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Silenced rRNA genes are activated and substitute for partially eliminated active homeologs in the recently formed allotetraploid Tragopogon mirus (Asteraceae)

机译:沉默的rRNA基因被激活并替代了最近形成的异源四倍体Tragopogon mirus(Asteraceae)中部分消除的活性同源物

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摘要

To study the relationship between uniparental rDNA (encoding 18S, 5.8S and 26S ribosomal RNA) silencing (nucleolar dominance) and rRNA gene dosage, we studied a recently emerged (within the last 80 years) allotetraploid Tragopogon mirus (2n=24), formed from the diploid progenitors T. dubius (2n=12, D-genome donor) and T. porrifolius (2n=12, P-genome donor). Here, we used molecular, cytogenetic and genomic approaches to analyse rRNA gene activity in two sibling T. mirus plants (33A and 33B) with widely different rRNA gene dosages. Plant 33B had ~400 rRNA genes at the D-genome locus, which is typical for T. mirus, accounting for ~25% of total rDNA. We observed characteristic expression dominance of T. dubius-origin genes in all organs. Its sister plant 33A harboured a homozygous macrodeletion that reduced the number of T. dubius-origin genes to about 70 copies (~4% of total rDNA). It showed biparental rDNA expression in root, flower and callus, but not in leaf where D-genome rDNA dominance was maintained. There was upregulation of minor rDNA variants in some tissues. The RNA polymerase I promoters of reactivated T. porrifolius-origin rRNA genes showed reduced DNA methylation, mainly at symmetrical CG and CHG nucleotide motifs. We hypothesise that active, decondensed rDNA units are most likely to be deleted via recombination. The silenced homeologs could be used as a ‘first reserve' to ameliorate mutational damage and contribute to evolutionary success of polyploids. Deletion and reactivation cycles may lead to bidirectional homogenisation of rRNA arrays in the long term.
机译:为了研究单亲rDNA(编码18S,5.8S和26S核糖体RNA)沉默(核仁显性)与rRNA基因剂量之间的关系,我们研究了最近出现的(最近80年内)同种四倍体Tragopogon mirus(2n = 24),来自二倍体祖细胞T. dubius(2n = 12,D基因组供体)和porrifolius(2n = 12,P基因组供体)。在这里,我们使用分子,细胞遗传学和基因组学方法来分析两种具有不同rRNA基因剂量的同胞三叶草植物(33A和33B)中的rRNA基因活性。植物33B在D基因组位点具有〜400个rRNA基因,这是T虫的典型特征,约占总rDNA的25%。我们观察到在所有器官中T. dubius起源基因的特征性表达优势。它的姊妹植物33A具有纯合的大缺失,可将杜比螺旋藻起源基因的数目减少到约70个拷贝(占总rDNA的4%)。它显示了根,花和愈伤组织中双亲rDNA的表达,但在维持D基因组rDNA优势的叶中却没有。在某些组织中存在轻微的rDNA变异体上调。重新激活的T. porrifolius起源的rRNA基因的RNA聚合酶I启动子显示减少的DNA甲基化,主要是在对称的CG和CHG核苷酸基序处。我们假设活性的,缩合的rDNA单元最有可能通过重组删除。沉默的同源物可以用作减轻突变损伤的“第一储备”,并有助于多倍体的进化成功。从长远来看,删除和重新激活周期可能导致rRNA阵列双向均质化。

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