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A Human Artificial Chromosome Recapitulates the Metabolism of Native Telomeres in Mammalian Cells

机译:人类人工染色体概括了哺乳动物细胞中天然端粒的代谢。

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摘要

Telomeric and subtelomeric regions of human chromosomes largely consist of highly repetitive and redundant DNA sequences, resulting in a paucity of unique DNA sequences specific to individual telomeres. Accordingly, it is difficult to analyze telomere metabolism on a single-telomere basis. To circumvent this problem, we have exploited a human artificial chromosome (HAC#21) derived from human chromosome 21 (hChr21). HAC#21 was generated through truncation of the long arm of native hChr21 by the targeted telomere seeding technique. The newly established telomere of HAC#21 lacks canonical subtelomere structures but possesses unique sequences derived from the target vector backbone and the internal region of hChr21 used for telomere targeting, which enabled us to molecularly characterize the single HAC telomere. We established HeLa and NIH-3T3 sub-lines containing a single copy of HAC#21, where it was robustly maintained. The seeded telomere is associated with telomeric proteins over a length similar to that reported in native telomeres, and is faithfully replicated in mid-S phase in HeLa cells. We found that the seeded telomere on HAC#21 is transcribed from the newly juxtaposed site. The transcript, HAC-telRNA, shares several features with TERRA (telomeric repeat-containing RNA): it is a short-lived RNA polymerase II transcript, rarely contains a poly(A) tail, and associates with chromatin. Interestingly, HAC-telRNA undergoes splicing. These results suggest that transcription into TERRA is locally influenced by the subtelomeric context. Taken together, we have established human and mouse cell lines that will be useful for analyzing the behavior of a uniquely identifiable, functional telomere.
机译:人类染色体的端粒和亚端粒区域主要由高度重复和冗余的DNA序列组成,导致个别端粒特有的独特DNA序列很少。因此,难以在单端粒的基础上分析端粒的代谢。为了解决这个问题,我们利用了源自人类21号染色体(hChr21)的人类人工染色体(HAC#21)。 HAC#21是通过靶向端粒接种技术将天然hChr21的长臂截短而产生的。新建立的HAC#21端粒缺乏规范的亚端粒结构,但具有源自靶载体主链和用于端粒靶向的hChr21内部区域的独特序列,这使我们能够分子表征单个HAC端粒。我们建立了包含单一HAC#21副本的HeLa和NIH-3T3子线,并在其中进行了维护。播种的端粒与端粒蛋白缔合的长度与天然端粒中报道的端粒相似,并在HeLa细胞的S期中期忠实复制。我们发现,HAC#21上的种子端粒是从新并置的位点转录而来的。转录本HAC-telRNA与TERRA(含端粒重复序列的RNA)具有几个特点:它是一种短暂的RNA聚合酶II转录本,很少包含poly(A)尾巴,并与染色质缔合。有趣的是,HAC-telRNA进行了剪接。这些结果表明,向TERRA的转录受亚端粒环境的局部影响。综上所述,我们已经建立了人类和小鼠细胞系,它们将用于分析独特可识别的功能性端粒的行为。

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