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Changes in Methylation Patterns of Kiss1 and Kiss1r Gene Promoters across Puberty
Author(s) -
Amanda Wyatt,
Monika Závodná,
Jean L. Viljoen,
JoAnn L. Stanton,
Neil J. Gemmell,
Christine L. Jasoni
Publication year - 2013
Publication title -
genetics and epigenetics
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.38
H-Index - 10
ISSN - 1179-237X
DOI - 10.4137/geg.s12897
Subject(s) - kisspeptin , epigenetics , dna methylation , biology , promoter , methylation , gene expression , gene , bisulfite sequencing , epigenetics of physical exercise , cpg site , regulation of gene expression , genetics , endocrinology , medicine , hormone
The initiation of mammalian puberty is underpinned by an increase in Kisspeptin (Kiss1) signaling via its receptor (Kiss1r/GPR54) on gonadotropin-releasing hormone (GnRH) neurons. Animals and humans with loss-of-function mutations in Kiss1 or Kiss1r fail to go through puberty. The timing of puberty is dependent on environmental factors, and malleability in puberty timing suggests a mechanism that can translate environmental signals into patterns of Kiss1/Kiss1r gene expression. Epigenetics is a powerful mechanism that can control gene expression in an environment-dependent manner. We investigated whether epigenetic DNA methylation is associated with gene expression changes at puberty. We used bisulfite-PCR-pyrosequencing to define the methylation in the promoters of Kiss1 and Kiss1r before and after puberty in female rats. Both Kiss1 and Kiss1r showed highly significant puberty-specific differential promoter methylation patterns. By identifying key differentially methylated residues associated with puberty, these findings will be important for further studies investigating the control of gene expression across the pubertal transition.

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