Label-free voltammetric detection of single-nucleotide mismatches recognized by the protein MutS

被引:37
|
作者
Masarik, Michal
Cahova, Katerina
Kizek, Rene
Palecek, Emil
Fojta, Miroslav [1 ]
机构
[1] Masaryk Univ, Fac Med, Inst Pathol Physiol, CS-66243 Brno, Czech Republic
[2] Acad Sci Czech Republ, Inst Biophys VVI, Brno 61265, Czech Republic
关键词
single-nucleotide polymorphism; point mutation; base mismatches; MutS; magnetic beads; protein electrochemistry; quartz-crystal microbalance;
D O I
10.1007/s00216-007-1181-7
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
MutS, a protein involved in DNA mismatch repair, recognizes mispaired and unpaired bases in duplex DNA. We have previously used MutS in an electrochemical double-surface technique (DST) for in-vitro detection of point mutations in DNA. The DST involved binding of unlabeled MutS to DNA heteroduplexes at the surface of magnetic beads followed by a highly sensitive electrochemical determination of the protein by measurement of a catalytic protein signal (peak H) at mercury electrodes. Detection of MutS using a peak resulting from oxidation of tyrosine and tryptophan residues of the protein at a carbon-paste electrode (CPE) was also possible but was approximately three orders of magnitude less sensitive. In this work we present an optimized technique for ex-situ voltammetric determination of MutS at a CPE. Choice of optimum experimental conditions (pH of supporting electrolyte, square-wave voltammetry settings, etc.) resulted in substantial improvement of the sensitivity of the assay, enabling detection of approximately 140 pg (1.6 fmol protein monomer) MutS in a 5-mu L sample. The sensitivity was increased further by acid hydrolysis of the protein before measurement. The hydrolyzed protein was detectable down to 5 pg (approx. 56 amol) MutS in 5 mu L solution. By using the DST combined with determination of the bound unlabeled MutS at the CPE we demonstrated selective interactions of the protein with single-base mismatches and discrimination among different base mispairs in 30-mer or 95-mer DNA duplexes. In agreement with previous studies, binding of the protein to the 30-mer substrates followed the trend G:T >> C:A > A:A > C:T > homoduplex. The electrochemical data were confirmed by use of an independent technique-a quartz-crystal microbalance for real-time monitoring of MutS interactions with DNA duplexes containing different base mispairs. By using the electrochemical DST a G:T mismatch was detectable in up to 1000-fold excess of homoduplex DNA.
引用
收藏
页码:259 / 270
页数:12
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