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细胞中凋亡诱导因子易位的实时空间和时间分析

Real-Time Spatial and Temporal Analysis of the Translocation of the Apoptosis-Inducing Factor in Cells.

作者信息

Park Sang-Hyun, Kim Sanggil, Lee Hyun Soo, Shin Injae

机构信息

Department of Chemistry, Yonsei University, Seoul 03722, Republic of Korea.

Department of Chemistry, Sogang University, Seoul 04107, Republic of Korea.

出版信息

ACS Chem Biol. 2021 Nov 19;16(11):2462-2471. doi: 10.1021/acschembio.1c00565. Epub 2021 Oct 25.

DOI:10.1021/acschembio.1c00565
PMID:34694772
Abstract

Translocation of the apoptosis-inducing factor (AIF) from the mitochondria to the nucleus is crucial for AIF-mediated apoptosis. However, the lack of methods for real-time spatial and temporal analysis of translocation of functional AIF is a large hurdle to gain a detailed understanding of this process. In this study, a genetic code expansion technique was developed to overcome this hurdle. Specifically, this technique was utilized to construct ANAP-AIF containing a small fluorescent amino acid (ANAP) at a specific site in cells. Additionally, we developed efficient fluorescence resonance energy-transfer systems consisting of ANAP-AIF and either yellow fluorescent protein (YFP)-fused cyclophilin A (CypA) or Hsp70, respective positive and negative regulators for AIF translocation to the nucleus. We found that apoptosis inducers, including apoptozole, 2-phenylethynesulfonamide (PES), myricetin, Bam7, reactivating p53 and inducing tumor apoptosis (RITA), brefeldin A, and carbonyl cyanide--trifluoromethoxyphenylhydrazone (FCCP) promote translocation of mitochondrial AIF to the cytosol after 4 h incubation, reaching a maximum after 6-7 h. However, these substances did not enhance AIF translocation to the nucleus through the interaction of AIF with Hsp70 in the cytosol. On the other hand, treatment with apoptosis inducers, such as paclitaxel, silibinin, doxorubicin, actinomycin D, and camptothecin caused AIF translocation to the nucleus after 4 h incubation through AIF binding to CypA, reaching saturation after 6-7 h. It was also found that Hsp70 and CypA regulate AIF translocation in a mutually exclusive manner because they do not interact with AIF simultaneously in cells undergoing apoptosis. The results demonstrate clearly that ANAP-incorporated proteins are powerful to obtain a more in-depth understanding of protein translocation.

摘要

凋亡诱导因子(AIF)从线粒体易位至细胞核对于AIF介导的细胞凋亡至关重要。然而,缺乏对功能性AIF易位进行实时空间和时间分析的方法是深入了解这一过程的一大障碍。在本研究中,开发了一种遗传密码扩展技术来克服这一障碍。具体而言,该技术用于构建在细胞特定位点含有小荧光氨基酸(ANAP)的ANAP-AIF。此外,我们开发了高效的荧光共振能量转移系统,该系统由ANAP-AIF与黄色荧光蛋白(YFP)融合的亲环素A(CypA)或热休克蛋白70(Hsp70)组成,它们分别是AIF易位至细胞核的正向和负向调节因子。我们发现,包括凋亡诱导剂、杨梅酮、巴佛洛霉素A1、重新激活p53并诱导肿瘤凋亡(RITA)、布雷菲德菌素A和羰基氰化物-三氟甲氧基苯腙(FCCP)在内的凋亡诱导剂在孵育4小时后促进线粒体AIF易位至细胞质,在6-7小时后达到最大值。然而,这些物质并未通过AIF与细胞质中Hsp70的相互作用增强AIF易位至细胞核。另一方面,用紫杉醇、水飞蓟宾、阿霉素、放线菌素D和喜树碱等凋亡诱导剂处理后,AIF在孵育4小时后通过与CypA结合易位至细胞核,在6-7小时后达到饱和。还发现Hsp70和CypA以互斥方式调节AIF易位,因为它们在凋亡细胞中不会同时与AIF相互作用。结果清楚地表明,掺入ANAP的蛋白质对于更深入了解蛋白质易位具有强大作用。

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