Simbulan-Rosenthal C M, Rosenthal D S, Iyer S, Boulares H, Smulson M E
Department of Biochemistry and Molecular Biology, Georgetown University School of Medicine, Washington, DC 20007, USA.
Mol Cell Biochem. 1999 Mar;193(1-2):137-48.
We have focused on the roles of PARP and poly(ADP-ribosyl)ation early in apoptosis, as well as during the early stages of differentiation-linked DNA replication. In both nuclear processes, a transient burst of PAR synthesis and PARP expression occurs early, prior to internucleosomal DNA cleavage before commitment to apoptosis as well as at the round of DNA replication prior to the onset of terminal differentiation. In intact human osteosarcoma cells undergoing spontaneous apoptosis, both PARP and PAR decreased after this early peak, concomitant with the inactivation and cleavage of PARP by caspase-3 and the onset of substantial DNA and nuclear fragmentation. Whereas 3T3-L1, osteosarcoma cells, and immortalized PARP +/+ fibroblasts exhibited this early burst of PAR synthesis during Fas-mediated apoptosis, neither PARP-depleted 3T3-L1 PARP-antisense cells nor PARP -/- fibroblasts showed this response. Consequently, whereas control cells progressed into apoptosis, as indicated by induction of caspase-3-like PARP-cleavage activity, PARP-antisense cells and PARP -/- fibroblasts did not, indicating a requirement for PARP and poly(ADP-ribosyl)ation of nuclear proteins at an early reversible stage of apoptosis. In parallel experiments, a transient increase in PARP expression and activity were also noted in 3T3-L1 preadipocytes 24 h after induction of differentiation, a stage at which approximately 95% of the cells were in S-phase, but not in PARP-depleted antisense cells, which were consequently unable to complete the round of DNA replication required for differentiation. PARP, a component of the multiprotein DNA replication complex (MRC) that catalyzes viral DNA replication in vitro, poly(ADP-ribosyl)ates 15 of approximately 40 MRC proteins, including DNA pol alpha, DNA topo I, and PCNA. Depletion of endogenous PARP by antisense RNA expression in 3T3-L1 cells results in MRCs devoid of any DNA pol alpha and DNA pol delta activities. Surprisingly, there was no new expression of PCNA and DNA pol alpha, as well as the transcription factor E2F-1 in PARP-antisense cells during entry into S-phase, suggesting that PARP may play a role in the expression of these proteins, perhaps by interacting with a site in the promoters for these genes.
我们重点研究了聚(ADP - 核糖)聚合酶(PARP)和聚(ADP - 核糖)基化在细胞凋亡早期以及与分化相关的DNA复制早期阶段所起的作用。在这两个核过程中,在细胞凋亡发生前核小体间DNA裂解之前以及终末分化开始前的一轮DNA复制期间,早期都会出现PAR合成和PARP表达的短暂爆发。在经历自发凋亡的完整人骨肉瘤细胞中,PARP和PAR在这个早期峰值后均下降,同时PARP被半胱天冬酶 - 3失活并裂解,大量DNA和核碎片化开始。而3T3 - L1细胞、骨肉瘤细胞和永生化PARP +/+ 成纤维细胞在Fas介导的细胞凋亡过程中表现出这种PAR合成的早期爆发,PARP缺失的3T3 - L1 PARP反义细胞和PARP -/- 成纤维细胞均未表现出这种反应。因此,虽然对照细胞如通过诱导类似半胱天冬酶 - 3的PARP裂解活性所示进入凋亡,但PARP反义细胞和PARP -/- 成纤维细胞则没有,这表明在细胞凋亡的早期可逆阶段需要PARP和核蛋白的聚(ADP - 核糖)基化。在平行实验中,在诱导分化24小时后的3T3 - L1前脂肪细胞中也观察到PARP表达和活性的短暂增加,此时约95%的细胞处于S期,但在PARP缺失的反义细胞中未观察到,因此这些细胞无法完成分化所需的一轮DNA复制。PARP是多蛋白DNA复制复合物(MRC)的一个组成部分,在体外催化病毒DNA复制,它对约40种MRC蛋白中的15种进行聚(ADP - 核糖)基化,包括DNA聚合酶α、DNA拓扑异构酶I和增殖细胞核抗原(PCNA)。通过在3T3 - L1细胞中反义RNA表达耗尽内源性PARP会导致MRC缺乏任何DNA聚合酶α和DNA聚合酶δ活性。令人惊讶的是,在进入S期期间,PARP反义细胞中PCNA、DNA聚合酶α以及转录因子E2F - 1均没有新的表达,这表明PARP可能在这些蛋白质的表达中起作用,也许是通过与这些基因启动子中的一个位点相互作用来实现的。
Zotero 插件