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Applied and Environmental Microbiology, July 2001, p. 3122-3126, Vol. 67, No. 7
Institute of Milk Hygiene, Milk Technology,
and Food Science, University of Veterinary
Medicine,1 and Roche
Diagnostics GmbH,2 1210 Vienna, Austria
Received 11 December 2000/Accepted 20 April 2001
Two different real-time quantitative PCR (RTQ-PCR) approaches were
applied for PCR-based quantification of Staphylococcus aureus cells by targeting the thermonuclease
(nuc) gene. Purified DNA extracts from pure cultures of
S. aureus were quantified in a LightCycler system using
SYBR Green I. Quantification proved to be less sensitive (60 nuc gene copies/µl) than using a fluorigenic TaqMan
probe (6 nuc gene copies/µl). Comparison of the
LightCycler system and the well-established ABI Prism 7700 SDS with
TaqMan probes revealed no statistically significant differences with respect to sensitivity and reproducibility. Application of the RTQ-PCR
assay to quantify S. aureus cells in artificially
contaminated cheeses of different types achieved sensitivities from
1.5 × 102 to 6.4 × 102 copies of
the nuc gene/2 g, depending on the cheese matrix. The coefficients of correlation between log CFU and nuc gene
copy numbers ranged from 0.979 to 0.998, thus enabling calculation of
the number of CFU of S. aureus in cheese by performing
RTQ-PCR.
Food poisoning caused by the
enterotoxins produced by Staphylococcus aureus is of major
concern in food hygiene. Many outbreaks involving contaminated milk and
milk products have been reported (2, 8, 12, 13, 21). The
natural habitat of S. aureus is warm-blooded animals,
including humans. Ten to 40% of people are asymptomatic carriers of
S. aureus, mostly at the mucosal membrane (20).
Food handlers with infected skin lesions and asymptomatic carriers are
often sources of food contamination, although with milk and milk
products the raw milk itself can be contaminated with S. aureus.
Once introduced into food-processing plants, bacteria can persist for a
long time. CFU of S. aureus numbering
106 to 108 per g or ml of
food must be present in order to produce sufficient amounts of toxins
for poisoning (13). The bacteria are readily destroyed by
heat, but the toxins are thermostable. Austrian national regulations
concerning the presence of S. aureus in milk and milk products apply three-class plans that define m
values to separate acceptable from marginally acceptable
products and M values to separate marginally acceptable from
defective-quality products; when numbers of bacteria are higher than
M values, the presence of enterotoxins has to be
investigated. The International Standardization Organization and
International Dairy Federation methods (3, 4, 5, 6) apply
conventional microbiological quantification techniques such as the
plate count method and the most-probable-number (MPN) method. Some of
these techniques require up to 6 days for quantification and detection,
thus being time-consuming. There are rapid alternative methods for
quantification of S. aureus cells. These comprise the
application of MPN-PCR (17), a rather laborious procedure,
and the quantification of the enzymatic activity of the bacterial
phosphatase (10), which is not specific and can therefore
be applied only to pure cultures.
Another rapid alternative is real-time quantitative PCR (RTQ-PCR)
(11), which quantifies DNA and thus has the potential for
accurate enumeration of microorganisms. To find the most convenient technique, two different approaches to RTQ-PCR-based quantification of
the nuc gene in S. aureus cells were performed
with a LightCycler system. This system combines an air thermocycler and
a fluorimeter, enabling rapid-cycle PCR. The first approach applies the
double-stranded DNA (dsDNA)-binding fluorescent dye SYBR Green I, and
the second approach applies a fluorescent probe called the TaqMan
probe. In addition, the sensitivity and repeatability of the results of
the RTQ-PCR assay employing the TaqMan probe in the LightCycler were
compared to those of the well-established ABI PRISM 7700 sequence
detection system (SDS), a heat block thermocycler with an
integrated fluorimeter. The application of different Taq DNA polymerases was tested. The optimized RTQ-PCR assay was used for quantification of the nuc gene of S. aureus cells
in artificially contaminated cheeses of different types.
Bacterial strains.
S. aureus DSM 1104 was used
for preparing the quantification standards for RTQ-PCR as well as for
contaminating the cheese samples. This strain was cultured at the
Institute for Milk Hygiene, Milk Technology and Food Science of the
University for Veterinary Medicine, Vienna, Austria, in a brain heart
infusion medium (Merck, Darmstadt, Germany) at 37°C for 15 h.
