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海七鳃鳗(Petromyzon marinus)血浆及血浆细胞外囊泡中的蛋白质翻译后脱亚氨基化特征

Post-translational protein deimination signatures in sea lamprey (Petromyzon marinus) plasma and plasma-extracellular vesicles.

作者信息

Rast Jonathan P, D'Alessio Stefania, Kraev Igor, Lange Sigrun

机构信息

Emory University School of Medicine, Pathology & Laboratory Medicine, Atlanta, GA, 30322, USA.

Tissue Architecture and Regeneration Research Group, School of Life Sciences, University of Westminster, London, W1W 6UW, UK.

出版信息

Dev Comp Immunol. 2021 Dec;125:104225. doi: 10.1016/j.dci.2021.104225. Epub 2021 Aug 3.

DOI:10.1016/j.dci.2021.104225
PMID:34358577
Abstract

Lampreys are a jawless vertebrate species belonging to an ancient vertebrate lineage that diverged from a common ancestor with humans ~500 million years ago. The sea lamprey (Petromyzon marinus) has a filter feeding ammocoete larval stage that metamorphoses into a parasitic adult, feeding both on teleost and elasmobranch fish. Lampreys are a valuable comparative model species for vertebrate immunity and physiology due to their unique phylogenetic position, unusual adaptive immune system, and physiological adaptions such as tolerance to salinity changes and urea. Peptidylarginine deiminases (PADs) are a phylogenetically conserved enzyme family which catalyses post-translational deimination/citrullination in target proteins, enabling proteins to gain new functions (moonlighting). The identification of deiminated protein targets in species across phylogeny may provide novel insights into post-translational regulation of physiological and pathophysiological processes. Extracellular vesicles (EVs) are membrane vesicles released from cells that carry cargos of small molecules and proteins for cellular communication, involved in both normal and pathological processes. The current study identified deimination signatures in proteins of both total plasma and plasma-EVs in sea lamprey and furthermore reports the first characterisation of plasma-EVs in lamprey. EVs were poly-dispersed in the size range of 40-500 nm, similar to what is observed in other taxa, positive for CD63 and Flotillin-1. Plasma-EV morphology was confirmed by transmission electron microscopy. Assessment of deimination/citrullination signatures in lamprey plasma and plasma-EVs, revealed 72 deimination target proteins involved in immunity, metabolism and gene regulation in whole plasma, and 37 target proteins in EVs, whereof 24 were shared targets. Furthermore, the presence of deiminated histone H3, indicative of gene-regulatory mechanisms and also a marker of neutrophil extracellular trap formation (NETosis), was confirmed in lamprey plasma. Functional protein network analysis revealed some differences in KEGG and GO pathways of deiminated proteins in whole plasma compared with plasma-EVs. For example, while common STRING network clusters in plasma and plasma-EVs included Peptide chain elongation, Viral mRNA translation, Glycolysis and gluconeogenesis, STRING network clusters specific for EVs only included: Cellular response to heat stress, Muscle protein and striated muscle thin filament, Nucleosome, Protein processing in endoplasmic reticulum, Nucleosome and histone deacetylase complex. STRING network clusters specific for plasma were: Adipokinetic hormone receptor activity, Fibrinogen alpha/beta chain family, peptidase S1A, Glutathione synthesis and recycling-arginine, Fructose 1,6-bisphosphate metabolic process, Carbon metabolism and lactate dehydrogenase activity, Post-translational protein phosphorylation, Regulation of insulin-like growth factor transport and clotting cascade. Overall, for the EV citrullinome, five STRING network clusters, 10 KEGG pathways, 15 molecular GO pathways and 29 Reactome pathways were identified, compared with nine STRING network clusters, six KEGG pathways, two Molecular GO pathways and one Reactome pathway specific for whole plasma; while further pathways were shared. The reported findings indicate that major pathways relevant for immunity and metabolism are targets of deimination in lamprey plasma and plasma-EVs, with some differences, and may help elucidating roles for the conserved PAD enzyme family in regulation of immune and metabolic function throughout phylogeny.

摘要

七鳃鳗是一种无颌脊椎动物,属于古老的脊椎动物谱系,约在5亿年前与人类从共同祖先分化而来。海七鳃鳗(Petromyzon marinus)有一个滤食性的沙隐虫幼虫阶段,会变态发育成寄生性成虫,以硬骨鱼和软骨鱼为食。由于七鳃鳗独特的系统发育位置、不寻常的适应性免疫系统以及诸如对盐度变化和尿素的耐受性等生理适应性,它们是研究脊椎动物免疫和生理学的宝贵比较模型物种。肽基精氨酸脱亚氨酶(PADs)是一个系统发育保守的酶家族,可催化靶蛋白的翻译后脱亚胺基化/瓜氨酸化,使蛋白质获得新功能(兼职功能)。在整个系统发育中的物种中鉴定瓜氨酸化蛋白靶标,可能为生理和病理生理过程的翻译后调控提供新见解。细胞外囊泡(EVs)是从细胞释放的膜囊泡,携带小分子和蛋白质货物用于细胞间通讯,参与正常和病理过程。当前研究鉴定了海七鳃鳗全血浆和血浆EVs中蛋白质的脱亚胺基化特征,并且进一步报道了七鳃鳗血浆EVs的首次表征。EVs在40 - 500nm大小范围内多分散,与在其他分类群中观察到的情况类似,对CD63和小窝蛋白-1呈阳性。通过透射电子显微镜确认了血浆EVs的形态。对七鳃鳗血浆和血浆EVs中脱亚胺基化/瓜氨酸化特征的评估,揭示了全血浆中有72个参与免疫、代谢和基因调控的脱亚胺基化靶蛋白,以及EVs中有37个靶蛋白,其中24个是共同靶标。此外,在七鳃鳗血浆中证实了瓜氨酸化组蛋白H3的存在,这表明了基因调控机制,也是中性粒细胞胞外诱捕网形成(NETosis)的标志物。功能蛋白网络分析显示,与血浆EVs相比,全血浆中脱亚胺基化蛋白的KEGG和GO途径存在一些差异。例如,虽然血浆和血浆EVs中常见的STRING网络簇包括肽链延伸、病毒mRNA翻译、糖酵解和糖异生,但仅EVs特有的STRING网络簇包括:细胞对热应激的反应、肌肉蛋白和横纹肌细肌丝、核小体、内质网中的蛋白质加工、核小体和组蛋白脱乙酰酶复合体。血浆特有的STRING网络簇包括:脂肪动激素受体活性、纤维蛋白原α/β链家族、肽酶S1A、谷胱甘肽合成与精氨酸循环利用、果糖1,6 - 二磷酸代谢过程、碳代谢和乳酸脱氢酶活性、翻译后蛋白质磷酸化、胰岛素样生长因子运输调节和凝血级联反应。总体而言,对于EV瓜氨酸化蛋白质组,鉴定出了5个STRING网络簇、10条KEGG途径、15条分子GO途径和29条Reactome途径,而全血浆特有的有9个STRING网络簇、6条KEGG途径、2条分子GO途径和1条Reactome途径;同时还有一些共享途径。报道的研究结果表明,与免疫和代谢相关的主要途径是七鳃鳗血浆和血浆EVs中脱亚胺基化的靶标,存在一些差异,这可能有助于阐明保守的PAD酶家族在整个系统发育中调节免疫和代谢功能的作用。

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