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Journal of Clinical Microbiology, May 2005, p. 2274-2276, Vol. 43, No. 5
0095-1137/05/$08.00+0 doi:10.1128/JCM.43.5.2274-2276.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.
Faculty of Tropical Medicine, Mahidol University, Bangkok, Thailand,1 Menzies School of Health Research, Charles Darwin University and Northern Territory Clinical School, Flinders University, Darwin, Australia,2 Medical Department, Sappasithiprasong Hospital, Ubon Ratchathani, Thailand,3 Centre for Clinical Vaccinology and Tropical Medicine, Nuffield Department of Clinical Medicine, University of Oxford, Churchill Hospital, Oxford OX3 7LJ, United Kingdom4
Received 22 November 2004/ Returned for modification 23 December 2004/ Accepted 19 January 2005
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105 CFU/ml from a neat sample. The overall in-hospital mortality rate was 45%. Patients with negative urine cultures had the lowest death rate (39%). Mortality rates rose with increasing B. pseudomallei counts in urine, from 58% for those with positive spun pellets only to 61% for those with between 103 CFU/ml and 105 CFU/ml and 71% for those with
105 CFU/ml. This was independent of age, presence of bacteremia, known risk factors for melioidosis such as diabetes, and the prior administration of antibiotics. The presence of B. pseudomallei in urine during systemic infection is associated with a poor prognosis. |
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Quantitative urine culture is a standard, inexpensive diagnostic test that is widely undertaken to provide laboratory evidence of urinary tract infection. The presence of
105 CFU/ml in urine culture is used to distinguish between a contaminated sample and one from a patient with urinary tract sepsis and is generally accepted as the gold standard for laboratory diagnosis (5). This interpretation is not applicable to patients with suspected melioidosis. B. pseudomallei is not a member of the human commensal flora, and the isolation of even a single colony in urine is both significant and sufficient to confirm the diagnosis of melioidosis. Furthermore, the significance of B. pseudomallei counts in urine is poorly understood. Although the urinary tract may be the primary source (especially in nephrolithiasis) of the organism or may become involved in the infective process, it is unclear whether the standard cutoff of
105 CFU/ml indicates an infection of the bladder, kidneys, or prostate. For this study, we explored the relationship between urinary symptoms and positive urine culture results for B. pseudomallei, determined whether the B. pseudomallei count in urine represents a marker for mortality risk, and defined the role of this simple, inexpensive technique in the diagnosis of melioidosis.
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Urine was collected into a sterile container and transported immediately to our on-site microbiology research laboratory. Using a sterile calibrated loop, we streaked 1 µl of fresh, unprocessed urine onto one half each of a MacConkey agar plate and an Ashdown's agar plate and then incubated the plates at 37°C for 2 days or 4 days, respectively. The remaining urine sample was centrifuged at 3,000 rpm for 5 min, excess supernatant was removed, and the pellet was cultured on one half of an Ashdown's agar plate. B. pseudomallei was identified by standard methodology as previously described (3).
For the purposes of analysis, urine culture results were divided into the following four groups based on the presence and number of B. pseudomallei cells: (i) no growth of B. pseudomallei from a neat sample or pellet, (ii) culture of B. pseudomallei from the centrifuged pellet only (<103 CFU/ml), (iii) detection of between 103 CFU/ml and 105 CFU/ml, or (iv) detection of
105 CFU/ml in a neat sample. Because renal tubular acidosis is endemic to this region, we specifically examined the profiles of a subgroup of patients with nondiabetic renal disease. Statistical analysis was performed with the statistical program Intercooled STATA, version 8.0 (College Station, Tex.). The trend across ordered groups was tested with a
2 test for trend. Logistic regression analysis was used to examine the independence of factors associated with quantitative urine cultures and the prognostic value of quantitative urine cultures for the survival outcome. Ethical approval for all clinical trials was obtained from the Ministry of Public Health, Royal Government of Thailand.
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Urine cultures that were positive for B. pseudomallei were analyzed from 171 patients (23%). Of these, 52 (30%) were positive from the spun pellet only (<103 CFU/ml), 51 (30%) contained between 103 CFU/ml and 105 CFU/ml, and 68 (40%) contained
105 CFU/ml. The urine culture was the only positive direct specimen in 70 cases. Nineteen of these (27%) were culture positive from the spun pellet only, and eight of these patients had negative blood cultures.
Positive urine cultures were significantly associated with increasing age, the presence of urinary symptoms, preexisting renal disease, and positive blood cultures upon both univariate and multiple-variable analyses. For both of these models, patients with diabetes and those who had received antibiotics which are active against B. pseudomallei prior to urine culture had lower rates of urine culture positivity (Table 1). The same factors predicted bacterial concentrations in the urine (data not shown). Only 41 patients (24%) with positive urine cultures had urinary symptoms.
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TABLE 1. Variables associated with positive urine cultures (n = 171) for 755 patients with melioidosisa
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In a multiple-variable model, a positive blood culture, a clinical diagnosis of pneumonia, and age were significantly associated with mortality, and diabetes and the prior administration of an effective antibiotic regimen were associated with survival. A positive urine culture was predictive of mortality independent of the prior receipt of active antibiotics, age, diabetes, blood culture positivity, and the presence of pneumonia. Furthermore, the magnitude of the urinary bacterial concentration was correlated with an increased risk of mortality compared to that of patients with negative urine cultures (
2 test for trend; P < 0.001) (Table 2).
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TABLE 2. Variables associated with in-hospital mortality (n = 337) for 755 patients with melioidosisa
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Genitourinary tract infections were previously thought to be infrequent in Thai patients compared with other population groups, such as those in northern Australia, where prostatic involvement has been described for 19% of male patients (2). During the 10-year period of this study, only 41 of 755 patients (5%) for whom urine culture was performed had both a positive urine culture and the clinical features of urinary tract sepsis. Since many patients did not have urine cultures performed and since patients with urinary symptoms were more likely to have cultures performed, it is likely that the true rate of urinary involvement is lower than that described in this study. The finding of asymptomatic bacteriuria has been considered to represent renal filtration of bacteria present in the blood, previously termed "spillover." We are currently investigating this assumption in a prospective study of simultaneous quantitative urine and blood cultures.
Chronic renal failure and/or renal calculi are well-recognized risk factors for melioidosis. In northeastern Thailand, renal tubular acidosis is endemic and is strongly associated with nephrolithiasis (4, 7). We found that patients with nondiabetic renal disease were more likely to have involvement of the urinary tract, probably reflecting calculi acting as a nidus of infection.
The observation that urinary symptoms are often absent from melioidosis patients with positive urine cultures indicates the utility of urine culture for the routine screening of patients with suspected disease. For one-third of patients with bacteriuria, B. pseudomallei would have been missed by standard urine culture techniques using undiluted urine since the cultures were positive for the spun urinary pellet alone. This indicates that the diagnostic sensitivity can be increased by using concentrating techniques prior to urine culture.
In conclusion, quantitative urine culture is a simple and inexpensive technique that has clinical utility for predicting the outcome of melioidosis independent of blood culture positivity and other potential confounders.
A.C. was supported by an Australian National Health and Medical Council Training Scholarship, and S.J.P. was supported by a Wellcome Trust Career Development Award in Clinical Tropical Medicine. This study was funded by the Wellcome Trust of Great Britain.
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