Time-Dependent pH Scanning of the Acid-Induced Unfolding of Human Serum Albumin Reveals Stabilization of the Native Form by Palmitic Acid Binding

Del Giudice, Alessandra; Dicko, Cedric; Galantini, Luciano; Pavel, Nicolae V.

Time-Dependent pH Scanning of the Acid-Induced Unfolding of Human Serum Albumin Reveals Stabilization of the Native Form by Palmitic Acid Binding

Mark

Del Giudice, Alessandra ; Dicko, Cedric ^LU

; Galantini, Luciano and Pavel, Nicolae V. (2017) In Journal of Physical Chemistry B 121(17). p.4388-4399

Abstract: The most abundant plasma protein, human serum albumin (HSA), is known to undergo several conformational transitions in an acidic environment. To avoid buffer effects and correlate global and local structural changes, we developed a continuous acidification method and simultaneously monitored the protein changes by both small-angle scattering (SAXS) and fluorescence. The progressive acidification, based on the hydrolysis of glucono-δ-lactone from pH 7 to pH 2.5, highlighted a multistep unfolding involving the putative F form (pH 4) and an extended and flexible conformation (pH < 3.5). The scattering profile of the F form was extracted by component analysis and further 3D modeled. The effect of acid unfolding at this intermediate stage... (More); The most abundant plasma protein, human serum albumin (HSA), is known to undergo several conformational transitions in an acidic environment. To avoid buffer effects and correlate global and local structural changes, we developed a continuous acidification method and simultaneously monitored the protein changes by both small-angle scattering (SAXS) and fluorescence. The progressive acidification, based on the hydrolysis of glucono-δ-lactone from pH 7 to pH 2.5, highlighted a multistep unfolding involving the putative F form (pH 4) and an extended and flexible conformation (pH < 3.5). The scattering profile of the F form was extracted by component analysis and further 3D modeled. The effect of acid unfolding at this intermediate stage was assigned to the rearrangement of the three albumin domains drifting apart toward a more elongated conformation, with a partial unfolding of one of the outer domains. To test the stabilizing effect of fatty acids, here palmitic acid, we compared the acid unfolding process of albumin with and without ligand. We found that when binding the ligand, the native conformation was favored up to lower pH values. Our approach solved the problem of realizing a continuous, homogeneous, and tunable acidification with simultaneous characterization applicable to study processes triggered by a pH decrease.
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Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/dbbf17a1-d47b-4a00-bd0f-32344d6f78de

author

Del Giudice, Alessandra ; Dicko, Cedric ^LU

; Galantini, Luciano and Pavel, Nicolae V.

organization

Pure and Applied Biochemistry

publishing date

2017-05-04

type

Contribution to journal

publication status

published

subject

Biophysics

in

Journal of Physical Chemistry B

volume

121

issue

17

pages

12 pages

publisher

The American Chemical Society (ACS)

external identifiers

pmid:28414449
wos:000400881300007
scopus:85020193318

ISSN

1520-6106

DOI

10.1021/acs.jpcb.7b01342

language

English

LU publication?

yes

id

dbbf17a1-d47b-4a00-bd0f-32344d6f78de

date added to LUP

2017-06-28 10:48:00

date last changed

2024-05-12 16:29:28

@article{dbbf17a1-d47b-4a00-bd0f-32344d6f78de,
  abstract     = {{<p>The most abundant plasma protein, human serum albumin (HSA), is known to undergo several conformational transitions in an acidic environment. To avoid buffer effects and correlate global and local structural changes, we developed a continuous acidification method and simultaneously monitored the protein changes by both small-angle scattering (SAXS) and fluorescence. The progressive acidification, based on the hydrolysis of glucono-δ-lactone from pH 7 to pH 2.5, highlighted a multistep unfolding involving the putative F form (pH 4) and an extended and flexible conformation (pH &lt; 3.5). The scattering profile of the F form was extracted by component analysis and further 3D modeled. The effect of acid unfolding at this intermediate stage was assigned to the rearrangement of the three albumin domains drifting apart toward a more elongated conformation, with a partial unfolding of one of the outer domains. To test the stabilizing effect of fatty acids, here palmitic acid, we compared the acid unfolding process of albumin with and without ligand. We found that when binding the ligand, the native conformation was favored up to lower pH values. Our approach solved the problem of realizing a continuous, homogeneous, and tunable acidification with simultaneous characterization applicable to study processes triggered by a pH decrease.</p>}},
  author       = {{Del Giudice, Alessandra and Dicko, Cedric and Galantini, Luciano and Pavel, Nicolae V.}},
  issn         = {{1520-6106}},
  language     = {{eng}},
  month        = {{05}},
  number       = {{17}},
  pages        = {{4388--4399}},
  publisher    = {{The American Chemical Society (ACS)}},
  series       = {{Journal of Physical Chemistry B}},
  title        = {{Time-Dependent pH Scanning of the Acid-Induced Unfolding of Human Serum Albumin Reveals Stabilization of the Native Form by Palmitic Acid Binding}},
  url          = {{http://dx.doi.org/10.1021/acs.jpcb.7b01342}},
  doi          = {{10.1021/acs.jpcb.7b01342}},
  volume       = {{121}},
  year         = {{2017}},
}

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Time-Dependent pH Scanning of the Acid-Induced Unfolding of Human Serum Albumin Reveals Stabilization of the Native Form by Palmitic Acid Binding