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6DPI

Crystal Structure of Bacillus Halodurans Ribonuclease H1 K196A in Complex with an RNA/DNA Hybrid: Reaction in 10 mM Mg2+ and 200 mM Rb+ for 40 s at 21 C

6DPI の概要
エントリーDOI10.2210/pdb6dpi/pdb
分子名称Ribonuclease H, 5'-R(*AP*CP*AP*U)-3' portion of intact RNA (5'-R(*AP*CP*AP*UP*CP*G)-3'), 5'-R(P*CP*G)-3' portion of intact RNA (5'-R(*AP*CP*AP*UP*CP*G)-3'), ... (10 entities in total)
機能のキーワードprotein-rna-dna complex, double helix, rna hydrolysis, in crystallo catalysis, metal dependent catalysis, monovalent cations, divalent cations, hydrolase-rna-dna complex, hydrolase/rna/dna
由来する生物種Bacillus halodurans
詳細
タンパク質・核酸の鎖数4
化学式量合計20892.77
構造登録者
Samara, N.L.,Yang, W. (登録日: 2018-06-09, 公開日: 2018-08-15, 最終更新日: 2023-10-11)
主引用文献Samara, N.L.,Yang, W.
Cation trafficking propels RNA hydrolysis.
Nat. Struct. Mol. Biol., 25:715-721, 2018
Cited by
PubMed Abstract: Catalysis by members of the RNase H superfamily of enzymes is generally believed to require only two Mg ions that are coordinated by active-site carboxylates. By examining the catalytic process of Bacillus halodurans RNase H1 in crystallo, however, we found that the two canonical Mg ions and an additional K failed to align the nucleophilic water for RNA cleavage. Substrate alignment and product formation required a second K and a third Mg, which replaced the first K and departed immediately after cleavage. A third transient Mg has also been observed for DNA synthesis, but in that case it coordinates the leaving group instead of the nucleophile as in the case of the RNase H1 hydrolysis reaction. These transient cations have no contact with the enzymes. Other DNA and RNA enzymes that catalyze consecutive cleavage and strand-transfer reactions in a single active site may similarly require cation trafficking coordinated by the substrate.
PubMed: 30076410
DOI: 10.1038/s41594-018-0099-4
主引用文献が同じPDBエントリー
実験手法
X-RAY DIFFRACTION (1.347 Å)
構造検証レポート
Validation report summary of 6dpi
検証レポート(詳細版)ダウンロードをダウンロード

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件を2024-10-30に公開中

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