Prospective Multicenter Evaluation of a New Immunoassay and Real-Time PCR for Rapid Diagnosis of Clostridium difficile-Associated Diarrhea i
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微生物临床杂志 2005年第10期
Department of Medical Microbiology, Center of Infectious Diseases, Leiden University Medical Center, Leiden
Department of Medical Microbiology and Infectious Diseases, Erasmus MC, University Medical Center, Rotterdam
Department of Medical Microbiology, VU University Medical Center, Amsterdam, The Netherlands
ABSTRACT
In a prospective multicenter study, 367 fecal samples from 300 patients with diarrhea were tested for Clostridium difficile-associated diarrhea (CDAD) with a new immunochromatography assay for toxins A and B (ICTAB), a real-time PCR on the toxin B gene, and the cell cytotoxicity assay. Twenty-three (6.2%) of the 367 fecal samples were positive by the cell cytotoxicity assay. With the cell cytotoxicity assay as the "gold standard," the sensitivity, specificity, positive predictive value, and negative predictive value for the ICTAB assay and real-time PCR were 91, 97, 70, and 99%, and 87, 96, 57 and 99%, respectively. In conclusion, both the ICTAB and the real-time PCR can be implemented as rapid screening methods for patients suspected of having CDAD.
TEXT
Clostridium difficile-associated diarrhea (CDAD) is the most important infectious cause of nosocomial diarrhea and pseudomembranous colitis. The enteropathogenicity depends on the production of enterotoxin A (308 kDa) and cytotoxin B (270 kDa). Several authors have suggested that all fecal samples for C. difficile from patients with diarrhea hospitalized for more than 72 h be investigated (3) irrespective of the physician's request, since length of hospitalization is simple to implement as an inclusion criterion. Conventional diagnostic methods for CDAD are the cell cytotoxicity assay and the enzyme immunoassays (EIA) to detect fecal toxins A (TcdA) and B (TcdB). The cell cytotoxicity assay is considered the "gold standard." However, with a turnaround time of more than 48 h, this method is laborious and time-consuming. Frequently, EIA are used because of their more rapid turnaround time. Rapid diagnosis of CDAD is important, since it may result in early treatment and prevention of nosocomial transmission.
A new rapid immunochromatography test, the ImmunoCard Toxins A&B (ICTAB; Meridian), has recently been introduced. The ICTAB is a single-test enzyme immunoassay for the detection of TcdA and TcdB in fecal samples within 20 min. No sample pretreatment is required, and an internal procedure control is integrated in each card. The performance of this rapid assay was evaluated in comparison with an in-house-developed, real-time PCR using tcdB and the cell cytotoxicity assay. A positive PCR result for a fecal sample is indicative of the presence of a C. difficile strain capable of producing TcdB.
Fecal samples were collected from October 2003 to February 2004 at the Department of Medical Microbiology of three university medical centers in The Netherlands: Erasmus Medical Center Rotterdam (Erasmus MC), Leiden University Medical Center (LUMC), and the VU University Medical Center Amsterdam (VUMC). Fecal samples from adult patients with diarrhea for whom there was a request for C. difficile diagnosis and samples from patients hospitalized for more than 72 h were included. All samples were stored within 6 hours after arrival at the laboratory at –20°C in two individual vials for subsequent testing by the cell cytotoxicity assay and real-time PCR at the LUMC. The ICTAB was performed in the Erasmus MC and the LUMC. All fecal samples were thawed only once for a specific test.
The ICTAB was performed according to the respective manufacturer's instructions. Briefly, enzyme conjugate was added to specimen diluent before the addition of 25 μl of the fecal sample or the control. After incubation at room temperature for 5 min, the specimen was added to the lower ports of the card. This was again incubated at room temperature for 5 min, after which wash reagent was added to the upper ports, followed by substrate addition. Results were read in the upper ports after a 5-min incubation at room temperature.