Preparation of the quantification standard.
One milliliter
of a pure culture of S. aureus DSM 1104 was subjected to DNA
isolation using a Puregene DNA isolation kit (Gentra Systems Inc.,
Minneapolis, Minn.) according to the manufacturer's instructions. DNA
concentration was measured fluorimetrically using a HoeferDyNA Quant200
apparatus (Pharmacia Biotech, San Francisco, Calif.). The copy
number of the nuc gene was determined by assuming that,
based on the molecular weight of the 2.7- to 2.8-mbp-sized genome of
S. aureus (18), 1 ng of DNA equals 6 × 105 times the entire genome and that the
nuc gene is a single-copy gene.
Oligonucleotides for RTQ-PCR.
The primers used for
amplifying a 269-bp fragment of the nuc gene in S. aureus cells have been previously published (9) and
were purchased from MWG Biotech (Ebersberg, Germany). In our work, the
sequence of the internal TaqMan probe was complementary to the sequence
of the published hybridization probe (9). At the 5' end,
the probe was labeled with 6-carboxy-fluorescein (FAM), and at
the 3' end, it was labeled with 6-carboxy-tetramethyl-rhodamine (TAMRA). It was synthesized by Metabion GmbH (Martinsried, Germany).
RTQ-PCR.
To quantify DNA by RTQ-PCR, an increase in
fluorescence emission during PCR proportional to the initial copy
number of the target gene is generated and detected. Both fluorescent
dsDNA-binding dyes and fluorigenic probes (either hybridization probes
or a TaqMan probe) can be applied. Fluorescence emission is detected for each PCR cycle. The threshold cycle
(CT) values must be determined. The
CT value is defined as the actual PCR
cycle when the fluorescence signal increases above the background
threshold. It indicates the number of target gene copies. PCR and
fluorescence detection can be performed in a combined thermocycler and fluorimeter.
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.7.3122-3126.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Comparison of Different Approaches To Quantify
Staphylococcus aureus Cells by Real-Time Quantitative
PCR and Application of This Technique for Examination of
Cheese
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
(i) SYBR Green I with the LightCycler.
RTQ-PCR with
SYBR Green I was performed using either the LightCycler-DNA Master SYBR
Green I Kit or, for hot-start PCR purposes, the
LightCycler-FastStart DNA Master SYBR Green I Kit (Roche Diagnostics GmbH, Mannheim, Germany) in a LightCycler. The 20-µl reaction mix
contained 1× LightCycler-DNA Master SYBR Green I or
LightCycler-FastStart DNA Master SYBR Green I; 5 or 4 mM
MgCl2; a 900, 600, or 300 nM concentration of
each primer; and 5 µl of the template. Times and temperatures applied
are shown in Table 1. For acquisition of
the fluorescent signal, channel F1 was used and the gain of F1 was set
at 5. For normalization of fluorescent data, the F1/1 ratio was
applied.
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(ii) TaqMan probe with the LightCycler and the ABI PRISM 7700 SDS.
RTQ-PCR using a TaqMan probe was performed in a LightCycler
by applying either the LightCycler-DNA Master Hybridization Probe Kit
or, for hot-start PCR purposes, the LightCycler-FastStart DNA Master
Hybridization Probe Kit (Roche Diagnostics GmbH). The 20-µl reaction
mix contained a 1× concentration of LightCycler-DNA Master
Hybridization probes or LightCycler-FastStart DNA Master Hybridization
probes, 4 mM MgCl2, a 300 nM concentration of the primer, a 100 nM concentration of the probe, and 5 µl of the
template. Times and temperatures are shown in Table
2. Channel F1 was used for data
acquisition, the gain of F1 was set at 2, and the F1 (FAM)/1 ratio was
applied for normalization of fluorescent data.
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Statistical procedures. When comparing the levels of performance of different reaction mixtures and different RTQ-PCR equipment, the CT values were first tested for outliers by the method of Nalimov as discussed by Kaiser and Gottschalk (14). The presence or absence of statistically significant differences between the approaches were investigated by F-test comparison of variances of the CT values.
