METHOD FOR TEMPLATE-BASED ENZYMATIC DNA SYNTHESIS USING PHOSPHORYL GUANIDINE OLIGONUCLEOTIDES AND REACTION MIXTURES FOR CARRYING OUT THE METHOD

METHOD FOR TEMPLATE-BASED ENZYMATIC DNA SYNTHESIS USING PHOSPHORYL GUANIDINE OLIGONUCLEOTIDES AND REACTION MIXTURES FOR CARRYING OUT THE METHOD

The invention relates to the development and optimization of PCR and RT-PCR systems used to detect nucleic acids, including the diagnosis of genetic, viral, and other diseases. The essence of the proposed method is that neutral derivatives of oligonucleotides, namely phosphoryl guanidines containing...

Ausführliche Beschreibung

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Bibliographische Detailangaben
Hauptverfasser: STETSENKO, DMITRY ALEKSANDROVICH, DMITRIENKO, ELENA VLADIMIROVNA, FILIPENKO, MAKSIM LEONIDOVICH, PYSHNAYA, INNA ALEKSEEVNA, RICHTER, VLADIMIR ALEKSANDROVICH, PYSHNYI, DMITRII VLADIMIROVICH, STEPANOV, GRIGORY ALEKSANDROVICH, IVANOV, MIKHAIL KONSTANTINOVICH, KUPRYUSHKIN, MAXIM SERGEEVICH, OSCORBIN, IGOR PETROVICH
Format: Patent
Sprache:eng
Schlagworte:
BEER
BIOCHEMISTRY
CHEMISTRY
DERIVATIVES THEREOF
ENZYMOLOGY
FERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIREDCHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERSFROM A RACEMIC MIXTURE
METALLURGY
MICROBIOLOGY
MUTATION OR GENETIC ENGINEERING
NUCLEIC ACIDS
NUCLEOSIDES
NUCLEOTIDES
ORGANIC CHEMISTRY
SPIRITS
SUGARS
VINEGAR
WINE
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Beschreibung
Zusammenfassung:The invention relates to the development and optimization of PCR and RT-PCR systems used to detect nucleic acids, including the diagnosis of genetic, viral, and other diseases. The essence of the proposed method is that neutral derivatives of oligonucleotides, namely phosphoryl guanidines containing one or more phosphate groups in which guanidine or substituted guanidine residue is introduced on the phosphorus atom, are used as primers for the template-based amplification, including polymerase chain reaction (PCR) and PCR combined with reverse transcription (RT-PCR). The invention allows to obtain more reliable, specific and selective results in the process of PCR, in particular, to increase the sensitivity of PCR by reducing the yield of by-products of DNA amplification and/or to control the yield of the PCR product, including intentionally suppressing, by using different combinations of the location and number of modified phosphate groups in the oligonucleotide primers.