Early Prediction of Bloodstream Infection with Complete Blood Count Parameters: an Ex-Vivo Human Whole Blood Model.

IF 0.7 4区医学 Q4 MEDICAL LABORATORY TECHNOLOGY Clinical laboratory Pub Date : 2024-04-01 DOI:10.7754/Clin.Lab.2023.231013

S. Ignak, Ozlem Unay-Demirel, Meral Yuksel

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Abstract

BACKGROUND Despite the advanced laboratory technologies available today, blood culture is the gold standard method in the diagnosis of bloodstream infections. Automated blood culture devices give blood culture results for laboratories approximately in 2 - 3 days up to 7 days. Moreover, some microorganisms like nonreproducible bacteria, fungi or viruses cannot be produced in culture. Among all samples taken for blood culture on suspicion of infection approximately 10% are determined as positive whereas the false positive rate due to contamination is 5%. Especially in life-threatening severe conditions such as sepsis early diagnosis and prompt treatment are crucial. Based on this the aim of this study is to investigate complete blood count parameters as potential early markers in Escherichia coli, Staphylococcus aureus and Candida albicans bloodstream infections using an ex vivo whole blood model. METHODS Blood samples collected from healthy donors (n = 10) were treated with suspensions containing a certain concentration of microorganisms (107 CFU/mL for both E. coli ATCC 25922 and S. aureus ATCC 29213, 106 CFU/mL for C. albicans ATCC 14053). After bacteremia and candidemia were induced, complete blood count parameters were analyzed hourly in the samples until the end of the 4th hour with a Mindray BC-6800 hematology analyzer. Statistical analysis was performed by Tukey-Kramer post-hoc multiple comparison test and statistical significance was accepted as p < 0.05. RESULTS When platelet derived parameter baseline values were compared to hourly values in E. coli and S. aureus induced whole blood samples, it was found that the decrease in PLT, P-LCC and the increase in IPF% was significant from the first hour whereas the increase in IMG% was found to be significant only from the 3rd hour onward. In the experiments with C. albicans, it was observed that the increase in IPF% and IMG% was significant from the 2nd and 3rd hour onward, respectively. There was no relationship between MPV, P-LCR, and NLR baseline and hourly results in any microorganism induced model. CONCLUSIONS IPF% can guide clinicians in the early diagnosis and management of treatment of infections caused by S. aureus, E. coli, and C. albicans.

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利用全血细胞计数参数早期预测血流感染：体外人体全血模型。

背景尽管当今的实验室技术非常先进，但血液培养仍是诊断血流感染的金标准方法。自动血液培养设备可在 2-3 天至 7 天内为实验室提供血液培养结果。此外，一些微生物如不可复制的细菌、真菌或病毒无法在培养过程中产生。在所有因怀疑感染而采集的血液培养样本中，约有 10%被确定为阳性，而因污染而导致的假阳性率为 5%。特别是在败血症等危及生命的严重情况下，早期诊断和及时治疗至关重要。基于此，本研究旨在利用体外全血模型研究全血细胞计数参数作为大肠杆菌、金黄色葡萄球菌和白色念珠菌血流感染的潜在早期标记物。方法用含有一定浓度微生物（大肠杆菌 ATCC 25922 和金黄色葡萄球菌 ATCC 29213 均为 107 CFU/mL，白色念珠菌 ATCC 14053 为 106 CFU/mL）的悬浮液处理从健康捐献者（n = 10）处采集的血样。诱发菌血症和念珠菌血症后，使用 Mindray BC-6800 血液分析仪每小时对样本的全血细胞计数参数进行分析，直至第 4 小时结束。结果将大肠杆菌和金黄色葡萄球菌诱导的全血样本中血小板衍生参数基线值与每小时值进行比较后发现，PLT、P-LCC 的下降和 IPF% 的增加从第一小时开始就很显著，而 IMG% 的增加仅从第三小时开始才显著。在白僵菌实验中，观察到 IPF% 和 IMG% 的增加分别从第 2 小时和第 3 小时开始显著。在任何微生物诱导的模型中，MPV、P-LCR 和 NLR 基线与每小时结果之间均无关系。

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来源期刊

Clinical laboratory 医学-医学实验技术

CiteScore

1.50

自引率

0.00%

发文量

494

审稿时长

3 months

期刊介绍： Clinical Laboratory is an international fully peer-reviewed journal covering all aspects of laboratory medicine and transfusion medicine. In addition to transfusion medicine topics Clinical Laboratory represents submissions concerning tissue transplantation and hematopoietic, cellular and gene therapies. The journal publishes original articles, review articles, posters, short reports, case studies and letters to the editor dealing with 1) the scientific background, implementation and diagnostic significance of laboratory methods employed in hospitals, blood banks and physicians'' offices and with 2) scientific, administrative and clinical aspects of transfusion medicine and 3) in addition to transfusion medicine topics Clinical Laboratory represents submissions concerning tissue transplantation and hematopoietic, cellular and gene therapies.

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