Phosphoryl guanidine oligonucleotides as primers for RNA-dependent DNA synthesis using murine leukemia virus reverse transcriptase

Phosphoryl guanidine oligonucleotides as primers for RNA-dependent DNA synthesis using murine leukemia virus reverse transcriptase

Modern approaches to the detection and analysis of low-copy-number RNAs are often based on the use of RNA-dependent DNA polymerases, for example, in reverse-transcription PCR. The accuracy and efficiency of cDNA synthesis in the reverse-transcription reaction catalyzed by reverse transcriptase (RNA-...

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Bibliographic Details
Main Authors: Dyudeeva, E.S (Author), Pyshnaya, I.A (Author)
Format: Article
Language:English
Published: Institute of Cytology and Genetics of Siberian Branch of the Russian Academy of Sciences 2022
Subjects:
MMLV H-
mouse leukemia virus reverse transcriptase
phosphoryl guanidine oligonucleotides
reverse transcriptase
reverse transcription
uncharged analogs of oligonucleotides
Online Access:View Fulltext in Publisher
LEADER 02743nam a2200217Ia 4500
001 10.18699-VJGB-22-02
008 220706s2022 CNT 000 0 und d
020 |a 25000462 (ISSN) 
245 1 0 |a Phosphoryl guanidine oligonucleotides as primers for RNA-dependent DNA synthesis using murine leukemia virus reverse transcriptase 
260 0 |b Institute of Cytology and Genetics of Siberian Branch of the Russian Academy of Sciences  |c 2022 
856 |z View Fulltext in Publisher  |u https://doi.org/10.18699/VJGB-22-02 
520 3 |a Modern approaches to the detection and analysis of low-copy-number RNAs are often based on the use of RNA-dependent DNA polymerases, for example, in reverse-transcription PCR. The accuracy and efficiency of cDNA synthesis in the reverse-transcription reaction catalyzed by reverse transcriptase (RNA-dependent DNA polymerase) significantly affect the correctness of the results of PCR diagnostic assays and/or RNA sequencing. In this regard, many studies are focused on the optimization of the reverse-transcription reaction, including the search for more perfect primers necessary to obtain a full-length DNA copy of RNA under study. The best-known completely uncharged analogs of oligonucleotides - morpholine oligonucleotides and peptide nucleic acids - cannot be substrates for enzymes that process nucleic acids. The aim of this work was to conduct a pilot study of uncharged phosphoryl guanidine oligodeoxyribonucleotides (PGOs) as primers for mouse leukemia virus reverse transcriptase (MMLV H-). Specific features of elongation of partially and completely uncharged PGO primers were investigated. It was demonstrated that PGOs can be elongated efficiently, e. g., in the presence of a fragment of human ribosomal RNA having complex spatial structure. It was shown that the proportion (%) of abortive elongation products of a PGO primer depends on buffer ionic strength, nucleotide sequence of the primer, and the presence and location of phosphoryl guanidine groups in the primer. The results indicate the suitability of PGOs, including completely electroneutral ones, as primers for reverse-transcription PCR, thereby opening up new prospects for the creation of experimental models for the analysis of highly structured RNA. © Dyudeeva E.S., Pyshnaya I.A., 2022 This work is licensed under a Creative Commons Attribution 4.0 License 
650 0 4 |a MMLV H- 
650 0 4 |a mouse leukemia virus reverse transcriptase 
650 0 4 |a phosphoryl guanidine oligonucleotides 
650 0 4 |a reverse transcriptase 
650 0 4 |a reverse transcription 
650 0 4 |a uncharged analogs of oligonucleotides 
700 1 |a Dyudeeva, E.S.  |e author 
700 1 |a Pyshnaya, I.A.  |e author 
773 |t Vavilovskii Zhurnal Genetiki i Selektsii 

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