Analytical characterization and purification of a commercial extract of enzymes: A case study
- Autores
- Llerena Suster, Carlos Rafael; Briand, Laura Estefanía; Morcelle del Valle, Susana Raquel
- Año de publicación
- 2014
- Idioma
- inglés
- Tipo de recurso
- artículo
- Estado
- versión publicada
- Descripción
- This paper presents a rational strategy to identify and quantify the components of a commercial extractof the lipase B of Candida antarctica that can be extended to the analytical investigation of other crudeextracts of enzymes. These information provided the fundamental knowledge for the development of amethodology to obtain highly pure and catalytically active CALB enzyme.The commercial extract Lipozyme®was subjected to a series of analytical techniques that alloweddetermining the presence of a non-soluble fraction; nucleic acids; benzoate and sorbate species and amixture of three proteins. Particularly, it is worth noticing that the Bradford assay using CALB as standardinstead of BSA proved to be a more reliable and accurate methodology to quantify the protein con-tent of the assayed enzymatic samples. Size exclusion chromatography coupled with anionic exchangechromatography using a non-conventional, easy to remove buffer system such as ammonia–ammoniumacetate afforded a sample that retains 47% of the proteins (being CALB the only enzymatic component ofthe purified sample) with a hydrolytic activity higher than the crude extract.
Centro de Investigación de Proteínas Vegetales - Materia
-
Biología
Protein purification
Protein quantification
CALBUV absorbance
Size exclusion chromatography
Ion exchange chromatography - Nivel de accesibilidad
- acceso abierto
- Condiciones de uso
- http://creativecommons.org/licenses/by/4.0/
- Repositorio
.jpg)
- Institución
- Universidad Nacional de La Plata
- OAI Identificador
- oai:sedici.unlp.edu.ar:10915/191968
Ver los metadatos del registro completo
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Analytical characterization and purification of a commercial extract of enzymes: A case studyLlerena Suster, Carlos RafaelBriand, Laura EstefaníaMorcelle del Valle, Susana RaquelBiologíaProtein purificationProtein quantificationCALBUV absorbanceSize exclusion chromatographyIon exchange chromatographyThis paper presents a rational strategy to identify and quantify the components of a commercial extractof the lipase B of Candida antarctica that can be extended to the analytical investigation of other crudeextracts of enzymes. These information provided the fundamental knowledge for the development of amethodology to obtain highly pure and catalytically active CALB enzyme.The commercial extract Lipozyme®was subjected to a series of analytical techniques that alloweddetermining the presence of a non-soluble fraction; nucleic acids; benzoate and sorbate species and amixture of three proteins. Particularly, it is worth noticing that the Bradford assay using CALB as standardinstead of BSA proved to be a more reliable and accurate methodology to quantify the protein con-tent of the assayed enzymatic samples. Size exclusion chromatography coupled with anionic exchangechromatography using a non-conventional, easy to remove buffer system such as ammonia–ammoniumacetate afforded a sample that retains 47% of the proteins (being CALB the only enzymatic component ofthe purified sample) with a hydrolytic activity higher than the crude extract.Centro de Investigación de Proteínas Vegetales2014-09-01info:eu-repo/semantics/articleinfo:eu-repo/semantics/publishedVersionArticulohttp://purl.org/coar/resource_type/c_6501info:ar-repo/semantics/articuloapplication/pdf11-20http://sedici.unlp.edu.ar/handle/10915/191968enginfo:eu-repo/semantics/altIdentifier/issn/0927-7765info:eu-repo/semantics/altIdentifier/doi/10.1016/j.colsurfb.2014.05.029info:eu-repo/semantics/openAccesshttp://creativecommons.org/licenses/by/4.0/Creative Commons Attribution 4.0 International (CC BY 4.0)reponame:SEDICI (UNLP)instname:Universidad Nacional de La Platainstacron:UNLP2026-03-26T09:21:46Zoai:sedici.unlp.edu.ar:10915/191968Institucionalhttp://sedici.unlp.edu.ar/Universidad públicaNo correspondehttp://sedici.unlp.edu.ar/oai/snrdalira@sedici.unlp.edu.arArgentinaNo correspondeNo correspondeNo correspondeopendoar:13292026-03-26 09:21:47.188SEDICI (UNLP) - Universidad Nacional de La Platafalse |
| dc.title.none.fl_str_mv |
Analytical characterization and purification of a commercial extract of enzymes: A case study |
| title |
Analytical characterization and purification of a commercial extract of enzymes: A case study |
| spellingShingle |