The cell cytotoxicity assay (1) was performed using Vero cells in a 24-well format. Fecal samples were diluted 1:4 in Eagle's minimum essential medium with 5% fetal bovine serum and centrifuged. Subsequently, the supernatant was filtered through a 0.45-μm-pore-size filter. Neutralization of the cytotoxic effect was performed by using specific C. difficile antitoxin (TechLab, Blacksburg, VA).
For real-time PCR, primers 398CLDs (5'-GAAAGTCCAAGTTTACGCTCAAT-3') and 399CLDas (5'-GCTGCACCTAAACTTACACCA-3') were designed to amplify 177 bp of the nonrepeat region of the tcdB gene. A specific 6-carboxyfluorescein-labeled Taqman probe (5'-ACAGATGCAGCCAAAGTTGTTGAATT-3') was used as an internal probe (8a). The amplification reactions were performed in a 50-μl final volume, containing 25 μl IQ supermix (Bio-Rad, Veenendaal, The Netherlands), 5 pmol of the forward primer, 10 pmol of the reverse primer, 4 mM MgCl2, 0.2 μM probe, and 5 μl of DNA. After an enzyme activation step of 3 min at 95°C, the protocol consisted of 50 cycles of 30 s at 94°C for denaturation, 30 s at 57°C for annealing, and 30 s at 72°C for elongation. The iCycler IQ real-time detection system (Bio-Rad) was used for amplification and analysis. DNA isolation from fecal samples was performed using stool-transport-and-recovery buffer pretreatment and subsequent automated isolation by use of a MagnaPure LC DNA isolation kit III (Roche, Almere, The Netherlands) in the MagnaPure System, according to the manufacturer's instructions. An internal control, the phocine herpesvirus, was included for detection of inhibition in the PCR, as has been described before (6). The sensitivity was 1 x 103 CFU/ml, and in feces the detection limit was 1 x 105 CFU/g feces.
In total, 367 samples were included from 300 patients: 183 samples from the Erasmus MC, 65 from the VUMC, and 119 from the LUMC. No significant differences were observed in age, gender, department, and number of days of hospitalization of the patients from the three participating centers (data not shown). Forty-three (11.7%) samples from 39 patients were positive in one or more assays, and 23 samples (6.3%) from 22 patients were positive by the cell cytotoxicity assay (Table 1). The highest percentage of positive cell cytotoxicity tests (43%) was found in the Erasmus MC, followed by the LUMC (35%) and the VUMC (22%). No inhibitory samples were present in the real-time PCR. The sensitivity, specificity, positive predictive value (PPV) and negative predictive value (NPV) were 91, 97, 70 and 99% for the ICTAB assay and 87, 96, 57 and 99% for the real-time PCR, respectively, using the cell cytotoxicity assay as the "gold standard" (Table 1). The concordance of cell cytotoxicity with ICTAB was 97%, and the concordance with real-time PCR was 95%. No large differences in sensitivity, specificity, PPV, and NPV for the two tests were observed between the three centers.
Discrepancy analysis was performed by culture of all samples positive for C. difficile in one or more assays. Culture is known as the most sensitive method (4) and can therefore be applied for discrepancy analysis. Culture was performed as described previously (10), and all isolated strains were tested by PCR for the presence of tcdA and tcdB (9). True-positive test results were defined as fecal samples positive for the presence of a toxinogenic C. difficile strain. Forty of the 43 samples positive in one or more assays were available for specific culture of toxinogenic C. difficile. The results of the discrepancy analysis are presented in Table 2. Real-time PCR showed a concordance with culture of 80% (32/40 samples). The concordance of the cell cytotoxicity assay and ICTAB with toxinogenic culture was 75% (30/40 samples) for both methods. Using the results of the discrepancy analysis, the recalculated sensitivity, specificity, PPV, and NPV were 79, 99, 90 and 98% for the ICTAB assay, 88, 99, 88 and 99% for the real-time PCR, and 70, 100, 100 and 97% for the cell cytotoxicity assay, respectively. The low sensitivity of the cell cytotoxicity assay (70% compared to 79% and 88% for the ICTAB and the real-time PCR, respectively) indicates the limitation of the cell cytotoxicity assay as the "gold standard." Additionally, it provides an explanation for the low PPVs of both the ICTAB and real-time PCR in comparison with the cell cytotoxicity assay, also given that the PPV was 20 and 33% higher for ICTAB and real-time PCR, respectively, in the discrepancy analysis. The relatively low number of positive samples underlines the need for a larger study to verify these results.
