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1,2-propanediol-trehalose mixture as a potent quantitative real-time PCR enhancer
H. Horáková, I. Polakovičová, GM. Shaik, J. Eitler, V. Bugajev, L. Dráberová, P. Dráber,
Jazyk angličtina Země Anglie, Velká Británie
Typ dokumentu časopisecké články, práce podpořená grantem
BioMedCentral Open Access od 2001
Directory of Open Access Journals od 2000
Free Medical Journals od 2001
PubMed Central od 2001
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ProQuest Central od 2009-01-01
Open Access Digital Library od 2000-01-01
Open Access Digital Library od 2001-01-01
Open Access Digital Library od 2001-04-01
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Health & Medicine (ProQuest) od 2009-01-01
ROAD: Directory of Open Access Scholarly Resources od 2001
Springer Nature OA/Free Journals od 2001-12-01
Odkazy
PubMed
21501492
DOI
10.1186/1472-6750-11-41
Knihovny.cz E-zdroje
- MeSH
- DNA chemie genetika MeSH
- fluorescenční barviva chemie MeSH
- lidé MeSH
- myši inbrední C57BL MeSH
- myši MeSH
- polymerázová řetězová reakce přístrojové vybavení MeSH
- propylenglykol chemie MeSH
- trehalosa chemie MeSH
- zvířata MeSH
- Check Tag
- lidé MeSH
- myši MeSH
- zvířata MeSH
- Publikační typ
- časopisecké články MeSH
- práce podpořená grantem MeSH
BACKGROUND: Quantitative real-time PCR (qPCR) is becoming increasingly important for DNA genotyping and gene expression analysis. For continuous monitoring of the production of PCR amplicons DNA-intercalating dyes are widely used. Recently, we have introduced a new qPCR mix which showed improved amplification of medium-size genomic DNA fragments in the presence of DNA dye SYBR green I (SGI). In this study we tested whether the new PCR mix is also suitable for other DNA dyes used for qPCR and whether it can be applied for amplification of DNA fragments which are difficult to amplify. RESULTS: We found that several DNA dyes (SGI, SYTO-9, SYTO-13, SYTO-82, EvaGreen, LCGreen or ResoLight) exhibited optimum qPCR performance in buffers of different salt composition. Fidelity assays demonstrated that the observed differences were not caused by changes in Taq DNA polymerase induced mutation frequencies in PCR mixes of different salt composition or containing different DNA dyes. In search for a PCR mix compatible with all the DNA dyes, and suitable for efficient amplification of difficult-to-amplify DNA templates, such as those in whole blood, of medium size and/or GC-rich, we found excellent performance of a PCR mix supplemented with 1 M 1,2-propanediol and 0.2 M trehalose (PT enhancer). These two additives together decreased DNA melting temperature and efficiently neutralized PCR inhibitors present in blood samples. They also made possible more efficient amplification of GC-rich templates than betaine and other previously described additives. Furthermore, amplification in the presence of PT enhancer increased the robustness and performance of routinely used qPCRs with short amplicons. CONCLUSIONS: The combined data indicate that PCR mixes supplemented with PT enhancer are suitable for DNA amplification in the presence of various DNA dyes and for a variety of templates which otherwise can be amplified with difficulty.
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