Genetically engineered horseradish peroxidase for facilitated purification from baculovirus cultures by cation-exchange chromatography

Levin, Gustavo Javier; Mendive, Fernando; Targovnik, Hector Manuel; Cascone, Osvaldo; Miranda, Maria Victoria

info:eu-repo/semantics/article

Fecha

2005-09-10

Registro en:

Levin, Gustavo Javier; Mendive, Fernando; Targovnik, Hector Manuel; Cascone, Osvaldo; Miranda, Maria Victoria; Genetically engineered horseradish peroxidase for facilitated purification from baculovirus cultures by cation-exchange chromatography; Elsevier Science; Journal of Biotechnology; 118; 4; 10-9-2005; 363-369

0168-1656

http://hdl.handle.net/11336/116258

CONICET Digital

CONICET

https://repositorioslatinoamericanos.uchile.cl/handle/2250/4401899

Autor

Levin, Gustavo Javier

Mendive, Fernando

Targovnik, Hector Manuel

Cascone, Osvaldo

Miranda, Maria Victoria

Institución

Consejo Nacional de Investigaciones Científicas y Tecnológicas (Argentina)

Resumen

An engineered horseradish peroxidase isozyme C (HRP C) gene was constructed by the addition of a 6xArg fusion tail to 6xHis-HRP C by the PCR strategy. The 6xHis-6xArg-HRP C cDNA was expressed in the Sf9 insect cell line from Spodoptera frugiperda infected with Autographa californica nuclear polyhedrosis virus. The recombinant peroxidase isoelectric point was 9.5 as judged by isoelectric focusing and was purified directly from the culture medium at day-6 post-infection by cation-exchange chromatography or immobilised metal ion-affinity chromatography. While the former technique gave a yield of 98.5% with a purification factor of 130, the latter gave only a 68% yield with a purification factor of 140. Results obtained provide evidence that the poly-Arg tag is more effective than the poly-His tag for peroxidase purification from a baculovirus expression system.

Materias

FUSION TAIL

IMMOBILISED METAL ION-AFFINITY CHROMATOGRAPHY

ION-EXCHANGE CHROMATOGRAPHY

PEROXIDASE

PURIFICATION

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