sPARP-1的特性。PARP-1基因的一种替代产物,具有不依赖于DNA链断裂的聚(ADP-核糖)聚合酶活性。
Characterization of sPARP-1. An alternative product of PARP-1 gene with poly(ADP-ribose) polymerase activity independent of DNA strand breaks.
作者信息
Sallmann F R, Vodenicharov M D, Wang Z Q, Poirier G G
机构信息
Poly(ADP-ribose) Metabolism Group, Health and Environment Unit, Laval University Medical Research Center, CHUQ, Laval University, Ste-Foy, Quebec, G1V 4G2 Canada.
出版信息
J Biol Chem. 2000 May 19;275(20):15504-11. doi: 10.1074/jbc.275.20.15504.
Poly(ADP-ribose) polymerase-1 (PARP-1) is an abundant nuclear enzyme that catalyzes the synthesis of poly(ADP-ribose) (pADPr) from its substrate NAD(+) upon binding to DNA strand breaks. Poly(ADP-ribosyl)ation has been implicated in many cellular processes including replication, transcription, and the maintenance of genomic stability. However, studies with mice and cells lacking PARP-1 reveal a critical role for the enzyme in the maintenance of genomic integrity only. Recently, a significant level of poly(ADP-ribose) polymerase activity has been detected in fibroblasts derived from mice lacking PARP-1 following treatment with genotoxic agents (Shieh, W. M., Amé, J-C., Wilson, M. V., Wang, Z-Q., Koh, D. W., Jacobson, M. K., and Jacobson, E. L. (1998) J. Biol. Chem. 273, 30069-30072). We have isolated a cDNA that originates from PARP-1 (-/-) fibroblasts and encodes a polypeptide of 493 amino acid residues bearing poly(ADP-ribose) polymerase activity. This protein, that we named sPARP-1 for short poly(ADP-ribose) polymerase-1, has a calculated mass of 55.3 kDa and is identical in deduced amino acid sequence to the catalytic domain of PARP-1. Radiation hybrid analysis assigned the sPARP-1 gene to the chromosome 1H5-H6 in an immediate proximity to the known location of PARP-1 gene, indicating that sPARP-1 and PARP-1 are most probably products of the same gene. Active sPARP-1 is present in both PARP-1 (+/+) and PARP-1 (-/-) cells as demonstrated by activity-Western blotting and immunostaining using a specific antibody developed against sPARP-1. Like PARP-1, sPARP-1 is localized in the cell nucleus, uses NAD(+) as a substrate and is inhibited by nicotinamide analogues. sPARP-1 produces pADPr of similar length and structure to that of PARP-1. However, contrary to PARP-1, sPARP-1 does not require DNA strand breaks for its activation, although it is stimulated following genotoxic treatments.
聚(ADP - 核糖)聚合酶 -1(PARP -1)是一种丰富的核酶,当它与DNA链断裂结合时,能催化从其底物烟酰胺腺嘌呤二核苷酸(NAD(+))合成聚(ADP - 核糖)(pADPr)。聚(ADP - 核糖基)化参与了许多细胞过程,包括复制、转录以及基因组稳定性的维持。然而,对缺乏PARP -1的小鼠和细胞的研究表明,该酶仅在维持基因组完整性方面起关键作用。最近,在用基因毒性剂处理后,在缺乏PARP -1的小鼠来源的成纤维细胞中检测到了显著水平的聚(ADP - 核糖)聚合酶活性(Shieh, W. M., Amé, J - C., Wilson, M. V., Wang, Z - Q., Koh, D. W., Jacobson, M. K., and Jacobson, E. L. (1998) J. Biol. Chem. 273, 30069 - 30072)。我们从PARP -1(- / -)成纤维细胞中分离出了一个cDNA,它编码一个含有493个氨基酸残基且具有聚(ADP - 核糖)聚合酶活性的多肽。这种蛋白质,我们简称为sPARP -1(短聚(ADP - 核糖)聚合酶 -1),计算分子量为55.3 kDa,其推导氨基酸序列与PARP -1的催化结构域相同。辐射杂交分析将sPARP -1基因定位到1H5 - H6染色体上,紧邻PARP -1基因的已知位置,这表明sPARP -1和PARP -1很可能是同一基因的产物。通过活性 - 蛋白质免疫印迹法以及使用针对sPARP -1制备的特异性抗体进行免疫染色证明,活性sPARP -1存在于PARP -1(+ / +)和PARP -1(- / -)细胞中。与PARP -1一样,sPARP -1定位于细胞核,以NAD(+)为底物,并受到烟酰胺类似物的抑制。sPARP -1产生的pADPr在长度和结构上与PARP -1产生的相似。然而,与PARP -1不同的是,sPARP -1的激活不需要DNA链断裂,尽管在基因毒性处理后它会被刺激。
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