A differential pulse voltammetry (DPV) method for amantadine (AT) determination is developed. To this end, all the chemical and instrumental variables affecting the determination of amantadine are optimized. These studies have used three types of glassy-carbon electrode, first electrode which has not undergone surface modification or coating, to then modify the working electrode surface with two kinds of suspensions: graphene and graphene-cucurbit[7]uril (CB[7]). From studies of the mechanisms governing the electrochemical response of amantadine, it was concluded that it is an electrochemically system with a diffusive reduction phenomenon. Under optimal conditions and with the appropriate electrode modification, we proceed to study the relation between the peak intensity with the analyte concentration. Thus, we find that when the electrode surface is covered with graphene-CB[7], two linear sections are obtained, the first one in the concentration range of between 0.05 μg·mL ﹣1 and 0.75 μg·mL ﹣1 ; and the second one between 1.00 μg·mL ﹣1 and 6.00 μg·mL ﹣1, with Er (%) = 87 and R.S.D. = 0.94% (n = 10 at 0.5 μg·mL ﹣1 level). The minimum detectable amount was 15 ng·mL ﹣1 while a concentration of 44 ng·mL ﹣1 was calculated as determination limit. The optimized method was applied to the determination of amantadine in biological fluids.
Amantadine is a semisynthetic derivative of petroleum hydrocarbons, is formed by rings after six carbon atoms each, it also has an amino group that is electrochemically active [
This molecule has been used in the fight against influenza A [
But it was in 1964, when Schwab, England, Poskaner and Young, described the first beneficial effects of amantadine against Parkinson's disease [
Despite the many applications that have this molecule, such as influenza A, hepatitis C, Alzheimer and Parkinson, in this article we wanted to focus on its action as influenza agent. To this end, we used biological fluids, namely human urine, as shown in the actual application of the method that is developed here [
In this paper, we have decided to take advantage of graphene properties [
Graphene is a carbon allotrope, forming a hexagonal lattice plane, where the carbon atoms are located at the vertices of the lattice, with the type of covalent generated by superimposing the sp2 hybrids bound carbons.
On a microscopic level, it can be considered that, the graphite is formed by superimposing a high number of graphene sheets.
The other substance used as a modifier in this article was the cucurbit[
CB[
CB[n]s are obtained by the acid-catalyzed condensation of n glycoluril molecules and formaldehyde to generate molecules with n-glycoluril units bridged by methylene groups. The diameter, and therefore cavity volume cavity depends on the number of glycoluril units repeated.
It is hardly demonstrated that CB[n]s are such efficient host molecules in molecular recognition and have a particularly high affinity for charged compounds.
In accordance with mentioned above, in this paper, the electrode of glassy-carbon surface has been modified with, firstly, a suspension of graphene, and secondly, with a suspension of graphene-cucurbit[
Pure standard of amantadine hydrochloride (AT) (>99%) and cucurbit[
The electrochemical measurements were performed using a Eco Chemie System General Purpose Electrochemical System (GPES) Potentiostat workstation. A conventional three electrode cell was used. In all experiments, a large area-coiled platinum wire was employed as a counter electrode, an Ag/AgCl/KCl 3 M as reference electrode and a glassy carbon electrode as the working electrode. For pH adjustment, a pH-meter Methrom C831 was employed.
AT stock solution (1000 μg∙mL−1) was prepared in methanol and stored at 4˚C ± 1˚C. A CB[
The preparation of the suspension of graphene was conducted by weighing 0.003 grams of graphene, using as solvent a mixture of 50% water and dimethylformamide (DMF), reaching a final volume of 1 mL. At Once done, and due to have a suspension as homogeneous as possible, we proceeded to sonicate for 15 - 20 minutes.
To prepare the second suspension, i.e. composed of graphene and CB, we followed the same mechanism as in the case of the suspension of graphene, i.e. graphene 0.03 mg and 0.03 mg of CB[
The application of the method developed in this article was conducted on biological fluids, specifically in human urine.
This sample underwent no treatment of extraction, purification. All what it was done was filtering the sample to remove any particulate matter that may have, as well as to adjust the pH chosen as the optimum for determination.
Once suspensions were prepared with graphene and grapheme-CB[
The electrochemical study of the amantadine was performed by differential pulse voltammetry (DPV) in order to determinate the best conditions for its determination.
