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对来自多糖裂解酶家族18的细菌海藻酸盐裂解酶N端延伸在成熟、底物识别和催化过程中作用的分子洞察。

Molecular insight into the role of the N-terminal extension in the maturation, substrate recognition, and catalysis of a bacterial alginate lyase from polysaccharide lyase family 18.

作者信息

Dong Sheng, Wei Tian-Di, Chen Xiu-Lan, Li Chun-Yang, Wang Peng, Xie Bin-Bin, Qin Qi-Long, Zhang Xi-Ying, Pang Xiu-Hua, Zhou Bai-Cheng, Zhang Yu-Zhong

机构信息

From the State Key Laboratory of Microbial Technology and the Marine Biotechnology Research Center, Shandong University, Jinan 250100, China.

From the State Key Laboratory of Microbial Technology and.

出版信息

J Biol Chem. 2014 Oct 24;289(43):29558-69. doi: 10.1074/jbc.M114.584573. Epub 2014 Sep 10.

Abstract

Bacterial alginate lyases, which are members of several polysaccharide lyase (PL) families, have important biological roles and biotechnological applications. The mechanisms for maturation, substrate recognition, and catalysis of PL18 alginate lyases are still largely unknown. A PL18 alginate lyase, aly-SJ02, from Pseudoalteromonas sp. 0524 displays a β-jelly roll scaffold. Structural and biochemical analyses indicated that the N-terminal extension in the aly-SJ02 precursor may act as an intramolecular chaperone to mediate the correct folding of the catalytic domain. Molecular dynamics simulations and mutational assays suggested that the lid loops over the aly-SJ02 active center serve as a gate for substrate entry. Molecular docking and site-directed mutations revealed that certain conserved residues at the active center, especially those at subsites +1 and +2, are crucial for substrate recognition. Tyr(353) may function as both a catalytic base and acid. Based on our results, a model for the catalysis of aly-SJ02 in alginate depolymerization is proposed. Moreover, although bacterial alginate lyases from families PL5, 7, 15, and 18 adopt distinct scaffolds, they share the same conformation of catalytic residues, reflecting their convergent evolution. Our results provide the foremost insight into the mechanisms of maturation, substrate recognition, and catalysis of a PL18 alginate lyase.

摘要

细菌海藻酸裂解酶是几个多糖裂解酶(PL)家族的成员,具有重要的生物学作用和生物技术应用。PL18海藻酸裂解酶的成熟、底物识别和催化机制在很大程度上仍然未知。一种来自假交替单胞菌属0524的PL18海藻酸裂解酶aly-SJ02具有β-果冻卷支架结构。结构和生化分析表明,aly-SJ02前体中的N端延伸可能作为分子内伴侣介导催化结构域的正确折叠。分子动力学模拟和突变分析表明,aly-SJ02活性中心上方的盖子环充当底物进入的门。分子对接和定点突变表明,活性中心的某些保守残基,特别是亚位点+1和+2处的残基,对底物识别至关重要。酪氨酸(353)可能同时起到催化碱和酸的作用。基于我们的结果,提出了aly-SJ02催化海藻酸解聚的模型。此外,尽管来自PL5、7、15和18家族的细菌海藻酸裂解酶采用不同的支架结构,但它们具有相同的催化残基构象,反映了它们的趋同进化。我们的结果为PL18海藻酸裂解酶的成熟、底物识别和催化机制提供了最前沿的见解。

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