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鉴定爱泼斯坦-巴尔病毒DNA复制所需的最小oriP。

Identification of minimal oriP of Epstein-Barr virus required for DNA replication.

作者信息

Shirakata M, Hirai K

机构信息

Department of Cell Regulation, Medical Research Institute, Tokyo Medical and Dental University.

出版信息

J Biochem. 1998 Jan;123(1):175-81. doi: 10.1093/oxfordjournals.jbchem.a021907.

Abstract

DNA replication from oriP of Epstein-Barr virus is mediated by the virus replication factor EBNA1 and cellular factors and occurs approximately once in each cell cycle. We have identified a minimal oriP element that is necessary and sufficient for DNA replication. We transfected plasmids containing several oriP fragments into HeLa cells expressing EBNA1 and analyzed their replication during four days after transfection using the methylation sensitive restriction endonuclease DpnI. All the oriP fragments containing the four EBNA1-binding sites known as the dyad symmetry sequence (DS) initiated DNA replication. The sequences flanking DS were not essential for DNA replication, but deletion of two or three EBNA1-binding sites in DS significantly reduced or totally abolished its replication activity. These results indicated that the four EBNA1-binding sites in DS constitute the minimal oriP element for DNA replication and suggest that DNA replication is initiated by recruitment of cellular replication factors onto or near the minimal oriP by EBNA1. We also found that the minimal oriP initiated DNA replication in mouse fibroblasts expressing EBNA1 but worked only at reduced efficiency, suggesting species specificity in DNA replication machineries.

摘要

爱泼斯坦-巴尔病毒oriP的DNA复制由病毒复制因子EBNA1和细胞因子介导,且在每个细胞周期中大约发生一次。我们已经鉴定出一个对DNA复制既必要又充分的最小oriP元件。我们将含有几个oriP片段的质粒转染到表达EBNA1的HeLa细胞中,并在转染后的四天内使用甲基化敏感限制性内切酶DpnI分析它们的复制情况。所有包含四个EBNA1结合位点(即二元对称序列,DS)的oriP片段都启动了DNA复制。DS两侧的序列对DNA复制并非必需,但DS中两个或三个EBNA1结合位点的缺失会显著降低或完全消除其复制活性。这些结果表明,DS中的四个EBNA1结合位点构成了DNA复制的最小oriP元件,并提示DNA复制是由EBNA1将细胞复制因子招募到最小oriP上或其附近而启动的。我们还发现,最小oriP在表达EBNA1的小鼠成纤维细胞中启动了DNA复制,但效率较低,这表明DNA复制机制存在物种特异性。

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