A Novel Signaling Strategy for an Ultrasensitive Photoelectrochemical Immunoassay Based on Electro-Fenton Degradation of Liposomes on a Photoelectrode.

A signaling strategy can directly determine the analytical performance and application scope of photoelectrochemical (PEC) immunoassays, so it is of great significance to develop an effective signaling strategy. The electro-Fenton reaction has been extensively used to degrade organic pollutants, but it has not been applied to PEC immunoassays. Herein, we report a novel signaling strategy for a PEC immunoassay based on electro-Fenton degradation of liposomes (Lip) on a photoelectrode. Lip vesicles are coated on Au@TiO core-shell photoactive material, which can prevent ascorbic acid (AA) from scavenging photogenerated holes. In the presence of a target, the immunomagnetic bead labels are converted to Fe for electro-Fenton reaction, and hydroxyl radicals generated by the electro-Fenton reaction can degrade the Lip vesicles on the photoelectrode. Because of the degradation of Lip vesicles, photogenerated holes can be scavenged more effectively by AA, leading to an increase in photocurrent. Based on the electro-Fenton-regulated interface electron transfer, the sensitive "signal on" PEC immunoassay of a carcinoembryonic antigen is achieved, which features a dynamic range from 0.05 to 5 × 10 pg mL and a detection limit of 0.01 pg mL. Our work provides a novel and efficient PEC immunoassay platform by introducing the electro-Fenton reaction into PEC analysis.