HDL Isolated by Immunoaffinity, Ultracentrifugation, or Precipitation is Compositionally and Functionally Distinct

Michael Holzer; Senka Ljubojevic-Holzer; Douglas Ricardo Souza Junior; Julia T Stadler; Alankrita Rani; Hubert Scharnagl; Graziella Eliza Ronsein; Gunther Marsche

doi:10.1016/j.jlr.2022.100307

HDL Isolated by Immunoaffinity, Ultracentrifugation, or Precipitation is Compositionally and Functionally Distinct

J Lipid Res. 2022 Dec;63(12):100307. doi: 10.1016/j.jlr.2022.100307. Epub 2022 Oct 29.

Authors

Michael Holzer¹, Senka Ljubojevic-Holzer², Douglas Ricardo Souza Junior³, Julia T Stadler⁴, Alankrita Rani⁴, Hubert Scharnagl⁵, Graziella Eliza Ronsein³, Gunther Marsche⁶

Affiliations

¹ Division of Pharmacology, Otto-Loewi Research Centre, Medical University of Graz, Graz, Austria; BioTechMed Graz, Graz, Austria. Electronic address: michael.holzer@medunigraz.at.
² BioTechMed Graz, Graz, Austria; Department of Cardiology, Medical University of Graz, Graz, Austria; Division of Molecular Biology and Biochemistry, Gottfried Schatz Research Center, Medical University of Graz, Graz, Austria.
³ Department of Biochemistry, Institute of Chemistry, University of São Paulo, São Paulo, Brazil.
⁴ Division of Pharmacology, Otto-Loewi Research Centre, Medical University of Graz, Graz, Austria.
⁵ Clinical Institute of Medical and Chemical Laboratory Diagnostics, Medical University of Graz, Graz, Austria.
⁶ Division of Pharmacology, Otto-Loewi Research Centre, Medical University of Graz, Graz, Austria; BioTechMed Graz, Graz, Austria.

Abstract

The HDL proteome has been widely recognized as an important mediator of HDL function. While a variety of HDL isolation methods exist, their impact on the HDL proteome and its associated function remain largely unknown. Here, we compared three of the most common methods for HDL isolation, namely immunoaffinity (IA), density gradient ultracentrifugation (UC), and dextran-sulfate precipitation (DS), in terms of their effects on the HDL proteome and associated functionalities. We used state-of-the-art mass spectrometry to identify 171 proteins across all three isolation methods. IA-HDL contained higher levels of paraoxonase 1, apoB, clusterin, vitronectin, and fibronectin, while UC-HDL had higher levels of apoA2, apoC3, and α-1-antytrypsin. DS-HDL was enriched with apoA4 and complement proteins, while the apoA2 content was very low. Importantly, size-exclusion chromatography analysis showed that IA-HDL isolates contained subspecies in the size range above 12 nm, which were entirely absent in UC-HDL and DS-HDL isolates. Analysis of these subspecies indicated that they primarily consisted of apoA1, IGκC, apoC1, and clusterin. Functional analysis revealed that paraoxonase 1 activity was almost completely lost in IA-HDL, despite high paraoxonase content. We observed that the elution conditions, using 3M thiocyanate, during IA resulted in an almost complete loss of paraoxonase 1 activity. Notably, the cholesterol efflux capacity of UC-HDL and DS-HDL was significantly higher compared to IA-HDL. Together, our data clearly demonstrate that the isolation procedure has a substantial impact on the composition, subclass distribution, and functionality of HDL. In summary, our data show that the isolation procedure has a significant impact on the composition, subclass distribution and functionality of HDL. Our data can be helpful in the comparison, replication and analysis of proteomic datasets of HDL.

Keywords: HDL subclass distribution; apolipoproteins; cholesterol/efflux; cholesterol/metabolism; density gradient ultracentrifugation; dextran-sulfate precipitation; lipoproteins; mass spectrometry; paraoxonase 1; proteomics.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Aryldialkylphosphatase
Cholesterol, HDL / metabolism
Clusterin*
Lipoproteins, HDL* / metabolism
Proteome
Proteomics
Ultracentrifugation

Substances

Lipoproteins, HDL
Clusterin
Aryldialkylphosphatase
Proteome
Cholesterol, HDL