Wang J, Satoh M, Pierani A, Schmitt J, Chou C H, Stunnenberg H G, Roeder R G, Reeves W H
Department of Medicine, University of North Carolina, Chapel Hill 27599-7280.
J Cell Sci. 1994 Nov;107 ( Pt 11):3223-33. doi: 10.1242/jcs.107.11.3223.
The Ku autoantigen is a heterodimer of 70 kDa (p70) and -80 kDa (p80) subunits that is the DNA-binding component of a DNA-dependent protein kinase (DNA-PK). The 350 kDa (p350) catalytic subunit of DNA-PK phosphorylates Sp-1, Oct-1, p53 and RNA polymerase II in vitro, but the precise cellular role of DNA-PK remains unclear. In the present studies, the assembly of p70/p80 heterodimers and the interaction of Ku with DNA was investigated using recombinant vaccinia viruses directing the synthesis of human p70 (p70-vacc) and p80 (p80-vacc), and monoclonal antibodies (mAbs). Expression of human Ku antigens in rabbit kidney (RK13) cells could be demonstrated by immunofluorescent staining because this cell line contains little endogenous Ku. A novel mAb designated 162 stained the nuclei of RK13 cells coinfected with p70-vacc and p80-vacc, but not cells that were infected with either virus alone, suggesting that it recognized the p70/p80 heterodimer but not monomeric p70 or p80. In agreement with the immunofluorescence data, 162 immunoprecipitated both p70 and p80 from extracts of coinfected cells, but did not immunoprecipitate either subunit by itself from extracts of cells infected with p70-vacc or p80-vacc, respectively. Conversely, the binding of 162 to Ku isolated from human K562 cells stabilized the p70/p80 heterodimer under conditions that normally dissociate p70 from p80. The nuclei of cells infected with p70-vacc alone could be stained with mAb N3H10 (anti-p70) and cells infected with p80-vacc alone could be stained with mAb 111 (anti-p80), indicating that the formation of p70/p80 heterodimers was not required for nuclear transport. Finally, free recombinant and cellular p70 both bound to DNA efficiently in vitro, suggesting that free p70, like the p70/p80 heterodimer, serves as a DNA-binding factor. Moreover, free human p70 could be released from the nuclei of p70-vacc-infected RK13 cells by deoxyribonuclease I treatment, suggesting that it was associated with chromatin in vivo. The nuclear transport of free p70 and the association of free p70 with chromatin in vivo raise the possibility that newly synthesized cellular p70 might undergo nuclear transport and DNA-binding prior to dimerization with p80 or assembly with p350.
Ku自身抗原是一种由70 kDa(p70)和80 kDa(p80)亚基组成的异源二聚体,它是DNA依赖性蛋白激酶(DNA-PK)的DNA结合成分。DNA-PK的350 kDa(p350)催化亚基在体外可使Sp-1、Oct-1、p53和RNA聚合酶II磷酸化,但DNA-PK在细胞中的具体作用仍不清楚。在本研究中,使用指导合成人p70(p70-痘苗病毒)和p80(p80-痘苗病毒)的重组痘苗病毒以及单克隆抗体(mAb),研究了p70/p80异源二聚体的组装以及Ku与DNA的相互作用。由于兔肾(RK13)细胞几乎不含内源性Ku,因此可以通过免疫荧光染色证明人Ku抗原在该细胞系中的表达。一种名为162的新型单克隆抗体可对同时感染p70-痘苗病毒和p80-痘苗病毒的RK13细胞的细胞核进行染色,但对单独感染任何一种病毒的细胞则无染色作用,这表明它识别的是p70/p80异源二聚体而非单体p70或p80。与免疫荧光数据一致,162可从共感染细胞的提取物中免疫沉淀p70和p80,但不能分别从感染p70-痘苗病毒或p80-痘苗病毒的细胞提取物中单独免疫沉淀任何一个亚基。相反,在通常会使p70与p80解离的条件下,162与从人K562细胞中分离出的Ku的结合稳定了p70/p80异源二聚体。单独感染p70-痘苗病毒的细胞的细胞核可用单克隆抗体N3H10(抗p70)染色,单独感染p80-痘苗病毒的细胞的细胞核可用单克隆抗体111(抗p80)染色,这表明核转运并不需要p70/p80异源二聚体的形成。最后,游离的重组p70和细胞内的p70在体外均能有效地与DNA结合,这表明游离的p70与p70/p80异源二聚体一样,可作为一种DNA结合因子。此外,用脱氧核糖核酸酶I处理可使游离的人p70从感染p70-痘苗病毒的RK13细胞的细胞核中释放出来,这表明它在体内与染色质相关。游离p70的核转运以及其在体内与染色质的结合增加了一种可能性,即新合成的细胞内p70在与p80二聚化或与p350组装之前可能会进行核转运并与DNA结合。