Previous results obtained in our laboratory show that the detection limit for culture (1 x 104 CFU/g feces) was slightly better than that for real-time PCR (1 x 105 CFU/g feces). This can offer an explanation for the fact that four of seven samples negative by real-time PCR were positive by toxinogenic culture. The sensitivity for detection of C. difficile can be further optimized by inclusion of a target such as the gluD gene, encoding glutamate dehydrogenase (GDH; a moderate, specific enzyme commonly produced by C. difficile), or a multiple-copy target (5). A different DNA extraction method can improve the sensitivity of our real-time PCR with tcdB.
Current laboratory diagnosis of CDAD is based on the cell cytotoxicity assay for its specificity, an enzyme-immunoassay for its fast turnaround time, or toxinogenic culture for its sensitivity (2, 4, 7). Recently, new rapid EIA have been evaluated for the detection of GDH in feces (8, 11, 12). Snell et al. (8) compared two GDH/toxin assays with toxinogenic culture, and for confirmation of toxinogenicity they used PCR (on the gluD gene) and the cell cytotoxicity assay. The cell cytotoxicity assay had the highest sensitivity and PPV, but testing in combination with GDH and toxin detection resulted in 100% correct diagnosis of CDAD. In the study by Zheng et al. (12), a new EIA (C. DIFF CHEK) for the detection of GDH was described and compared to a homemade PCR using gluD and with toxinogenic culture. The PCR outperformed culture and showed a comparable result to the C. DIFF CHEK assay in sensitivity and specificity. However, the disadvantage of methods based on GDH or gluD is the inability to differentiate between toxin-positive and -negative strains, necessitating subsequent testing by other methods. Despite the excellent test statistics of the ICTAB compared to the cell cytotoxicity assay and real-time PCR, a comparison with other rapid EIA should be performed.
ICTAB results can be obtained within 20 min, and results for real-time PCR can be obtained within one working day. We conclude that, based on the excellent sensitivity, NPV, and rapidity, the new diagnostic ICTAB assay and in-house real-time PCR can be used as methods for first screening for CDAD.
ACKNOWLEDGMENTS
This work was supported by a grant from the Foundation Microbiology Leiden.
We thank Hadi Ameen for his technical support and Kate Templeton for her support and assistance with the manuscript.
REFERENCES
Delmee, M. 2001. Laboratory diagnosis of Clostridium difficile disease. Clin. Microbiol. Infect.7:411-416.
Fekety, R. 1997. Guidelines for the diagnosis and management of Clostridium difficile-associated diarrhea and colitis. American College of Gastroenterology, Practice Parameters Committee. Am. J. Gastroenterol. 92:739-750.
Gerding, D. N., S. Johnson, L. R. Peterson, M. E. Mulligan, and J. Silva, Jr. 1995. Clostridium difficile-associated diarrhea and colitis. Infect. Control Hosp. Epidemiol. 16:459-477.
Johnson, S., and D. N. Gerding. 1998. Clostridium difficile-associated diarrhea. Clin. Infect. Dis. 26:1027-1034.
Mackay, I. M. 2004. Real-time PCR in the microbiology laboratory. Clin. Microbiol. Infect. 10:190-212.
Niesters, H. G. 2002. Clinical virology in real time. J. Clin. Virol. 25(Suppl. 3):S3-2.
