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膜特异性自旋捕获剂,5-十二烷基碳酰胺-5-N-十二烷基乙酰胺-1-吡咯啉-N-氧化物(diCPO):理论、生物正交荧光成像和 EPR 研究。

Membrane-specific spin trap, 5-dodecylcarbamoyl-5-N-dodecylacetamide-1-pyroline-N-oxide (diCPO): theoretical, bioorthogonal fluorescence imaging and EPR studies.

机构信息

Department of Biological Chemistry and Pharmacology, College of Medicine, The Ohio State University, Columbus, OH 43210, USA.

Davis Heart and Lung Research Institute, Department of Internal Medicine, College of Medicine, The Ohio State University, Columbus, OH 43210, USA.

出版信息

Org Biomol Chem. 2019 Sep 7;17(33):7694-7705. doi: 10.1039/c9ob01334b. Epub 2019 Jul 22.

DOI:10.1039/c9ob01334b
PMID:31328213
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6703941/
Abstract

Membranous organelles are major endogenous sources of reactive oxygen and nitrogen species. When present at high levels, these species can cause macromolecular damage and disease. To better detect and scavenge free radical forms of the reactive species at their sources, we investigated whether nitrone spin traps could be selectively targeted to intracellular membranes using a bioorthogonal imaging approach. Electron paramagnetic resonance imaging demonstrated that the novel cyclic nitrone 5-dodecylcarbamoyl-5-N-dodecylacetamide-1-pyroline-N-oxide (diCPO) could be used to target the nitrone moiety to liposomes composed of phosphatidyl choline. To test localization with authentic membranes in living cells, fluorophores were introduced via strain-promoted alkyne-nitrone cycloaddition (SPANC). Two fluorophore-conjugated alkynes were investigated: hexynamide-fluoresceine (HYA-FL) and dibenzylcyclooctyne-PEG4-5/6-sulforhodamine B (DBCO-Rhod). Computational and mass spectrometry experiments confirmed the cycloadduct formation of DBCO-Rhod (but not HYA-FL) with diCPO in cell-free solution. Confocal microscopy of bovine aortic endothelial cells treated sequentially with diCPO and DBCO-Rhod demonstrated clear localization of fluorescence with intracellular membranes. These results indicate that targeting of nitrone spin traps to cellular membranes is feasible, and that a bioorthogonal approach can aid the interrogation of their intracellular compartmentalization properties.

摘要

膜细胞器是活性氧和氮物种的主要内源性来源。当这些物质水平较高时,它们可能会导致大分子损伤和疾病。为了更好地在其来源处检测和清除活性物质的自由基形式,我们使用生物正交成像方法研究了是否可以使用硝酮自旋捕获物选择性地靶向细胞内膜。电子顺磁共振成像表明,新型环状硝酮 5-十二烷基氨基甲酰基-5-N-十二烷基乙酰胺-1-吡咯啉-N-氧化物(diCPO)可用于将硝酮部分靶向由磷脂酰胆碱组成的脂质体。为了测试活细胞中真实膜的定位,通过应变促进的炔烃-硝酮环加成(SPANC)引入荧光团。研究了两种荧光团缀合的炔烃:己二酰胺-荧光素(HYA-FL)和二苄基环辛炔-PEG4-5/6-磺基罗丹明 B(DBCO-Rhod)。计算和质谱实验证实了 DBCO-Rhod(而不是 HYA-FL)与 diCPO 在无细胞溶液中的环加成产物的形成。用 diCPO 和 DBCO-Rhod 顺序处理的牛主动脉内皮细胞的共焦显微镜显示,荧光明显定位于细胞内膜。这些结果表明,将硝酮自旋捕获物靶向细胞膜是可行的,并且生物正交方法可以帮助研究它们的细胞内区室化特性。

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