Discrimination of A1555G and C1494T point mutations in the mitochondrial 12S rRNA gene by on/off switch |
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| Authors: | Guo Zi-Fen Guo Wu-Shuang Xiao Li Gao Guo-Qiang Lan Fen Lu Xue-Guan Li Kai Liao Duan-Fang |
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| Institution: | (1) Institute of Pharmacy and Pharmacology, University of South China, Hengyang, Hunan, 421001, China;(2) Department of Pharmacology, Medical College, Soochow University, Suzhou, Jiangsu, 215123, China;(3) Molecular Medicine Center, the Second Affiliated Hospital of Soochow University, Suzhou, Jiangsu, 215004, China;(4) Department of Traditional Chinese Diognotics, School of Pharmacy, Hunan University of Chinese Medicine, Changsha, Hunan, 410208, China; |
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| Abstract: | The objective of this study was to apply the “on/off” switch consisting of 3′ phosphorothioate-modified allele specific primers
and exo+ polymerase in single base discrimination of A1555G and C1494T mutations in the highly conserved sites of the mitochondrial
12S rRNA. The two point mutations are the hotspot mutations associated with either aminoglycoside antibiotics induced deafness
or inherited nonsyndromic hearing loss. The PCR products of mitochondrial DNA (mtDNA) 12S rRNA gene were inserted into the
pMD19-T vector for transformation into Escherichia coli JM109 competent cells for preparing wild-type pMD19-T/mt vector. Inverse PCR was carried out for mtDNA 12S rRNA gene C1494T
and A1555G mutagenesis and DpnI endonuclease degradating methylated pMD19-T/mt vector existing in the inverse PCR products
was carried out to construct the mutation-type pMD19-T/mtM vector. These constructed vectors were confirmed by DNA sequencing.
Allelic specific primers targeting wild-type and mutation-type templates were designed with 3′ terminal phosphorothioate modification.
Two-directional primer extension was performed using Pfu polymerases. Amplified by exo+ polymerase, allelic specific primers perfectly matching wild-type allele were extended while no products were produced from
primers targeting point-mutated deafness-related allele. Similarly, allelic specific primers perfectly matching point-mutated
deafness-related mutation-type allele were extended and no products were yielded from primers targeting wild-type allele.
No specific product was observed in the primer extension reaction mediated by on/off switch in screening the mtDNA 12S rRNA
gene harboring either C1494T or A1555G mutation in 40 healthy volunteers tested. These data suggest that the “off switch”
mediated by exo+ polymerase is highly reliable in the diagnosis of monogenic diseases and the novel “on/off” switch has enormous applications
in systematic and extended screening of the12S rRNA gene A1555G and C1494T mutations. The established assay can be widely
used not only for hearing loss patients but also for normal subjects before the use of aminoglycoside antibiotics. |
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