菌血症
细菌
荧光原位杂交
微生物学
大肠杆菌
全血
生物
多路复用
血培养
聚合酶链反应
原位杂交
原位
化学
免疫学
抗生素
生物化学
生物信息学
有机化学
基因表达
基因
遗传学
染色体
作者
Min Seok Lee,Hwi Hyun,Inwon Park,Sungho Kim,Dong-Hyun Jang,Seonghye Kim,Jae-Kyeong Im,Hajin Kim,Jae Hyuk Lee,Taejoon Kwon,Joo H. Kang
标识
DOI:10.1002/smtd.202101239
摘要
The current diagnosis of bacteremia mainly relies on blood culture, which is inadequate for the rapid and quantitative determination of most bacteria in blood. Here, a quantitative, multiplex, microfluidic fluorescence in situ hybridization method (μFISH) is developed, which enables early and rapid (3-h) diagnosis of bacteremia without the need for prior blood culture. This novel technology employs mannose-binding lectin-coated magnetic nanoparticles, which effectively opsonize a broad range of pathogens, magnetically sequestering them in a microfluidic device. Therein, μFISH probes, based on unique 16S rRNA sequences, enable the identification and quantification of sequestered pathogens both in saline and whole blood, which is more sensitive than conventional polymerase chain reaction. Using μFISH, Escherichia coli (E. coli) is detected in whole blood collected from a porcine disease model and from E. coli-infected patients. Moreover, the proportion of E. coli, relative to other bacterial levels in the blood, is accurately and rapidly determined, which is not possible using conventional diagnostic methods. Blood from E. coli-infected patients is differentiated from healthy donors' blood using cutoff values with a 0.05 significance level. Thus, μFISH is a versatile method that can be used to rapidly identify pathogens and determine their levels relative to other culturable and nonculturable bacteria in biological samples.
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