Affiliation:
1. Laboratory of Developmental Genetics and Imprinting, Developmental Genetics Programme, The Babraham Institute, Cambridge CB2 4AT, United Kingdom
Abstract
ABSTRACT
Igf2
and
H19
are reciprocally imprinted genes on mouse distal chromosome 7. They share several regulatory elements, including a differentially methylated region (DMR) upstream of
H19
that is paternally methylated throughout development. The
cis-
acting sequence requirements for targeting DNA methylation to the DMR remain unknown; however, it has been suggested that direct tandem repeats near DMRs could be involved. Previous studies of the imprinted
Rasgrf1
locus demonstrate indeed that a direct repeat element adjacent to a DMR is responsible for establishing paternal allele-specific methylation at the DMR and therefore allelic expression of the
Rasgrf1
transcript. We identified a prominent and conserved direct tandem repeat 1 kb upstream of the
H19
DMR and proposed that it played a similar role in imprinted regulation of
H19
. To test our hypothesis, we generated mice harboring a 1.7-kb targeted deletion of the direct repeat element and analyzed fetal growth, allelic expression, and methylation within the
Igf2-H19
region. Surprisingly the deletion had no effect on imprinting. These results together with deletions of other repeats close to imprinted genes suggest that direct repeats may not be important for the targeting of methylation at the majority of imprinted loci and that the
Rasgrf1
locus may be an exception to this rule.
Publisher
American Society for Microbiology
Subject
Cell Biology,Molecular Biology
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