In order to select the optimum pH was employed a range of pH between pH 2 and pH 11. The buffers used were phosphate buffer for pH 2, 3, 7 and 11; and acetic buffer for pH 4 and 5. The concentration of all of the buffers was 0.5 M.
In
The same behavior was observed in the study of the pH with a glassy-carbon electrode without its active surface has been coated or modified was repeated when the working electrode surface was coated with (1), and graphene (2) with graphene-cucurbit[
From the standpoint of electrochemistry and the results, pH 2 was chosen for further studies.
When comparing the recorded voltammograms for the three cases discussed in this article, shows that, although the intensity of the signal, when the electrode is modified with graphene, is much higher, also, the residual current greatly increases, reducing the method selectivity (
Analyzing the behavior of the potential peak, with 1) the unmodified electrode, 2) modified with graphene and 3) modified with graphene and CB
[
Once the study of the chemical variables, it was proceeded to the optimization of the instrumental variables by differential pulse voltammetry (DPV) and keeping the pH constant and the concentration of analyte (10 μg∙mL−1).
The instrumental variables study was performed with a commercial electrode Glassy-Carbon 1) unmodified, 2) covering the active surface with a suspension graphene and 3) covering the electrode surface with a suspension of graphene and cucurbit[
The variables studied were the accumulation time, accumulation potential, scan rate and pulse amplitude, all by DPV.
When the influence of accumulation potential in the electrochemical signal was studied, the following results were obtained. In the case of unmodified electrode, the potential of providing the best accumulation signal from the electrochemical standpoint was −200 mV.
For the electrode covered with graphene, the suitable potential accumulation corresponded to a value of ?350 mV, but in this case it was observed that as the potential accumulation moved towards more positive values, a preadsorption wave appeared, which provoked the decreased sensitivity of the electrochemical signal of the molecule under study in this paper. For this reason, the influence of the accumulation potential when the surface of the working electrode is covered with a suspension of graphene and CB[
The criteria that we followed, and maintained in all studies referenced in this article, to choose the optimal value of the variable under study were: 1) stronger signal; 2) lower semi-peak width and 3) lower residual current.
A similar event occurred when we studied the influence of accumulation time, the results were 1) unmodified electrode 90 s accumulation time and 2) 120 s for the electrode covered with graphene, but with increasing accumulation time appeared a preadsorption wave, which lowered the sensitivity of the electrochemical signal.
When the electrode is modified with the suspension composed of graphene-CB[
The procedure followed in this study was the same as in previous studies, i.e. remain constant all variables except the one we are studying at this time, the pulse amplitude.
In addition, we have followed the selection criteria pulse amplitude value discussed above.
According to the discussion in this section, the pulse amplutide values chosen for further study are: 1) for nude electrode surface 50 mV; 2) 100 mV for the graphene electrode and 3) 50 mV when the electrode surface is covered with the graphene-CB[
The pulse amplitude follows a linear trend that fit to the equation, 1) uncover electrode ip(A) = 0.134 DE(V) − 0.2142, 2) electrode covered with grapheme ip(A) = 0.2476 DE(V) − 0.4848 and 3) electrode covered with graphene-CB[
It should be noted that when the electrode surface was covered with graphene and CB[
When we studied the influence of the scanning velocity was observed that in all three cases studied (electrode unmodified, modified and modified graphene and graphene CB[
(1) unmodified electrode: ip(A) = 0.1606v (mV∙s−1)(1/2) + 1.9787
(2) electrode covered with graphene: ip(A) = 0.9538v (mV∙s−1)(1/2) + 7.8026
(3) electrode covered with graphene-CB[
The sweep speed values chosen in accordance with the selection criteria outlined above, were: 1) for the unmodified electrode 8 mV∙s−1, 2) to the electrode 10 mV∙s−1 graphene and 3) for the electrode modified with graphene and CB[
The mole ratio variation method was employed in order to study the stoichiometry of the formed complex between amantadine and cucurbit[
Instrumental variables used in the electrochemical study of complex AT with CB[
After choosing the most suitable measurement conditions for determining the compound under study, it was conducted to study the influence of analyte concentration using the following conditions
(1) Unmiodified electrode: pH = 2; accumulation potential = −200 mV; accumulation time = 90 s; scan rate = 8 mV∙s−1 and pulse amplitude = 50 mV
(2) Electrode modified with graphene: pH = 2; accumulation potential= −350 mV; accumulation time = 120 s; scan rate = 10 mV∙s−1 and pulse amplitude = 100 mV
(3) Electrode coated with graphene-CB[
The analytical performance of the differential pulse voltammetry method developed for amantadine determination was evaluated. From the voltammograms recording for increasing amounts of AT using the optimized parameters described above, it was observed that the peak current increases with the analyte concentration in the range between 0.1 μg∙mL−1 to 0.6 μg∙mL−1 with a good linearity according to ip(A) = 0.668C (μg∙mL−1) + 2.4458; r = 0.998 with an Er (%) = 0.75% and R.S.D. = 1.05% (n = 10 at 0.5 μg∙mL−1 level). The minimum detectable amount was 55 ng∙mL−1 while a concentration of 0.1 μg∙mL−1 was calculated as determination limit.
