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香蕉主要过敏原内切-β-1,3-葡聚糖酶1.45埃分辨率的晶体结构,作为乳胶-水果综合征的分子基础。

Crystal structure at 1.45-A resolution of the major allergen endo-beta-1,3-glucanase of banana as a molecular basis for the latex-fruit syndrome.

作者信息

Receveur-Bréchot Véronique, Czjzek Mirjam, Barre Annick, Roussel Alain, Peumans Willy J, Van Damme Els J M, Rougé Pierre

机构信息

Architecture et Fonction des Macromolécules Biologiques, Marseille, France.

出版信息

Proteins. 2006 Apr 1;63(1):235-42. doi: 10.1002/prot.20876.

Abstract

Resolution of the crystal structure of the banana fruit endo-beta-1,3-glucanase by synchrotron X-ray diffraction at 1.45-A resolution revealed that the enzyme possesses the eightfold beta/alpha architecture typical for family 17 glycoside hydrolases. The electronegatively charged catalytic central cleft harbors the two glutamate residues (Glu94 and Glu236) acting as hydrogen donor and nucleophile residue, respectively. Modeling using a beta-1,3 linked glucan trisaccharide as a substrate confirmed that the enzyme readily accommodates a beta-1,3-glycosidic linkage in the slightly curved catalytic groove between the glucose units in positions -2 and -1 because of the particular orientation of residue Tyr33 delimiting subsite -2. The location of Phe177 in the proximity of subsite +1 suggested that the banana glucanase might also cleave beta-1,6-branched glucans. Enzymatic assays using pustulan as a substrate demonstrated that the banana glucanase can also cleave beta-1,6-glucans as was predicted from docking experiments. Similar to many other plant endo-beta-1,3-glucanases, the banana glucanase exhibits allergenic properties because of the occurrence of well-conserved IgE-binding epitopes on the surface of the enzyme. These epitopes might trigger some cross-reactions toward IgE antibodies and thus account for the IgE-binding cross-reactivity frequently reported in patients with the latex-fruit syndrome.

摘要

通过同步辐射X射线衍射以1.45埃分辨率解析香蕉果实内切β-1,3-葡聚糖酶的晶体结构,结果表明该酶具有17家族糖苷水解酶典型的八重β/α结构。带负电荷的催化中心裂隙中含有两个谷氨酸残基(Glu94和Glu236),分别作为氢供体和亲核残基。以β-1,3连接的葡聚糖三糖为底物进行建模证实,由于界定亚位点-2的残基Tyr33的特定取向,该酶能够在-2和-1位葡萄糖单元之间略微弯曲的催化凹槽中轻松容纳β-1,3-糖苷键。Phe177位于亚位点+1附近,这表明香蕉葡聚糖酶也可能切割β-1,6-分支的葡聚糖。以 pustulan 为底物的酶活性测定表明,香蕉葡聚糖酶也能够切割β-1,6-葡聚糖,这与对接实验的预测结果一致。与许多其他植物内切β-1,3-葡聚糖酶类似,香蕉葡聚糖酶因其表面存在保守的IgE结合表位而具有致敏特性。这些表位可能引发一些针对IgE抗体的交叉反应,从而解释了乳胶-水果综合征患者中频繁报道的IgE结合交叉反应性。

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