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紫外线B照射的拟南芥根中分裂细胞对复制应激的耐受性:DNA跨损伤聚合酶η和ζ的需求

Tolerance of dividing cells to replication stress in UVB-irradiated Arabidopsis roots: requirements for DNA translesion polymerases eta and zeta.

作者信息

Curtis Marc J, Hays John B

机构信息

Department of Environmental and Molecular Toxicology, Oregon State University, Corvallis, OR, United States.

出版信息

DNA Repair (Amst). 2007 Sep 1;6(9):1341-58. doi: 10.1016/j.dnarep.2007.03.004. Epub 2007 May 7.

Abstract

In tissues of multicellular organisms, DNA lesions that block replication can disrupt division of the transiently amplifying (TA) cells and stem cells that drive growth. To study how tissue growth is maintained despite DNA damage, stem cells and other cell types must be clearly identifiable. In plants, root growth depends directly on cell divisions in the root meristem. In Arabidopsis thaliana, cell identities in root meristems are unambiguously defined by position relative to the quiescent center and are readily visualized by microscopy. We evaluated roles of two DNA translesion polymerases, AtPoleta (Eta) and AtPolzeta (Zeta), in resistance of dividing root cells to a model genotoxin, UVB-radiation. The major UV photoproducts in DNA, cyclobutane pyrimidine dimers (CPDs), were induced to roughly 0.03CPD/kb by a threshold dose (0.28 kJ m(-2)) that minimally affected wild-type roots. In roots lacking AtPoleta and/or AtPolzeta, this dose inhibited cell division and tissue growth and specifically killed stem cells; severities of all three phenotypes increased in the order eta-<zeta-<eta-zeta-. One to 2 days after CPDs had disappeared from eta-zeta- roots, TA cell pools were depleted and there were novel cell divisions in the quiescent center. This delayed "secondary" response to genotoxic stress may reflect changes in the balance of proliferation and differentiation signals. In eta-zeta- roots, death of stem cells was substantial even in the absence of irradiation. The lethality of Polzeta ablation in mice had confined most previous analyses of Polzeta (and concomitant Poleta) function to unicellular (yeast) and chicken-cell culture models, so these studies illustrate the advantages afforded by the Arabidopsis-root model system in studies of growth and development of multicellular tissues.

摘要

在多细胞生物体的组织中,阻碍复制的DNA损伤会扰乱驱动生长的瞬时扩增(TA)细胞和干细胞的分裂。为了研究尽管存在DNA损伤,组织生长是如何维持的,干细胞和其他细胞类型必须能够被清晰识别。在植物中,根的生长直接依赖于根分生组织中的细胞分裂。在拟南芥中,根分生组织中的细胞身份通过相对于静止中心的位置明确界定,并且通过显微镜很容易观察到。我们评估了两种DNA跨损伤聚合酶AtPoleta(Eta)和AtPolzeta(Zeta)在根分裂细胞对模型基因毒素UVB辐射的抗性中的作用。DNA中的主要紫外线光产物——环丁烷嘧啶二聚体(CPD),通过一个阈值剂量(0.28 kJ m(-2))被诱导至大约0.03 CPD/kb,该剂量对野生型根的影响最小。在缺乏AtPoleta和/或AtPolzeta的根中,这个剂量抑制细胞分裂和组织生长,并特异性地杀死干细胞;所有这三种表型的严重程度按eta-<zeta-<eta-zeta-的顺序增加。在CPD从eta-zeta-根中消失1至2天后,TA细胞池被耗尽,并且在静止中心出现了新的细胞分裂。这种对基因毒性应激的延迟“二次”反应可能反映了增殖和分化信号平衡的变化。在eta-zeta-根中,即使没有辐射,干细胞的死亡也很严重。Polzeta缺失在小鼠中的致死性使得之前对Polzeta(以及伴随的Poleta)功能的大多数分析局限于单细胞(酵母)和鸡细胞培养模型,因此这些研究说明了拟南芥根模型系统在多细胞组织生长和发育研究中的优势。

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