Rapid and sensitive detection of Chlamydia trachomatis using a ligatable binary RNA probe and Qβ replicase

被引：2

作者：

Stefano, JE ^{[1
]}

Cenovese, L ^{[1
]}

An, Q ^{[1
]}

Lu, L ^{[1
]}

McCarty, J ^{[1
]}

Du, Y ^{[1
]}

Stefano, K ^{[1
]}

Burg, JL ^{[1
]}

King, W ^{[1
]}

Lane, DJ ^{[1
]}

机构：

[1] GENE TRAK Inc, Framingham, MA 01701 USA

来源：

MOLECULAR AND CELLULAR PROBES | 1997年 / 11卷 / 06期

关键词：

Q beta replicase; T4 DNA ligase; exponential amplification; nucleic acid diagnostics; C-trachomatis;

D O I：

10.1006/mcpr.1997.0135

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

A simple assay format was developed for the direct detection of C. trachomatis rRNA utilizing ligation of recombinant MDV-1 probe RNA fragments hybridized to 23S rRNA after capture and release from a solid support. Assay background (equivalent to 10(4) targets) was suppressed by blocking sequences in the 5' MDV reporter probe fragment complementary to the 3' fragment by prehybridization of a DNA oligonucleotide. A pair of reporter fragments bearing a deletion within the region, obtained by a hydrid-selection-amplification protocol, yielded a low level of assay background which was reduced to < 2 % with a blocker directed against the remaining pairing sequence. This probe set showed a sensitivity of 10(3) molecules of 23S rRNA (> 95 % responding) and could detect a single elementary body (EB) of Chlamydia trachomatis or 1 - 10 EB added to a clinical matrix of pooled negative human cervical swab samples. The time of first appearance of amplification products by real-time fluorescence detection showed a linear response to log increases in the target lever over a 10(5)-fold range, permitting the determination of target level within an order of magnitude. The assay showed similar to 10(9)-fold discrimination over Chlamydia pneumonae (TWAR) rRNA. High levels of cultured C. albicans, E. coli, S. aureus, or N. gonorrhoeae had no detectable effect on assay background or the ability to detect a single elementary body. (C) 1997 Academic Press Limited.

引用

页码：407 / 426

页数：20

共 35 条

[1] COMPARISON OF CHARACTERISTICS OF Q-BETA REPLICASE-AMPLIFIED ASSAY WITH COMPETITIVE PCR ASSAY FOR CHLAMYDIA-TRACHOMATIS
AN, Q
LIU, J
OBRIEN, W
RADCLIFFE, G
BUXTON, D
POPOFF, S
KING, W
VERAGARCIA, M
LU, L
SHAH, J
KLINGER, J
OLIVE, DM
[J]. JOURNAL OF CLINICAL MICROBIOLOGY, 1995, 33 (01) : 58 - 63
[2] COLIPHAGE Q-BETA RNA REPLICATION - RNA CATALYTIC FOR SINGLE-STRAND RELEASE
AXELROD, VD
BROWN, E
PRIANO, C
MILLS, DR
[J]. VIROLOGY, 1991, 184 (02) : 595 - 608
[3] INVITRO RECOMBINATION AND TERMINAL ELONGATION OF RNA BY Q-BETA REPLICASE
BIEBRICHER, CK
LUCE, R
[J]. EMBO JOURNAL, 1992, 11 (13) : 5129 - 5135
[4] Burg JL, 1996, MOL CELL PROBE, V10, P257
[5] REAL-TIME FLUORESCENCE DETECTION OF RNA AMPLIFIED BY Q-BETA REPLICASE
BURG, JL
CAHILL, PB
KUTTER, M
STEFANO, JE
MAHAN, DE
[J]. ANALYTICAL BIOCHEMISTRY, 1995, 230 (02) : 263 - 272
[6] Accurate quantification of hepatitis C virus (HCV) RNA from all HCV genotypes by using branched-DNA technology
Detmer, J
Lagier, R
Flynn, J
Zayati, C
Kolberg, J
Collins, M
Urdea, M
SanchezPescador, R
[J]. JOURNAL OF CLINICAL MICROBIOLOGY, 1996, 34 (04) : 901 - 907
[7] DIMOND RL, 1991, Patent No. 09776
[8] A NEW PROCEDURE FOR THE SIMULTANEOUS LARGE-SCALE PURIFICATION OF BACTERIOPHAGE-T4-INDUCED POLYNUCLEOTIDE KINASE, DNA-LIGASE, RNA LIGASE AND DNA-POLYMERASE
DOLGANOV, GM
CHESTUKHIN, AV
SHEMYAKIN, MF
[J]. EUROPEAN JOURNAL OF BIOCHEMISTRY, 1981, 114 (02): : 247 - 254
[9] RNA-CATALYZED SYNTHESIS OF COMPLEMENTARY-STRAND RNA
DOUDNA, JA
SZOSTAK, JW
[J]. NATURE, 1989, 339 (6225) : 519 - 522
[10] A novel method for real time quantitative RT PCR
Gibson, UEM
Heid, CA
Williams, PM
[J]. GENOME RESEARCH, 1996, 6 (10): : 995 - 1001

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