Oldfield, E. C., III. 2004. Clostridium difficile-associated diarrhea: risk factors, diagnostic methods, and treatment. Rev. Gastroenterol. Disord. 4:186-195.
Snell, H., M. Ramos, S. Longo, M. John, and Z. Hussain. 2004. Performance of the TechLab C. DIFF CHEK-60 enzyme immunoassay (EIA) in combination with the C. difficile Tox A/B II EIA kit, the Triage C. difficile panel immunoassay, and a cytotoxin assay for diagnosis of Clostridium difficile-associated diarrhea. J. Clin. Microbiol. 42:4863-4865.
van den Berg, R. J., E. J. Kuijper, E. S. Bruijnesteijn van Coppenraet, and E. C. J. Claas. Clin. Microbiol. Infect., in press.
van den Berg, R. J., E. C. Claas, D. H. Oyib, C. H. Klaassen, L. Dijkshoorn, J. S. Brazier, and E. J. Kuijper. 2004. Characterization of toxin A-negative, toxin B-positive Clostridium difficile isolates from outbreaks in different countries by amplified fragment length polymorphism and PCR ribotyping. J. Clin. Microbiol. 42:1035-1041.
van den Berg, R. J., H. A. Ameen, T. Furusawa, E. C. Claas, E. R. van der Vorm, and E. J. Kuijper. 2005. Coexistence of multiple PCR-ribotype strains of Clostridium difficile in faecal samples limits epidemiological studies. J. Med. Microbiol. 54:173-179.
Wilkins, T. D., and D. M. Lyerly. 2003. Clostridium difficile testing: after 20 years, still challenging. J. Clin. Microbiol. 41:531-534.
Zheng, L., S. F. Keller, D. M. Lyerly, R. J. Carman, C. W. Genheimer, C. A. Gleaves, S. J. Kohlhepp, S. Young, S. Perez, and K. Ye. 2004. Multicenter evaluation of a new screening test that detects Clostridium difficile in fecal specimens. J. Clin. Microbiol. 42:3837-3840.(Renate J. van den Berg, L)
Department of Medical Microbiology and Infectious Diseases, Erasmus MC, University Medical Center, Rotterdam
Department of Medical Microbiology, VU University Medical Center, Amsterdam, The Netherlands
ABSTRACT
In a prospective multicenter study, 367 fecal samples from 300 patients with diarrhea were tested for Clostridium difficile-associated diarrhea (CDAD) with a new immunochromatography assay for toxins A and B (ICTAB), a real-time PCR on the toxin B gene, and the cell cytotoxicity assay. Twenty-three (6.2%) of the 367 fecal samples were positive by the cell cytotoxicity assay. With the cell cytotoxicity assay as the "gold standard," the sensitivity, specificity, positive predictive value, and negative predictive value for the ICTAB assay and real-time PCR were 91, 97, 70, and 99%, and 87, 96, 57 and 99%, respectively. In conclusion, both the ICTAB and the real-time PCR can be implemented as rapid screening methods for patients suspected of having CDAD.
TEXT
Clostridium difficile-associated diarrhea (CDAD) is the most important infectious cause of nosocomial diarrhea and pseudomembranous colitis. The enteropathogenicity depends on the production of enterotoxin A (308 kDa) and cytotoxin B (270 kDa). Several authors have suggested that all fecal samples for C. difficile from patients with diarrhea hospitalized for more than 72 h be investigated (3) irrespective of the physician's request, since length of hospitalization is simple to implement as an inclusion criterion. Conventional diagnostic methods for CDAD are the cell cytotoxicity assay and the enzyme immunoassays (EIA) to detect fecal toxins A (TcdA) and B (TcdB). The cell cytotoxicity assay is considered the "gold standard." However, with a turnaround time of more than 48 h, this method is laborious and time-consuming. Frequently, EIA are used because of their more rapid turnaround time. Rapid diagnosis of CDAD is important, since it may result in early treatment and prevention of nosocomial transmission.
