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top1beta基因表达降低诱导胡萝卜培养细胞程序性细胞死亡并改变抗坏血酸代谢。

Reduced expression of top1beta gene induces programmed cell death and alters ascorbate metabolism in Daucus carota cultured cells.

作者信息

Locato Vittoria, Balestrazzi Alma, De Gara Laura, Carbonera Daniela

机构信息

Department of Plant Biology and Pathology, University of Bari, Via Orabona 4, I-70125 Bari, Italy.

出版信息

J Exp Bot. 2006;57(8):1667-76. doi: 10.1093/jxb/erj194. Epub 2006 May 22.

DOI:10.1093/jxb/erj194
PMID:16717060
Abstract

Topoisomerase I (topo I) is a nuclear enzyme which plays a fundamental role in several pathways involving changes in DNA topology. The topo I-mediated reaction is accomplished by the transient covalent binding of the enzyme to DNA (topo I-DNA complex). Stabilization of the topo I-DNA complex, leading to irreversible double-strand breaks, has been reported to occur in animal cells under oxidative stress conditions and during apoptosis. In order to study the existence of a putative link between the topo I-mediated DNA damage and ascorbate (ASC) metabolism, also involved in the responses against oxidative stress and in the apoptotic process in plants, Daucus carota cells showing reduced expression of the top1beta gene encoding the topo Ibeta isoform were produced, using an antisense RNA strategy. Two independent transgenic lines (AT1-beta/22 and beta/36), characterized by a slow growth phenotype, resistance to camptothecin, a specific inhibitor of topo I, but sensitivity to etoposide, an inhibitor of topo II, were investigated in this study. In the absence of external stimuli, AT1-beta/22 and beta/36 cells underwent programmed cell death (PCD) in a precocious phase of the growth curve. ASC metabolism showed remarkable differences in AT1-beta/22 and beta/36 cells, compared with control, and the observed alterations were similar to those occurring in tobacco Yellow Bright-2 cells induced to enter PCD by exogenous stimuli. However, differently from other studied examples of PCD, overproduction of reactive oxygen species was not detected in AT1-beta/22 and beta/36 cells. The relevance of these findings in relation to the signalling pathways leading to PCD is discussed.

摘要

拓扑异构酶I(topo I)是一种核酶,在涉及DNA拓扑结构变化的多种途径中发挥着重要作用。topo I介导的反应是通过该酶与DNA的瞬时共价结合(topo I-DNA复合物)来完成的。据报道,在氧化应激条件下和细胞凋亡过程中,动物细胞中会发生topo I-DNA复合物的稳定化,导致不可逆的双链断裂。为了研究topo I介导的DNA损伤与抗坏血酸(ASC)代谢之间可能存在的联系(ASC代谢也参与植物对氧化应激的反应和凋亡过程),采用反义RNA策略培育了胡萝卜细胞,其编码topo Iβ同工型的top1β基因表达降低。本研究对两个独立的转基因株系(AT1-β/22和β/36)进行了研究,它们具有生长缓慢的表型,对topo I的特异性抑制剂喜树碱具有抗性,但对topo II的抑制剂依托泊苷敏感。在没有外部刺激的情况下,AT1-β/22和β/36细胞在生长曲线的早熟阶段经历了程序性细胞死亡(PCD)。与对照相比,AT1-β/22和β/36细胞中的ASC代谢表现出显著差异,观察到的变化与外源刺激诱导进入PCD的烟草黄亮-2细胞中发生的变化相似。然而,与其他研究的PCD例子不同,在AT1-β/22和β/36细胞中未检测到活性氧的过量产生。本文讨论了这些发现与导致PCD的信号通路的相关性。

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