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Label-free detection of nosocomial bacteria using a nanophotonic interferometric biosensor

机译:使用纳秒干涉生成生物传感器无标记检测医院细菌

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Nosocomial infections are a major concern at the worldwide level. Early and accurate identification of nosocomial pathogens is crucial to provide timely and adequate treatment. A prompt response also prevents the progression of the infection to life-threatening conditions, such as septicemia or generalized bloodstream infection. We have implemented two highly sensitive methodologies using an ultrasensitive photonic biosensor based on a bimodal waveguide interferometer (BiMW) for the fast detection of Pseudomonas aeruginosa and methicillin-resistant Staphylococcus aureus (MRSA), two of the most prevalent bacteria associated with nosocomial infections. For that, we have developed a biofunctionalization strategy based on the use of a PEGylated silane (silane-PEG-COOH) which provides a highly resistant and bacteria-repelling surface, which is crucial to specifically detect each bacterium. Two different biosensor assays have been set under standard buffer conditions: one based on a specific direct immunoassay employing polyclonal antibodies for the detection of P. aeruginosa and another one employing aptamers for the direct detection of MRSA. The biosensor immunoassay for P. aeruginosa is fast (it only takes 12 min) and specific and has experimentally detected concentrations down to 800 cfu mL~(-1) (cfu: colony forming unit). The second one relies on the use of an aptamer that specifically detects penicillin-binding protein 2a (PBP2a), a protein only expressed in the MRSA mutant, providing a photonic biosensor with the ability to identify the resistant pathogen MRSA and differentiate it from methicillin-susceptible S. aureus (MSSA). Direct, label-free, and selective detection of whole MRSA bacteria has been achieved, making possible the direct detection of also 800 cfu mL~(-1). According to the signal-to-noise (S/N) ratio of the device, a theoretical limit of detection (LOD) of around 49 and 29 cfu mL~(-1) was estimated for P. aeruginosa and MRSA, respectively. Both resu
机译:医院感染是全球范围内的主要问题。早期准确地鉴定医院病原体至关重要,提供及时和充分的治疗。迅速反应还可以防止感染进程对生命威胁的病症,例如败血症或广义血流感染。我们利用基于双峰波导干涉仪(BIMW)的超敏感光子生物传感器来实现两种高敏感的方法,用于快速检测假单胞菌铜绿假单胞菌和耐甲氧西林金黄色葡萄球菌(MRSA),其中两种与医院感染相关的最普遍的细菌。为此,我们开发了基于使用聚乙二醇化硅烷(硅烷-PEG-COOH)的生物官能化策略,该硅烷(硅烷-PEG-COOH)提供高抗性和细菌排斥的表面,这对于特异性检测每个细菌至关重要。在标准缓冲条件下设定了两种不同的生物传感器测定:基于采用多克隆抗体的特异性直接免疫测定,用于检测P.铜绿假单胞菌和用于直接检测MRSA的适体的另一个。用于P.铜绿假单胞菌的生物传感器免疫测定快(仅需要12分钟)和特异性,并实验地检测到800cfu ml〜(-1)(CFU:菌落形成单元)的浓度。第二个依赖于使用特异性检测青霉素结合蛋白2a(PBP2a)的适体,仅在MRSA突变体中表达的蛋白质,提供光子生物传感器,其能够鉴定抗性病原体MRSA并将其与甲氧西林分化易感金黄色葡萄球菌(MSSA)。已经实现了直接,无标记和选择性检测全MRSA细菌,使得可以直接检测800 CFU ML〜(-1)。根据装置的信号 - 噪声(S / N)比例,分别估计了49和29cFu ml〜(-1)的检测(LOD)的理论极限分别用于P.铜绿假单胞菌和MRSA。兼顾

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