A Rapid and Sensitive Diagnosis of Typhoid Fever Based On Nested PCR-Voltammetric DNA Biosensor Using Flagellin Gene Fragment
Author(s) -
Yeni Wahyuni Hartati,
Santhy Wyantuti,
M. Lutfi Firdaus,
Nurul Auliany,
Rini Surbakti,
Shabarni Gaffar
Publication year - 2017
Publication title -
indonesian journal of chemistry
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.273
H-Index - 14
eISSN - 2460-1578
pISSN - 1411-9420
DOI - 10.22146/ijc.21182
Subject(s) - chemistry , flagellin , primer dimer , biosensor , nested polymerase chain reaction , microbiology and biotechnology , dna , polymerase chain reaction , differential pulse voltammetry , typhoid fever , agarose gel electrophoresis , genomic dna , gene , chromatography , virology , biochemistry , electrode , electrochemistry , biology , cyclic voltammetry , multiplex polymerase chain reaction
Typhoid fever caused by Salmonella typhi is an important issue for public health in the world. Laboratory methods for rapid and sensitive diagnosis are very important for disease management. The purpose of this study was to determine the performance of nested PCR–voltammetric DNA biosensor using flagellin gene (fla) of S. typhi as a marker. The differential pulse voltammetry using pencil graphite electrode was applied to measure the guanine oxidation signal of probes vs synthetic target stDNA and probes vs fla PCR product hybridizations. The probe DNA selectivity was examined by hybridized probes vs non-complementary sequence. The result showed that the first round nested PCR product can not be visualized by agarose electrophoresis, whereas using the voltammetric biosensor methods can be detected both for the first or second round nested PCR product. The average peak current of hybridized probe vs first and second round of PCR product was 2.32 and 1.47 μA respectively, at 0.9 V. Detection of the DNA sequences of the infectious diseases from PCR amplified real sample was also carried out using this voltammetric DNA biosensor methods.
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