Reproducibility and Variability of Protein Analytes Measured Using a Multiplexed Modified Aptamer Assay

Author:

Tin Adrienne12,Yu Bing3,Ma Jianzhong3,Masushita Kunihiro12,Daya Natalie12,Hoogeveen Ron C4,Ballantyne Christie M4,Couper David5,Rebholz Casey M12,Grams Morgan E16,Alonso Alvaro7,Mosley Thomas8,Heiss Gerardo9,Ganz Peter10,Selvin Elizabeth12,Boerwinkle Eric311,Coresh Josef12

Affiliation:

1. Department of Epidemiology, Johns Hopkins Bloomberg School of Public Health, Baltimore, MD

2. Welch Center for Prevention, Epidemiology and Clinical Research, Johns Hopkins University, Baltimore MD

3. Department of Epidemiology, Human Genetics and Environmental Sciences, School of Public Health, University of Texas Health Science Center at Houston, Houston, TX

4. Section of Cardiovascular Research, Department of Medicine, Baylor College of Medicine, Houston TX

5. Department of Biostatistics, Gillings School of Global Public Health, University of North Carolina, Chapel Hill, NC

6. Division of Nephrology, Johns Hopkins School of Medicine, Baltimore, MD

7. Department of Epidemiology, Rollins School of Public Health, Emory University, Atlanta, GA

8. Department of Neurology, The University of Mississippi Medical Center, Jackson, MS

9. Department of Epidemiology, Gillings School of Global Public Health, University of North Carolina, Chapel Hill, NC

10. Division of Cardiology, San Francisco General Hospital, University of California, San Francisco, CA

11. Human Genome Sequencing Center, Baylor College of Medicine, Houston, TX

Abstract

Abstract Background There is growing interest in the use of multiplexed aptamer-based assays for large-scale proteomic studies. However, the analytic, short- and long-term variation of the measured proteins is largely uncharacterized. Methods We quantified 4001 plasma protein analytes from 42 participants in the Atherosclerosis Risk in Communities (ARIC) Study in split samples and at multiple visits using a multiplexed modified aptamer assay. We calculated the CV, Spearman correlation, and intraclass correlation (ICC) between split samples and evaluated the short-term (4–9 weeks) and long-term (approximately 20 years) variability using paired t-tests with log-transformed protein concentrations and Bonferroni-corrected significance thresholds. We performed principal component (PC) analysis of protein analyte concentrations and evaluated their associations with age, sex, race, and estimated glomerular filtration rate (eGFR). Results The mean baseline age was 57 years at the first visit, 43% of participants were male and 57% were white. Among 3693 protein analytes that passed quality control, half (n = 1846) had CVs < 5.0%, Spearman correlations > 0.89, and ICCs > 0.96 among the split samples. Over the short term, only 1 analyte had a statistically significant difference between the 2 time points, whereas, over approximately 20 years, 866 analytes (23.4%) had statistically significant differences (P < 1.4 × 10−5, 681 increased, 185 decreased). PC1 had high correlations with age (−0.73) and eGFR (0.60). PC2 had moderate correlation with male sex (0.18) and white race (0.31). Conclusions Multiplexed modified aptamer technology can assay thousands of proteins with excellent precision. Our results support the potential for large-scale studies of the plasma proteome over the lifespan.

Funder

National Heart, Lung, and Blood Institute

NIH

National Institute of Diabetes and Digestive and Kidney Diseases

Publisher

Oxford University Press (OUP)

Subject

General Medicine

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