Artificial contamination of cheese. Tilsiter-type semisoft cheese made from pasteurized milk and French Camembert made from raw milk were purchased at a local supermarket. Fresh cheese made from raw goat's milk was obtained from a local farm. All cheese types tested negative by RTQ-PCR for the presence of S. aureus DNA.
A pure culture of S. aureus DSM 1104 in brain heart infusion medium was subjected to a 10-fold dilution series in buffered peptone water, and the number of CFU of each dilution step was obtained by the plate count method using Baird Parker agar plates (Merck). One milliliter of each dilution step was added to 2 g of cheese with 45 ml of digestion buffer (100 mM Tris-HCl, 100 mM EDTA, 0.5% sodium dodecyl sulfate [pH 8.0]) diluted 1:10.DNA isolation from artificially contaminated cheese. DNA isolation from artificially contaminated cheese was performed as previously described (1), apart from the following modifications. Two grams of cheese was added to 45 ml of digestion buffer diluted 1:10 and containing 12 U of pronase (Fluka Chemie, Buchs, Switzerland) per ml, homogenized in a Laboratory Blender Stomacher 400 (Seward, London, United Kingdom) for 1 min, and subsequently incubated at 40°C for 3 h. After centrifugation at 5,700 × g for 15 min at 4°C, the fat layer and aqueous phase were discarded and the pellet was washed three times with TE buffer (10 mM Tris-HCl, 1 mM EDTA [pH 7.5]) and once with PCR buffer (50 mM KCl, 1.5 mM MgCl2, 10 mM Tris-HCl [pH 8.4]). Finally, the pellet was resolved in 25 µl (Tilsiter, cheese from goat's milk) or 250 µl (Camembert) of PCR buffer and 143 U of lysostaphin (Sigma-Aldrich GmbH, Steinheim, Germany) per ml was added. This solution was incubated at room temperature for 15 min. After addition of 8 U of proteinase K (Roche Diagnostics GmbH) per ml, samples were held at 60°C for 1 h and afterwards incubated for 15 min at 95°C. Cell debris was removed by centrifugation at 13,000 × g for 5 min. Five microliters of the supernatant was subjected to RTQ-PCR.
Calculation of the nuc gene copy number per 2 g of cheese. Calculation of the nuc gene copy number per 2 g of cheese was performed by multiplying the number of nuc gene copies per PCR with the ratio of the final suspension volume of the DNA isolated from 2 g of cheese and 5, as 5 µl of the final DNA suspension was subjected to PCR.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Setup of RTQ-PCR. A 269-bp fragment of the nuc gene was chosen as a target for detection and quantification in S. aureus cells by RTQ-PCR. This gene codes for an extracellular thermonuclease, which is produced at a frequency similar to that of the coagulase. The primers and probe had been used previously for amplification and identification of the fragment by conventional PCR. The specificities of the oligonucleotides have been demonstrated elsewhere (9). Preliminary testing proved these oligonucleotides to be suited for RTQ-PCR (data not shown).
Comparison of two different approaches for quantification of S. aureus cells by RTQ-PCR using a LightCycler. (i) SYBR Green I with the LightCycler. A 10-fold dilution series of pure DNA from S. aureus DSM 1104 ranging from 6 × 105 to 6 × 100 copies of the nuc gene/µl was quantified by RTQ-PCR with SYBR Green I. Detection of the amplicon was performed by examination of the Tms of the amplicons after PCR. The Tm of the specific 269-bp amplicon was 81°C. Nonspecific side products and primer dimers showed lower Tms. The detection limit was improved from 6,000 copies of the nuc gene/µl of the template to 60 copies by decreasing stepwise the concentrations of the primers from 900 to 300 nM and of MgCl2 from 5 to 4 mM and increasing the annealing temperature from 60 to 62°C. For samples containing less than 60 copies/µl of the template, no specific amplicon was generated. Application by hot-start PCR using a modified form of the thermostable recombinant Taq DNA polymerase, inactive at room temperature, improved the detection limit of the RTQ-PCR assay to 6 nuc gene copies/µl of the template. However, for samples containing less than 60 nuc gene copies/µl, more nonspecific side products than specific amplicons were generated. Binding of SYBR Green I to both the undesired PCR side products and the specific amplicon masked the signal of the latter, thus hindering accurate quantification of low copy numbers. Therefore, further experiments concentrated on the performance of a TaqMan probe for the quantification of S. aureus.
