Project Details
Mechanism and regulation of the Dnmt1 DNA methyltransferase
Applicant
Professor Dr. Albert Jeltsch
Subject Area
Biochemistry
Term
from 2012 to 2015
Project identifier
Deutsche Forschungsgemeinschaft (DFG) - Project number 225439244
Dnmt1 is a large multidomain enzyme which specifically methylates hemimethylated CpG sites after DNA replication and thereby copies exiting DNA methylation patterns through cell divisions which is a key epigenetic event involved in several biological processes. In our proposal, we like to address the question that the in vitro activity of Dnmt1 is not sufficient to explain the speed of remethylation of DNA after DNA replication in cells. Preliminary data from our lab suggest that the in vitro rate of Dnmt1 is underestimated, because the enzyme exists in different conformations. Novel structural data indeed show that Dnmt1 can adopt different autoinhibitory conformations, in which other domains block access of the DNA to the catalytic domain. We plan to carry out single enzyme kinetics and determine the DNA methylation activity of Dnmt1 in its most active conformation after DNA has been bound. In addition, we aim to measure if a possible direct movement of Dnmt1 along DNA in cells (as opposed to the random walk on DNA in vitro) could further speed up DNA methylation. The starting point of the second part of our proposal is that the in vitro specificity of Dnmt1 is obviously not sufficient to ensure correct copying of methylation patterns without additional regulation, because the enzyme also shows activity towards unmethylated CpG sites. This is particularly critical outside of S-phase, when no correct hemimethylated CpG substrate sites are available. Therefore, we aim to study if cell cycle coupled regulation of Dnmt1 occurs. To this end, we plan to identify post-translational modifications of Dnmt1 and study their cell cycle connection. In the case of phosphorylations and lysine methylations we will further study, whether they influence the enzymes activity or specificity or its interaction with other protein. We will also investigate if the modifications affect the sub-cellular and sub-nuclear localisation of Dnmt1. We are convinced that our project will contribute important pieces to the understanding of the maintenance of DNA methylation patterns a fundamental process in molecular epigenetics.
DFG Programme
Research Grants