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Amplification of histone genes by circular chromosome formation in Saccharomyces cerevisiae

机译:酿酒酵母中通过环状染色体形成扩增组蛋白基因

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Proper histone levels are critical for transcription, chromosome segregation, and other chromatin-mediated processes(1-7). In Saccharomyces cerevisiae, the histones H2A and H2B are encoded by two gene pairs, named HTA1-HTB1 and HTA2-HTB2 (ref. 8). Previous studies have demonstrated that when HTA2-HTB2 is deleted, HTA1-HTB1 dosage compensates at the transcriptional level(4,9). Here we show that a different mechanism of dosage compensation, at the level of gene copy number, can occur when HTA1-HTB1 is deleted. In this case, HTA2-HTB2 amplifies via creation of a new, small, circular chromosome. This duplication, which contains 39 kb of chromosome II, includes HTA2-HTB2, the histone H3-H4 locus HHT1-HHF1, a centromere and origins of replication. Formation of the new chromosome occurs by recombination between two Ty1 retrotransposon elements that flank this region. Following meiosis, recombination between these two particular Ty1 elements occurs at a greatly elevated level in hta1-htb1 Delta mutants, suggesting that a decreased level of histones H2A and H2B specifically stimulates this amplification of histone genes. Our results demonstrate another mechanism by which histone gene dosage is controlled to maintain genomic integrity.
机译:适当的组蛋白水平对于转录,染色体分离和其他染色质介导的过程至关重要(1-7)。在酿酒酵母中,组蛋白H2A和H2B由两个基因对编码,分别称为HTA1-HTB1和HTA2-HTB2(参考文献8)。以前的研究表明,删除HTA2-HTB2后,HTA1-HTB1剂量会在转录水平上补偿(4,9)。在这里我们表明,删除HTA1-HTB1时,可能在基因拷贝数的水平上发生不同的剂量补偿机制。在这种情况下,HTA2-HTB2通过创建新的小圆形染色体进行扩增。包含39 kb II号染色体的该重复序列包括HTA2-HTB2,组蛋白H3-H4基因座HHT1-HHF1,着丝粒和复制起点。新染色体的形成是通过位于该区域两侧的两个Ty1反转录转座子元件之间的重组而发生的。减数分裂后,在hta1-htb1 Delta突变体中,这两个特定的Ty1元件之间的重组以大大升高的水平发生,这表明组蛋白H2A和H2B的水平降低会特异性地刺激组蛋白基因的这种扩增。我们的结果证明了控制组蛋白基因剂量以维持基因组完整性的另一种机制。

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