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酿酒酵母CDC6基因产物的细胞内定位。

Intracellular location of the Saccharomyces cerevisiae CDC6 gene product.

作者信息

Jong A, Young M, Chen G C, Zhang S Q, Chan C

机构信息

Department of Pediatrics and Microbiology, University of Southern California School of Medicine, Los Angeles 90027, USA.

出版信息

DNA Cell Biol. 1996 Oct;15(10):883-95. doi: 10.1089/dna.1996.15.883.

Abstract

The CDC6 gene product from Saccharomyces cerevisiae is required for transition from late G1 to S phase of the cell cycle. We have investigated the subcellular localization of the CDC6 protein in yeast to explore where Cdc6p exerts its gene function (s). Using affinity-purified sera we localized Cdc6p to the cytoplasm and the nuclear matrix by both subcellular fractionation and indirect immunofluorescence microscopy. The nuclear localization was confirmed to be in the nuclear scaffold by the low-salt extraction method. The Cdc6p cannot be detected in the mitochondrial or plasma membrane fractions. Using indirect immunofluorescence, we found that a subpopulation of Cdc6p migrated into the nucleus after G1/S transition and diminished after M phase, suggesting its temporal role in nuclear DNA replication. The predicted Cdc6p polypeptide contains a conserved nuclear localization, 27PLKRKKL33, similar to that of the SV40 large T antigen and other nuclear proteins. To test whether this peptide segment plays a role in mediating nuclear transport, we have carried out site-directed mutagenesis to alter the conserved 29Lys to Thr and Arg. The wild-type nuclear localization signal of Cdc6p was found to mediate the LacZ reporter gene fused to CDC6 efficiently to the nucleus, but not the mutated versions of the nuclear localization motif. The results suggested that 29Lys is important in mediating nuclear localization, the 29Thr and 29Arg mutant versions of the CDC6 gene were also unable to complement the cdc6 temperature-sensitive mutant. However, when these mutants were expressed from a multicopy plasmid, the mutated genes could complement the mutation. Similar results were obtained in the cdc6-disrupted cells. Taken together, we suggest that (i) Cdc6p is predominantly located in the cytoplasm, (ii) the nuclear entry of Cdc6p is cell cycle dependent, and (iii) nuclear entry of Cdc6p is mediated by its nuclear localization signal. The presence of Cdc6p in both the nucleus and the cytoplasm suggests a model that Cdc6p exerts its gene function in DNA replication and mitotic restraint in the cell cycle.

摘要

酿酒酵母的CDC6基因产物是细胞周期从G1晚期过渡到S期所必需的。我们研究了酵母中CDC6蛋白的亚细胞定位,以探索Cdc6p在何处发挥其基因功能。通过亚细胞分级分离和间接免疫荧光显微镜技术,利用亲和纯化的血清,我们将Cdc6p定位到细胞质和核基质中。通过低盐提取法证实其核定位在核支架中。在线粒体或质膜组分中未检测到Cdc6p。利用间接免疫荧光,我们发现一部分Cdc6p在G1/S期转换后迁移到细胞核中,并在M期后减少,这表明其在核DNA复制中的时间作用。预测的Cdc6p多肽包含一个保守的核定位序列27PLKRKKL33,类似于SV40大T抗原和其他核蛋白的核定位序列。为了测试该肽段是否在介导核转运中起作用,我们进行了定点诱变,将保守的29位赖氨酸突变为苏氨酸和精氨酸。发现Cdc6p的野生型核定位信号能有效地将与CDC6融合的LacZ报告基因介导到细胞核中,但不能将核定位基序的突变版本介导到细胞核中。结果表明29位赖氨酸在介导核定位中很重要,CDC6基因的29位苏氨酸和29位精氨酸突变版本也不能互补cdc6温度敏感突变体。然而,当这些突变体从多拷贝质粒表达时,突变基因可以互补该突变。在cdc6缺失的细胞中也获得了类似的结果。综上所述,我们认为:(i)Cdc6p主要位于细胞质中;(ii)Cdc6p的核进入是细胞周期依赖性的;(iii)Cdc6p的核进入是由其核定位信号介导的。Cdc6p在细胞核和细胞质中的存在提示了一种模型,即Cdc6p在细胞周期的DNA复制和有丝分裂抑制中发挥其基因功能。

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