Expression of the Caldariomyces fumago chloroperoxidase in Aspergillus niger and characterization of the recombinant enzyme

article





Conesa, A.

Velde, F. van de

Rantwijk, F. van

Sheldon, R.A.

Hondel, C.A.M.J.J. van den

Punt, P.J.
The Caldariomyces fumago chloroperoxidase was successfully expressed in Aspergillus niger. The recombinant enzyme was produced in the culture medium as an active protein and could be purified by a three-step purification procedure. The catalytic behavior of recombinant chloroperoxidase (rCPO) was studied and compared with that of native CPO. The specific chlorination activity (47 units/nmol) of rCPO and its pH optimum (pH 2.75) were very similar to those of native CPO. rCPO catalyzes the oxidation of various substrates in comparable yields and selectivities to native CPO. Indole was oxidized to 2-oxindole with 99% selectivity and thioanisole to the corresponding R-sulfoxide (enantiomeric excess >98%). Incorporation of 18O from labeled H218O2 into the oxidized products was 100% in both cases. Molecular Sequence Numbers: GENBANK: AJ300448; Chemicals/CAS: chloride peroxidase, 9055-20-3; hydrogen, 12385-13-6, 1333-74-0; indole, 120-72-9; oxindole, 59-48-3; oxygen, 7782-44-7; sulfoxide, 120-62-7; thioanisole, 100-68-5; Chloride Peroxidase, EC 1.11.1.10; Fungal Proteins; Recombinant Proteins
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AspergillusAspergillus nigerFungiLeptoxyphium fumagoCaldariomycesAspergillus nigerCatalysisChloride PeroxidaseFungal ProteinsRecombinant ProteinsSubstrate Specificity
TNO Identifier
72309
Repository link
https://resolver.tno.nl/uuid:dab9006e-3932-4a2f-a46f-9c65c077b9bd
ISSN
00219258
Source
Journal of Biological Chemistry, 276(21), pp. 17635-17640.
Pages
17635-17640
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