Molecular recognition of proteolytic activity in metastatic cancer cells using fluorogenic gold nanoprobes.

Biosens Bioelectron

Department of Radiology, College of Medicine, Yonsei University, Seoul 120-752, Republic of Korea; Severance Integrative Research Institute for Cerebral & Cardiovascular Diseases, Yonsei University Health System, Seoul 120-752, Republic of Korea; YUHS-KRIBB Medical Convergence Research Institute, Seoul 120-752, Republic of Korea. Electronic address:

Published: July 2014

AI Article Synopsis

  • The study focuses on developing specialized nanoprobes that can detect and measure the activity of a specific protein linked to invasive cancer cells, known as MT1-MMP.
  • Researchers confirmed the aggressive nature of certain cancer cell lines (HT1080 and MCF7) through various tests, while designing gold nanoparticles to improve the accuracy of this detection.
  • The results showed that these gold nanoparticles can generate fluorescence when they interact with MT1-MMP, allowing for precise observation of cancer cell activity using advanced imaging techniques.

Article Abstract

We describe the development of biomarker-sensitive nanoprobes based on nanoparticle surface energy transfer (NSET) effect that enabling recognition of the expression of membrane type-1 matrix metalloproteinase (MT1-MMP) anchored on invasive cancer cells and its proteolytic activity simultaneously. First of all, we confirmed invasiveness of cancer cell lines (HT1080 and MCF7) via migration and invasion assay. We also prepared gold nanoparticle (GNP) acts as a quencher for fluorescein isothiocyanate (FITC). This FITC is conjugated in end-terminal of activatable fluorogenic peptide (ActFP). The ActFP attach to surface of GNP (GNP-ActFP) for a targeting moiety and proteolytic activity ligand toward MT1-MMP. The GNP-ActFP can generate fluorescence signal when ActFP is cleaved by proteolytic activity after targeting toward MT1-MMP. In order to study specificity for MT1-MMP, GNP-ActFP is treated to HT1080 and MCF7 cells, and then, we determine the in vitro targeting potential and fluorogenic activity of GNP-ActFP for MT1-MMP via fluorescence multi-reader. We also confirmed fluorogenic activity of GNP-ActFP via confocal microscopic imaging, and finally, endocytosis of GNP-ActFP is observed via cellular transmission electron microscopic imaging.

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http://dx.doi.org/10.1016/j.bios.2014.02.011DOI Listing

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