(ii) TaqMan probe with the LightCycler. The detection limit of the TaqMan probe was 60 copies of the nuc gene/µl. Once again, application of hot-start PCR improved the detection limit to 6 nuc gene copies/µl of the template DNA. Contrary to what occurred in SYBR Green I-based quantification, the signal generation through cleavage of the TaqMan probe was strictly specific. Therefore, an accurate quantification of low copy numbers was possible. All further experiments were then conducted by applying the TaqMan probe.
Quantification sensitivity and repeatability of RTQ-PCR results using either a commercial kit or an in-house reaction mix formula. To this point, all experiments had been performed using commercially available RTQ-PCR kits. The same quantification sensitivity as that obtained with the TaqMan probe and the kit for hot-start PCR was achieved when we used a PCR mix including Platinum Taq DNA polymerase (6 nuc gene copies/µl of the template DNA). This enzyme is inactive at room temperature as well. Further experiments compared the repeatability of the results obtained with the commercially available kit with those obtained with the PCR mix containing Platinum Taq DNA polymerase.
For each step of a 10-fold dilution series ranging from 6 × 104 to 6 × 100 copies/µl, the nuc gene of S. aureus was quantified six times after both polymerases were applied. Mean CT values and standard deviations are shown in Table 3. No statistically significant differences between the methods were observed. However, mean CT values were 1.03 to 2.07 lower when we used Platinum Taq DNA polymerase, indicating higher RTQ-PCR efficiency. Although both PCR mixtures worked satisfactorily, the in-house procedure was used for all further experiments due to budget limitations.
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TaqMan probe with the LightCycler versus TaqMan probe with the ABI PRISM 7700 SDS. As the LightCycler system is rather new equipment, its performance was compared to that of the well-established ABI PRISM 7700 SDS. Experiments to measure the quantification sensitivity and repeatability of results were conducted on both systems. Mean CT values and standard deviations for the measurements (repeated six times) of a 10-fold dilution series of the nuc gene of S. aureus ranging from 6 × 103 to 6 × 100 copies/µl are shown in Table 3. Regarding repeatability, no significant distinction was found between the two machines. The sensitivity of the RTQ-PCR assay in the ABI PRISM 7700 SDS was 6 copies of the nuc gene. The mean CT values were 0.38 to 0.98 higher than in the LightCycler, suggesting a slightly lower efficiency for the RTQ-PCR.
In summary, the TaqMan probe-LightCycler configuration was found to be the most appropriate for quantification of the nuc gene of S. aureus. Therefore, it was used for applicability testing in a cheese model.Quantification of S. aureus in artificially
contaminated cheese with the TaqMan probe-LightCycler
configuration.
Cheeses of three different types (Tilsiter-style
cheese, French Camembert made from raw milk, and fresh cheese made from
raw goat's milk) were artificially contaminated with different
concentrations of a pure culture of S. aureus DSM 1104. The
samples were then subjected to DNA isolation in triplicate, and
nuc gene copy numbers were measured twice by RTQ-PCR (Table
4). Mean nuc gene copy numbers
were compared to the numbers of CFU determined by the plate count
method. Quantification of S. aureus cells in Tilsiter and
goat's cheese consistently revealed nuc gene copy numbers comparable to numbers of CFU. Using Camembert, copy numbers were 1 log unit higher than numbers of CFU. The calculated coefficients of
correlation (r2) between log copy
numbers of the nuc gene and log CFU were 0.979 for Tilsiter,
0.996 for Camembert, and 0.998 for goat's cheese. The limit of
quantification was 3.8 × 102 nuc
gene copies/2 g of Tilsiter, 6.4 × 102
copies/2 g of Camembert, and 1.5 × 102
copies/2 g of goat's cheese. Samples containing lower copy numbers did
not reveal consistent quantification results.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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SYBR Green I with the LightCycler versus the TaqMan probe with the LightCycler. The dsDNA-binding dye SYBR Green I and a TaqMan probe were tested in different RTQ-PCR systems (LightCyler and ABI PRISM 7700 SDS) to determine the number of copies of the S. aureus nuc gene.
