Study of cell and drug interactions based on dual-mode detection using SPR and fluorescence imaging

Lulu Zhang; Runye Liu; Luyao Liu; Xiaoxing Xing; Haoyuan Cai; Yongdong Fu; Jianhai Sun; Wang Ruan; Jian Chen; Xianbo Qiu; Duli Yu

doi:10.1016/j.saa.2024.124170

Study of cell and drug interactions based on dual-mode detection using SPR and fluorescence imaging

Spectrochim Acta A Mol Biomol Spectrosc. 2024 Jun 5:314:124170. doi: 10.1016/j.saa.2024.124170. Epub 2024 Mar 17.

Authors

Lulu Zhang¹, Runye Liu², Luyao Liu², Xiaoxing Xing², Haoyuan Cai³, Yongdong Fu², Jianhai Sun³, Wang Ruan³, Jian Chen³, Xianbo Qiu², Duli Yu²

Affiliations

¹ College of Information Science and Technology, Beijing University of Chemical Technology, Beijing 100029, China. Electronic address: llzhang@buct.edu.cn.
² College of Information Science and Technology, Beijing University of Chemical Technology, Beijing 100029, China.
³ State Key Laboratory of Transducer Technology, Aerospace Information Research Institute, Chinese Academy of Sciences, Beijing 100190, China.

PMID: 38513319
DOI: 10.1016/j.saa.2024.124170

Abstract

The investigation of the interactions between cells and drugs forms a crucial aspect of biological and clinical medical studies. Generally, single-cell or local-cellular studies require a microscopic imaging system with high magnifications, which suffers from low detection throughputs and poor time responses. The study presented in this paper combined SPR and fluorescence to achieve cell localization, real-time monitoring of cell images and quantitative analysis of drugs. In order to obtain more comprehensive, accurate and real-time data, a dual-mode system based on surface plasmon resonance (SPR) and fluorescence was constructed based on a 4× magnification lens. This enables simultaneous studies of an entire cell and a specific region of the cell membrane. An adaptive adjustment algorithm was established for distorted SPR images, achieving temporal and spatial matching of the dual-mode detection. The combination of SPR and fluorescence not only achieved micro-detection but also complemented the qualitative or quantitative limitations of SPR or fluorescence method alone. In system characterization, the response signal of SPR was noticed to increase with the increasing concentration of EGF in stimulated cells. It indicated that this platform could be employed for quantitative detection of the cell membrane region. Upon addition of EGF, a peak in the SPR curve was observed, and the cells in the corresponding SPR image turned whiter. This indicated that the platform can simultaneously monitor the SPR response signal and image changes. The response time of fluorescence in EGF testing was several seconds earlier than SPR, revealing that signal transduction first occurred in the whole cell and then propagated to the cell membrane region. The inhibitory ability of Gefitinib on cells was verified in a fast and real-time manner within 20 min. The results indicated that the detection limit of this method was 20 IU/mL for EGF and 10 µg/mL for Gefitinib. In conclusion, this study demonstrates the advantages of SPR and fluorescence dual-mode techniques in the analysis of cell-drug interactions, as well as their strong potential in drug screening.

Keywords: Cell-drug interactions; Dual-mode detection; Fluorescence; Surface plasmon resonance.

MeSH terms

Biosensing Techniques*
Drug Interactions
Epidermal Growth Factor
Gefitinib
Optical Imaging
Surface Plasmon Resonance* / methods

Substances

Epidermal Growth Factor
Gefitinib