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真菌烟曲霉中表二硫二氧哌嗪二硫醇吉妥毒素螯合锌的系统影响:天然产物功能的新方向。

Systems impact of zinc chelation by the epipolythiodioxopiperazine dithiol gliotoxin in Aspergillus fumigatus: a new direction in natural product functionality.

机构信息

Department of Biology, Maynooth University, Co. Kildare, Ireland.

出版信息

Metallomics. 2018 Jun 20;10(6):854-866. doi: 10.1039/c8mt00052b.

DOI:10.1039/c8mt00052b
PMID:29897360
Abstract

The non-ribosomal peptide gliotoxin, which autoinduces its own biosynthesis, has potent anti-fungal activity, especially in the combined absence of the gliotoxin oxidoreductase GliT and bis-thiomethyltransferase GtmA. Dithiol gliotoxin (DTG) is a substrate for both of these enzymes. Herein we demonstrate that DTG chelates Zn2+ (m/z 424.94), rapidly chelates Zn2+ from Zn(4-(2-pyridylazo)-resorcinol) (Zn(PAR)2) and also inhibits a Zn2+-dependent alkaline phosphatase (AP). Zn2+ addition rescues AP function following DTG-associated inhibition, and pre-incubation of DTG with Zn2+ completely protects AP activity. Zn2+ (1-50 μM) also significantly relieves the potent gliotoxin-mediated inhibition of Aspergillus fumigatus ΔgliT::ΔgtmA (p < 0.05), which infers in vivo dithiol gliotoxin-mediated sequestration of free Zn2+ or chelation from intracellular metalloenzymes as inhibitory mechanisms. Quantitative proteomic analysis revealed that excess Zn2+ alters the effect of gliotoxin on A. fumigatus ΔgliT, with differential abundance of secondary metabolism-associated proteins in the combinatorial condition. GtmA abundance increased 18.8 fold upon co-addition of gliotoxin and Zn2+ compared to gliotoxin alone, possibly to compensate for disruption to GtmA activity, as seen in in vitro assays. Furthermore, DTG effected significant in vitro aggregation of a number of protein classes, including Zn2+-dependent enzymes, while proteins were protected from aggregation by pre-incubating DTG with Zn2+. We conclude that DTG can act in vivo as a Zn2+ chelator, which can significantly impede A. fumigatus growth in the absence of GliT and GtmA.

摘要

非核糖体肽Gliotoxin 能够自动诱导自身生物合成,具有很强的抗真菌活性,尤其是在Gliotoxin 氧化还原酶GliT 和双硫甲基转移酶 GtmA 同时缺失的情况下。二硫代Gliotoxin (DTG) 是这两种酶的底物。本文中,我们证明 DTG 螯合 Zn2+(m/z 424.94),能够迅速从 Zn(4-(2-吡啶偶氮)-间苯二酚) (Zn(PAR)2) 中螯合 Zn2+,还能抑制依赖 Zn2+的碱性磷酸酶 (AP)。DTG 相关抑制作用后,添加 Zn2+可恢复 AP 功能,而 DTG 与 Zn2+预孵育则完全保护 AP 活性。Zn2+(1-50 μM)还能显著缓解Gliotoxin 对 Aspergillus fumigatus ΔgliT::ΔgtmA 的强烈抑制作用(p < 0.05),这意味着在体内,二硫代 Gliotoxin 通过螯合游离 Zn2+或从细胞内金属酶中螯合 Zn2+来抑制,是其抑制机制之一。定量蛋白质组学分析显示,过量的 Zn2+ 改变了 Gliotoxin 对 A. fumigatus ΔgliT 的影响,在组合条件下,次级代谢相关蛋白的丰度发生变化。与单独使用 Gliotoxin 相比,当 Gliotoxin 和 Zn2+ 同时添加时,GtmA 的丰度增加了 18.8 倍,这可能是为了补偿 GtmA 活性的破坏,就像在体外测定中看到的那样。此外,DTG 会显著影响多种蛋白类别的体外聚集,包括依赖 Zn2+的酶,而蛋白类在与 DTG 预孵育 Zn2+时则能免受聚集的影响。我们得出结论,DTG 在体内可作为 Zn2+螯合剂,在没有 GliT 和 GtmA 的情况下,可显著阻碍 A. fumigatus 的生长。

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