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1XLM

D254E, D256E MUTANT OF D-XYLOSE ISOMERASE COMPLEXED WITH AL3 AND XYLITOL

1XLM の概要
エントリーDOI10.2210/pdb1xlm/pdb
分子名称D-XYLOSE ISOMERASE, Xylitol, ALUMINUM ION, ... (4 entities in total)
機能のキーワードisomerase, al, substrate induced metal ion movement, xylose metabolism, pentose shunt
由来する生物種Arthrobacter sp. NRRL
細胞内の位置Cytoplasm: P12070
タンパク質・核酸の鎖数2
化学式量合計86886.66
構造登録者
Gerczei, T.,Bocskei, Z.S.,Szabo, E.,Naray-Szabo, G.,Asboth, B. (登録日: 1997-07-22, 公開日: 1998-01-28, 最終更新日: 2024-05-22)
主引用文献Gerczei, T.,Bocskei, Z.,Szabo, E.,Asboth, B.,Naray-Szabo, G.
Structure determination and refinement of the Al3+ complex of the D254,256E mutant of Arthrobacter D-xylose isomerase at 2.40 A resolution. Further evidence for inhibitor-induced metal ion movement.
Int.J.Biol.Macromol., 25:329-336, 1999
Cited by
PubMed Abstract: The structure of the D254.256E double mutant of Arthrobacter xylose isomerase with Al3+ at both metal-binding sites was determined by the molecular replacement method at a conventional R-factor of 0.179. Binding of the two Al3+ does not alter the overall structure significantly. However, there are local rearrangements in the octahedral co-ordination sphere of the Al3+. The inhibitor molecule moves somewhat away from the active site. Furthermore, evidence was revealed for metal ion movement from site 2(1) to site 2(2) upon double mutation. Xylose isomerase requires two divalent metal cations for activation. The catalytic metal ion is translocated 1.8 A away from its initial position during the catalytic reaction. The fact that both activating and inactivating metals (including Al3+) were found exclusively at a single location in the double mutant was an indication that the consequently missing shuttle may account for the crippled catalytic efficiency.
PubMed: 10456773
DOI: 10.1016/S0141-8130(99)00051-3
主引用文献が同じPDBエントリー
実験手法
X-RAY DIFFRACTION (2.4 Å)
構造検証レポート
Validation report summary of 1xlm
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2026-04-29に公開中

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