病性的对虾的优良品系。
    Vibriosis is one of the most serious diseases that commonly occurs in aquatic animals, thus, shaping a steady inherited resistance trait in organisms has received the highest priority in aquaculture. Whereas, the mechanisms underlying the development of such a resistance trait are mostly elusive. In this study, we constructed vibriosis-resistant and susceptible families of the Pacific white shrimp Litopenaeus vannamei after four generations of artificial selection. Microbiome sequencing indicated that shrimp can successfully develop a colonization resistance trait against Vibrio infections. This trait was characterized by a microbial community structure with specific enrichment of a single probiotic species (namely Shewanella algae), and notably, its formation was inheritable and might be memorized by host epigenetic remodeling. Regardless of the infection status, a group of genes was specifically activated in the resistant family through disruption of complete methylation. Specifically, hypo-methylation and hyper-expression of genes related to lactate dehydrogenase (LDH) and iron homeostasis might provide rich sources of specific carbon (lactate) and ions for the colonization of S. algae, which directly results in the reduction of Vibrio load in shrimp. Lactate feeding increased the survival of shrimp, while knockdown of LDH gene decreased the survival when shrimp was infected by Vibrio pathogens. In addition, treatment of shrimp with the methyltransferase inhibitor 5-azacytidine resulted in upregulations of LDH and some protein processing genes, significant enrichment of S. algae, and simultaneous reduction of Vibrio in shrimp. Our results suggest that the colonization resistance can be memorized as epigenetic information by the host, which has played a pivotal role in vibriosis resistance. The findings of this study will aid in disease control and the selection of superior lines of shrimp with high disease resistance.
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