单链和双链DNA结合蛋白协同作用以保存端粒DNA核心序列。

Q4 Biochemistry, Genetics and Molecular Biology

Genome Integrity Pub Date : 2011-01-14 DOI:10.1186/2041-9414-2-2

Jenny Rhodin Edsö, Cecilia Gustafsson, Marita Cohn

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引用次数: 24

摘要

背景:端粒是线性真核生物染色体末端的保护帽结构，通过屏蔽降解和染色体融合为基因组提供稳定性。端粒帽由端粒特异性蛋白质组成，这些蛋白质分别与端粒序列的单链和双链部分结合。除了染色质结构的成核外，端粒结合蛋白还参与了端粒长度的调节。然而，端粒序列在酵母菌种之间是高度分化的。在进化过程中，这种高分化率对端粒结合蛋白的序列识别提出了挑战。结果:我们发现，端粒长度负调节因子castellii Saccharomyces protein Rap1在双链端粒DNA中结合一个12-mer的最小结合位点(minimum binding site, MBS)。序列特异性依赖于与两个5个核苷酸基序的相互作用，具有6个核苷酸的中心到中心间距。分离的dna结合域与相同的MBS结合，并保留与全长Rap1蛋白相同的基序结合特性。然而，在某些核苷酸位置上，序列特异性依赖的程度存在一些偏差。有趣的是，对于全长Rap1蛋白序列特异性结合最重要的位置与3'悬垂结合蛋白Cdc13所利用的4个核苷酸中的3个重合。这些核苷酸在酵母高度分化的端粒序列中非常保守。结论:Rap1和Cdc13是两种非常不同的dna结合蛋白，具有高度独立的功能。它们通过明显不同类型的DNA结合域结构与双链和单链端粒DNA相互作用。然而，我们表明，它们依赖于重合的核苷酸位置，它们的序列特异性结合到端粒序列。因此，我们得出结论，在分子进化过程中，它们共同作用以保存端粒DNA的核心序列。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

Single- and double-stranded DNA binding proteins act in concert to conserve a telomeric DNA core sequence.

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Single- and double-stranded DNA binding proteins act in concert to conserve a telomeric DNA core sequence.

Background: Telomeres are protective cap structures at the ends of the linear eukaryotic chromosomes, which provide stability to the genome by shielding from degradation and chromosome fusions. The cap consists of telomere-specific proteins binding to the respective single- and double-stranded parts of the telomeric sequence. In addition to the nucleation of the chromatin structure the telomere-binding proteins are involved in the regulation of the telomere length. However, the telomeric sequences are highly diverged among yeast species. During the evolution this high rate of divergency presents a challenge for the sequence recognition of the telomere-binding proteins.

Results: We found that the Saccharomyces castellii protein Rap1, a negative regulator of telomere length, binds a 12-mer minimal binding site (MBS) within the double-stranded telomeric DNA. The sequence specificity is dependent on the interaction with two 5 nucleotide motifs, having a 6 nucleotide centre-to-centre spacing. The isolated DNA-binding domain binds the same MBS and retains the same motif binding characteristics as the full-length Rap1 protein. However, it shows some deviations in the degree of sequence-specific dependence in some nucleotide positions. Intriguingly, the positions of most importance for the sequence-specific binding of the full-length Rap1 protein coincide with 3 of the 4 nucleotides utilized by the 3' overhang binding protein Cdc13. These nucleotides are very well conserved within the otherwise highly divergent telomeric sequences of yeasts.

Conclusions: Rap1 and Cdc13 are two very distinct types of DNA-binding proteins with highly separate functions. They interact with the double-stranded vs. the single-stranded telomeric DNA via significantly different types of DNA-binding domain structures. However, we show that they are dependent on coinciding nucleotide positions for their sequence-specific binding to telomeric sequences. Thus, we conclude that during the molecular evolution they act together to preserve a core sequence of the telomeric DNA.

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Genome Integrity Biochemistry, Genetics and Molecular Biology-Genetics

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