Institute of Experimental Pharmacology and Toxicology, University Medical Center Hamburg-Eppendorf, Hamburg, Germany.
DZHK (German Centre for Cardiovascular Research), partner site Hamburg/Kiel/Lübeck, Hamburg, Germany.
Autophagy. 2021 Oct;17(10):3124-3139. doi: 10.1080/15548627.2020.1856493. Epub 2020 Dec 27.
The ubiquitin-proteasome system (UPS) and autophagy-lysosomal pathway (ALP) are two major protein degradation pathways in eukaryotic cells. Initially considered as two independent pathways, there is emerging evidence that they can work in concert. As alterations of UPS and ALP function can contribute to neurodegenerative disorders, cancer and cardiac disease, there is great interest in finding targets that modulate these catabolic processes. We undertook an unbiased, total genome high-throughput screen to identify novel effectors that regulate both the UPS and ALP. We generated a stable HEK293 cell line expressing a UPS reporter (Ub-mCherry) and an ALP reporter (GFP-LC3) and screened for genes for which knockdown increased both Ub-mCherry intensity and GFP-LC3 puncta. With stringent selection, we isolated 80 candidates, including the transcription factor ZNF418 (ZFP418 in rodents). After screen validation with overexpression in HEK293 cells, we evaluated knockdown and overexpression in neonatal rat ventricular myocytes (NRVMs). Endogenous and overexpressed ZFP418 were localized in the nucleus. Subsequent experiments showed that ZFP418 negatively regulates UPS and positively regulates ALP activity in NRVMs. RNA-seq from knockdown revealed altered gene expression of numerous ubiquitinating and deubiquitinating enzymes, decreased expression of autophagy activators and initiators and increased expression of autophagy inhibitors. We found that ZPF418 activated the promoters of and , which are involved in autophagy. RNA-seq from knockdown revealed accumulation of several genes involved in cardiac development and/or hypertrophy. In conclusion, our study provides evidence that ZNF418 activates the ALP, inhibits the UPS and regulates genes associated with cardiomyocyte structure/function. ACTN2, actinin alpha 2; ALP, autophagy-lysosomal pathway; COPB1, COPI coat complex subunit beta 1; DAPK2, death associated protein kinase 2; FYCO1, FYVE and coiled-coil domain autophagy adaptor 1; HEK293, human embryonic kidney cells 293; HTS, high-throughput screen; LC3, microtubule associated protein 1 light chain 3; NRVMs, neonatal rat ventricular myocytes; RNA-seq, RNA sequencing; RPS6, ribosomal protein S6; TNNI3, troponin I, cardiac 3; UPS, ubiquitin-proteasome system; shRNA, short hairpin RNA; SQSTM1/p62, sequestosome 1; VPS28, VPS28 subunit of ESCRT-I; ZNF418/ZFP418, zinc finger protein 418.
泛素-蛋白酶体系统 (UPS) 和自噬溶酶体途径 (ALP) 是真核细胞中两种主要的蛋白质降解途径。最初被认为是两种独立的途径,有证据表明它们可以协同工作。由于 UPS 和 ALP 功能的改变可能导致神经退行性疾病、癌症和心脏病,因此人们对寻找调节这些分解代谢过程的靶点非常感兴趣。我们进行了一项无偏见的全基因组高通量筛选,以鉴定调节 UPS 和 ALP 的新效应物。我们生成了一种稳定的表达 UPS 报告基因 (Ub-mCherry) 和 ALP 报告基因 (GFP-LC3) 的 HEK293 细胞系,并筛选出敲低后能同时增加 Ub-mCherry 强度和 GFP-LC3 斑点的基因。经过严格的选择,我们分离出 80 个候选基因,包括转录因子 ZNF418(啮齿动物中的 ZFP418)。在 HEK293 细胞中过表达进行筛选验证后,我们评估了在新生大鼠心室肌细胞 (NRVMs) 中的 敲低和过表达。内源性和过表达的 ZFP418 定位于细胞核内。随后的实验表明,ZFP418 负调节 UPS 并正调节 NRVMs 中的 ALP 活性。从 敲低的 RNA-seq 显示出许多泛素化和去泛素化酶的基因表达改变,自噬激活剂和起始子的表达减少,自噬抑制剂的表达增加。我们发现 ZPF418 激活了与自噬相关的 和 的启动子。从 敲低的 RNA-seq 显示出与心脏发育和/或肥大相关的几个基因的积累。总之,我们的研究提供了证据,证明 ZNF418 激活 ALP、抑制 UPS 并调节与心肌细胞结构/功能相关的基因。ACTN2,肌动蛋白 alpha 2;ALP,自噬溶酶体途径;COPB1,COP 衣壳复合物亚基 beta 1;DAPK2,死亡相关蛋白激酶 2;FYCO1,FYVE 和卷曲螺旋结构域自噬衔接子 1;HEK293,人胚肾细胞 293;HTS,高通量筛选;LC3,微管相关蛋白 1 轻链 3;NRVMs,新生大鼠心室肌细胞;RNA-seq,RNA 测序;RPS6,核糖体蛋白 S6;TNNI3,肌钙蛋白 I,心脏 3;UPS,泛素-蛋白酶体系统;shRNA,短发夹 RNA;SQSTM1/p62,自噬体 1;VPS28,VPS28 亚基 ESCRT-I;ZNF418/ZFP418,锌指蛋白 418。
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