Biodegradation of polyurethanes by Serratia liquefaciens L135 and its polyurethanase: In silico and in vitro analyses

Cleonice Aparecida Salgado; Júnio Gonçalves Silva; Felipe Alves de Almeida; Maria Cristina Dantas Vanetti

doi:10.1016/j.envpol.2023.122016

Biodegradation of polyurethanes by Serratia liquefaciens L135 and its polyurethanase: In silico and in vitro analyses

Environ Pollut. 2023 Sep 15:333:122016. doi: 10.1016/j.envpol.2023.122016. Epub 2023 Jun 18.

Authors

Cleonice Aparecida Salgado¹, Júnio Gonçalves Silva², Felipe Alves de Almeida³, Maria Cristina Dantas Vanetti⁴

Affiliations

¹ Department of Microbiology, Universidade Federal de Viçosa (UFV), Viçosa, MG, Brazil. Electronic address: cleonice.salgado@ufv.br.
² Department of Chemistry, Universidade Federal de Minas Gerais (UFMG), Belo Horizonte, MG, Brazil. Electronic address: junio.ufv@gmail.com.
³ Instituto de Laticínios Cândido Tostes (ILCT), Empresa de Pesquisa Agropecuária de Minas Gerais (EPAMIG), Juiz de Fora, MG, Brazil. Electronic address: felipe.almeida@epamig.br.
⁴ Department of Microbiology, Universidade Federal de Viçosa (UFV), Viçosa, MG, Brazil. Electronic address: mvanetti@ufv.br.

PMID: 37339733
DOI: 10.1016/j.envpol.2023.122016

Abstract

Polyurethanes (PUs) are found in many everyday products and their disposal leads to environmental accumulation. Therefore, there is an urgent need to develop ecologically sustainable techniques to biodegrade and recycle this recalcitrant polymer and replace traditional methods that form harmful by-products. Serratia liquefaciens L135 secretes a polyurethanase with lipase activity, and this study explores the biodegradation of PUs by this bacterium and its enzyme through in silico and in vitro analyses. PUs monomers and tetramers were constructed in silico and tested with modeled and validated structure of the polyurethanase from S. liquefaciens. The molecular docking showed that all PUs monomers presented favorable interactions with polyurethanase (values of binding energy between -84.75 and -121.71 kcal mol^-1), including PU poly[4,4'-methylenebis (phenyl isocyanate)-alt-1,4-butanediol/di (propylene glycol)/polycaprolactone] (PCLMDI). Due to repulsive steric interactions, tetramers showed less favorable interactions (values between 24.26 and -45.50 kcal mol^-1). In vitro analyses evaluated the biodegradation of PUs: Impranil® and PCLMDI; this latter showed high binding energy with this polyurethanase in silico. The biodegradation of Impranil® by S. liquefaciens and its partially purified polyurethanase was confirmed in agar by forming a transparent halo. Impranil® disks inoculated with S. liquefaciens and incubated at 30 °C for six days showed rupture of the PU structure, possibly due to the formation of cracks visualized by scanning electron microscopy (SEM). PCLMDI films were also biodegraded by S. liquefaciens after 60 days of incubation, with the formation of pores and cracks visualized by SEM. The biodegradation may have occurred due to the action of polyurethanase produced by this bacterium. This work provides essential information on the potential of S. liquefaciens to biodegrade PUs through in silico analyses combined with in vitro analyses.

Keywords: Biofilm; Impranil; Lipase; Molecular docking; Polymer.

MeSH terms

Biodegradation, Environmental
Humans
Molecular Docking Simulation
Polyurethanes / chemistry
Serratia liquefaciens* / metabolism
Suppuration

Substances

Polyurethanes