Accurate quantification of low copy numbers of the nuc gene of S. aureus using SYBR Green I was hindered due to the accumulation of primer dimers and nonspecific side products which were bound by the SYBR Green I dye. Measurement of the ratio of specific to nonspecific PCR products by determining the melting peak integration enabled quantification of low copy numbers (22). However, this procedure requires further post-PCR analysis of the data. In another publication, fluorescence data collection at a temperature above the Tms of nonspecific PCR products minimized biased quantification of low copy numbers of the gene (19). In our study, the Tms of nonspecific side products exceeded 72°C. Thus, the procedure would have required another PCR step subsequent to primer extension. To improve the sensitivity, an addition of tRNA to the PCR mix (23) may further reduce nonspecific side products. To overcome the shortcomings of SYBR Green I for the quantification of the nuc gene of S. aureus, a TaqMan probe was applied. Optimization included testing two different Taq DNA polymerases with respect to the 5'-3' exonuclease activities of the enzymes for cleavage of the probe. The FastStart Taq DNA polymerase, included in a commercial kit designed to be used in conjunction with hybridization probes (15) (which represents a slightly different approach to RTQ-PCR using fluorogenic probes), proved to be sufficient for sensitive quantification of the nuc gene using the TaqMan probe. Application of an in-house PCR mix containing Platinum Taq DNA polymerase also enabled sensitive quantification, with which, according to the product information, no 5'-3' exonuclease activity should be present. Moreover, CT values were 1.03 to 2.07 lower when this enzyme was applied, suggesting a higher efficiency of cleavage of the TaqMan probe. A recently published study used the same DNA polymerase for quantification of bcr and abl fusion transcripts by a TaqMan probe (15). When our assay configuration was applied to the LightCycler, repeatability was in accordance with recently published data (7, 16).TaqMan probe with the LightCycler versus TaqMan probe with the ABI PRISM 7700 SDS. The performance of the air-heated LightCycler was compared to that of the well-established ABI PRISM 7700 SDS 96-well block cycler. The algorithms for calculation of the initial target copy number and acquisition of fluorescence emission data differ substantially between both systems. In the ABI PRISM 7700 SDS, the increase in fluorescence emission of the reporter dye, generated by cleavage of the probe, is normalized either to the fluorescence emission of an additional fluorescent dye or to that of the quencher dye. Normalization to the emission of a separately added fluorescent dye is not feasible in the LightCycler. Excitation and data acquisition in the ABI PRISM 7700 SDS are performed continuously in parallel for all samples via fiber optic cables. In the LightCycler a high-precision stepper motor positions each sample above the fluorimetric optics, thus enabling data acquisition from each sample by the same optical device. However, both approaches led to comparable results in the present study. For high-throughput applications, the 96-well machine may be advantageous. For establishing new RTQ-PCR assays or examining smaller numbers of samples, the 32-capillary LightCycler may be preferable as it enables performance of PCR in less than 1 h and is much less expensive.
Quantification of S. aureus cells in cheese by RTQ-PCR. When we compared nuc gene copy numbers in S. aureus cells and numbers of CFU, matrix-dependent effects were observed. In the case of Tilsiter and fresh goat's cheese, CFU and nuc gene copy numbers were nearly identical. In the Camembert, about 1 log unit more nuc gene copies than CFU was detected. This result suggests different extraction efficiencies. Application of MPN-PCR for quantification of the enterotoxin c1 gene in fresh cheese revealed a copy number 2 log units higher than the number of CFU (17). Mäntynen et al. explained the bias by the detection of dead and stressed unculturable bacterial cells through PCR. The difference of 1 log unit in the Camembert suggests that only 10% of bacterial cells were culturable and therefore detectable by the plate count method. As fresh overnight cultures were applied for contamination, this should not have been the case in our experiments. Another explanation may be that S. aureus formed clusters during multiplication. They may not have been sufficiently broken up before the samples were plated onto agar plates. In this case 1 CFU would originate from more than one bacterial cell. However, the coefficients of correlation between copy numbers and numbers of CFU ranged from 0.979 to 0.998 for all cheese matrices tested. Therefore, the calculation of the number of CFU of S. aureus via determination of nuc gene copy numbers is possible.
