Erchen Zhang, Lei Peng, Kejia Yuan, Zexian Ding, Qi Yi
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引用次数: 0
Abstract
Background: α thalassemia/mental retardation syndrome X-linked (ATRX) serves as a part of the sucrose nonfermenting 2 (SNF2) chromatin-remodeling complex. In interphase, ATRX localizes to pericentromeric heterochromatin, contributing to DNA double-strand break repair, DNA replication, and telomere maintenance. During mitosis, most ATRX proteins are removed from chromosomal arms, leaving a pool near the centromere region in mammalian cells, which is critical for accurate chromosome congression and sister chromatid cohesion protection. However, the function and localization mechanisms of ATRX at mitotic centromeres remain largely unresolved.
Methods: The clustered regularly interspaced short palindromic repeats with CRISPR-associated protein 9 (CRISPR-Cas9) system and overexpression approaches were employed alongside immunofluorescence to investigate the mechanism of ATRX localization at the centromere. To study the binding mechanism between ATRX and heterochromatin protein 1 (HP1), both full-length and truncated mutants of hemagglutinin (HA)-ATRX were generated for co-immunoprecipitation and glutathione S-transferase (GST)-pull assays. Wild-type ATRX and HP1 binding-deficient mutants were created to investigate the role of ATRX binding to HP1 during mitosis, with the Z-Leu-Leu-Leu-al (MG132) maintenance assay, cohesion function assay, and kinetochore distance measurement.
Results and conclusions: Our research demonstrated that HP1α, HP1β, and HP1γ facilitate the positioning of ATRX within the mitotic centromere area through their interaction with the first two [P/L]-X-V-X-[M/L/V] (PxVxL)motifs at the N-terminus of ATRX. ATRX deficiency causes aberrant mitosis and decreased centromeric cohesion. Furthermore, reducing Wapl activity can bypass the need for ATRX to protect centromeric cohesion. These results provide insights into the mechanism of ATRX's centromeric localization and its critical function in preserving centromeric cohesion by reducing Wapl activity in human cells.
背景:α地中海贫血/智力低下综合征x连锁(ATRX)是蔗糖非发酵2 (SNF2)染色质重塑复合体的一部分。在间期,ATRX定位于中心周围异染色质,参与DNA双链断裂修复、DNA复制和端粒维持。在有丝分裂过程中,大多数ATRX蛋白从染色体臂上被移除,在哺乳动物细胞中在着丝粒区域附近留下一个池,这对于染色体准确聚集和姐妹染色单体内聚保护至关重要。然而,ATRX在有丝分裂着丝粒中的功能和定位机制在很大程度上仍未得到解决。方法:采用CRISPR-Cas9 (CRISPR-associated protein 9, CRISPR-Cas9)系统和过表达方法,结合免疫荧光技术研究ATRX在着丝粒定位的机制。为了研究ATRX与异染色质蛋白1 (HP1)的结合机制,我们制备了血凝素(HA)-ATRX的全长突变体和截短突变体,用于共免疫沉淀和谷胱甘肽s -转移酶(GST)拉取试验。通过z - leu - leu - leu - leu -al (MG132)维持实验、内聚功能实验和着丝点距离测量,构建野生型ATRX和HP1结合缺陷突变体,研究ATRX在有丝分裂过程中与HP1结合的作用。结果和结论:我们的研究表明,HP1α、HP1β和HP1γ通过与ATRX n端前两个[P/L]- x -V- x -[M/L/V] (PxVxL)基序相互作用,促进ATRX在有丝分裂着丝粒区域内的定位。ATRX缺乏导致有丝分裂异常和着丝粒内聚减少。此外,减少Wapl活性可以绕过ATRX保护着心性内聚的需要。这些结果为ATRX的着丝粒定位机制及其通过降低Wapl活性保持着丝粒内聚的关键功能提供了新的见解。
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