Replicated effects of sex and genotype on gene expression in human lymphoblastoid cell lines

doi:10.1093/hmg/ddl456

Human Molecular Genetics Advance Access originally published online on December 12, 2006
Human Molecular Genetics 2007 16(4):364-373; doi:10.1093/hmg/ddl456

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Replicated effects of sex and genotype on gene expression in human lymphoblastoid cell lines

Allan F. McRae¹^,8^,*^,, Nicholas A. Matigian²^,3^,, Lata Vadlamudi⁴^,5, John C. Mulley⁶^,7, Bryan Mowry³, Nicholas G. Martin¹, Sam F. Berkovic⁴, Nicholas K. Hayward² and Peter M. Visscher¹^,8

¹ Genetic Epidemiology Group and ² Human Genetics Laboratory, Queensland Institute of Medical Research, Herston, QLD 4029, Australia, ³ Queensland Centre for Mental Health Research, The Park Centre for Mental Health, Wacol, QLD 4076, Australia, ⁴ Epilepsy Research Centre, Department of Medicine (Neurology), University of Melbourne, Austin Health, Heidelberg, Victoria, Australia, ⁵ Academic Unit of Medicine (Neurology), The Australian National University, Canberra, Australia, ⁶ Department of Genetic Medicine, Women's and Children's Hospital, North Adelaide, Australia, ⁷ Department of Molecular Biosciences, University of Adelaide, Adelaide, South Australia, Australia, ⁸ Institute of Evolutionary Biology, University of Edinburgh, Edinburgh EH9 3JT, UK

^* To whom correspondence should be addressed. Tel: +61 733620190; Fax: +61 733620101; Email: allan.mcrae{at}qimr.edu.au

Received July 4, 2006; Revised September 26, 2006; Accepted December 4, 2006

The expression level for 15 887 transcripts in lymphoblastoidcell lines from 19 monozygotic twin pairs (10 male, 9 female)were analysed for the effects of genotype and sex. On an average,the effect of twin pairs explained 31% of the variance in normalizedgene expression levels, consistent with previous broad senseheritability estimates. The effect of sex on gene expressionlevels was most noticeable on the X chromosome, which contained15 of the 20 significantly differentially expressed genes. Ahigh concordance was observed between the sex difference teststatistics and surveys of genes escaping X chromosome inactivation.Notably, several autosomal genes showed significant differencesin gene expression between the sexes despite much of the cellularenvironment differences being effectively removed in the celllines. A publicly available gene expression data set from theCEPH families was used to validate the results. The heritabilityof gene expression levels as estimated from the two data setsshowed a highly significant positive correlation, particularlywhen both estimates were close to one and thus had the smalleststandard error. There was a large concordance between the genessignificantly differentially expressed between the sexes inthe two data sets. Analysis of the variability of probe bindingintensities within a probe set indicated that results are robustto the possible presence of polymorphisms in the target sequences.

The authors wish it to be known that, in their opinion, thefirst two authors should be regarded as joint First Authors.

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