The quantification limits of 20 and 290 CFU/2 g in raw milk Camembert and fresh goat's cheese, respectively, are sufficient for examination according to the national regulations (m = 1,000/g and M = 10,000/g). On the other hand, as Tilsiter is made from pasteurized milk, an m of 100/g and an M of 1,000/g apply. Therefore, the sensitivity of 350 CFU/2 g is sufficient only for detecting a transgression of the M value. When applying PCR-based quantification methods to heat-processed products, it must be considered that the DNAs from bacteria are detected whether they are alive or dead. In foodstuffs S. aureus is reliably killed when it is subjected to appropriate pasteurization conditions. However, the enterotoxins are still harmful due to their heat stability. Therefore PCR-based quantification methods which display the total contamination level of a toxin-producing pathogen present a distinct advantage over conventional microbiological methods. In conclusion, the suitability of RTQ-PCR for fast quantification of S. aureus cells in cheese using this particular technique was demonstrated. With regard to the different RTQ-PCR configurations, it was shown (i) that TaqMan probes are superior to SYBR Green I with respect to quantification of low copy numbers of the target gene by RTQ-PCR and (ii) that both types of RTQ-PCR equipment, the LightCycler and the ABI PRISM 7700 SDS, lead to comparable results despite differences in hardware and software.| |
ACKNOWLEDGMENT |
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This research was supported by the Hochschuljubiläumsstiftung, Vienna, Austria.
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FOOTNOTES |
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* Corresponding author. Mailing address: Institute of Milk Hygiene, Milk Technology and Food Science, University of Veterinary Medicine, Veterinärplatz 1, 1210 Vienna, Austria. Phone: 431250773511. Fax: 431250773590. E-mail: Ingeborg.Hein{at}vu-wien.ac.at.
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Applied and Environmental Microbiology, July 2001, p. 3122-3126, Vol. 67, No. 7
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.7.3122-3126.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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[Abstract] [Full Text] -
Park, T.-G., de Salas, M. F., Bolch, C. J. S., Hallegraeff, G. M.
(2007). Development of a Real-Time PCR Probe for Quantification of the Heterotrophic Dinoflagellate Cryptoperidiniopsis brodyi (Dinophyceae) in Environmental Samples. Appl. Environ. Microbiol.
73: 2552-2560
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Hierro, N., Esteve-Zarzoso, B., Gonzalez, A., Mas, A., Guillamon, J. M.
(2006). Real-Time Quantitative PCR (QPCR) and Reverse Transcription-QPCR for Detection and Enumeration of Total Yeasts in Wine. Appl. Environ. Microbiol.
72: 7148-7155
[Abstract] [Full Text] -
Monnet, C., Correia, K., Sarthou, A.-S., Irlinger, F.
(2006). Quantitative Detection of Corynebacterium casei in Cheese by Real-Time PCR. Appl. Environ. Microbiol.
72: 6972-6979
[Abstract] [Full Text] -
Ward, L. N., Bej, A. K.
(2006). Detection of Vibrio parahaemolyticus in Shellfish by Use of Multiplexed Real-Time PCR with TaqMan Fluorescent Probes.. Appl. Environ. Microbiol.
72: 2031-2042
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Yu, Z., Michel, F. C. Jr, Hansen, G., Wittum, T., Morrison, M.
(2005). Development and Application of Real-Time PCR Assays for Quantification of Genes Encoding Tetracycline Resistance. Appl. Environ. Microbiol.
71: 6926-6933
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Simon, H. M., Jahn, C. E., Bergerud, L. T., Sliwinski, M. K., Weimer, P. J., Willis, D. K., Goodman, R. M.
(2005). Cultivation of Mesophilic Soil Crenarchaeotes in Enrichment Cultures from Plant Roots. Appl. Environ. Microbiol.
71: 4751-4760
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Guilbaud, M., de Coppet, P., Bourion, F., Rachman, C., Prevost, H., Dousset, X.
(2005). Quantitative Detection of Listeria monocytogenes in Biofilms by Real-Time PCR. Appl. Environ. Microbiol.
71: 2190-2194
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Hachiya, A., Kobayashi, A., Yoshida, Y., Kitahara, T., Takema, Y., Imokawa, G.
(2004). Biphasic Expression of Two Paracrine Melanogenic Cytokines, Stem Cell Factor and Endothelin-1, in Ultraviolet B-Induced Human Melanogenesis. Am. J. Pathol.
165: 2099-2109
[Abstract] [Full Text] -
Audemard, C., Reece, K. S., Burreson, E. M.
