Suppression of the poly(ADP-ribose) polymerase activity by DNA-dependent protein kinase in vitro

Author:

Ariumi, Y.

Masutani, M.

Copeland, T. D.

Mimori, T.

Sugimura, T.

Shimotohno, K.

Ueda, K.

Hatanaka, M.

Noda, M.
Author Address

Ariumi Y Kyoto Univ, Inst Virus Res, Sakyo Ku Kyoto 6068507 Japan Kyoto Univ, Inst Virus Res, Sakyo Ku Kyoto 6068507 Japan Natl Canc Ctr, Res Inst, Div Biochem Tokyo 1040045 Japan NCI, ABL Basic Res Program, Frederick Canc Res & Dev Ctr Frederick, MD 21702 USA Keio Univ, Sch Med Tokyo 1600016 Japan Kyoto Univ, Chem Res Inst Kyoto 6110011 Japan Kyoto Univ, Grad Sch Med, Dept Mol Oncol Kyoto 6068501 Japan

Abstract:

It has been suggested that DNA-dependent protein kinase (DNA-PK) is a central component of DNA double-strand-break repair. The mechanism of DNA-PK action, however, has not been fully understood. Poly(ADP-ribose) polymerase (PARP) is another nuclear enzyme which has high affinity to DNA ends. In this study, we analysed the interaction between these tao enzymes. First, DNA-PK was found to suppress the PARP activity and alters the pattern of poly(ADP-ribosyl)ation. Although DNA-PK phosphorylates PARP in a DNA-dependent manner, this modification is unlikely to be responsible for the suppression of PARP activity, since this suppression occurs even in the absence of ATP. Conversely, PARP was found to ADP-ribosylate DNA-PK in vitro. However, the autophosphorylation activity of DNA-PK was not influenced by this modification. In a competitive electrophoretic mobility shift assay, Ku 70/80 complex, the DNA binding component of DNA-PK, was found to have higher affinity to a short fragment of DNA than does PARP. Furthermore, co-immunoprecipitation analysis suggested direct or close association between Ku and PARP. Thus, DNA-PK suppresses PARP activity, probably through direct binding and/or sequestration of DNA-ends which serve as an important stimulator for both enzymes. [References: 49]

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