Kan Kültüründe Kalite Güvence Göstergelerinin ve Kontaminasyon Oranının Değerlendirilmesi

Year 2021, Volume: 13 Issue: 3, 557 - 562, 18.10.2021

Şükrü Öksüz Betül Dönmez Banu Keskin Nagihan Memiş Zeynep Dilara Karamurat Emel Çalışkan Cihadiye Öztürk İdris Şahin

https://doi.org/10.18521/ktd.858764

Cited By: 1

Abstract

Amaç: Kan kültürü, sepsise neden olan mikroorganizmaların üretilmesini ve tanımlanmasını sağladığı, antibiyotik tedavisini zamanında başlamayı ve mortalite ve morbiditeyi azalttığı için hasta takibinde hayati öneme sahiptir. Bu çalışmada hastanemiz mikrobiyoloji laboratuvarında otomatik kan kültür sisteminde üretilen mikroorganizmaların kalite göstergeleri açısından değerlendirilmesi amaçlanmıştır.
Metod: Bu çalışmada, XXX Üniversitesi Tıbbi Mikrobiyoloji Laboratuvarına gönderilen kan kültürü örneklerinden otomatize kan kültürü BACTEC-9120 (Becton Dickinson, ABD) sisteminde üreyen mikroorganizmalar retrospektif değerlendirilmiştir. Bu amaçla kan kültürü istemi yapılan örneklerin reddedilme ve kontaminasyon oranı, Gram boyama sonucu-son identifikasyon uyum oranı, tek şişe gönderilen örnek sayısı ve inkübasyon sonrası mikroorganizmaların üreme süreleri belirlenmiştir.
Bulgular: Laboratuvara çeşitli kliniklerden gönderilen 5037 kan kültür örneği dahil edilmiştir. Bu örneklerden %1.7’si uygunsuz numune olarak reddedilmiştir. Gram boyama -son identifikasyon uyumu araştırılmış ve %97,8 olarak saptanmıştır. Gönderilen örneklerin tek şişe sayısı 511 olarak bulunmuştur. Çalışmaya alınan 5037 örneğin, %20.7’sinde üreme saptanmış, bunların %10.2’si kontaminant olarak kabul edilmiştir. Araştırmamızda üreme süresi incelenen etkenlerin ortalama üreme süresi 30,29 saat olarak saptanmıştır.
Sonuç: Sonuç olarak, kan kültürlerinde gerçek patojenleri kontaminant ajanlardan ayırt etmek için altın standart yoktur.

Keywords

kan kültürü, bakteriyemi, kalite göstergeleri

Evaluation of Quality Assurance Indicators and Contamination Rate in Blood Culture

Abstract

Objective: Blood culture are of vital importance in patient follow-up, as they enable the identification and production of sepsis causative microorganisms, initiate antibiotic treatment in a timely manner and reduce mortality and morbidity. In this study, it is aimed to evaluate the microorganisms grown in the automated blood culture in the microbiology laboratory of the hospital in terms of quality indicators.
Method: In this study, microorganisms grown from automated blood culture BACTEC-9120 (Becton Dickinson, USA) system from the blood culture samples sent to XXX University Medical Microbiology Laboratory were evaluated retrospectively. For this purpose, the rejection and contamination rate of the samples for which blood culture was requested, the result of Gram staining-final identification compliance, the number of samples sent from a single bottle, and the growth times of microorganisms after incubation were determined.
Result: 5037 blood culture samples were sent to the laboratory from various clinics. 1.7% of these samples were rejected as inappropriate samples. Gram stain-final identification compatibility of blood cultures was investigated and it was determined as 97.8%. The single bottle number of the samples sent was found to be 511. For the 5037 samples included in the study, growth was detected in 20.7%, of which 10.2% were considered as contaminants. In our study, the average breeding time of the factors examined for breeding time was determined to be 30.29 hours.
Conclusion: As conclusion, there is no gold standard to distinguish true pathogens from contaminant agents in blood cultures.

Keywords

blood culture, bacteremia, quality indicators

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