complementation of Rts1 RepA with phage p1 RepA protein

• Project/Area Number: 05454191
• Research Category: Grant-in-Aid for General Scientific Research (B)
• Allocation Type: Single-year Grants
• Research Field: Bacteriology (including Mycology)
• Research Institution: School of Medicine, Shinshu University
• Principal Investigator: TERAWAKI Yoshiro School of Med, Shinshu Univ., Professor, 医学部, 教授 (10014333)
• Co-Investigator(Kenkyū-buntansha): TABUCHI Akira School of Med, Shinshu Univ., Research Associate, 医学部, 助手 (50236725)
• Project Period (FY): 1993 – 1994
• Project Status: Completed (Fiscal Year 1994)
• Budget Amount: ¥6,400,000 (Direct Cost: ¥6,400,000); Fiscal Year 1994: ¥1,700,000 (Direct Cost: ¥1,700,000); Fiscal Year 1993: ¥4,700,000 (Direct Cost: ¥4,700,000)
• Keywords: Plasmid Rts1 / Phage P1 / Initiator protein RepA / Hybrid protein / ori activation / Autorepression / DNA binding / Replication inhibition / オートリプレッション / キメラ蛋白質 / 機能的ドメイン / DNA結合能 / 不和合性

Research Abstract

The RepA protein of the plasmid Rts1, consisting of 288 amino acids, is a trans-acting protein essential for initiation of replication. To study the functional domains of RepA,hybrid proteins were constructed of Rts1 RepA with the RepA initiator protein of plasmid P1 such that the N-terminal portion was from Rts1 RepA and the C-terminal portion from P1 RepA.Six hybrid protein were examined for function.
The minimal region of Rts1 RepA required for the in trans activation of Rts1 origin encompassed the N-terminal 206 amino acids while only 129 N-terminal amino acids were required for binding to the Rts1 ori region in vitro. Both in vivo and in vitro studies showed that the N-terminal 257 amino acids fragment was required for autorepressor activity. These results cleary indicate that the N-terminal region of the RepA molecule of Rts1 is involved in the activation of the replication origin of Rts1.
Among the hybrid proteins, RepAX15 consisting of the N-terminal 145 amino acids of Rts1 RepA and 142 amino acids from P1 RepA is most interesting, since it showed strong interference with both Rts1 and P1 replication, although the protein could not bind in vitro to P1 ori efficiently. It should be also stressed that no hybrid RepA activated P1 ori. These results suggest that the C-terminal region of both Rts1 and P1 RepA is involved in protein-protein interaction, perhaps in dimer formation.

Research Products

• [Publications] Terawaki,Y.: "Function of the N-terminal half of RepA in activation of Rts1 ori" J.Bacteriol.174. 6904-6910 (1992)
  • Description: 「研究成果報告書概要(和文)」より
• [Publications] 田渕晃 他: "Rts1とP1とのhybrid RepA蛋白の作成と機能的ドメインの解析" 日本細菌学雑誌. 49. 219 (1994)
  • Description: 「研究成果報告書概要(和文)」より
• [Publications] Tabuchi,A.: "Analysis of functional domains of Rts1 RepA by constructing a series of hybrid proteins--" J.Bacteriol.(submitted).
  • Description: 「研究成果報告書概要(和文)」より
• [Publications] Terawaki, Y.: "Function of the N-terminal half of RepA in activation of Rts1 ori" J.Bacteriol.174. 6904-6910 (1992)
  • Description: 「研究成果報告書概要(欧文)」より
• [Publications] Tabuchi, A.: "Analysis of functional domains of Rts1 RepA by constructing a series of hybrid proteins with P1 RepA" J.Bacteriol.(submitted).
  • Description: 「研究成果報告書概要(欧文)」より
• [Publications] 田渕 晃 他: "Rts1とP1とのhybrid RepA蛋白の作成と機能的ドメインの解析" 日本細菌学雑誌. 49. 219 (1994)
• [Publications] 田渕 晃 他: "プラスミドRts1の複製開始蛋白質RepAの機能" 日本細菌学雑誌. 50. 197 (1995)
• [Publications] Tabuchi,A.: "Analysis of functional domains of Rst1 RepA by‐‐‐‐" J.Bacteriol.submitted,in revision.
• [Publications] Terawaki,Y.: "Function of the N-terminal half of RepA in activation of Rts1 ori" J.Bacteriol.174. 6904-6910 (1992)
• [Publications] 寺脇良郎: "プラスミドRts1の複製開始蛋白質の機能的ドメイン" 日本細菌学雑誌. 48. 144 (1993)