On‐line high‐performance liquid chromatography coupled with biochemical detection method for screening of <i>α</i>‐glucosidase inhibitors in green tea

Guo, Peng-Cheng; Shen, Hua-Dan; Fang, Jiangji; Ding, Tian-Ming; Ding, Xuehua; Liu, Junfeng

doi:10.1002/bmc.4281

Cited by 6 publications

(1 citation statement)

References 33 publications

(43 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…In the early 1990s, direct post-column coupling of a continuous-flow enzyme assay to a liquid chromatographic (LC) system with UV-Vis, fluorescence or mass spectrometry (MS) detection received attention since it eliminated the fractionation steps ( Greis, 2007 ; Shi et al, 2009 ; Malherbe et al, 2012 ; Zhang et al, 2013 ; Peng et al, 2015 ; De-qiang et al, 2016 ; Zhao et al, 2016 ). This post-column screening format coupled with MS detection is a relevant tool for online enzymatic activity/affinity screening and was subsequently used to identify bioactive compounds in NP crude extracts ( Schenk et al, 2003 ; van Elswijk et al, 2003 ; Kool et al, 2011 ; Guo et al, 2018 ; Wu et al, 2018 ).…”

Section: Introductionmentioning

confidence: 99%

A Comprehensive 2D-LC/MS Online Platform for Screening of Acetylcholinesterase Inhibitors

Seidl

Lima

Leme

et al. 2022

Front. Mol. Biosci.

View full text Add to dashboard Cite

The continuous interest in discovering new bioactive molecules derived from natural products (NP) has stimulated the development of improved screening assays to help overcome challenges in NP-based drug discovery. Here, we describe a unique platform for the online screening of acetylcholinesterase inhibitors without the need for pre-treating the sample. In the current study, we have demonstrated the ability to combine reversed-phase separation with a capillary immobilized enzyme reactor (cIMER) in two-dimensional liquid chromatography system coupled with mass spectrometry detection. We systematically investigated the effects of method parameters that are of practical significance and are known to affect the enzyme assay and interfere in the analysis such as: bioreactor dimensions, loop sizes, amount of immobilized enzyme, second dimension flow rates, reaction time, substrate concentration, presence of organic modifier, limit of detection and signal suppression. The performance of this new platform was evaluated using a mixture containing three known AChE inhibitors (tacrine, galanthamine and donepezil) and an ethanolic extract obtained from the dry bulbs of Hippeastrum calyptratum (Amaryllidaceae) was investigated to provide a proof of concept of the applicability of the platform for the analysis of complex mixtures such as those derived from NPs.

show abstract