Luminescent Ln(III)-Metallopeptide Sensors for Monitoring Pseudomonas aeruginosa Elastase B Activity in Complex Biological Media

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Sánchez-Fernández, Rosalía
Sandá Ares, Martín
Lamas, Nerea
Cuesta, Trinidad
Martínez, José Luis

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Sánchez-Fernández, R.; Sandá-Ares, M.; Lamas, N.; Cuesta, T.; Martínez, J. L.; Fernandez-Trillo, P.; Pazos, E. Luminescent Ln(III)-Metallopeptide Sensors for Monitoring Pseudomonas Aeruginosa Elastase B Activity in Complex Biological Media. ACS Sens. 2024, 9 (10), 5052–5057. https://doi.org/10.1021/acssensors.4c00986

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Abstract

[Abstract] The detection and monitoring of Pseudomonas aeruginosa and its virulence factors, such as the LasB protease, are crucial for managing bacterial infections. Traditional fluorescent sensors for this protease face limitations in bacterial cultures due to interference from pigments like pyoverdine secreted by this opportunistic pathogen. We report here a Ln(III)-metallopeptide that combines a DO3A-Ln(III) complex and a sensitizing unit via a short peptide sequence as a simple, tunable, and selective probe for detecting P. aeruginosa’s LasB. The probe’s luminescence switches off in the presence of P. aeruginosa’s secretome due to LasB cleavage but remains stable in other bacterial environments, such as non-LasB-secreting P. aeruginosa strains or E. coli cultures. It also resists degradation by other proteases, like human leukocyte elastase and trypsin, and remains stable in the presence of bioanalytes related to P. aeruginosa infections, such as glutathione, H2O2, and pyocyanin, and in complex media like FBS. Importantly, time-gated experiments completely remove the background fluorescence of P. aeruginosa pigments, thus demonstrating the potential of the developed Ln(III)-metallopeptide for real-time monitoring of LasB activity in bacterial cultures.

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Financiado para publicación en acceso aberto: Universidade da Coruña/CISUG

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Atribución 3.0 España
Atribución 3.0 España

Except where otherwise noted, this item's license is described as Atribución 3.0 España