A new rapid immunochromatography test, the ImmunoCard Toxins A&B (ICTAB; Meridian), has recently been introduced. The ICTAB is a single-test enzyme immunoassay for the detection of TcdA and TcdB in fecal samples within 20 min. No sample pretreatment is required, and an internal procedure control is integrated in each card. The performance of this rapid assay was evaluated in comparison with an in-house-developed, real-time PCR using tcdB and the cell cytotoxicity assay. A positive PCR result for a fecal sample is indicative of the presence of a C. difficile strain capable of producing TcdB.
Fecal samples were collected from October 2003 to February 2004 at the Department of Medical Microbiology of three university medical centers in The Netherlands: Erasmus Medical Center Rotterdam (Erasmus MC), Leiden University Medical Center (LUMC), and the VU University Medical Center Amsterdam (VUMC). Fecal samples from adult patients with diarrhea for whom there was a request for C. difficile diagnosis and samples from patients hospitalized for more than 72 h were included. All samples were stored within 6 hours after arrival at the laboratory at –20°C in two individual vials for subsequent testing by the cell cytotoxicity assay and real-time PCR at the LUMC. The ICTAB was performed in the Erasmus MC and the LUMC. All fecal samples were thawed only once for a specific test.
The ICTAB was performed according to the respective manufacturer's instructions. Briefly, enzyme conjugate was added to specimen diluent before the addition of 25 μl of the fecal sample or the control. After incubation at room temperature for 5 min, the specimen was added to the lower ports of the card. This was again incubated at room temperature for 5 min, after which wash reagent was added to the upper ports, followed by substrate addition. Results were read in the upper ports after a 5-min incubation at room temperature.
The cell cytotoxicity assay (1) was performed using Vero cells in a 24-well format. Fecal samples were diluted 1:4 in Eagle's minimum essential medium with 5% fetal bovine serum and centrifuged. Subsequently, the supernatant was filtered through a 0.45-μm-pore-size filter. Neutralization of the cytotoxic effect was performed by using specific C. difficile antitoxin (TechLab, Blacksburg, VA).
For real-time PCR, primers 398CLDs (5'-GAAAGTCCAAGTTTACGCTCAAT-3') and 399CLDas (5'-GCTGCACCTAAACTTACACCA-3') were designed to amplify 177 bp of the nonrepeat region of the tcdB gene. A specific 6-carboxyfluorescein-labeled Taqman probe (5'-ACAGATGCAGCCAAAGTTGTTGAATT-3') was used as an internal probe (8a). The amplification reactions were performed in a 50-μl final volume, containing 25 μl IQ supermix (Bio-Rad, Veenendaal, The Netherlands), 5 pmol of the forward primer, 10 pmol of the reverse primer, 4 mM MgCl2, 0.2 μM probe, and 5 μl of DNA. After an enzyme activation step of 3 min at 95°C, the protocol consisted of 50 cycles of 30 s at 94°C for denaturation, 30 s at 57°C for annealing, and 30 s at 72°C for elongation. The iCycler IQ real-time detection system (Bio-Rad) was used for amplification and analysis. DNA isolation from fecal samples was performed using stool-transport-and-recovery buffer pretreatment and subsequent automated isolation by use of a MagnaPure LC DNA isolation kit III (Roche, Almere, The Netherlands) in the MagnaPure System, according to the manufacturer's instructions. An internal control, the phocine herpesvirus, was included for detection of inhibition in the PCR, as has been described before (6). The sensitivity was 1 x 103 CFU/ml, and in feces the detection limit was 1 x 105 CFU/g feces.
