QUANTITATIVE PCR AS A METHOD FOR MONITORING RETROVIRAL INFECTION ON THE GENE LEVEL

被引：4

作者：

YOLOV, AA

KOZLOVA, AV

YAROSLAVTSEVA, NG

MEDNIKOV, BM

KARAMOV, EV

机构：

[1] DI IVANOVSKII INST VIROL,MOSCOW 123098,RUSSIA

[2] MOSCOW MV LOMONOSOV STATE UNIV,AN BELOZERSKY INST PHYSICOCHEM BIOL,MOSCOW,RUSSIA

来源：

VIRUS GENES | 1995年 / 10卷 / 01期

关键词：

RETROVIRAL INFECTION; HIV; QUANTITATIVE PCR; AIDS THERAPY; RECOMBINANT DNA;

D O I：

10.1007/BF01724296

中图分类号：

Q3 [遗传学];

学科分类号：

071007 ; 090102 ;

摘要：

For monitoring retroviral infection on the gene level, we propose the use of quantitative PCR with two internal standards: one for a fragment of the viral genome and the other for the host cell marker gene. The standards (one for HIV and the other for a human DNA marker gene HLA-DQ alpha) were constructed by PCR-mediated joining of DNA fragments and were found to be effective in quantitative PCR despite rather different structures of amplified fragments in target and standard DNAs. The number of HIV DNA copies was found to be 2-500 per 1000 lymphocytes in blood from HIV-infected patients and up to 5000 + per 1000 cells in chronically infected cell lines. The degree of infection thus measured was found to change over the course of treatment.

引用

收藏

页码：45 / 51

页数：7

相关论文

共 18 条

[1] FREQUENCY OF CELLS POSITIVE FOR HIV-1 SEQUENCES ASSESSED BY IN-SITU POLYMERASE CHAIN-REACTION [J].

BAGASRA, O ;

SESHAMMA, T ;

OAKES, JW ;

POMERANTZ, RJP .

AIDS, 1993, 7 :S7-S10

[2] ABSOLUTE MESSENGER-RNA QUANTIFICATION USING THE POLYMERASE CHAIN-REACTION (PCR) - A NOVEL-APPROACH BY A PCR AIDED TRANSCRIPT TITRATION ASSAY (PATTY) [J].

BECKERANDRE, M ;

HAHLBROCK, K .

NUCLEIC ACIDS RESEARCH, 1989, 17 (22) :9437-9446

[3] POLYMERASE-CHAIN REACTION - ANALYSIS OF DNA DNA HYBRIDIZATION BY CAPILLARY ELECTROPHORESIS [J].

BIANCHI, N ;

MISCHIATI, C ;

FERIOTTO, G ;

GAMBARI, R .

NUCLEIC ACIDS RESEARCH, 1993, 21 (15) :3595-3596

[4] USE OF COMPETITIVE POLYMERASE CHAIN-REACTION TO DETERMINE HIV-1 LEVELS IN RESPONSE TO ANTIVIRAL TREATMENTS [J].

BRUISTEN, SM ;

KOPPELMAN, MHGM ;

ROOS, MTL ;

LOELIGER, AE ;

REISS, P ;

BOUCHER, CAB ;

HUISMAN, HG .

AIDS, 1993, 7 :S15-S20

[5] QUANTITATION OF UNINTEGRATED HIV-1 DNA IN ASYMPTOMATIC PATIENTS IN THE PRESENCE OR ABSENCE OF ANTIRETROVIRAL THERAPY [J].

BUSH, CE ;

DONOVAN, RM ;

SMERECK, SM ;

STRANG, D ;

MARKOWITZ, N ;

SARAVOLATZ, LD .

AIDS RESEARCH AND HUMAN RETROVIRUSES, 1993, 9 (02) :183-187

[6]

DAQUILLA RT, 1992, PERKIN ELMER BIOTECH, P14

[7]

DAQUILLA RT, 1991, NUCLEIC ACIDS RES, V19, P749

[8] A NOVEL PROCEDURE FOR QUANTITATIVE POLYMERASE CHAIN-REACTION BY COAMPLIFICATION OF COMPETITIVE TEMPLATES [J].

DIVIACCO, S ;

NORIO, P ;

ZENTILIN, L ;

MENZO, S ;

CLEMENTI, M ;

BIAMONTI, G ;

RIVA, S ;

FALASCHI, A ;

GIACCA, M .

GENE, 1992, 122 (02) :313-320

[9] GENERATION OF SINGLE-STRANDED-DNA BY THE POLYMERASE CHAIN-REACTION AND ITS APPLICATION TO DIRECT SEQUENCING OF THE HLA-DQA LOCUS [J].

GYLLENSTEN, UB ;

ERLICH, HA .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (20) :7652-7656

[10] ENGINEERING HYBRID GENES WITHOUT THE USE OF RESTRICTION ENZYMES - GENE-SPLICING BY OVERLAP EXTENSION [J].

HORTON, RM ;

HUNT, HD ;

HO, SN ;

PULLEN, JK ;

PEASE, LR .

GENE, 1989, 77 (01) :61-68