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Dive into the research topics where Takashi Tsuyama is active.

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Featured researches published by Takashi Tsuyama.


Nucleic Acids Research | 2005

Licensing for DNA replication requires a strict sequential assembly of Cdc6 and Cdt1 onto chromatin in Xenopus egg extracts

Takashi Tsuyama; Shusuke Tada; Saori Watanabe; Masayuki Seki; Takemi Enomoto

Replication origins are licensed for a single initiation event by the loading of Mcm2-7 proteins during late mitosis and G1. Sequential associations of origin recognition complex, Cdc6 and Mcm2-7 are essential for completion of the licensing. Although Cdt1 also binds to the chromatin when the licensing reaction takes place, whether the binding is a requirement for Cdt1 to function is unclear. To analyze the relevance of the chromatin association of Cdt1, we carried out chromatin transfer experiments using either immunodepleted Xenopus egg extracts or purified proteins. Licensing assay and immunoblotting analyses indicated that Cdt1 could only license DNA replication and load Mcm2-7 onto DNA when it binds to chromatin that has already associated with Cdc6. These results provide evidence supporting that Cdc6 and Cdt1 must bind to chromatin in a strict order for DNA licensing to occur.


Protein Science | 2009

Structure of the Cdt1 C-terminal domain: Conservation of the winged helix fold in replication licensing factors

Bulat I. Khayrutdinov; Won Jin Bae; Young Mi Yun; Jie Hye Lee; Takashi Tsuyama; Jung Joo Kim; Eunha Hwang; Kyoung-Seok Ryu; Hae-Kap Cheong; Chaejoon Cheong; Jung-Soon Ko; Takemi Enomoto; P. Andrew Karplus; Peter Güntert; Shusuke Tada; Young Ho Jeon; Yunje Cho

In eukaryotic replication licensing, Cdt1 plays a key role by recruiting the MCM2‐7 complex onto the origin of chromosome. The C‐terminal domain of mouse Cdt1 (mCdt1C), the most conserved region in Cdt1, is essential for licensing and directly interacts with the MCM2‐7 complex. We have determined the structures of mCdt1CS (mCdt1C_small; residues 452 to 557) and mCdt1CL (mCdt1C_large; residues 420 to 557) using X‐ray crystallography and solution NMR spectroscopy, respectively. While the N‐terminal 31 residues of mCdt1CL form a flexible loop with a short helix near the middle, the rest of mCdt1C folds into a winged helix structure. Together with the middle domain of mouse Cdt1 (mCdt1M, residues 172–368), this study reveals that Cdt1 is formed with a tandem repeat of the winged helix domain. The winged helix fold is also conserved in other licensing factors including archaeal ORC and Cdc6, which supports an idea that these replication initiators may have evolved from a common ancestor. Based on the structure of mCdt1C, in conjunction with the biochemical analysis, we propose a binding site for the MCM complex within the mCdt1C.


Molecular Biology of the Cell | 2008

Repression of Nascent Strand Elongation by Deregulated Cdt1 during DNA Replication in Xenopus Egg Extracts

Takashi Tsuyama; Saori Watanabe; Ayako Aoki; Yunje Cho; Masayuki Seki; Takemi Enomoto; Shusuke Tada

Excess Cdt1 reportedly induces rereplication of chromatin in cultured cells and Xenopus egg extracts, suggesting that the regulation of Cdt1 activity by cell cycle-dependent proteolysis and expression of the Cdt1 inhibitor geminin is crucial for the inhibition of chromosomal overreplication between S phase and metaphase. We analyzed the consequences of excess Cdt1 for DNA replication and found that increased Cdt1 activity inhibited the elongation of nascent strands in Xenopus egg extracts. In Cdt1-supplemented extracts, overreplication was remarkably induced by the further addition of the Cdt1-binding domain of geminin (Gem79-130), which lacks licensing inhibitor activity. Further analyses indicated that fully active geminin, as well as Gem79-130, restored nascent strand elongation in Cdt1-supplemented extracts even after the Cdt1-induced stalling of replication fork elongation had been established. Our results demonstrate an unforeseen, negative role for Cdt1 in elongation and suggest that its function in the control of replication should be redefined. We propose a novel surveillance mechanism in which Cdt1 blocks nascent chain elongation after detecting illegitimate activation of the licensing system.


Biochimica et Biophysica Acta | 2007

Possible involvement of RecQL4 in the repair of double-strand DNA breaks in Xenopus egg extracts

Yuji Kumata; Shusuke Tada; Yumie Yamanada; Takashi Tsuyama; Takayuki Kobayashi; Yu-Peng Dong; Kyoko Ikegami; Hiromu Murofushi; Masayuki Seki; Takemi Enomoto


Journal of Biological Chemistry | 2005

Caenorhabditis elegans geminin homologue participates in cell cycle regulation and germ line development.

Ken-ichiro Yanagi; Takeshi Mizuno; Takashi Tsuyama; Shusuke Tada; Yumi Iida; Asako Sugimoto; Toshihiko Eki; Takemi Enomoto; Fumio Hanaoka


Journal of Cell Science | 2002

Focus-formation of replication protein A, activation of checkpoint system and DNA repair synthesis induced by DNA double-strand breaks in Xenopus egg extract

Takayuki Kobayashi; Shusuke Tada; Takashi Tsuyama; Hiromu Murofushi; Masayuki Seki; Takemi Enomoto


DNA Repair | 2006

Analyses of the interaction of WRNIP1 with Werner syndrome protein (WRN) in vitro and in the cell.

Yoh-ichi Kawabe; Masayuki Seki; Akari Yoshimura; Katsuaki Nishino; Tomoko Hayashi; Takashi Takeuchi; Sohta Iguchi; Yumiko Kusa; Makoto Ohtsuki; Takashi Tsuyama; Osamu Imamura; Takehisa Matsumoto; Yasuhiro Furuichi; Shusuke Tada; Takemi Enomoto


Biochemical and Biophysical Research Communications | 2006

Chromatin loading of Smc5/6 is induced by DNA replication but not by DNA double-strand breaks

Takashi Tsuyama; Katsutoshi Inou; Masayuki Seki; Takahiko Seki; Yuji Kumata; Takayuki Kobayashi; Keiji Kimura; Fumio Hanaoka; Takemi Enomoto; Shusuke Tada


The Japanese Biochemical Society/The Molecular Biology Society of Japan | 2017

Enhancement of apoptosis via increase of ICERII by O -GlcNAc-modified protein

Yutaro Azuma; Hitomi Enosawa; Takashi Tsuyama; Shusuke Tada


The Molecular Biology Society of Japan | 2016

Inhibitory effect of Cdt1 on the nascent strand elongation during DNA replication in Xenopus egg extracts

Yuta Nakazaki; Takashi Tsuyama; Yutaro Azuma; Mikiko Takahashi; Shusuke Tada

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Yunje Cho

Pohang University of Science and Technology

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