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玉米黑粉菌的REC1基因编码一种3'→5'核酸外切酶,它将DNA修复及DNA合成的完成与有丝分裂检查点联系起来。

The REC1 gene of Ustilago maydis, which encodes a 3'-->5' exonuclease, couples DNA repair and completion of DNA synthesis to a mitotic checkpoint.

作者信息

Onel K, Koff A, Bennett R L, Unrau P, Holloman W K

机构信息

Hearst Microbiology Research Center, Cornell University Medical College, New York, New York 10021, USA.

出版信息

Genetics. 1996 May;143(1):165-74. doi: 10.1093/genetics/143.1.165.

Abstract

Mutation in the REC1 gene of Ustilago maydis results in extreme sensitivity to killing by ultraviolet light. The lethality of the rec1-1 mutant was found to be partially suppressed if irradiated cells were held artificially in G2-phase by addition of a microtubule inhibitor. This mutant was also found to be sensitive to killing when DNA synthesis was inhibited by external means through addition of hydroxyurea or by genetic control in a temperature-sensitive mutant strain defective in DNA synthesis. Flow cytometric analysis of exponentially growing cultures indicated that wild-type cells accumulated in G2 after UV irradiation, while rec1-1 cells appeared to exit from G2 and accumulate in G1/S. Analysis of mRNA levels in synchronized cells indicated that the REC1 gene is periodically expressed with the cell cycle and reaches maximal levels at G1/S. The results are interpreted to mean that a G2-M checkpoint is disabled in the rec1-1 mutant. It is proposed that the REC1 gene product functions in a surveillance system operating during S-phase and G2 to find and repair stretches of DNA with compromised integrity and to communicate with the cell cycle apparatus.

摘要

玉米黑粉菌REC1基因的突变导致其对紫外线杀伤极度敏感。如果通过添加微管抑制剂将受照射细胞人工阻滞在G2期,rec1-1突变体的致死性会得到部分抑制。当通过添加羟基脲从外部抑制DNA合成或在DNA合成缺陷的温度敏感突变菌株中通过遗传控制抑制DNA合成时,也发现该突变体对杀伤敏感。对指数生长培养物的流式细胞术分析表明,野生型细胞在紫外线照射后积累在G2期,而rec1-1细胞似乎从G2期退出并积累在G1/S期。对同步化细胞中mRNA水平的分析表明,REC1基因随细胞周期周期性表达,并在G1/S期达到最高水平。这些结果被解释为意味着rec1-1突变体中的G2-M检查点被禁用。有人提出,REC1基因产物在S期和G2期运行的监测系统中发挥作用,以发现和修复完整性受损的DNA片段,并与细胞周期机制进行通信。

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