double haploid population

  • 文章类型: Journal Article
    由土壤传播的真菌枯萎病引起的水稻叶鞘枯萎病(SB)每年导致10-30%的全球产量损失,在严重爆发时可达到50%。许多抗病基因和受体样激酶(RLK)在宿主植物早期被募集以响应病原体。壁相关受体激酶(WAKs),受体样激酶亚家族,已被证明在真菌防御中起作用。水稻基因WAK91(OsWAK91),共同位于9号染色体上主要的SB抗性QTL区域,被我们确定为防御水稻纹枯病的候选者。在易感水稻品种Cocodrie(CCDR)和抗性品系MCR010277(MCR)中鉴定出WAK91基因中的SNP突变T/C。抗性等位基因C的结果是终止密码子丢失,导致具有额外62个氨基酸的开放阅读框,携带更长的蛋白激酶结构域和额外的磷酸化位点。我们对父母CCDR和MCR以及双单倍体SB群体的前20名个体的基因型和表型分析与SNP强烈相关。易感等位基因T存在于粳稻亚种以及大多数热带和温带粳稻系中。具有粳稻背景的多个美国商业水稻品种携带易感等位基因,并且以SB易感性而闻名。这一发现开启了将抗性等位基因引入高产商业品种以减少纹枯病引起的产量损失的可能性。
    Leaf sheath blight disease (SB) of rice caused by the soil-borne fungus Rhizoctonia solani results in 10-30% global yield loss annually and can reach 50% under severe outbreaks. Many disease resistance genes and receptor-like kinases (RLKs) are recruited early on by the host plant to respond to pathogens. Wall-associated receptor kinases (WAKs), a subfamily of receptor-like kinases, have been shown to play a role in fungal defense. The rice gene WAK91 (OsWAK91), co-located in the major SB resistance QTL region on chromosome 9, was identified by us as a candidate in defense against rice sheath blight. An SNP mutation T/C in the WAK91 gene was identified in the susceptible rice variety Cocodrie (CCDR) and the resistant line MCR010277 (MCR). The consequence of the resistant allele C is a stop codon loss, resulting in an open reading frame with extra 62 amino acid carrying a longer protein kinase domain and additional phosphorylation sites. Our genotype and phenotype analysis of the parents CCDR and MCR and the top 20 individuals of the double haploid SB population strongly correlate with the SNP. The susceptible allele T is present in the japonica subspecies and most tropical and temperate japonica lines. Multiple US commercial rice varieties with a japonica background carry the susceptible allele and are known for SB susceptibility. This discovery opens the possibility of introducing resistance alleles into high-yielding commercial varieties to reduce yield losses incurred by the sheath blight disease.
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  • 文章类型: Journal Article
    西利克长度(SL)是重要的产量性状,与每个西利克种子和种子重量呈正相关。在本研究中,两个双单倍体(DH)种群,从杂交中双11×R11(ZR)和R1×R2(RR)建立,包含280和95条DH线,分别,用于绘制SL的数量性状位点(QTL)。构建了ZR种群的高密度遗传图谱,包括19个连锁群上的14,658个bin,图长为2,198.85cM,平均标记距离为0.15cM。通过使用锚定在19条染色体上的2,046个定位标记,具有2,217-cM的图谱长度和1.08cM的平均标记距离,构建了RR种群的遗传连锁图。从ZR和RR种群中鉴定出A09上的主要QTLqSL_ZR_A09和qSL_RR_A09b,分别。两种QTL均可在四种环境中稳定检测。QTLqSL_RR_A09b和qSL_ZR_A09位于68.5-70.8cM和91.33-91.94cM区间,RR和ZR种群的R2值为14.99-39.07%和15.00-20.36%,分别。基于拟南芥中qSL_ZR_A09侧翼的单核苷酸多态性(SNP)标记的物理位置和基因注释,鉴定了26个在亲本之间具有SNP/Indel变异的基因,并且选择两个基因(BnaA09g41180D和BnaA09g41380D)作为候选基因。表达分析进一步显示BnaA09g41180D,编码拟南芥fasciclin样阿拉伯半乳聚糖蛋白(FLA3)的同源物,作为qSL_ZR_A09最有希望的候选基因。QTL鉴定和候选基因分析将为控制甘蓝型油菜SL的基因组区域以及QTL基础的候选基因提供新的见解。
    Silique length (SL) is an important yield trait and positively correlates with seeds per silique and seed weight. In the present study, two double haploid (DH) populations, established from crosses Zhongshuang11 × R11 (ZR) and R1 × R2 (RR), containing 280 and 95 DH lines, respectively, were used to map quantitative trait loci (QTL) for SL. A high-dense genetic map from ZR population was constructed comprising 14,658 bins on 19 linkage groups, with map length of 2,198.85 cM and an average marker distance of 0.15 cM. Genetic linkage map from RR population was constructed by using 2,046 mapped markers anchored to 19 chromosomes with 2,217-cM map length and an average marker distance of 1.08 cM. Major QTL qSL_ZR_A09 and qSL_RR_A09b on A09 were identified from ZR and RR populations, respectively. Both QTL could be stably detected in four environments. QTL qSL_RR_A09b and qSL_ZR_A09 were located on 68.5-70.8 cM and 91.33-91.94 cM interval with R2 values of 14.99-39.07% and 15.00-20.36% in RR and ZR populations, respectively. Based on the physical positions of single nucleotide polymorphism (SNP) markers flanking qSL_ZR_A09 and gene annotation in Arabidopsis, 26 genes were identified with SNP/Indel variation between parents and two genes (BnaA09g41180D and BnaA09g41380D) were selected as the candidate genes. Expression analysis further revealed BnaA09g41180D, encoding homologs of Arabidopsis fasciclin-like arabinogalactan proteins (FLA3), as the most promising candidate gene for qSL_ZR_A09. The QTL identification and candidate gene analysis will provide new insight into the genomic regions controlling SL in Brassica napus as well as candidate genes underlying the QTL.
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