Back to Search Start Over

Measurement of Telomere Length for Longitudinal Analysis: Implications of Assay Precision.

Authors :
Nettle, Daniel
Gadalla, Shahinaz M
Lai, Tsung-Po
Susser, Ezra
Bateson, Melissa
Aviv, Abraham
Source :
American Journal of Epidemiology; Jul2021, Vol. 190 Issue 7, p1406-1413, 8p
Publication Year :
2021

Abstract

Researchers increasingly wish to test hypotheses concerning the impact of environmental or disease exposures on telomere length (TL), and they use longitudinal study designs to do so. In population studies, TL is usually measured with a quantitative polymerase chain reaction (qPCR)-based method. This method has been validated by calculating its correlation with a gold standard method such as Southern blotting (SB) in cross-sectional data sets. However, in a cross-section, the range of true variation in TL is large, and measurement error is introduced only once. In a longitudinal study, the target variation of interest is small, and measurement error is introduced at both baseline and follow-up. In this paper, we present results from a small data set (n  = 20) in which leukocyte TL was measured twice 6.6 years apart by means of both qPCR and SB. The cross-sectional correlations between qPCR and SB were high at both baseline (r  = 0.90) and follow-up (r  = 0.85), yet their correlation for TL change was poor (r  = 0.48). Moreover, the qPCR data but not the SB data showed strong signatures of measurement error. Through simulation, we show that the statistical power gain from performing a longitudinal analysis is much greater for SB than for qPCR. We discuss implications for optimal study design and analysis. [ABSTRACT FROM AUTHOR]

Details

Language :
English
ISSN :
00029262
Volume :
190
Issue :
7
Database :
Complementary Index
Journal :
American Journal of Epidemiology
Publication Type :
Academic Journal
Accession number :
151248300
Full Text :
https://doi.org/10.1093/aje/kwab025