Analytical characterization and purification of a commercial extract of enzymes: A case study Llerena Suster, Carlos Rafael Biología Protein purification Protein quantification CALBUV absorbance Size exclusion chromatography Ion exchange chromatography |
| title_short |
Analytical characterization and purification of a commercial extract of enzymes: A case study |
| title_full |
Analytical characterization and purification of a commercial extract of enzymes: A case study |
| title_fullStr |
Analytical characterization and purification of a commercial extract of enzymes: A case study |
| title_full_unstemmed |
Analytical characterization and purification of a commercial extract of enzymes: A case study |
| title_sort |
Analytical characterization and purification of a commercial extract of enzymes: A case study |
| dc.creator.none.fl_str_mv |
Llerena Suster, Carlos Rafael Briand, Laura Estefanía Morcelle del Valle, Susana Raquel |
| author |
Llerena Suster, Carlos Rafael |
| author_facet |
Llerena Suster, Carlos Rafael Briand, Laura Estefanía Morcelle del Valle, Susana Raquel |
| author_role |
author |
| author2 |
Briand, Laura Estefanía Morcelle del Valle, Susana Raquel |
| author2_role |
author author |
| dc.subject.none.fl_str_mv |
Biología Protein purification Protein quantification CALBUV absorbance Size exclusion chromatography Ion exchange chromatography |
| topic |
Biología Protein purification Protein quantification CALBUV absorbance Size exclusion chromatography Ion exchange chromatography |
| dc.description.none.fl_txt_mv |
This paper presents a rational strategy to identify and quantify the components of a commercial extractof the lipase B of Candida antarctica that can be extended to the analytical investigation of other crudeextracts of enzymes. These information provided the fundamental knowledge for the development of amethodology to obtain highly pure and catalytically active CALB enzyme.The commercial extract Lipozyme®was subjected to a series of analytical techniques that alloweddetermining the presence of a non-soluble fraction; nucleic acids; benzoate and sorbate species and amixture of three proteins. Particularly, it is worth noticing that the Bradford assay using CALB as standardinstead of BSA proved to be a more reliable and accurate methodology to quantify the protein con-tent of the assayed enzymatic samples. Size exclusion chromatography coupled with anionic exchangechromatography using a non-conventional, easy to remove buffer system such as ammonia–ammoniumacetate afforded a sample that retains 47% of the proteins (being CALB the only enzymatic component ofthe purified sample) with a hydrolytic activity higher than the crude extract. Centro de Investigación de Proteínas Vegetales |
| description |
This paper presents a rational strategy to identify and quantify the components of a commercial extractof the lipase B of Candida antarctica that can be extended to the analytical investigation of other crudeextracts of enzymes. These information provided the fundamental knowledge for the development of amethodology to obtain highly pure and catalytically active CALB enzyme.The commercial extract Lipozyme®was subjected to a series of analytical techniques that alloweddetermining the presence of a non-soluble fraction; nucleic acids; benzoate and sorbate species and amixture of three proteins. Particularly, it is worth noticing that the Bradford assay using CALB as standardinstead of BSA proved to be a more reliable and accurate methodology to quantify the protein con-tent of the assayed enzymatic samples. Size exclusion chromatography coupled with anionic exchangechromatography using a non-conventional, easy to remove buffer system such as ammonia–ammoniumacetate afforded a sample that retains 47% of the proteins (being CALB the only enzymatic component ofthe purified sample) with a hydrolytic activity higher than the crude extract. |
| publishDate |
2014 |
| dc.date.none.fl_str_mv |
2014-09-01 |
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info:eu-repo/semantics/article info:eu-repo/semantics/publishedVersion Articulo http://purl.org/coar/resource_type/c_6501 info:ar-repo/semantics/articulo |
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article |
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publishedVersion |
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http://sedici.unlp.edu.ar/handle/10915/191968 |
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eng |
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eng |
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