New insights into the altered binding capacity of pharmaceutical-grade human serum albumin: site-specific binding studies by induced circular dichroism spectroscopy

Anna Tramarin; Daniele Tedesco; Marina Naldi; Maurizio Baldassarre; Carlo Bertucci; Manuela Bartolini

doi:10.1016/j.jpba.2018.09.022

New insights into the altered binding capacity of pharmaceutical-grade human serum albumin: site-specific binding studies by induced circular dichroism spectroscopy

J Pharm Biomed Anal. 2019 Jan 5:162:171-178. doi: 10.1016/j.jpba.2018.09.022. Epub 2018 Sep 12.

Authors

Anna Tramarin¹, Daniele Tedesco¹, Marina Naldi², Maurizio Baldassarre³, Carlo Bertucci¹, Manuela Bartolini⁴

Affiliations

¹ Department of Pharmacy and Biotechnology, Alma Mater Studiorum - University of Bologna, Via Belmeloro 6, 40126 Bologna, Italy.
² Department of Pharmacy and Biotechnology, Alma Mater Studiorum - University of Bologna, Via Belmeloro 6, 40126 Bologna, Italy; Center for Applied Biomedical Research (CRBA), S. Orsola-Malpighi Hospital, Via Massarenti 9, 40138 Bologna, Italy.
³ Center for Applied Biomedical Research (CRBA), S. Orsola-Malpighi Hospital, Via Massarenti 9, 40138 Bologna, Italy; Department of Medical and Surgical Sciences, Alma Mater Studiorum - University of Bologna, Via Massarenti 9, 40138 Bologna, Italy.
⁴ Department of Pharmacy and Biotechnology, Alma Mater Studiorum - University of Bologna, Via Belmeloro 6, 40126 Bologna, Italy. Electronic address: manuela.bartolini3@unibo.it.

PMID: 30248608
DOI: 10.1016/j.jpba.2018.09.022

Abstract

The ADMET profile of drugs is strongly affected by human serum albumin (HSA), due to its leading role as carrier of poorly soluble compounds in plasma; a critical assessment of the binding capacity of HSA and the evaluation of binding competition between drugs are therefore pivotal for a reliable pharmacokinetic and pharmacodynamic characterization. In clinical practice, a potential source of impairment in the binding properties of HSA is the use of octanoate and N-acetyltryptophan as stabilizers during the production of pharmaceutical-grade HSA for infusion (i-HSA), which is currently administered in the treatment of a growing range of pathological conditions. The peculiar sensitivity of circular dichroism (CD) spectroscopy towards the stereochemical features of high-affinity binding events is herein exploited to achieve a site-specific assessment of the effect of stabilizers on the binding properties of i-HSA. The binding affinity and capacity of fatty-acid-free HSA towards site-selective induced circular dichroism (ICD) markers for the three high-affinity binding sites of HSA was compared to that of i-HSA submitted to ultrafiltration and dialysis to remove both stabilizers. Results showed a considerable impairment of the binding capacity of i-HSA at site II and a relatively lower influence on the binding properties of site I. Ultrafiltration proved to be ineffective in depleting octanoate, while the proposed dialysis protocol, which involves a pH-induced reversible unfolding of the protein, resulted in a total clearance of both stabilizers, confirmed by the full restoration of the binding properties of HSA at all binding sites. The outcomes of this study proved that CD spectroscopy is a suitable technique to evaluate the binding properties of i-HSA, ensuring an assessment of the availability of the binding sites and the possibility of monitoring the clearance of stabilizers. Eventually, the proposed method for their depletion might constitute a connection bridge between albumin in vitro studies and its clinical applications.

Keywords: Binding capacity; Dialysis; Human serum albumin; Induced circular dichroism; N-Acetyltryptophan; Octanoate.

MeSH terms

Binding Sites
Caprylates / chemistry
Chemistry, Pharmaceutical / methods*
Circular Dichroism*
Dialysis / methods
Hydrogen-Ion Concentration
Protein Binding
Protein Conformation
Protein Stability
Protein Unfolding
Serum Albumin, Human / chemistry
Serum Albumin, Human / metabolism*
Structure-Activity Relationship
Tryptophan / analogs & derivatives
Tryptophan / chemistry
Ultrafiltration / methods

Substances

Caprylates
N-acetyltryptophan
Tryptophan
octanoic acid
Serum Albumin, Human