Electrochemical fingerprinting of cephalosporin antibiotics and its applications for investigations of hydrolysis behavior.

Cephalosporin, as one of the most widely used antibiotics, study of its hydrolysis process is important for predicting their environmental persistence. Two critical factors are considered has the first priority, which are hydrolysis rate constant (kh) and half-life (t1/2). To date, many efforts have been made by using various analytical techniques to obtain the data for calculating kh and t1/2. However, the typical techniques such as UV/vis spectrophotometry and liquid chromatography are of significant challenges like low accuracy and timely operations. Herein, we explored an electrochemical method by identifying the characteristic peaks with the same parent nuclear structure through square wave voltammetry (SWV). This proposed electrochemical fingerprinting was able to track the hydrolysis of intact cephalosporin molecules, ß-lactam ring, and transformation product. The kh and t1/2 of cefadroxil (CDX) under pH = 7 and 25 °C by electrochemical (0.0640 d-1 and 11.0 d) were consistent with those of high-performance liquid chromatography-UV/vis (HPLC-UV/vis) (0.0660 d-1 and 10.7 d). The t1/2 ranged from 3.40 to 36.2 d, 7.33 d-43.7 d and 9.63 d-45.3 d for base-catalyzed, neutral pH and acid-catalyzed hydrolysis hydrolyzed, respectively, indicating that base-catalyzed hydrolysis rates were the greatest under alkaline conditions. Meanwhile, hydrolysis rates increased 2.50-3.60-fold for every 10 °C raise in temperature. Besides, the electrochemical fingerprinting could realize cephalosporin and ß-lactam ring hydrolysis rates close to 100% in-situ hydrolysis process monitoring. This present work provides a powerful technology for understanding the environmental fate and predicting the environmental behavior of antibiotics with fast, high accuracy, specific recognition, and in situ monitoring.

Dual-labeling ratiometric electrochemical strategy initiated with ISDPR for accurate screening MecA gene.

An outstanding dual-labeling ratiometric electrochemical biosensor based on isothermal strand displacement polymerization reaction (ISDPR) for highly sensitive and selective detection of mecA gene has been proposed. Concretely, in the presence of mecA gene, the addition of methylene blue (MB)-labeled primer and polymerase induced recycling amplification to change the structure of the ferrocene (Fc)-labeled hairpin probe, thereby releasing abundant target gene to realize the signal amplification and dual-signal output. Through this process, the electrochemical responses of Fc (IFc) and MB (IMB) were both substantially reduced and increased proportionally, ensuring that the value of IMB/IFc can accurately reflect the true detection level of mecA gene. Benefiting from the "signal-on/off" strategy, the fabricated biosensor exhibited outstanding sequence specificity to discriminate mismatched mecA gene, which verified to be 2.72 times that of single-label detection for perfect match/single base mismatch (PM/MM) discrimination ratio. This strategy effectively integrated the advantages of signal amplification and ratiometric modes, making the biosensor exhibit a broad working range with 10 fM - 3000 pM and a limit of detection (LOD) with 3.33 fM (S/N = 3). Moreover, the proposed biosensor has good feasibility for mecA gene determination in water samples due to acceptable recoveries (95-115%) and repeatability relative standard deviations (RSD) value of 4%. This will provide a powerful sensing platform for improving accuracy and decreasing background signal of sensor for ARGs screening in environmental monitoring.