SIX transcription factors are necessary for the activation of DUX4 expression in facioscapulohumeral muscular dystrophy.

IF 5.3 2区医学 Q2 CELL BIOLOGY

Skeletal Muscle Pub Date : 2024-12-03 DOI:10.1186/s13395-024-00361-3

Amelia Fox, Jonathan Oliva, Rajanikanth Vangipurapu, Francis M Sverdrup

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引用次数: 0

Abstract

Background: Facioscapulohumeral muscular dystrophy (FSHD) is a common and progressive muscle wasting disease that is characterized by muscle weakness often first noticed in the face, the shoulder girdle and upper arms before progressing to the lower limb muscles. FSHD is caused by the misexpression of the Double Homeobox 4 (DUX4) transcription factor in skeletal muscle. While epigenetic derepression of D4Z4 macrosatellite repeats underlies DUX4 misexpression, our understanding of the complex transcriptional activation of DUX4 is incomplete.

Methods: To identify potential DUX4-regulatory factors, we used small interfering RNAs (siRNAs) to knockdown SIX family transcription factors (SIX1, 2, 4, 5) in patient-derived FSHD1 and FSHD2 myoblasts that were differentiated to form multinucleated myotubes. Quantitative real-time polymerase chain reaction was used to measure changes in DUX4 mRNA, DUX4 target gene expression and myogenic markers. Staining for SIX1 and SIX2 with specific antibodies was performed in FSHD myoblasts and myotubes. To assess reciprocal effects of DUX4 on SIX1, 2, and 4 expression, we utilized a doxycycline-inducible DUX4 myoblast cell line.

Result: We show that SIX1, 2 and 4 transcription factors, regulators of embryonic development, muscle differentiation, regeneration and homeostasis, are necessary for myogenic differentiation-dependent DUX4 expression in FSHD muscle cells. Using siRNA, we demonstrate SIX1, SIX2, and SIX4 to be critical factors involved in the induction of DUX4 transcription in differentiating FSHD myotubes in vitro. siRNA dual knockdown of SIX1 and SIX2 resulted in a ~ 98% decrease of DUX4 and DUX4 target genes, suggesting that SIX1 and SIX2 are the most critical in promoting DUX4 expression. Importantly, we show that DUX4 downregulates SIX RNA levels, suggesting negative feedback regulation.

Conclusions: In this study, we identified a family of developmental regulators that promote aberrant DUX4 expression in FSHD1 and FSHD2 differentiating muscle cells. Our findings highlight the critical involvement of SIX transcription factors (SIX1, 2, 4) in the pathogenesis of FSHD by serving as necessary factors that function in the promotion of DUX4 expression following epigenetic derepression of the D4Z4 repeats.

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6个转录因子是激活DUX4在面肩肱肌营养不良症中的表达所必需的。

背景：面肩肱骨肌营养不良症（FSHD）是一种常见的进行性肌肉萎缩疾病，其特征是肌肉无力，通常首先出现在面部、肩带和上臂，然后进展到下肢肌肉。FSHD是由骨骼肌双同源盒4 （DUX4）转录因子的错误表达引起的。虽然D4Z4大卫星重复序列的表观遗传抑制是DUX4错误表达的基础，但我们对DUX4复杂转录激活的理解尚不完整。方法：为了鉴定潜在的dux4调节因子，我们在分化成多核肌管的患者源性FSHD1和FSHD2肌母细胞中，使用小干扰rna （sirna）敲低SIX家族转录因子（SIX1, 2,4,5）。采用实时定量聚合酶链反应测定DUX4 mRNA、DUX4靶基因表达及肌生成标志物的变化。在FSHD成肌细胞和肌管中对SIX1和SIX2进行特异性抗体染色。为了评估DUX4对SIX1、six2和six4表达的相互作用，我们使用了强力霉素诱导的DUX4成肌细胞系。结果：我们发现SIX1, 2和4转录因子是胚胎发育，肌肉分化，再生和稳态的调节因子，是肌源性分化依赖的DUX4在FSHD肌肉细胞中的表达所必需的。利用siRNA，我们证明SIX1、SIX2和SIX4是诱导体外FSHD肌管分化DUX4转录的关键因子。siRNA双敲低SIX1和SIX2导致DUX4和DUX4靶基因减少98%，表明SIX1和SIX2在促进DUX4表达中最为关键。重要的是，我们发现DUX4下调了SIX RNA水平，提示负反馈调控。结论：在这项研究中，我们发现了一个促进FSHD1和FSHD2分化肌肉细胞中DUX4异常表达的发育调节因子家族。我们的研究结果强调了SIX转录因子（SIX1, 2,4）在FSHD发病机制中的关键作用，它们是在D4Z4重复序列表观遗传降低后促进DUX4表达的必要因子。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Skeletal Muscle CELL BIOLOGY-

CiteScore

9.10

自引率

0.00%

发文量

审稿时长

12 weeks

期刊介绍： The only open access journal in its field, Skeletal Muscle publishes novel, cutting-edge research and technological advancements that investigate the molecular mechanisms underlying the biology of skeletal muscle. Reflecting the breadth of research in this area, the journal welcomes manuscripts about the development, metabolism, the regulation of mass and function, aging, degeneration, dystrophy and regeneration of skeletal muscle, with an emphasis on understanding adult skeletal muscle, its maintenance, and its interactions with non-muscle cell types and regulatory modulators. Main areas of interest include: -differentiation of skeletal muscle- atrophy and hypertrophy of skeletal muscle- aging of skeletal muscle- regeneration and degeneration of skeletal muscle- biology of satellite and satellite-like cells- dystrophic degeneration of skeletal muscle- energy and glucose homeostasis in skeletal muscle- non-dystrophic genetic diseases of skeletal muscle, such as Spinal Muscular Atrophy and myopathies- maintenance of neuromuscular junctions- roles of ryanodine receptors and calcium signaling in skeletal muscle- roles of nuclear receptors in skeletal muscle- roles of GPCRs and GPCR signaling in skeletal muscle- other relevant aspects of skeletal muscle biology. In addition, articles on translational clinical studies that address molecular and cellular mechanisms of skeletal muscle will be published. Case reports are also encouraged for submission. Skeletal Muscle reflects the breadth of research on skeletal muscle and bridges gaps between diverse areas of science for example cardiac cell biology and neurobiology, which share common features with respect to cell differentiation, excitatory membranes, cell-cell communication, and maintenance. Suitable articles are model and mechanism-driven, and apply statistical principles where appropriate; purely descriptive studies are of lesser interest.