Expression and characterization of plant aspartic protease nepenthesin-1 from Nepenthes gracilis
Language English Country United States Media print-electronic
Document type Journal Article, Research Support, Non-U.S. Gov't
PubMed
24365662
DOI
10.1016/j.pep.2013.12.005
PII: S1046-5928(13)00274-X
Knihovny.cz E-resources
- Keywords
- Carnivorous plant, Nepenthesin, Plant aspartic protease, Protease characterization, Protein stability, Recombinant protein,
- MeSH
- Aspartic Acid Proteases chemistry genetics metabolism MeSH
- Disulfides MeSH
- Hydrogen-Ion Concentration MeSH
- Magnoliopsida enzymology genetics MeSH
- Carnivory MeSH
- Reducing Agents MeSH
- Recombinant Proteins chemistry genetics metabolism MeSH
- Plant Proteins chemistry genetics metabolism MeSH
- Enzyme Stability MeSH
- Temperature MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
- Names of Substances
- Aspartic Acid Proteases MeSH
- Disulfides MeSH
- Reducing Agents MeSH
- Recombinant Proteins MeSH
- Plant Proteins MeSH
Carnivorous plants of the genus Nepenthes produce their own aspartic proteases, nepenthesins, to digest prey trapped in their pitchers. Nepenthesins differ significantly in sequence from other aspartic proteases in the animal or even plant kingdoms. This difference, which also brings more cysteine residues into the structure of these proteases, can be a cause of uniquely high temperature and pH stabilities of nepenthesins. Their detailed structure characterization, however, has not previously been possible due to low amounts of protease present in the pitcher fluid and also due to limited accessibility of Nepenthes plants. In the present study we describe a convenient way for obtaining high amounts of nepenthesin-1 from Nepenthes gracilis using heterologous production in Escherichia coli. The protein can be easily refolded in vitro and its characteristics are very close to those described for a natural enzyme isolated from the pitcher fluid. Similarly to the natural enzyme, recombinant nepenthesin-1 is sensitive to denaturing and reducing agents. It also has maximal activity around pH 2.5, shows unusual stability at high pH and its activity is not irreversibly inhibited even after prolonged incubation in the basic pH range. On the other hand, temperature stability of the recombinant enzyme is lower in comparison with the natural enzyme, which can be attributed to missing N-glycosylation in the recombinant protein.
Department of Biochemistry and Molecular Biology University of Calgary Calgary Alberta Canada
Institute of Microbiology v v i Academy of Sciences of the Czech Republic Prague Czech Republic
References provided by Crossref.org
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Structural Dynamics of Lytic Polysaccharide Monooxygenase during Catalysis
Regulation of enzyme activities in carnivorous pitcher plants of the genus Nepenthes
Addressing proteolytic efficiency in enzymatic degradation therapy for celiac disease
Crystallization of nepenthesin I using a low-pH crystallization screen
