Previous Article | Next Article 
Journal of Clinical Microbiology, September 1998, p. 2766-2768, Vol. 36, No. 9
Department of Pathology, University of Texas
Medical Branch, Galveston, Texas 77555-0740
Received 26 March 1998/Returned for modification 1 June
1998/Accepted 10 June 1998
The reliability of the BDProbeTec MTB Test (Becton Dickinson,
Sparks, Md.) for direct detection of Mycobacterium
tuberculosis in respiratory specimens was evaluated by comparing
results to those of conventional mycobacterial culture, with the BACTEC
TB 460 and Middlebrook 7H11 biplates. Patients known to have
tuberculosis were excluded from analysis. Of 523 specimens from 277 patients, 53 grew a mycobacterium: 24 specimens of M. tuberculosis and 29 specimens of nontuberculous mycobacteria.
After initial testing, 42 specimens were positive by the BDProbeTec,
for overall sensitivity, specificity, and positive and negative
predictive values of 95.8, 96.2, 54.8, and 99.8%, respectively. After
resolution of discrepancies, 28 specimens were positive by the
BDProbeTec, for overall sensitivity, specificity, and positive and
negative predictive values of 100, 99.2, 85.7, and 100%, respectively.
These same values were 100, 80.8, 93.4, and 100%, respectively, for
smear-positive samples and 100, 99.4, 75.0, and 100%, respectively,
for smear-negative specimens.
Tuberculosis remains a public health
problem in the United States, despite a declining incidence during the
past several years. One of the most critical aspects of tuberculosis
control is rapid identification of infectious patients, a process which
for many years was based on staining smears for acid-fast bacilli (AFB) and culturing samples for mycobacteria with a liquid and a solid medium. AFB smear results generally are available in 24 h or less, but a positive result is not specific for tuberculosis. Mycobacterial culture and identification results, which provide a specific diagnosis, are not available for 2 to 3 weeks or longer. In response to the need
for a more rapid diagnostic test, several manufacturers have developed
nucleic acid amplification tests specific for Mycobacterium tuberculosis complex (MTBC) (9). Currently, two such
tests (Amplified Mycobacterium tuberculosis Direct Test [Gen-Probe, Inc., San Diego, Calif.] and AMPLICOR Mycobacterium tuberculosis PCR
assay [Roche Molecular Systems, Branchburg, N.J.]) are commercially available in the United States for detection of MTBC in AFB
smear-positive specimens (1-6, 8, 10).
Becton Dickinson (Sparks, Md.) recently developed a semiautomated
system Specimens.
Respiratory specimens (expectorated and induced
sputum samples, tracheal aspirates, bronchial washings, and
bronchoalveolar lavage fluids) submitted to the clinical microbiology
laboratory at the University of Texas Medical Branch for detection of
mycobacteria from April through June 1997 were included in the study.
Samples from patients receiving therapy for previously diagnosed
tuberculosis were excluded from analysis.
Specimen processing and culture.
Specimens were decontaminated
with 1% sodium hydroxide (final
concentration)-N-acetylcysteine and concentrated by
centrifugation at 3,000 × g for 20 min, according to a
standard procedure (7). Approximately 0.2 µl of the
sediment was used to prepare a smear for staining with auramine O. Phosphate-buffered saline was added to the remaining sediment to give a
volume of 2.0 ml. For mycobacterial culture, 0.5 ml of the suspension
was inoculated into a BACTEC 12B bottle and 0.2 ml was inoculated onto
each side of a Middlebrook 7H11 selective biplate. The remainder of the
specimen was stored at BDProbeTec MTB Test.
Frozen samples were thawed, vigorously
agitated on a vortex mixer, and processed according to the
manufacturer's directions. Briefly, 500 µl of specimen was added to
1.0 ml of sample diluent A (which had been heated for 1 h in a
50°C water bath), agitated on a vortex mixer, and centrifuged at
12,200 × g for 3 min. The supernatant was discarded,
and the pellet was washed three times as follows: 1.0 ml of sample
diluent B was added, the pellet was resuspended by being mixed on a
vortex mixer, and the suspension was centrifuged at 12,200 × g for 3 min. After the third wash, the supernatant was
discarded, and one sample processing capsule, one glass bead, and 400 µl of sample diluent B were added to the pellet. The mixture was
vigorously agitated on a vortex mixer and then frozen at
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Clinical Evaluation of the BDProbeTec Strand
Displacement Amplification Assay for Rapid Diagnosis of
Tuberculosis
ABSTRACT
Top
Abstract
Text
References
TEXT
Top
Abstract
Text
References
the BDProbeTECfor the rapid detection of MTBC in respiratory
specimens. The enabling chemistry utilized is a thermophilic version of
strand displacement amplification, which enzymatically replicates
target nucleic acid sequences exponentially to detectable levels.
