TY - JOUR
T1 - Examination of the DNA substrate selectivity of DNA cytosine methyltransferases using mass tagging
AU - Rusmintratip, Valaiporn
AU - Riggs, Arthur D.
AU - Sowers, Lawrence C.
PY - 2000/9/15
Y1 - 2000/9/15
N2 - The biological significance of cytosine methylation is as yet incompletely understood, but substantial and growing evidence strongly suggests that perturbation of methylation patterns, resulting from the infidelity of DNA cytosine methyltransferase, is an important component of the development of human cancer. We have developed a novel in vitro assay that allows us to quantitatively determine the DNA substrate preferences of cytosine methylases. This approach, which we call mass tagging, involves the labeling of target cytosine residues in synthetic DNA duplexes with stable isotopes, such as 15N. Methylation is then measured by the formation of 5-methylcytosine (5mC) by gas chromatography/mass spectrometry. The DNA substrate selectivity is determined from the mass spectrum of the product 5mC. With the non-symmetrical duplex DNA substrate examined in this study we find that the bacterial methyltransferase Hpall (duplex DNA recognition sequence CCGG) methylates the one methylatable cytosine of each strand similarly. Introduction of an A-C mispair at the methylation site shifts methylation exclusively to the mispaired cytosine residue. In direct competition assays with Hpall methylase we observe that the mispaired substrate is methylated more extensively than the fully complementary, normal substrate, although both have one Hpall methylation site. Through the use of this approach we will be able to learn more about the mechanisms by which methylation patterns can become altered.
AB - The biological significance of cytosine methylation is as yet incompletely understood, but substantial and growing evidence strongly suggests that perturbation of methylation patterns, resulting from the infidelity of DNA cytosine methyltransferase, is an important component of the development of human cancer. We have developed a novel in vitro assay that allows us to quantitatively determine the DNA substrate preferences of cytosine methylases. This approach, which we call mass tagging, involves the labeling of target cytosine residues in synthetic DNA duplexes with stable isotopes, such as 15N. Methylation is then measured by the formation of 5-methylcytosine (5mC) by gas chromatography/mass spectrometry. The DNA substrate selectivity is determined from the mass spectrum of the product 5mC. With the non-symmetrical duplex DNA substrate examined in this study we find that the bacterial methyltransferase Hpall (duplex DNA recognition sequence CCGG) methylates the one methylatable cytosine of each strand similarly. Introduction of an A-C mispair at the methylation site shifts methylation exclusively to the mispaired cytosine residue. In direct competition assays with Hpall methylase we observe that the mispaired substrate is methylated more extensively than the fully complementary, normal substrate, although both have one Hpall methylation site. Through the use of this approach we will be able to learn more about the mechanisms by which methylation patterns can become altered.
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U2 - 10.1093/nar/28.18.3594
DO - 10.1093/nar/28.18.3594
M3 - Article
C2 - 10982881
AN - SCOPUS:0034666342
SN - 0305-1048
VL - 28
SP - 3594
EP - 3599
JO - Nucleic acids research
JF - Nucleic acids research
IS - 18
ER -