Air-Liquid Interface Microfluidic Monitoring Sensor Platform for Studying Autophagy Regulation after PM2.5 Exposure.
Lulu ZhengZhijin YangZhiwei XueMengya ChenYule ZhangShuqi CaiKejie ZhengBo DaiSixiu LiuSonglin ZhuangGuodong SuiDa-Wei ZhangPublished in: ACS sensors (2024)
Undoubtedly, a deep understanding of PM 2.5 -induced tumor metastasis at the molecular level can contribute to improving the therapeutic effects of related diseases. However, the underlying molecular mechanism of fine particle exposure through long noncoding RNA (lncRNA) regulation in autophagy and, ultimately, lung cancer (LC) metastasis remains elusive; on the other hand, the related monitoring sensor platform used to investigate autophagy and cell migration is lacking. Herein, this study performed an air-liquid interface microfluidic monitoring sensor (AIMMS) platform to analyze human bronchial epithelial cells after PM 2.5 stimulation. The multiomics analysis [RNA sequencing (RNA-seq) on lncRNA and mRNA expressions separately] showed that MALAT1 was highly expressed in the PM 2.5 treatment group. Furthermore, RNA-seq analysis demonstrated that autophagy-related pathways were activated. Notably, the main mRNAs associated with autophagy regulation, including ATG4D, ATG12, ATG7, and ATG3, were upregulated. Inhibition or downregulation of MALAT1 inhibited autophagy via the ATG4D/ATG12/ATG7/ATG3 pathway after PM 2.5 exposure and ultimately suppressed LC metastasis. Thus, based on the AIMMS platform, we found that MALAT1 might become a promising therapeutic target. Furthermore, this low-cost AIMMS system as a fluorescence sensor integrated with the cell-monitor module could be employed to study LC migration after PM 2.5 exposure. With the fluorescence cell-monitoring module, the platform could be used to observe the migration of LC cells and construct the tumor metastasis model. In the future, several fluorescence probes, including nanoprobes, could be used in the AIMMS platform to investigate many other biological processes, especially cell interaction and migration, in the fields of toxicology and pharmacology.
Keyphrases
- single cell
- rna seq
- high throughput
- air pollution
- particulate matter
- cell death
- endoplasmic reticulum stress
- signaling pathway
- long noncoding rna
- polycyclic aromatic hydrocarbons
- oxidative stress
- induced apoptosis
- heavy metals
- water soluble
- single molecule
- cell migration
- low cost
- simultaneous determination
- endothelial cells
- mass spectrometry
- long non coding rna
- cell proliferation
- liquid chromatography
- high glucose
- risk assessment
- stem cells
- fluorescence imaging
- living cells
- circulating tumor cells
- photodynamic therapy
- binding protein
- high resolution mass spectrometry
- solid phase extraction