In total, 367 samples were included from 300 patients: 183 samples from the Erasmus MC, 65 from the VUMC, and 119 from the LUMC. No significant differences were observed in age, gender, department, and number of days of hospitalization of the patients from the three participating centers (data not shown). Forty-three (11.7%) samples from 39 patients were positive in one or more assays, and 23 samples (6.3%) from 22 patients were positive by the cell cytotoxicity assay (Table 1). The highest percentage of positive cell cytotoxicity tests (43%) was found in the Erasmus MC, followed by the LUMC (35%) and the VUMC (22%). No inhibitory samples were present in the real-time PCR. The sensitivity, specificity, positive predictive value (PPV) and negative predictive value (NPV) were 91, 97, 70 and 99% for the ICTAB assay and 87, 96, 57 and 99% for the real-time PCR, respectively, using the cell cytotoxicity assay as the "gold standard" (Table 1). The concordance of cell cytotoxicity with ICTAB was 97%, and the concordance with real-time PCR was 95%. No large differences in sensitivity, specificity, PPV, and NPV for the two tests were observed between the three centers.
Discrepancy analysis was performed by culture of all samples positive for C. difficile in one or more assays. Culture is known as the most sensitive method (4) and can therefore be applied for discrepancy analysis. Culture was performed as described previously (10), and all isolated strains were tested by PCR for the presence of tcdA and tcdB (9). True-positive test results were defined as fecal samples positive for the presence of a toxinogenic C. difficile strain. Forty of the 43 samples positive in one or more assays were available for specific culture of toxinogenic C. difficile. The results of the discrepancy analysis are presented in Table 2. Real-time PCR showed a concordance with culture of 80% (32/40 samples). The concordance of the cell cytotoxicity assay and ICTAB with toxinogenic culture was 75% (30/40 samples) for both methods. Using the results of the discrepancy analysis, the recalculated sensitivity, specificity, PPV, and NPV were 79, 99, 90 and 98% for the ICTAB assay, 88, 99, 88 and 99% for the real-time PCR, and 70, 100, 100 and 97% for the cell cytotoxicity assay, respectively. The low sensitivity of the cell cytotoxicity assay (70% compared to 79% and 88% for the ICTAB and the real-time PCR, respectively) indicates the limitation of the cell cytotoxicity assay as the "gold standard." Additionally, it provides an explanation for the low PPVs of both the ICTAB and real-time PCR in comparison with the cell cytotoxicity assay, also given that the PPV was 20 and 33% higher for ICTAB and real-time PCR, respectively, in the discrepancy analysis. The relatively low number of positive samples underlines the need for a larger study to verify these results.
Previous results obtained in our laboratory show that the detection limit for culture (1 x 104 CFU/g feces) was slightly better than that for real-time PCR (1 x 105 CFU/g feces). This can offer an explanation for the fact that four of seven samples negative by real-time PCR were positive by toxinogenic culture. The sensitivity for detection of C. difficile can be further optimized by inclusion of a target such as the gluD gene, encoding glutamate dehydrogenase (GDH; a moderate, specific enzyme commonly produced by C. difficile), or a multiple-copy target (5). A different DNA extraction method can improve the sensitivity of our real-time PCR with tcdB.
Current laboratory diagnosis of CDAD is based on the cell cytotoxicity assay for its specificity, an enzyme-immunoassay for its fast turnaround time, or toxinogenic culture for its sensitivity (2, 4, 7). Recently, new rapid EIA have been evaluated for the detection of GDH in feces (8, 11, 12). Snell et al. (8) compared two GDH/toxin assays with toxinogenic culture, and for confirmation of toxinogenicity they used PCR (on the gluD gene) and the cell cytotoxicity assay. The cell cytotoxicity assay had the highest sensitivity and PPV, but testing in combination with GDH and toxin detection resulted in 100% correct diagnosis of CDAD. In the study by Zheng et al. (12), a new EIA (C. DIFF CHEK) for the detection of GDH was described and compared to a homemade PCR using gluD and with toxinogenic culture. The PCR outperformed culture and showed a comparable result to the C. DIFF CHEK assay in sensitivity and specificity. However, the disadvantage of methods based on GDH or gluD is the inability to differentiate between toxin-positive and -negative strains, necessitating subsequent testing by other methods. Despite the excellent test statistics of the ICTAB compared to the cell cytotoxicity assay and real-time PCR, a comparison with other rapid EIA should be performed.
