Plasma lipoproteome in Alzheimer’s disease: a proof-of-concept study

Danni Li; Fangying Huang; Yingchun Zhao; Peter W. Villata; Timothy J. Griffin; Lin Zhang; Ling Li; Fang Yu

doi:10.1186/s12014-018-9207-z

Clinical Proteomics (Sep 2018)

Plasma lipoproteome in Alzheimer’s disease: a proof-of-concept study

Danni Li,
Fangying Huang,
Yingchun Zhao,
Peter W. Villata,
Timothy J. Griffin,
Lin Zhang,
Ling Li,
Fang Yu

Affiliations

Danni Li: Department of Laboratory Medicine and Pathology, University of Minnesota
Fangying Huang: Department of Laboratory Medicine and Pathology, University of Minnesota
Yingchun Zhao: Masonic Cancer Center, University of Minnesota
Peter W. Villata: Masonic Cancer Center, University of Minnesota
Timothy J. Griffin: Department of Biochemistry, Molecular Biology, and Biophysics, University of Minnesota
Lin Zhang: Department of Biostatistics, University of Minnesota
Ling Li: Department of Experimental and Clinical Pharmacology, University of Minnesota
Fang Yu: School of Nursing, University of Minnesota

DOI: https://doi.org/10.1186/s12014-018-9207-z
Journal volume & issue: Vol. 15, no. 1
pp. 1 – 8

Abstract

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Abstract Background Although total plasma lipoproteome consists of proteins that have shown promises as biomarkers that can identify Alzheimer’s disease (AD), effect sizes are modest. The objective of this study is to provide initial proof-of-concept that the plasma lipoproteome more likely differ between AD cases and controls when measured in individual plasma lipoprotein fractions than when measured as total in immunodepleted plasma. Methods We first developed a targeted proteomics method based on selected reaction monitoring (SRM) and liquid chromatography and tandem mass spectrometry for measurement of 120 tryptic peptides from 79 proteins that are commonly present in plasma lipoproteins. Then in a proof-of concept case–control study of 5 AD cases and 5 sex- and age-matched controls, we applied the targeted proteomic method and performed relatively quantification of 120 tryptic peptides in plasma lipoprotein fractions (fractionated by sequential gradient ultracentrifugation) and in immunodepleted plasma (of albumin and IgG). Unadjusted p values from two-sample t-tests and overall fold change was used to evaluate a peptide relative difference between AD cases and controls, with lower p values ( 1.05 or 1.05 or < 0.95, compared to only 6 tryptic peptides in immunodepleted plasma. The overall comparisons, therefore, suggested greater peptide/protein differences in plasma lipoproteome when measured in individual plasma lipoproteins than as total in immunodepleted plasma. Specifically, protein complement C3’s peptide IHWESASLLR, had unadjusted p values of 0.00007, 0.00012, and 0.0006 and overall 1.25, 1.17, 1.14-fold changes in VLDL, IDL, and LDL, respectively. After positive False Discovery Rate (pFDR) adjustment, the complement C3 peptide IHWESASLLR in VLDL remained statistically different (adjusted p value < 0.05). Discussion The findings may warrant future studies to investigate plasma lipoproteome when measured in individual plasma lipoprotein fractions for AD diagnosis.

Published in Clinical Proteomics

ISSN: 1559-0275 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine
Website: https://clinicalproteomicsjournal.biomedcentral.com/

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