PENCIL GRAPHITE ELECTRODE AS A PROMISING TOOL FOR ELECTROANALYSIS OF METHYLGUANINES

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Authors

TŘÍSKOVÁ Iveta BOSÁKOVÁ Markéta TRNKOVÁ Libuše

Year of publication 2017
Type Article in Proceedings
Conference XVII. Workshop of Physical Chemists and Electrochemists
MU Faculty or unit

Faculty of Science

Citation
Field Physical chemistry and theoretical chemistry
Keywords epigenetic modifications; DNA methylation; methylguanines; voltammetry; PeGE
Description Nowadays, epigenetics is among the top disciplines of biomedicine. It is actually because epigentic modifications, especially methylation of nucleic acids (NAs), are linked with many diseases and dysfunctions, such as human carcinomas (lung, thyroid, prostate and pancreas), leukemia, etc.[1-4]. Guanine (G), one of the two essential nucleic bases, plays a key role in the DNA oxidation by various types of oxidants and free radicals [5-7]. Although guanine, compared with cytosine, is not a typical recipient of methyl groups, methylated guanines attract the attention as potential drugs and/or markers. Specifically, N7-methyl modification of G is a well-established biomarker for the detection and determination of DNA methylation [8]. Only few examples can be found in the literature regarding to the electrochemical determination of this alkylmodification of G. The electrochemical reduction of 7-methylguanine derivatives (7-methylguanosine and 7-methylguanosine-5‘-phosphate) at the mercury electrode [3, 9, 10] was completed with the study of oxidation behavior of 7-methylguanine at boron-doped diamond electrode and carbon electrodes (glassy carbon electrode and screen printed graphite electrodes)[8]. There are some papers regarding electrochemical behavior of 7N-methylguanine (7N-mG), linked with epigenetic modifications of DNA chain, but there are not any publications regarding other methylated guanine derivatives, such as 1N-, 3N- or 9N-methylguanines. In our research the oxidation processes of methylated guanine derivatives on a polymer pencil graphite electrode (pPeGE) in dependence on pH (phosphate – acetate buffer; pH 3.16 – 7.52) and the position of methyl group in the G molecule (pyrimidine ring vs. imidazole ring) were investigated.
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