Sediments of decontaminated and concentrated clinical specimens are
processed off-line, with several washes to remove inhibitors, followed
by heat inactivation and mechanical agitation to lyse the mycobacteria.
Processed specimens are then placed onto the BDProbeTec sample handling
unit, where they are robotically introduced to the
decontamination-amplification devices (DADs), which are disposable,
single-use reagent cartridges that allow for amplicon decontamination
followed by subsequent amplification (by strand displacement
amplification) of the target and provide an internal amplification
control. Once amplification is complete, the amplified material is
harvested, and product is detected via target-specific sandwich
hybridization assays, which occur in disposable, single-use assay
devices (ADs). Amplification is demonstrated via a chemiluminescent
signal that is detected in a luminometer. The purpose of this study was
to evaluate the performance of the BDProbeTec MTB Test for direct
detection of MTBC in respiratory specimens in a clinical setting.
20°C for batch testing by the BDProbeTec MTB
Test. BACTEC bottles were incubated at 37°C in 8% CO2
and monitored for growth for 8 weeks by the BACTEC 460 TB instrument
according to the manufacturer's recommendations, as described in
detail elsewhere (7). Plates were incubated at 37°C in 8%
CO2 and examined weekly for growth for 8 weeks. Isolates of
mycobacteria were identified by DNA probes (AccuProbe [Gen-Probe,
Inc.] for MTBC, Mycobacterium avium complex, Mycobacterium kansasii, and Mycobacterium
gordonae) or by conventional biochemical tests (for rapidly
growing mycobacteria), performed according to the standard protocol
(7). Isolates not identified by these procedures were
referred to the Texas Department of Health for identification by
high-performance liquid chromatography and/or conventional biochemical
tests.
20°C.
Prior to BDProbeTec testing, samples were thawed at room temperature.
Two positive and three negative controls were prepared by adding 400 µl of sample diluent B to each. Samples and controls were lysolyzed
for 30 min at 105°C, and samples only were agitated in the CellPrep
instrument for 45 s at 5.0 m/s. Both samples and controls were
pulse-centrifuged for 15 s and then transferred to the BDProbeTec
instrument, which was programmed according to the manufacturer's
directions to transfer an aliquot of each patient sample and control to
the DAD and then to the AD. Within 10 min after the BDProbeTec process
was completed, trays containing samples and controls were manually
transferred to the luminometer for reading.
Discrepant analysis. If the culture and BDProbeTec results were discordant, a second aliquot of the frozen sample that had been processed for amplification was tested by the BDProbeTec. If the results remained discrepant, the patient's medical record was reviewed (if available).
A total of 526 specimens were included in the study. For 24 of these specimens, the initial BDProbeTec result could not be interpreted due to failure of the internal amplification control. After testing of a second aliquot from these 24 samples, 3 remained uninterpretable due to failure of the internal control. These latter three specimens were excluded from the analysis, leaving 523 evaluable specimens from 277 patients. Fifty-three specimens (10.1%) grew a mycobacterium: 24 specimens of MTBC (from nine patients) and 29 of nontuberculous mycobacteria (NTM), including 12 of M. avium complex, 9 of Mycobacterium fortuitum-chelonae complex, 2 of M. gordonae, 1 of M. kansasii, and 5 of Mycobacterium nonchromogenicum. The smear for AFB was positive in 20 cases (12 patients), of which 15 were from a culture that grew MTBC and 5 were from a culture that grew NTM (two of M. avium complex, two of M. fortuitum-chelonae complex, and one of M. nonchromogenicum). On initial testing, 42 of the 523 specimens from 27 patients were positive for MTBC by the BDProbeTec. Twenty-three of these were MTBC culture positive, three grew NTM, and the rest were culture negative. Based on these results, the initial overall sensitivity, specificity, and positive and negative predictive values of the BDProbeTec for diagnosis of tuberculosis were 95.8, 96.2, 54.8, and 99.8%, respectively. These same values were 100, 80.0, 93.8, and 100%, respectively, for the 20 AFB smear-positive specimens and 88.9, 96.4, 30.8, and 99.8%, respectively, for the AFB smear-negative samples. The one false-positive BDProbeTec result for smear-positive specimens was from a specimen that grew M. fortuitum-chelonae complex. On testing of a second aliquot of the 20 specimens that yielded discordant BDProbeTec and culture results, one specimen failed due to fluid in the device and was excluded from analysis. Of the remaining 522 evaluable samples, 28 samples from 16 patients were BDProbeTec positive (Table 1). Based on these data, the overall revised sensitivity, specificity, and positive and negative predictive values were 100, 99.2, 85.7, and 100%, respectively. These same values were 100, 80.0, 93.4, and 100%, respectively, for AFB smear-positive specimens and 100, 99.4, 75.0, and 100%, respectively, for smear-negative samples. Of the four patients with discrepant culture and BDProbeTec results, charts of two were available for review, and both had pulmonary disease caused by M. fortuitum-chelonae complex.