It was proceeded in the same way when the glassy-carbon electrode surface was coated with graphene and with graphene-cucurbit[
Thus, we find that when the electrode surface is covered with graphene, two linear sections are obtained, the first in the concentration range of between 0.05 μg∙mL−1 and 1 μg∙mL−1 according to ip(A) = 1.2859C (μg∙mL−1) + 3.6206; r = 0.992, and the second between 1 μg∙mL−1 and 10 μg∙mL−1, according to ip(A) = 0.065C (μg∙mL−1) + 4.2371; r = 0.989. The sensitivity of the method was inferred from the LOD (3s) (20 ng∙mL−1) and LOQ (3s) (50 ng∙mL−1) values. On the other hand, the RSD and Er values of 0.96% and 0.84% respectively (n = 10 at 5 ng∙mL−1 level) indicated the accuracy and reproducibility of the proposed method.
A similar event occurs when the surface of the working electrode is modified with the suspension graphene and cucurbit[
Finally, for carrying out the method here proposed on a real sample biological, it was imperative picking out which glassy-carbon electrode modification gave the highest selectivity. So, if we compare the voltammograms shown in the figure, it is sighted that although the signal belonging to the electrode covered with graphene-CB[
Because one of the main applications of amantadine, is to treat influenza, in this article we have tried to develop a fast, simple way to determine the degree of removal that has this drug once the patient has ingested it.
Under the selected conditions and with a glassy-carbon work electrode coated with the graphene-cucur- bit[
To perform this experiment it was used the standard addition method, Therefore, sub-samples of 2.0 mL non- fortified and fortified at different concentration levels (0.5, 1.0, 2.5 and 5.0 μg∙mL−1) were diluted to a final volume of 10.0 mL with supporting electrolyte and the corresponding square wave voltammograms were recorded. The linear relationship between peak current and AT concentration of AT obeyed the following equation
ip = 0.3397C (μg∙mL−1) + 0.6893, with a correlation coefficient of R = 0.9947, when the glassy-carbon electrode surface is coated with graphene-CB[
When the current data obtained are extrapolate into the equation of calibration curve [C1] , the concentration of amantadine obtained was 9.57 μg∙mL−1. Therefore, the degree of extraction of amantadine in human urine is 95.67%.
The second peak, which appears at 600 mV, may be due to many of the compounds present in the urine, because as mentioned before, the sample has not undergone any pretreatment of extraction or derivatization
To corroborate the results obtained electrochemically is employed the method described by A. Sultan, Maha [
The results obtained by ultraviolet-visible spectroscopy, being the wavelength of 520 nm, are fully in of the line with those obtained by the electrochemical study amantadine. That is, the detected concentration of AT in human urine was 9.87 µg∙mL−1.
A sensitive differential pulse voltammetry (DPV) method to analyze amantadine has been developed in this paper. The proposed method can be applied to the determination of the studied molecule, amantadine, in biological fluids excreted by patients who have previously ingested pharmaceutical preparations against influenza, with the inherent advantages of the electrochemical techniques, such as more economical and easy instrumentation with high accuracy and reproducibility as shown from the obtained results
AT (amantadine)
CB[
DMF (dimethylformamide)
AO (ascorbic acid)
DPV (differential pulse voltammetry)
[C1] En el texto solo se dice que dopas con un nivel de concentración de 10 ppm que, en el electrodo modificado con cb queda fuera del intervalo respuesta lineal. Debes dar información de como has hecho la adicion estándar, no se dice volumen de alícuota sin dopar, ni concentraciones¿has hecho una adición estantar simple? Aclarar. En la figura debería aparecer la muestra sin dopar. Si no es solo valor de recuperación lo que estás dando (creo entender que es eso lo que se ha hecho) no determinación por adicion estándar.