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Genomic and molecular analyses of the core DNA replication machinery in plants.

机译:植物核心DNA复制机制的基因组和分子分析。

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摘要

Accurate and complete DNA replication is essential for maintaining the integrity of the genome. In eukaryotes, this process requires the coordinated action of numerous molecular machines. Based on yeast and animal model systems, we defined a set of fifty-one core DNA replication proteins” that are integral to the initiation, DNA synthesis, and Okazaki fragment maturation functions of DNA replication. We used computational analyses to identify putative homologs in the genomes of two plants, Arabidopsis thaliana (Arabidopsis) and Oryza sativa (rice), providing the first comprehensive view of the core DNA replication machinery in plants. Our results indicated that the overall composition of this apparatus is conserved, but plants are unique in that multiple DNA replication genes exist as small gene families. Fourteen of the genes we annotated in this study have not been previously reported in the literature, and we have provided revised gene models for seventeen plant proteins. To better understand how the DNA replication machinery functions in plants, we cloned multiple subunits of the pre-replication complex (pre-RC) from Arabidopsis and generated antibodies against four key components of this complex—AtORC1, AtORC2, AtMCM5, and AtMCM7. We demonstrated that the pre-RC is developmentally regulated in Arabidopsis and, consistent with a role in DNA replication, is abundant in proliferating tissues. We used immunocytochemical and biochemical methods to characterize MCM7 in plants. We observed two distinct localization patterns for plant MCM7 proteins. In most cells, MCM7 was nuclear and colocalized with DNA. In a small fraction of cells, MCM7 was dispersed throughout the cytoplasmic compartment. Biochemical analysis confirmed that MCM7 binds to chromatin and that it is present in the nucleus at least during the G1, S and G2 cell cycle stages. Together, these analyses support a model where the MCM complex is loaded onto DNA in late M and early G1, released into the nucleoplasm during S phase followed by a brief dispersion into the cytoplasmic compartment concurrent with nuclear envelope breakdown in mitosis.
机译:准确而完整的DNA复制对于维持基因组的完整性至关重要。在真核生物中,该过程需要众多分子机器的协同作用。基于酵母和动物模型系统,我们定义了一组51个核心DNA复制蛋白”,它们是DNA复制的起始,DNA合成和冈崎片段成熟功能不可或缺的。我们使用计算分析来鉴定拟南芥(Arabidopsis)和水稻(水稻)两种植物基因组中的推定同源物,从而首次全面了解了植物中核心DNA复制机制。我们的结果表明该装置的总体组成是保守的,但是植物的独特之处在于多个DNA复制基因作为小基因家族存在。我们在这项研究中注释的基因中有14个以前没有在文献中报道过,并且我们提供了17种植物蛋白的改良基因模型。为了更好地了解DNA复制机制如何在植物中发挥作用,我们从拟南芥中克隆了复制前复合体(pre-RC)的多个亚基,并产生了针对该复合体的四个关键成分的抗体-AtORC1,AtORC2,AtMCM5和AtMCM7。我们证明了pre-RC在拟南芥中受到发育调节,并且与DNA复制中的作用一致,在增殖组织中含量很高。我们使用免疫细胞化学和生化方法来表征植物中的MCM7。我们观察到了植物MCM7蛋白的两种不同的定位模式。在大多数细胞中,MCM7是有核的,并与DNA共定位。在一小部分细胞中,MCM7分散在整个细胞质区室中。生化分析证实,MCM7与染色质结合,并且至少在G1,S和G2细胞周期阶段它存在于细胞核中。这些分析共同支持一个模型,该模型将MCM复合物加载到M期晚期和G1期早期的DNA上,并在S期释放到核质中,然后短暂分散到细胞质区室中,同时在有丝分裂中核被膜破裂。

著录项

  • 作者

    Shultz, Randall William.;

  • 作者单位

    North Carolina State University.;

  • 授予单位 North Carolina State University.;
  • 学科 Biology Molecular.;Health Sciences Oncology.;Biology Botany.
  • 学位 Ph.D.
  • 年度 2007
  • 页码 253 p.
  • 总页数 253
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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