In Vivo Brain Sampling Using a Microextraction Probe Reveals Metabolic Changes in Rodents after Deep Brain Stimulation

微透析 化学 体内 固相微萃取 代谢物 代谢组学 脑深部刺激 色谱法 生物化学 质谱法 内科学 气相色谱-质谱法 生物 医学 细胞外 生物技术 疾病 帕金森病
作者
Nathaly Reyes-Garcés,Mustansir Diwan,Ezel Boyacı,Germán Augusto Gómez-Ríos,Barbara Bojko,José N. Nobrega,Francis Rodriguez Bambico,Clement Hamani,Janusz Pawliszyn
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:91 (15): 9875-9884 被引量:44
标识
DOI:10.1021/acs.analchem.9b01540
摘要

Brain metabolomics is an emerging field that complements the more traditional approaches of neuroscience. However, typical brain metabolomics workflows require that animals be sacrificed and tend to involve tedious sample preparation steps. Microdialysis, the standard technique to study brain metabolites in vivo, is encumbered by significant limitations in the analysis of hydrophobic metabolites, which are prone to adsorption losses on microdialysis equipment. An alternative sampling method suitable for in vivo brain studies is solid-phase microextraction (SPME). In SPME, a small probe coated with a biocompatible polymer is employed to extract/enrich analytes from biological matrices. In this work, we report the use of SPME and liquid chromatography-mass spectrometry for untargeted in vivo analysis of rodent's brains after deep brain stimulation (DBS). First, metabolite changes occurring in brain hippocampi after application of 3 h of DBS to the animals' prefrontal cortex were monitored with the proposed approach. As SPME allows for nonlethal sampling, the same group of animals was sampled again after 8 days of daily DBS therapy. After acute DBS, we detected changes in a broad range of metabolites, including the amino acid citrulline, which may reflect changes in nitric oxide production, as well as various phospho- and glycosphingolipids. Measurements conducted after chronic DBS showed a decrease in hippocampal corticosterone, indicating that DBS may have a regulatory effect in the hypothalamic-pituitary-adrenal axis. Our findings demonstrate the potential of in vivo SPME as a tool of scientific and clinical interest capable of revealing changes in a wide range of metabolites in brain tissue.
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