Tn3とγδのキメラトランスポゼ-スを用いたトランスポゼ-スの逆向き繰り返し配列(IR)に対する結合特異性決定部位の解析〔英文〕
スポンサーリンク
概要
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To analyze the region that determines the specificity of binding of the Tn3 transposase to the terminal inverted repeat sequences (IR), we first determined the nucleotide sequence of a Tn3-family transposon, γδ, which is supposed to encode a transposase similar to that of Tn3. γδ was 5981 bp in length and contained three coding frames: Two were the genes, tupA and tnpR, encoding transposase (1002 amino acids) and resolvase/repressor (183 amino acids), respectively, and the third, named tnpX, encoding a protein (698 amino acids) of unknown function but containing two NTP-binding motifs. Utilizing the tnpA sequence, we then constructed a series of Tn3-γδ hybrid genes encoding chimeric proteins in the N-terminal segments of the transposases (amino acid position 1 to 242 of Tn3 or 1 to 243 of γδ), which has been previously shown to be responsible for specific binding of transposase to IR sequences in Tn3. Examination of their DNA-binding activities revealed that the subsegment of the N-terminus from amino acid position 1 to 109 determines the specificity of binding to the IR sequences. The third coding frame found in γδ, tnpX, is located downstream of tnpR and is expressed from the tnpR promoter in the absence of the tnpR gene product, resolvase/repressor, to produce a protein that inhibits the growth of the host cells. Possible roles of this protein are discussed.
- 日本遺伝学会の論文
- 1994-06-25
著者
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Maekawa Takafumi
Institute Of Molecular And Cellular Biosciences The University Of Tokyo
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Ohtsubo Eiichi
Institute Of Molecular And Cellular Biosciences The University Of Tokyo
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大坪 栄一
Institute of Applied Microbiology, University of Tokyo
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前川 隆文
Institute of Molecular and Cellular Biosciences, The University of Tokyo
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