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Colorimetric Detection of Escherichia coli Based on the Enzyme-Induced Metallization of Gold Nanorods

机译:基于酶诱导的金纳米棒金属化比色法检测大肠杆菌

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摘要

A novel enzyme-induced metallization colorimetric assay is developed to monitor and measure beta-galactosidase (beta-gal) activity, and is further employed for colorimetric bacteriophage (phage)-enabled detection of Escherichia coli (E. coli). This assay relies on enzymatic reaction-induced silver deposition on the surface of gold nanorods (AuNRs). In the presence of beta-gal, the substrate p-aminophenyl beta-D-galactopyranoside is hydrolyzed to produce p-aminophenol (PAP). Reduction of silver ions by PAP generates a silver shell on the surface of AuNRs, resulting in the blue shift of the longitudinal localized surface plasmon resonance peak and multicolor changes of the detection solution from light green to orange-red. Under optimized conditions, the detection limit for beta-gal is 128 pM, which is lower than the conventional colorimetric assay. Additionally, the assay has a broader dynamic range for beta-gal detection. The specificity of this assay for the detection of beta-gal is demonstrated against several protein competitors. Additionally, this technique is successfully applied to detect E. coli bacteria cells in combination with bacteriophage infection. Due to the simplicity and short incubation time of this enzyme-induced metallization colorimetric method, the assay is well suited for the detection of bacteria in low-resource settings.
机译:开发了一种新型的酶诱导的金属比色测定法,以监测和测量β-半乳糖苷酶(β-gal)活性,并进一步用于大肠杆菌(E. coli)的比色噬菌体(噬菌体)检测。该测定法依赖于酶反应诱导的银在金纳米棒(AuNRs)表面上的沉积。在β-gal存在下,底物对氨基苯基β-D-吡喃半乳糖苷水解生成对氨基苯酚(PAP)。通过PAP还原银离子,会在AuNRs的表面上产生一个银壳,从而导致纵向局部表面等离振子共振峰发生蓝移,并使检测溶液的颜色从浅绿色变为橙红色。在最佳条件下,β-gal的检出限为128 pM,低于常规比色测定法。此外,该测定法具有更广的β-gal检测动态范围。针对几种蛋白质竞争者证明了该检测β-gal的特异性。此外,该技术已成功应用于结合噬菌体感染的大肠杆菌细胞检测。由于这种酶诱导的金属比色法的简便性和较短的孵育时间,因此该方法非常适合在低资源环境中检测细菌。

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