(2004). Real-Time PCR for Detection and Quantification of the Protistan Parasite Perkinsus marinus in Environmental Waters. Appl. Environ. Microbiol.
70: 6611-6618
[Abstract] [Full Text] -
O'Mahony, J., Hill, C.
(2004). Rapid Real-Time PCR Assay for Detection and Quantitation of Mycobacterium avium subsp. paratuberculosis DNA in Artificially Contaminated Milk. Appl. Environ. Microbiol.
70: 4561-4568
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Labrenz, M., Brettar, I., Christen, R., Flavier, S., Botel, J., Hofle, M. G.
(2004). Development and Application of a Real-Time PCR Approach for Quantification of Uncultured Bacteria in the Central Baltic Sea. Appl. Environ. Microbiol.
70: 4971-4979
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Sharkey, F. H., Banat, I. M., Marchant, R.
(2004). Detection and Quantification of Gene Expression in Environmental Bacteriology. Appl. Environ. Microbiol.
70: 3795-3806
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Inglis, G. D., Kalischuk, L. D.
(2004). Direct Quantification of Campylobacter jejuni and Campylobacter lanienae in Feces of Cattle by Real-Time Quantitative PCR. Appl. Environ. Microbiol.
70: 2296-2306
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Skovhus, T. L., Ramsing, N. B., Holmstrom, C., Kjelleberg, S., Dahllof, I.
(2004). Real-Time Quantitative PCR for Assessment of Abundance of Pseudoalteromonas Species in Marine Samples. Appl. Environ. Microbiol.
70: 2373-2382
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Wolffs, P., Knutsson, R., Norling, B., Radstrom, P.
(2004). Rapid Quantification of Yersinia enterocolitica in Pork Samples by a Novel Sample Preparation Method, Flotation, Prior to Real-Time PCR. J. Clin. Microbiol.
42: 1042-1047
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Panicker, G., Myers, M. L., Bej, A. K.
(2004). Rapid Detection of Vibrio vulnificus in Shellfish and Gulf of Mexico Water by Real-Time PCR. Appl. Environ. Microbiol.
70: 498-507
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Phister, T. G., Mills, D. A.
(2003). Real-Time PCR Assay for Detection and Enumeration of Dekkera bruxellensis in Wine. Appl. Environ. Microbiol.
69: 7430-7434
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Burtscher, C., Wuertz, S.
(2003). Evaluation of the Use of PCR and Reverse Transcriptase PCR for Detection of Pathogenic Bacteria in Biosolids from Anaerobic Digestors and Aerobic Composters. Appl. Environ. Microbiol.
69: 4618-4627
[Abstract] [Full Text] -
Bleve, G., Rizzotti, L., Dellaglio, F., Torriani, S.
(2003). Development of Reverse Transcription (RT)-PCR and Real-Time RT-PCR Assays for Rapid Detection and Quantification of Viable Yeasts and Molds Contaminating Yogurts and Pasteurized Food Products. Appl. Environ. Microbiol.
69: 4116-4122
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Kolb, S., Knief, C., Stubner, S., Conrad, R.
(2003). Quantitative Detection of Methanotrophs in Soil by Novel pmoA-Targeted Real-Time PCR Assays. Appl. Environ. Microbiol.
69: 2423-2429
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Malinen, E., Kassinen, A., Rinttila, T., Palva, A.
(2003). Comparison of real-time PCR with SYBR Green I or 5'-nuclease assays and dot-blot hybridization with rDNA-targeted oligonucleotide probes in quantification of selected faecal bacteria. Microbiology
149: 269-277
[Abstract] [Full Text] -
Nicolas, L., Prina, E., Lang, T., Milon, G.
(2002). Real-Time PCR for Detection and Quantitation of Leishmania in Mouse Tissues. J. Clin. Microbiol.
40: 1666-1669
[Abstract] [Full Text] -
Gouarin, S., Gault, E., Vabret, A., Cointe, D., Rozenberg, F., Grangeot-Keros, L., Barjot, P., Garbarg-Chenon, A., Lebon, P., Freymuth, F.
(2002). Real-Time PCR Quantification of Human Cytomegalovirus DNA in Amniotic Fluid Samples from Mothers with Primary Infection. J. Clin. Microbiol.
40: 1767-1772
[Abstract] [Full Text]
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