ICTAB results can be obtained within 20 min, and results for real-time PCR can be obtained within one working day. We conclude that, based on the excellent sensitivity, NPV, and rapidity, the new diagnostic ICTAB assay and in-house real-time PCR can be used as methods for first screening for CDAD.
ACKNOWLEDGMENTS
This work was supported by a grant from the Foundation Microbiology Leiden.
We thank Hadi Ameen for his technical support and Kate Templeton for her support and assistance with the manuscript.
REFERENCES
Delmee, M. 2001. Laboratory diagnosis of Clostridium difficile disease. Clin. Microbiol. Infect.7:411-416.
Fekety, R. 1997. Guidelines for the diagnosis and management of Clostridium difficile-associated diarrhea and colitis. American College of Gastroenterology, Practice Parameters Committee. Am. J. Gastroenterol. 92:739-750.
Gerding, D. N., S. Johnson, L. R. Peterson, M. E. Mulligan, and J. Silva, Jr. 1995. Clostridium difficile-associated diarrhea and colitis. Infect. Control Hosp. Epidemiol. 16:459-477.
Johnson, S., and D. N. Gerding. 1998. Clostridium difficile-associated diarrhea. Clin. Infect. Dis. 26:1027-1034.
Mackay, I. M. 2004. Real-time PCR in the microbiology laboratory. Clin. Microbiol. Infect. 10:190-212.
Niesters, H. G. 2002. Clinical virology in real time. J. Clin. Virol. 25(Suppl. 3):S3-2.
Oldfield, E. C., III. 2004. Clostridium difficile-associated diarrhea: risk factors, diagnostic methods, and treatment. Rev. Gastroenterol. Disord. 4:186-195.
Snell, H., M. Ramos, S. Longo, M. John, and Z. Hussain. 2004. Performance of the TechLab C. DIFF CHEK-60 enzyme immunoassay (EIA) in combination with the C. difficile Tox A/B II EIA kit, the Triage C. difficile panel immunoassay, and a cytotoxin assay for diagnosis of Clostridium difficile-associated diarrhea. J. Clin. Microbiol. 42:4863-4865.
van den Berg, R. J., E. J. Kuijper, E. S. Bruijnesteijn van Coppenraet, and E. C. J. Claas. Clin. Microbiol. Infect., in press.
van den Berg, R. J., E. C. Claas, D. H. Oyib, C. H. Klaassen, L. Dijkshoorn, J. S. Brazier, and E. J. Kuijper. 2004. Characterization of toxin A-negative, toxin B-positive Clostridium difficile isolates from outbreaks in different countries by amplified fragment length polymorphism and PCR ribotyping. J. Clin. Microbiol. 42:1035-1041.
van den Berg, R. J., H. A. Ameen, T. Furusawa, E. C. Claas, E. R. van der Vorm, and E. J. Kuijper. 2005. Coexistence of multiple PCR-ribotype strains of Clostridium difficile in faecal samples limits epidemiological studies. J. Med. Microbiol. 54:173-179.
Wilkins, T. D., and D. M. Lyerly. 2003. Clostridium difficile testing: after 20 years, still challenging. J. Clin. Microbiol. 41:531-534.
Zheng, L., S. F. Keller, D. M. Lyerly, R. J. Carman, C. W. Genheimer, C. A. Gleaves, S. J. Kohlhepp, S. Young, S. Perez, and K. Ye. 2004. Multicenter evaluation of a new screening test that detects Clostridium difficile in fecal specimens. J. Clin. Microbiol. 42:3837-3840.(Renate J. van den Berg, L)