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人多聚(ADP - 核糖)聚合酶1在酿酒酵母中的表达:对生存、同源重组的影响以及参与细胞内定位的基因的鉴定。

Expression of human poly (ADP-ribose) polymerase 1 in Saccharomyces cerevisiae: Effect on survival, homologous recombination and identification of genes involved in intracellular localization.

作者信息

La Ferla Marco, Mercatanti Alberto, Rocchi Giulia, Lodovichi Samuele, Cervelli Tiziana, Pignata Luca, Caligo Maria Adelaide, Galli Alvaro

机构信息

Yeast Genetics and Genomics, Institute of Clinical Physiology, National Council of Research (CNR), via Moruzzi 1, 56122 Pisa, Italy.

Section of Genetic Oncology, University Hospital and University of Pisa, via Roma 57, 56125 Pisa, Italy.

出版信息

Mutat Res. 2015 Apr;774:14-24. doi: 10.1016/j.mrfmmm.2015.02.006. Epub 2015 Mar 6.

Abstract

The poly (ADP-ribose) polymerase 1 (PARP-1) actively participates in a series of functions within the cell that include: mitosis, intracellular signaling, cell cycle regulation, transcription and DNA damage repair. Therefore, inhibition of PARP1 has a great potential for use in cancer therapy. As resistance to PARP inhibitors is starting to be observed in patients, thus the function of PARP-1 needs to be studied in depth in order to find new therapeutic targets. To gain more information on the PARP-1 activity, we expressed PARP-1 in yeast and investigated its effect on cell growth and UV induced homologous recombination. To identify candidate genes affecting PARP-1 activity and cellular localization, we also developed a yeast genome wide genetic screen. We found that PARP-1 strongly inhibited yeast growth, but when yeast was exposed to the PARP-1 inhibitor 6(5-H) phenantridinone (PHE), it recovered from the growth suppression. Moreover, we showed that PARP-1 produced PAR products in yeast and we demonstrated that PARP-1 reduced UV-induced homologous recombination. By genome wide screening, we identified 99 mutants that suppressed PARP-1 growth inhibition. Orthologues of human genes were found for 41 of these yeast genes. We determined whether the PARP-1 protein level was altered in strains which are deleted for the transcription regulator GAL3, the histone H1 gene HHO1, the HUL4 gene, the deubiquitination enzyme gene OTU1, the nuclear pore protein POM152 and the SNT1 that encodes for the Set3C subunit of the histone deacetylase complex. In these strains the PARP-1 level was roughly the same as in the wild type. PARP-1 localized in the nucleus more in the snt1Δ than in the wild type strain; after UV radiation, PARP-1 localized in the nucleus more in hho1 and pom152 deletion strains than in the wild type indicating that these functions may have a role on regulating PARP-1 level and activity in the nucleus.

摘要

聚(ADP - 核糖)聚合酶1(PARP - 1)积极参与细胞内的一系列功能,包括:有丝分裂、细胞内信号传导、细胞周期调控、转录和DNA损伤修复。因此,抑制PARP1在癌症治疗中具有很大的应用潜力。由于在患者中已开始观察到对PARP抑制剂的耐药性,因此需要深入研究PARP - 1的功能以寻找新的治疗靶点。为了获得更多关于PARP - 1活性的信息,我们在酵母中表达了PARP - 1,并研究了其对细胞生长和紫外线诱导的同源重组的影响。为了鉴定影响PARP - 1活性和细胞定位的候选基因,我们还开展了全基因组酵母遗传筛选。我们发现PARP - 1强烈抑制酵母生长,但当酵母暴露于PARP - 1抑制剂6(5 - H)菲啶酮(PHE)时,它从生长抑制中恢复。此外,我们表明PARP - 1在酵母中产生PAR产物,并且我们证明PARP - 1降低了紫外线诱导的同源重组。通过全基因组筛选,我们鉴定出99个抑制PARP - 1生长抑制的突变体。在这些酵母基因中的41个中发现了人类基因的直系同源物。我们确定了在缺失转录调节因子GAL3、组蛋白H1基因HHO1、HUL4基因、去泛素化酶基因OTU1、核孔蛋白POM152以及编码组蛋白脱乙酰酶复合物Set3C亚基的SNT1的菌株中PARP - 1蛋白水平是否发生改变。在这些菌株中,PARP - 1水平与野生型大致相同。与野生型菌株相比,PARP - 1在snt1Δ中更多地定位于细胞核;紫外线辐射后,与野生型相比,PARP - 1在hho1和pom152缺失菌株中更多地定位于细胞核,表明这些功能可能在调节细胞核中PARP - 1的水平和活性方面发挥作用。

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