The kinetics of fluorescent DNA labeling using PCR with different Taq polymerases depends on the chemical structures of modified nucleotides

T. S. Lisitsa; V. E. Shershov; M. A. Spitsyn; T. O. Guseinov; A. Yu. Ikonnikova; D. O. Fesenko; S. A. Lapa; A. S. Zasedatelev; A. V. Chudinov; T. V. Nasedkina

doi:10.1134/S0006350917030095

The kinetics of fluorescent DNA labeling using PCR with different Taq polymerases depends on the chemical structures of modified nucleotides

Autores: Lisitsa T.S.¹, Shershov V.E.¹, Spitsyn M.A.¹, Guseinov T.O.¹, Ikonnikova A.Y.¹, Fesenko D.O.¹, Lapa S.A.¹, Zasedatelev A.S.¹, Chudinov A.V.¹, Nasedkina T.V.¹
Afiliações:
1. Engelhardt Institute of Molecular Biology
Edição: Volume 62, Nº 3 (2017)
Páginas: 366-372
Seção: Molecular Biophysics
URL: https://ogarev-online.ru/0006-3509/article/view/152299
DOI: https://doi.org/10.1134/S0006350917030095
ID: 152299

Citar

Texto integral

Acesso aberto
Acesso é fechado

Acesso está concedido
Acesso é fechado

Somente assinantes

Resumo
Sobre autores
Bibliografia
Arquivos suplementares
Estatísticas

Resumo

The kinetics of DNA labeling during PCR using six fluorescent derivatives of 2′-deoxyuridine 5′-triphosphate has been studied. These compounds differ in their chemical structure, total electric charge and the length of the linker between a dye and the C5 position of a pyrimidine base. The efficiency of the incorporation of the fluorescent derivatives into a growing DNA chain by four commercially available Taq DNA polymerases with 5′→3′ exonuclease and hot start activity has been determined using real-time PCR with a TaqMan probe and the subsequent electrophoretic analysis of the reaction products. Modified deoxyuridines with a total positive or negative charge of the chromophore were practically not incorporated by Taq polymerases during PCR. The modified deoxyuridines with a neutral charge of the chromophore were effectively incorporated into DNA. The extended length of the linker between the pyrimidine base and the chromophore led to a lower PCR inhibition and a more effective inclusion of modified nucleotides in the growing DNA chain. This fact can be explained by the reduced steric effects that were caused by the dye. As a result, the most promising combinations of fluorescently labeled nucleotide and Taq polymerase have been chosen for further use in fluorescent DNA labeling.

Palavras-chave

fluorescence, modified nucleotides, cyanine dyes, real-time PCR, PCR efficiency

Arquivos suplementares

Ação

1. JATS XML

Baixar

Nome de usuário
Senha
Lembrar usuário

Esqueceu a senha?	Cadastro

Nome de usuário
Senha
Lembrar usuário

Esqueceu a senha?	Cadastro

The kinetics of fluorescent DNA labeling using PCR with different Taq polymerases depends on the chemical structures of modified nucleotides

Texto integral

Resumo

Palavras-chave

Sobre autores

T. Lisitsa

V. Shershov

M. Spitsyn

T. Guseinov

A. Ikonnikova

D. Fesenko

S. Lapa

A. Zasedatelev

A. Chudinov

T. Nasedkina

Arquivos suplementares