METHOD OF INDIRECT DETERMINATION OF THE COMPLETENESS OF RABIES VIRUS ANTIGEN INACTIVATION USING REVERSE-TRANSCRIPTASE POLYMERASE CHAIN REACTION FOLLOWED BY ELECTROPHORESIS OF AMPLICONS IN AGAROSE GEL

FIELD: biotechnology.SUBSTANCE: method of indirect determination of the completeness of inactivation of the rabies virus antigen using reverse transcriptase polymerase chain reaction (hereinafter - RT-PCR) followed by electrophoresis of amplicons in agarose gel is described. The completeness of inac...

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Hauptverfasser:	Mikhalishin Dmitrij Valerevich, Starikov Vyacheslav Alekseevich, Doronin Maksim Igorevich, Shulpin Mikhail Ivanovich, Nazarov Nikolaj Alekseevich, Chupin Sergej Aleksandrovich, Borisov Aleksej Valerevich
Format:	Patent
Sprache:	eng ; rus
Schlagworte:	BEER BIOCHEMISTRY CHEMISTRY COMPOSITIONS OR TEST PAPERS THEREFOR CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL ORENZYMOLOGICAL PROCESSES ENZYMOLOGY HUMAN NECESSITIES HYGIENE MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEICACIDS OR MICROORGANISMS MEDICAL OR VETERINARY SCIENCE METALLURGY MICROBIOLOGY MUTATION OR GENETIC ENGINEERING PREPARATIONS FOR MEDICAL, DENTAL, OR TOILET PURPOSES PROCESSES OF PREPARING SUCH COMPOSITIONS SPIRITS VINEGAR WINE
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Zusammenfassung:	FIELD: biotechnology.SUBSTANCE: method of indirect determination of the completeness of inactivation of the rabies virus antigen using reverse transcriptase polymerase chain reaction (hereinafter - RT-PCR) followed by electrophoresis of amplicons in agarose gel is described. The completeness of inactivation of the rabies virus antigen is determined by RT-PCR using 5 systems of original primers (Shift Oligo-NR1069 (for the site of the highly conserved gene N of the rabies virus); PF1807-MR3020 (for the site that captures the genes P and M of the rabies virus); GF3471-ΨR5520 (for the site of the variable fragment of the G gene and the Ψ-area of the rabies virus); LF5499-LR6290 and LF8085-LR9954 (for the sites of the L gene of the rabies virus carrying information about RNA-dependent DNA polymerase)). Detection of the results of completeness of inactivation of the rabies virus is carried out in an ultraviolet light flux at a wavelength of 312 nm after horizontal electrophoresis in 1.5% agarose gel with the addition of 0.0005% ethidium bromide. In the presence of fluorescent amplicons obtained in PCR using 5 systems of original primers, the sample is virulent; in the absence of luminous PCR products in all 5 systems of primers, the sample is inactivated.EFFECT: present invention makes it possible to assess quickly and with a high degree of confidence the completeness of inactivation of the rabies virus antigen using a reverse transcriptase polymerase chain reaction followed by electrophoresis of amplicons in an agarose gel.8 cl, 8 tbl, 4 ex, 7 dwg Изобретение относится к области биотехнологии. Описан способ опосредованного определения полноты инактивации антигена вируса бешенства с применением обратно-транскриптазной полимеразной цепной реакции (ОТ-ПЦР) с последующим электрофорезом ампликонов в агарозном геле. Полноту инактивации антигена вируса бешенства определяют методом ОТ-ПЦР с использованием 5 систем оригинальных праймеров (Shift_Oligo-NR1069 (для участка высококонсервативного гена N вируса бешенства); PF1807-MR3020 (для участка, захватывающего гены Р и М вируса бешенства); GF3471-ΨR5520 (для участка вариабельного фрагмента гена G и Ψ-региона вируса бешенства); LF5499-LR6290 и LF8085-LR9954 (для участков L-гена вируса бешенства, несущего информацию о РНК-зависимой ДНК-полимеразе)). Детекцию результатов полноты инактивации вируса бешенства осуществляют в потоке ультрафиолетового света при длине волны 312 нм после проведения горизонтального электрофореза в