|
| |
ACKNOWLEDGMENTS |
|---|
This study was supported by Becton, Dickinson and Company. G.L.W. is supported in part by a Tuberculosis Academic Award from the National Heart, Lung, and Blood Institute (K07 HL03335).
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: Department of Pathology, University of Texas Medical Branch, Galveston, TX 77555-0740. Phone: (409) 772-4851. Fax: (409) 772-5683. E-mail: GWOODS{at}UTMB.EDU.
| |
REFERENCES |
|---|
|
Top
Abstract
Text
References
|
|---|
| 1. | American Thoracic Society Workshop. 1997. Rapid diagnostic tests for tuberculosis. What is the appropriate use? Am. J. Respir. Crit. Care Med. 155:1804-1814[Abstract]. |
| 2. | Bergmann, J. S., and G. L. Woods. 1996. Clinical evaluation of the Roche Amplicor PCR Mycobacterium tuberculosis test for detection of M. tuberculosis in respiratory specimens. J. Clin. Microbiol. 34:1083-1085[Abstract]. |
| 3. | Dalovisio, J. R., S. Montenegro-James, S. A. Kemmerly, C. F. Genre, R. Chambers, D. Greer, G. A. Pankey, D. M. Failla, K. G. Haydel, L. Hutchinson, M. F. Lindley, B. M. Nunez, A. Praba, K. D. Eisenach, and E. S. Cooper. 1996. Comparison of the Amplified Mycobacterium tuberculosis (MTB) Direct Test, Amplicor MTB PCR, and IS6110-PCR for detection of MTB in respiratory specimens. Clin. Infect. Dis. 23:1099-1106[Medline]. |
| 4. | Gamboa, F., J. M. Manterola, B. Vinado, L. Matas, M. Gimenez, J. Lonca, J. R. Manzano, C. Rodrigo, P. J. Cardona, E. Padilla, J. Dominguez, and V. Ausina. 1997. Direct detection of Mycobacterium tuberculosis complex in nonrespiratory specimens by Gen-Probe Amplified Mycobacterium Tuberculosis Direct Test. J. Clin. Microbiol. 35:307-310[Abstract]. |
| 5. | Ichiyama, S., Y. Iinuma, Y. Tawada, S. Yamora, Y. Hasegawa, K. Shimokata, and N. Nakashima. 1996. Evaluation of Gen-Probe Amplified Mycobacterium Tuberculosis Direct Test and Roche PCR-microwell plate hybridization method (Amplicor Mycobacterium) for direct detection of mycobacteria. J. Clin. Microbiol. 34:130-133[Abstract]. |
| 6. | Moore, D. F., and J. I. Curry. 1995. Detection and identification of Mycobacterium tuberculosis directly from sputum sediments by Amplicor PCR. J. Clin. Microbiol. 33:2686-2691[Abstract]. |
| 7. | Nolte, F. S., and B. Metchock. 1995. Mycobacterium, p. 400-437. In P. R. Murray, E. J. Baron, M. A. Pfaller, F. C. Tenover, and R. H. Yolken (ed.), Manual of clinical microbiology, 6th ed. ASM Press, Washington, D.C. |
| 8. | Piersimoni, C., A. Callegaro, D. Nista, S. Bornigia, F. DeConti, G. Santini, and G. DeSio. 1997. Comparative evaluation of two commercial amplification assays for direct detection of Mycobacterium tuberculosis complex in respiratory specimens. J. Clin. Microbiol. 35:193-196[Abstract]. |
| 9. |
Walker, G. T.,
J. G. Nadeau,
P. A. Spears,
J. L. Schram,
C. M. Nycz, and D. D. Shank.
1994.
