RESUMO
This study introduces an innovative electrochemical sensor designed to detect glutamate using a nonenzymatic approach. The sensor utilizes a porous network metal-organic framework (Ni-MOF)-NiO-Ni-Carbon nanocomposite (PNM-NiO-Ni-Carbon) as an electrode modifier, which was synthesized and assessed for its effectiveness. Cyclic voltammetry measurements demonstrated that the PNM-NiO-Ni-Carbon nanocomposite, synthesized at 450 °C, displayed remarkable electrocatalytic activity for glutamate oxidation. The linear range for detection spanned from 5 to 960 µmol/L, and the sensor achieved a low detection limit of 320 nmol/L (S/N = 3), which was comparable to previously reported data. Moreover, the sensor exhibited high accuracy and favorable recovery rates when tested with real samples, thus, demonstrating its potential for rapid glutamate detection. The real samples were analyzed using both electrochemical and high-performance liquid chromatography methods, and the results obtained from the two methods did not differ significantly, validating the sensor's excellent practical performance. Based on our findings, the PNM-NiO-Ni-Carbon system exhibits potential for a wide range of biomedical applications.
RESUMO
The release of the cargo from soft vesicles, an essential process for chemical delivery, is mediated by multiple factors. Among them, the regulation by the interaction between the chemical cargo species and the vesicular membrane, widely existing in all vesicles, has not been investigated to date. Yet, these interactions hold the potential to complicate the release process. We used liposomes loaded with different monoamines, dopamine (DA) and serotonin (5-HT), to simulate vesicular release and to monitor the dynamics of chemical release from isolated vesicles during vesicle impact electrochemical cytometry (VIEC). The release of DA from liposomes presents a longer release time compared to 5-HT. Modelling the release time showed that DA filled vesicles had a higher percentage of events where the time for the peak fall was better fit to a double exponential (DblExp) decay function, suggesting multiple kinetic steps in the release. By fitting to a desorption-release model, where the transmitters adsorbed to the vesicle membrane, the dissociation rates of DA and 5-HT from the liposome membrane were estimated. DA has a lower desorption rate constant, which leads to slower DA release than that observed for 5-HT, whereas there is little difference in pore size. The alteration of vesicular release dynamics due to the interaction between the chemical cargo and vesicle membrane lipids provides an important mechanism to regulate vesicular release in chemical and physiological processes. It is highly possible that this introduces a fundamental chemical regulation difference between transmitters during exocytosis.
RESUMO
An innovative label-free electrochemical aptasensing platform has been designed for detection of insulin using functionalized mesoporous silica thin-film (MSTF) coated on a glassy carbon electrode through the one-step electrochemically assisted self-assembly (EASA) method. This strategy is contingent upon the covalent attachment of a complementary DNA (cDNA) oligonucleotide sequence on the mesoporous silica surface, for which further hybridization with its labeled aptamer as a gating molecule restricts the diffusion of the electroactive probe (Fe(CN)63-/4-) toward the electrode surface by the closing of mesochannels. Upon insulin introduction as the stimulus target molecule, hybridization between aptamer and cDNA is efficiently destroyed, which triggers the opening of nanochannels to facilitate redox probe diffusion toward the electrode with a noticeable increase in differential pulse voltammetry signal. The proposed aptasensor showed a wide detection ranging from 10.0 to 350.0 nM and a suitable detection limit of 3.0 nM. This method offers the sensitive and rapid detection of insulin without the need for cargo (dye/fluorophore) as an electrochemical marker inside the pore, at low cost and with a fast modification time.
