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Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing

INTRODUCTION: Pituitary autoantibodies can be determined both in patients with pituitary disease as well as patients with autoimmune endocrine diseases. The purpose of the study was to isolate and purify pituitary autoantigen using sera of patients and the microsomal fraction of the pituitary. MATER...

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Autores principales: Gut, Paweł, Fischbach, Jakub, Ziemnicka, Katarzyna, Bączyk, Maciej, Baszko-Błaszyk, Daria, Wrotkowska, Elżbieta, Ruchała, Marek
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Polish Society of Experimental and Clinical Immunology 2014
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4439984/
https://www.ncbi.nlm.nih.gov/pubmed/26155099
http://dx.doi.org/10.5114/ceji.2014.42122
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author Gut, Paweł
Fischbach, Jakub
Ziemnicka, Katarzyna
Bączyk, Maciej
Baszko-Błaszyk, Daria
Wrotkowska, Elżbieta
Ruchała, Marek
author_facet Gut, Paweł
Fischbach, Jakub
Ziemnicka, Katarzyna
Bączyk, Maciej
Baszko-Błaszyk, Daria
Wrotkowska, Elżbieta
Ruchała, Marek
author_sort Gut, Paweł
collection PubMed
description INTRODUCTION: Pituitary autoantibodies can be determined both in patients with pituitary disease as well as patients with autoimmune endocrine diseases. The purpose of the study was to isolate and purify pituitary autoantigen using sera of patients and the microsomal fraction of the pituitary. MATERIAL AND METHODS: To isolate a pituitary autoantigen, patient sera were used, which showed a strong immune response to pituitary antigens. Pituitary microsomal fractions were prepared from pituitary tissue homogenates. In the study, sera of patients with pituitary disease, Addison and Graves’ disease were used. The initial stages were carried out by affinity chromatography on CN -Br sepharose column whereas purification was continued by column liquid chromatography on AcA54 Ultrogel. Chromatofocusing was performed by Polybuffer exchanger PBE 94. RESULTS: (125)I-labeled pituitary antigens after isolation appeared in column chromatography in three peaks. The first peak contained 50-70 kDa proteins, the second peak – 17 to 22 kDa proteins and the third peak contains (125)-iodides. Three fractions obtained from filtration on Ultrogel were separated in a polyacrylamide gel. In the first peak two bands 67 and 55 kDa appeared. The second peak contained low molecular weight substances, and the third peak contained (125)I. The first peak from Ultrogel was isolated by chromatofocusing – the first peak with pH 5.9 and the second one with pH 4.9. CONCLUSIONS: Isolation and purification of pituitary autoantigen with the use of column liquid chromatography and chromatofocusing resulted in obtainment of two antigenic proteins of specific gravity of 67 and 55 kDa.
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spelling pubmed-44399842015-07-07 Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing Gut, Paweł Fischbach, Jakub Ziemnicka, Katarzyna Bączyk, Maciej Baszko-Błaszyk, Daria Wrotkowska, Elżbieta Ruchała, Marek Cent Eur J Immunol Original Article INTRODUCTION: Pituitary autoantibodies can be determined both in patients with pituitary disease as well as patients with autoimmune endocrine diseases. The purpose of the study was to isolate and purify pituitary autoantigen using sera of patients and the microsomal fraction of the pituitary. MATERIAL AND METHODS: To isolate a pituitary autoantigen, patient sera were used, which showed a strong immune response to pituitary antigens. Pituitary microsomal fractions were prepared from pituitary tissue homogenates. In the study, sera of patients with pituitary disease, Addison and Graves’ disease were used. The initial stages were carried out by affinity chromatography on CN -Br sepharose column whereas purification was continued by column liquid chromatography on AcA54 Ultrogel. Chromatofocusing was performed by Polybuffer exchanger PBE 94. RESULTS: (125)I-labeled pituitary antigens after isolation appeared in column chromatography in three peaks. The first peak contained 50-70 kDa proteins, the second peak – 17 to 22 kDa proteins and the third peak contains (125)-iodides. Three fractions obtained from filtration on Ultrogel were separated in a polyacrylamide gel. In the first peak two bands 67 and 55 kDa appeared. The second peak contained low molecular weight substances, and the third peak contained (125)I. The first peak from Ultrogel was isolated by chromatofocusing – the first peak with pH 5.9 and the second one with pH 4.9. CONCLUSIONS: Isolation and purification of pituitary autoantigen with the use of column liquid chromatography and chromatofocusing resulted in obtainment of two antigenic proteins of specific gravity of 67 and 55 kDa. Polish Society of Experimental and Clinical Immunology 2014-04-17 2014 /pmc/articles/PMC4439984/ /pubmed/26155099 http://dx.doi.org/10.5114/ceji.2014.42122 Text en Copyright © Central European Journal of Immunology 2014 http://creativecommons.org/licenses/by-nc-nd/3.0/ This is an Open Access article distributed under the terms of the Creative Commons Attribution-Noncommercial 3.0 Unported License, permitting all non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Original Article
Gut, Paweł
Fischbach, Jakub
Ziemnicka, Katarzyna
Bączyk, Maciej
Baszko-Błaszyk, Daria
Wrotkowska, Elżbieta
Ruchała, Marek
Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing
title Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing
title_full Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing
title_fullStr Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing
title_full_unstemmed Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing
title_short Purification of pituitary autoantigen by column liquid chromatography and chromatofocusing
title_sort purification of pituitary autoantigen by column liquid chromatography and chromatofocusing
topic Original Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4439984/
https://www.ncbi.nlm.nih.gov/pubmed/26155099
http://dx.doi.org/10.5114/ceji.2014.42122
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