2021
DOI: 10.1016/j.ekir.2021.01.010
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Association of Local Unit Sampling and Microbiology Laboratory Culture Practices With the Ability to Identify Causative Pathogens in Peritoneal Dialysis-Associated Peritonitis in Thailand

Abstract: Introduction This describes variations in facility peritoneal dialysis (PD) effluent (PDE) culture techniques and local microbiology laboratory practices, competencies, and quality assurance associated with peritonitis, with a specific emphasis on factors associated with culture-negative peritonitis (CNP). Methods Peritonitis data were prospectively collected from 22 Thai PD centers between May 2016 and October 2017 as part of the Peritoneal Dialysis Outcomes and Practi… Show more

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Cited by 17 publications
(21 citation statements)
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“…144,145 The specimens should arrive at the laboratory within 6 h. If immediate delivery to the laboratory is not possible, the inoculated culture bottles should ideally be incubated at 37 C. Inoculated bottles should not be refrigerated or frozen, since it may kill or retard the growth of some microorganisms. 146 The solid media should be incubated in aerobic, microaerophilic and anaerobic environments. To fully assess yeast and filamentous fungal pathogens, appropriate fungal media should be selected; incubation of inoculated media under two temperature conditions (room temperature and 35-37 C) can increase the diagnostic yield.…”
Section: Identification Of Causative Organismsmentioning
confidence: 99%
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“…144,145 The specimens should arrive at the laboratory within 6 h. If immediate delivery to the laboratory is not possible, the inoculated culture bottles should ideally be incubated at 37 C. Inoculated bottles should not be refrigerated or frozen, since it may kill or retard the growth of some microorganisms. 146 The solid media should be incubated in aerobic, microaerophilic and anaerobic environments. To fully assess yeast and filamentous fungal pathogens, appropriate fungal media should be selected; incubation of inoculated media under two temperature conditions (room temperature and 35-37 C) can increase the diagnostic yield.…”
Section: Identification Of Causative Organismsmentioning
confidence: 99%
“…146 Notably, experience of the centre is important because culture-negative peritonitis rates frequently show an inverse relationship with the PD centre size. 38,146 When cultures remain negative after 3-5 days of incubation, PD effluent should be sent for repeat cell count, differential count, fungal and mycobacterial culture. In addition, subculture on media with aerobic, anaerobic and microaerophilic incubation conditions for a further 3-4 days may help to identify slow-growing fastidious bacteria and yeasts that are undetectable in some automated culture systems.…”
Section: Identification Of Causative Organismsmentioning
confidence: 99%
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“…This finding may have reflected a lack of clinician appreciation of the virulence of mold peritonitis in Thailand. Since most Thai PD facilities (91%) have limited ability to culture filamentous mold [ 28 ], the attending nephrologists may also have had limited experience treating fungal peritonitis and limited access to infectious disease specialists. Moreover, some facilities might have had limited facility HD backup support, resulting in a reluctance to remove the PD catheter and subsequent deviation in practice from the ISPD Guideline recommendation.…”
Section: Resultsmentioning
confidence: 99%
“…Cultivation of this specific organism in media with a high water activity (>0.98) or at a higher temperature than 30 °C (maximal temperature of 37 °C) significantly slow its growth [ 16 ]; therefore, traditional bacterial broth (water activity, 0.99) incubated at 37 °C may prevent growth of this rare yeast. Appropriate media should be selected to detect fungal pathogens, and incubation at different temperature conditions are recommended (room temperature and 35–37 °C) [ 19 ].…”
Section: Discussionmentioning
confidence: 99%