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由两种先前注释错误的非血红素铁加氧酶催化的有机膦酸盐降解新微生物途径。

A New Microbial Pathway for Organophosphonate Degradation Catalyzed by Two Previously Misannotated Non-Heme-Iron Oxygenases.

作者信息

Rajakovich Lauren J, Pandelia Maria-Eirini, Mitchell Andrew J, Chang Wei-Chen, Zhang Bo, Boal Amie K, Krebs Carsten, Bollinger J Martin

出版信息

Biochemistry. 2019 Mar 26;58(12):1627-1647. doi: 10.1021/acs.biochem.9b00044. Epub 2019 Mar 7.

DOI:10.1021/acs.biochem.9b00044
PMID:30789718
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6503667/
Abstract

The assignment of biochemical functions to hypothetical proteins is challenged by functional diversification within many protein structural superfamilies. This diversification, which is particularly common for metalloenzymes, renders functional annotations that are founded solely on sequence and domain similarities unreliable and often erroneous. Definitive biochemical characterization to delineate functional subgroups within these superfamilies will aid in improving bioinformatic approaches for functional annotation. We describe here the structural and functional characterization of two non-heme-iron oxygenases, TmpA and TmpB, which are encoded by a genomically clustered pair of genes found in more than 350 species of bacteria. TmpA and TmpB are functional homologues of a pair of enzymes (PhnY and PhnZ) that degrade 2-aminoethylphosphonate but instead act on its naturally occurring, quaternary ammonium analogue, 2-(trimethylammonio)ethylphosphonate (TMAEP). TmpA, an iron(II)- and 2-(oxo)glutarate-dependent oxygenase misannotated as a γ-butyrobetaine (γbb) hydroxylase, shows no activity toward γbb but efficiently hydroxylates TMAEP. The product, ( R)-1-hydroxy-2-(trimethylammonio)ethylphosphonate [( R)-OH-TMAEP], then serves as the substrate for the second enzyme, TmpB. By contrast to its purported phosphohydrolytic activity, TmpB is an HD-domain oxygenase that uses a mixed-valent diiron cofactor to enact oxidative cleavage of the C-P bond of its substrate, yielding glycine betaine and phosphate. The high specificities of TmpA and TmpB for their N-trimethylated substrates suggest that they have evolved specifically to degrade TMAEP, which was not previously known to be subject to microbial catabolism. This study thus adds to the growing list of known pathways through which microbes break down organophosphonates to harvest phosphorus, carbon, and nitrogen in nutrient-limited niches.

摘要

将生化功能赋予假设的蛋白质面临着许多蛋白质结构超家族内功能多样化的挑战。这种多样化在金属酶中尤为常见,使得仅基于序列和结构域相似性的功能注释不可靠且常常错误。明确的生化特征描述以界定这些超家族内的功能亚组将有助于改进功能注释的生物信息学方法。我们在此描述了两种非血红素铁加氧酶TmpA和TmpB的结构和功能特征,它们由在超过350种细菌中发现的一对基因组聚集基因编码。TmpA和TmpB是一对降解2-氨基乙基膦酸盐的酶(PhnY和PhnZ)的功能同源物,但它们作用于其天然存在的季铵类似物2-(三甲基铵)乙基膦酸盐(TMAEP)。TmpA是一种依赖铁(II)和2-(氧代)戊二酸的加氧酶,被错误注释为γ-丁基甜菜碱(γbb)羟化酶,对γbb无活性,但能有效地将TMAEP羟基化。产物(R)-1-羟基-2-(三甲基铵)乙基膦酸盐[(R)-OH-TMAEP]随后作为第二种酶TmpB的底物。与其声称的磷酸水解活性相反,TmpB是一种HD结构域加氧酶,它使用混合价态的二铁辅因子对其底物的C-P键进行氧化裂解,产生甘氨酸甜菜碱和磷酸盐。TmpA和TmpB对其N-三甲基化底物的高特异性表明它们已经专门进化以降解TMAEP,而TMAEP以前并不被认为会受到微生物分解代谢的作用。因此,这项研究增加了已知的微生物分解有机膦酸盐以在营养有限的生态位中获取磷、碳和氮的途径的数量。

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