Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.

Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.

Human serum albumin presents in its primary structure only one free cysteine (Cys34) which constitutes the most abundant thiol of plasma. An antioxidant role can be attributed to this thiol, which is located in domain I of the protein. Herein we expressed domain I as a secretion protein using the ye...

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Main Authors: Martina Steglich, Rodrigo Lombide, Ignacio López, Madelón Portela, Martín Fló, Mónica Marín, Beatriz Alvarez, Lucía Turell
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2020-01-01
Series:PLoS ONE
Online Access:https://doi.org/10.1371/journal.pone.0240580
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spelling doaj-8c5b75083ae840548c43ce96268bfde32021-03-04T11:10:45ZengPublic Library of Science (PLoS)PLoS ONE1932-62032020-01-011510e024058010.1371/journal.pone.0240580Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.Martina SteglichRodrigo LombideIgnacio LópezMadelón PortelaMartín FlóMónica MarínBeatriz AlvarezLucía TurellHuman serum albumin presents in its primary structure only one free cysteine (Cys34) which constitutes the most abundant thiol of plasma. An antioxidant role can be attributed to this thiol, which is located in domain I of the protein. Herein we expressed domain I as a secretion protein using the yeast Pichia pastoris. In the initial step of ammonium sulfate precipitation, a brown pigment co-precipitated with domain I. Three chromatographic methods were evaluated, aiming to purify domain I from the pigment and other contaminants. Purification was achieved by cation exchange chromatography. The protein behaved as a non-covalent dimer. The primary sequence of domain I and the possibility of reducing Cys34 to the thiol state while avoiding the reduction of internal disulfides were confirmed by mass spectrometry. The reactivity of the thiol towards the disulfide 5,5´-dithiobis(2-nitrobenzoate) was studied and compared to that of full-length albumin. A ~24-fold increase in the rate constant was observed for domain I with respect to the entire protein. These results open the door to further characterization of the Cys34 thiol and its oxidized derivatives.https://doi.org/10.1371/journal.pone.0240580
collection DOAJ
language English
format Article
sources DOAJ
author Martina Steglich
Rodrigo Lombide
Ignacio López
Madelón Portela
Martín Fló
Mónica Marín
Beatriz Alvarez
Lucía Turell
spellingShingle Martina Steglich
Rodrigo Lombide
Ignacio López
Madelón Portela
Martín Fló
Mónica Marín
Beatriz Alvarez
Lucía Turell
Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.
PLoS ONE
author_facet Martina Steglich
Rodrigo Lombide
Ignacio López
Madelón Portela
Martín Fló
Mónica Marín
Beatriz Alvarez
Lucía Turell
author_sort Martina Steglich
title Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.
title_short Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.
title_full Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.
title_fullStr Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.
title_full_unstemmed Expression, purification and initial characterization of human serum albumin domain I and its cysteine 34.
title_sort expression, purification and initial characterization of human serum albumin domain i and its cysteine 34.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2020-01-01
description Human serum albumin presents in its primary structure only one free cysteine (Cys34) which constitutes the most abundant thiol of plasma. An antioxidant role can be attributed to this thiol, which is located in domain I of the protein. Herein we expressed domain I as a secretion protein using the yeast Pichia pastoris. In the initial step of ammonium sulfate precipitation, a brown pigment co-precipitated with domain I. Three chromatographic methods were evaluated, aiming to purify domain I from the pigment and other contaminants. Purification was achieved by cation exchange chromatography. The protein behaved as a non-covalent dimer. The primary sequence of domain I and the possibility of reducing Cys34 to the thiol state while avoiding the reduction of internal disulfides were confirmed by mass spectrometry. The reactivity of the thiol towards the disulfide 5,5´-dithiobis(2-nitrobenzoate) was studied and compared to that of full-length albumin. A ~24-fold increase in the rate constant was observed for domain I with respect to the entire protein. These results open the door to further characterization of the Cys34 thiol and its oxidized derivatives.
url https://doi.org/10.1371/journal.pone.0240580
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