Multiplex strand displacement amplification (SDA) and detection of DNA sequences from Mycobacterium tuberculosis and other mycobacteria.
Nucleic Acids Res.
22:2670-2677 |
| 10. | Wobeser, W. L., M. Kradjden, J. Conly, H. Simpson, B. Yim, M. D'Costa, M. Fuksa, C. Hian-Cheong, M. Patterson, A. Phillips, R. Bannatyne, A. Haddad, J. L. Brunton, and S. Krajden. 1996. Evaluation of Roche Amplicor PCR assay for Mycobacterium tuberculosis. J. Clin. Microbiol. 34:134-139[Abstract]. |
Journal of Clinical Microbiology, September 1998, p. 2766-2768, Vol. 36, No. 9
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
This article has been cited by other articles:
-
Bean, D. C., Hills, A., Ryan, T., Aitken, J.
(2007). Evaluation of the BD ProbeTec ET System for Direct Detection of Mycobacterium bovis in Veterinary Specimens. J. Clin. Microbiol.
45: 3434-3435
[Abstract] [Full Text] -
Huang, T.-S., Liu, Y.-C., Tu, H.-Z., Sy, C.-L., Chen, Y.-S., Chen, B.-C.
(2007). Rapid Purity Check Method for Susceptibility Testing of M. tuberculosis Complex with the MGIT 960 System. Annals of Clinical & Laboratory Science
37: 323-329
[Abstract] [Full Text] -
Dubaniewicz, A., Dubaniewicz-Wybieralska, M., Sternau, A., Zwolska, Z., Izycka-Swieszewska, E., Augustynowicz-Kopec, E., Skokowski, J., Singh, M., Zimnoch, L.
(2006). Mycobacterium tuberculosis Complex and Mycobacterial Heat Shock Proteins in Lymph Node Tissue from Patients with Pulmonary Sarcoidosis.. J. Clin. Microbiol.
44: 3448-3451
[Abstract] [Full Text] -
Palomino, J. C.
(2005). Nonconventional and new methods in the diagnosis of tuberculosis: feasibility and applicability in the field. Eur Respir J
26: 339-350
[Abstract] [Full Text] -
Chakravorty, S., Tyagi, J. S.
(2005). Novel Multipurpose Methodology for Detection of Mycobacteria in Pulmonary and Extrapulmonary Specimens by Smear Microscopy, Culture, and PCR. J. Clin. Microbiol.
43: 2697-2702
[Abstract] [Full Text] -
Wang, S. X., Sng, L. H., Tay, L.
(2004). Preliminary study on rapid identification of Mycobacterium tuberculosis complex isolates by the BD ProbeTec ET system. J Med Microbiol
53: 57-59
[Abstract] [Full Text] -
Piersimoni, C., Scarparo, C.
(2003). Relevance of Commercial Amplification Methods for Direct Detection of Mycobacterium tuberculosis Complex in Clinical Samples. J. Clin. Microbiol.
41: 5355-5365
[Full Text] -
Mazzarelli, G., Rindi, L., Piccoli, P., Scarparo, C., Garzelli, C., Tortoli, E.
(2003). Evaluation of the BDProbeTec ET System for Direct Detection of Mycobacterium tuberculosis in Pulmonary and Extrapulmonary Samples: a Multicenter Study. J. Clin. Microbiol.
41: 1779-1782
[Abstract] [Full Text] -
Bergmann, J. S., Keating, W. E., Woods, G. L.
(2000). Clinical Evaluation of the BDProbeTec ET System for Rapid Detection of Mycobacterium tuberculosis. J. Clin. Microbiol.
38: 863-865
[Abstract] [Full Text]
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
Copyright © 2009 by the American Society for Microbiology. For an alternate route to Journals.ASM.org, visit: http://intl-journals.asm.org | More Info»