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Open AccessJournal ArticleDOI

Gene reactivation: a tool for the isolation of mammalian DNA methylation mutants.

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TLDR
It is proposed that the phenotype of tsm cells is due to a mutation involved in the regulation of DNA methylation, and the further characterization of this and other mammalian mutants should help to clarify the physiological role of DNAmethylation, as well as its regulation.
Abstract
We report the isolation and characterization of a mammalian strain (tsm) that has a temperature-sensitive mutation in DNA methylation. The isolation procedure was based on the observation that treatment of a CHO TK- MT- cell line with demethylating agents introduces up to 46% demethylation, resulting in phenotypic reversion and transcriptional activation of the thymidine kinase (TK) and metallothionein (MT) genes at frequencies ranging from 1% to 59%. Seven thousand individual colonies from an EMS-mutagenized CHO TK- MT- population were screened for spontaneous reversion to TK+ phenotype after treatment at 39 degrees C. Successful isolates were subsequently examined for MT+ reversion. A single clone (tsm) was obtained that showed temperature-dependent reactivation of both TK and MT genes at frequencies of 7.2 X 10(-4) and 6 X 10(-4), respectively. The tsm cells were viable at 39 degrees C and showed no increased mutation frequency. Reactivation correlated with transcriptional activation of the respective genes, whereas backreversion to the TK- phenotype was associated with transcriptional inactivation. TK- backrevertants were reactivable again with demethylating agents. Although demethylation in tsm cells was not detectable by HPLC, Southern blot analysis revealed that reactivants, irrespective of their mode of generation, showed specific demethylation of both TK and MT genes. Also, after about 150 cell generations after treatment, reactivants from both temperature-induced tsm and cells exposed to demethylating agents gained 60% and 23%, respectively, in 5-methylcytosine (5mC). It is proposed that the phenotype of tsm cells is due to a mutation involved in the regulation of DNA methylation. The further characterization of this and other mammalian mutants should help to clarify the physiological role of DNA methylation, as well as its regulation.

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Book ChapterDOI

Mechanisms of genomic imprinting in mammals.

TL;DR: The chapter presents an analysis of DNA methylation in somatic tissues and germ cells during embryonic and post-natal development that reveals dynamic changes, particularly during gametogenesis and early embryogenesis that suggest thatDNA methylation may be involved in genomic imprinting.
Journal ArticleDOI

Methods for DNA methylation analysis and applications in colon cancer.

TL;DR: The goal of this review is to describe the most widely used methylation methods in the study of cancer, as well as the potential clinical applications of DNA methylation biomarkers in colorectal cancer.
Journal ArticleDOI

Region-specific methylation of the parathyroid hormone-related peptide gene determines its expression in human renal carcinoma cell lines.

TL;DR: Using a system of 12 human renal carcinoma cell lines, it was found that the expression of the PTHrP gene in these cell lines is controlled at the transcriptional level, and the functional importance of this mechanism of control was confirmed by the ability of the demethylating agent, 5-azacytidine, to induce P THrP mRNA expression in previously nonexpressing cell lines.
Journal Article

Coregulation of the human O6-methylguanine-DNA methyltransferase with two unrelated genes that are closely linked.

TL;DR: It appears that methyltransferase expression may in some instances be coordinately regulated with the tk and glk loci which are closely linked on human chromosome 17.
References
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Journal ArticleDOI

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Journal ArticleDOI

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TL;DR: A model based on DNA methylation is proposed to explain the initiation and maintenance of mammalian X inactivation and certain aspects of other permanent events in eukaryotic cell differentiation using sequence-specific DNA methylases that methylate unmethylated sites with great difficulty but easily methylate half-methylated sites.