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Expression of a Cutinase of Moniliophthora roreri with Polyester and PET-Plastic Residues Degradation Activity
- Source :
- Microbiology Spectrum, Microbiology Spectrum, Vol 9, Iss 3 (2021)
- Publication Year :
- 2021
- Publisher :
- American Society for Microbiology, 2021.
-
Abstract
- Cutinases are enzymes produced by phytopathogenic fungi like Moniliophthora roreri. The three genome-located cutinase genes of M. roreri were amplified from cDNA of fungi growing in different induction culture media for cutinase production. The mrcut1 gene was expressed in the presence of a cacao cuticle, while the mrcut2 and mrcut3 genes were expressed when an apple cuticle was used as the inducer. The sequences of all genes were obtained and analyzed by bioinformatics tools to determine the presence of signal peptides, introns, glycosylation, and regulatory sequences. Also, the theoretical molecular weight and pI were obtained and experimentally confirmed. Finally, cutinase 1 from M. roreri (MRCUT1) was selected for heterologous expression in Escherichia coli. Successful overexpression of MRCUT1 was observed with the highest enzyme activity of 34,036 U/mg under the assay conditions at 40°C and pH 8. Furthermore, the degradation of different synthetic polyesters was evaluated; after 21 days, 59% of polyethylene succinate (PES), 43% of polycaprolactone (PCL), and 31% of polyethylene terephthalate (PET) from plastic residues were degraded. IMPORTANCE Plastic pollution is exponentially increasing; even the G20 has recognized an urgent need to implement actions to reduce it. In recent years, searching for enzymes that can degrade plastics, especially those based on polyesters such as PET, has been increasing as they can be a green alternative to the actual plastic degradation process. A promising option in recent years refers to biological tools such as enzymes involved in stages of partial and even total degradation of some plastics. In this context, the MRCUT1 enzyme can degrade polyesters contained in plastic residues in a short time. Besides, there is limited knowledge about the biochemical properties of cutinases from M. roreri. Commonly, fungal enzymes are expressed as inclusion bodies in E. coli with reduced activity. Interestingly, the successful expression of one cutinase of M. roreri in E. coli with enhanced activity is described.
- Subjects :
- Microbiology (medical)
Cutinase
polyester degradation
Glycosylation
Physiology
Polyesters
Moniliophthora roreri
Gene Expression
Context (language use)
medicine.disease_cause
Microbiology
chemistry.chemical_compound
Genetics
medicine
Escherichia coli
Amino Acid Sequence
cutinase
chemistry.chemical_classification
Cacao
General Immunology and Microbiology
Ecology
biology
Base Sequence
Polyethylene Terephthalates
Gene Amplification
Succinates
Cell Biology
biology.organism_classification
QR1-502
Enzyme assay
Infectious Diseases
Enzyme
Biodegradation, Environmental
chemistry
Biochemistry
biology.protein
Environmental Pollutants
Heterologous expression
Polyethylenes
Agaricales
Environmental Pollution
Carboxylic Ester Hydrolases
Nucleic Acid Amplification Techniques
Plastics
Research Article
Subjects
Details
- Language :
- English
- ISSN :
- 21650497
- Volume :
- 9
- Issue :
- 3
- Database :
- OpenAIRE
- Journal :
- Microbiology Spectrum
- Accession number :
- edsair.doi.dedup.....5f21c5611db7696b00670ef521a9f096