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糖苷酶 BcX 活性位点的双模态底物结合。

Bimodal substrate binding in the active site of the glycosidase BcX.

机构信息

Leiden Institute of Chemistry, Leiden University, The Netherlands.

出版信息

FEBS J. 2024 Oct;291(19):4222-4239. doi: 10.1111/febs.17251. Epub 2024 Aug 26.

DOI:10.1111/febs.17251
PMID:39185686
Abstract

Bacillus circulans xylanase (BcX) from the glycoside hydrolase family 11 degrades xylan through a retaining, double-displacement mechanism. The enzyme is thought to hydrolyze glycosidic bonds in a processive manner and has a large, active site cleft, with six subsites allowing the binding of six xylose units. Such an active site architecture suggests that oligomeric xylose substrates can bind in multiple ways. In the crystal structure of the catalytically inactive variant BcX E78Q, the substrate xylotriose is observed in the active site, as well as bound to the known secondary binding site and a third site on the protein surface. Nuclear magnetic resonance (NMR) titrations with xylose oligomers of different lengths yield nonlinear chemical shift trajectories for active site nuclei resonances, indicative of multiple binding orientations for these substrates for which binding and dissociation are in fast exchange on the NMR timescale, exchanging on the micro- to millisecond timescale. Active site binding can be modeled with a 2 : 1 model with dissociation constants in the low and high millimolar range. Extensive mutagenesis of active site residues indicates that tight binding occurs in the glycon binding site and is stabilized by Trp9 and the thumb region. Mutations F125A and W71A lead to large structural rearrangements. Binding at the glycon site is sensed throughout the active site, whereas the weak binding mostly affects the aglycon site. The interactions with the two active site locations are largely independent of each other and of binding at the secondary binding site.

摘要

生淀粉环糊精酶(BcX)属于糖苷水解酶家族 11,通过保留、双置换机制降解木聚糖。该酶被认为以渐进的方式水解糖苷键,具有较大的活性位点裂缝,有六个亚位点允许结合六个木糖单元。这种活性位点结构表明,寡糖木糖底物可以以多种方式结合。在催化失活变体 BcX E78Q 的晶体结构中,观察到底物木三糖存在于活性位点中,以及与已知的次级结合位点和蛋白质表面上的第三个位点结合。用不同长度的木糖寡糖进行核磁共振(NMR)滴定,活性位点核共振的化学位移轨迹呈非线性,表明这些底物有多种结合取向,其结合和解离在 NMR 时间尺度上快速交换,在微秒至毫秒时间尺度上交换。活性位点的结合可以用 2:1 模型进行建模,解离常数在低毫摩尔和高毫摩尔范围内。对活性位点残基的广泛突变表明,紧密结合发生在糖基结合位点,并由色氨酸 9 和拇指区域稳定。F125A 和 W71A 突变导致了较大的结构重排。糖基结合位点的结合在整个活性位点都能被感知,而弱结合主要影响非糖基结合位点。与两个活性位点位置的相互作用在很大程度上是相互独立的,与次级结合位点的结合也是相互独立的。

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引用本文的文献

1
Terminal spin labeling of xylotriose strongly affects interactions in the active site of xylanase BcX.木三糖的末端自旋标记强烈影响木聚糖酶BcX活性位点的相互作用。
J Biomol NMR. 2025 Jun;79(2):99-113. doi: 10.1007/s10858-025-00459-w.