Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein

The tissue of insects, pests, and fungi has a chitin layer followed by protein in the cell membrane. The complete biodegradation of chitin and protein-present in the waste requires the action of two enzymes, namely chitinase, and protease. Combining chitinase and protease in a single protein/enzyme...

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Autores principales: Nilpa, Patel, Chintan, Kapadia, Sayyed, R. Z., El Enshasy, Hesham, El Adawi, Hala, Alhazmi, Alaa, Almalki, Atiah H., Haque, Shafiul
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2022
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8975109/
https://www.ncbi.nlm.nih.gov/pubmed/35363796
http://dx.doi.org/10.1371/journal.pone.0265969
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author Nilpa, Patel
Chintan, Kapadia
Sayyed, R. Z.
El Enshasy, Hesham
El Adawi, Hala
Alhazmi, Alaa
Almalki, Atiah H.
Haque, Shafiul
author_facet Nilpa, Patel
Chintan, Kapadia
Sayyed, R. Z.
El Enshasy, Hesham
El Adawi, Hala
Alhazmi, Alaa
Almalki, Atiah H.
Haque, Shafiul
author_sort Nilpa, Patel
collection PubMed
description The tissue of insects, pests, and fungi has a chitin layer followed by protein in the cell membrane. The complete biodegradation of chitin and protein-present in the waste requires the action of two enzymes, namely chitinase, and protease. Combining chitinase and protease in a single protein/enzyme will serve as a bifunctional enzyme that can efficiently degrade the chitin and protein-rich biomass. The present study was aimed to fuse these two enzymes to produce a single protein and study the kinetics of the recombinant fusion protein. A chitinase and alkaline protease genes were isolated, cloned, and expressed successfully as a fusion product in heterologous host Escherichia coli. The two native genes were successfully fused in E.coli by using flexible glycine–serine (G(4)S)(2) linker (GGGGS, GS linker). The recombinant fusion protein in E.coli showed hydrolyzed chitin and protein on chitin and bovine serum albumin agar plates confirming the successful cloning and expression of chitinase and protease enzymes in a single fusion protein. The common pUC18-T7 mini vector with the ompA signal sequence helps the extracellular expression of fusion protein efficiently. The native gel electrophoresis revealed a molecular mass of purified protein as 92.0 kDa. The fusion protein’s maximal chitinase and protease activity occurred at pH 5.0 and 8.0 and 30 (0)C, respectively resembling the individual enzymes’. In the kinetic studies of the fusion protein, it was observed that the presence of metal ions such as Cu(2+), Na(2+), and Ca(2+); significantly enhanced the enzyme activities while organic solvents oxidants and chemicals have drastically affected the activities of both the enzymes in the fusion protein. No such fusion protein has been produced in a heterologous host yet. The reports on fusion protein with biomass-degrading capacity are also scarce. This is probably the first report of a bifunctional chitinase/protease expressed in E. coli.
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spelling pubmed-89751092022-04-02 Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein Nilpa, Patel Chintan, Kapadia Sayyed, R. Z. El Enshasy, Hesham El Adawi, Hala Alhazmi, Alaa Almalki, Atiah H. Haque, Shafiul PLoS One Research Article The tissue of insects, pests, and fungi has a chitin layer followed by protein in the cell membrane. The complete biodegradation of chitin and protein-present in the waste requires the action of two enzymes, namely chitinase, and protease. Combining chitinase and protease in a single protein/enzyme will serve as a bifunctional enzyme that can efficiently degrade the chitin and protein-rich biomass. The present study was aimed to fuse these two enzymes to produce a single protein and study the kinetics of the recombinant fusion protein. A chitinase and alkaline protease genes were isolated, cloned, and expressed successfully as a fusion product in heterologous host Escherichia coli. The two native genes were successfully fused in E.coli by using flexible glycine–serine (G(4)S)(2) linker (GGGGS, GS linker). The recombinant fusion protein in E.coli showed hydrolyzed chitin and protein on chitin and bovine serum albumin agar plates confirming the successful cloning and expression of chitinase and protease enzymes in a single fusion protein. The common pUC18-T7 mini vector with the ompA signal sequence helps the extracellular expression of fusion protein efficiently. The native gel electrophoresis revealed a molecular mass of purified protein as 92.0 kDa. The fusion protein’s maximal chitinase and protease activity occurred at pH 5.0 and 8.0 and 30 (0)C, respectively resembling the individual enzymes’. In the kinetic studies of the fusion protein, it was observed that the presence of metal ions such as Cu(2+), Na(2+), and Ca(2+); significantly enhanced the enzyme activities while organic solvents oxidants and chemicals have drastically affected the activities of both the enzymes in the fusion protein. No such fusion protein has been produced in a heterologous host yet. The reports on fusion protein with biomass-degrading capacity are also scarce. This is probably the first report of a bifunctional chitinase/protease expressed in E. coli. Public Library of Science 2022-04-01 /pmc/articles/PMC8975109/ /pubmed/35363796 http://dx.doi.org/10.1371/journal.pone.0265969 Text en © 2022 Nilpa et al https://creativecommons.org/licenses/by/4.0/This is an open access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Nilpa, Patel
Chintan, Kapadia
Sayyed, R. Z.
El Enshasy, Hesham
El Adawi, Hala
Alhazmi, Alaa
Almalki, Atiah H.
Haque, Shafiul
Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein
title Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein
title_full Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein
title_fullStr Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein
title_full_unstemmed Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein
title_short Formation of recombinant bifunctional fusion protein: A newer approach to combine the activities of two enzymes in a single protein
title_sort formation of recombinant bifunctional fusion protein: a newer approach to combine the activities of two enzymes in a single protein
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8975109/
https://www.ncbi.nlm.nih.gov/pubmed/35363796
http://dx.doi.org/10.1371/journal.pone.0265969
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