Imprinted Polymer – Modified Hanging Mercury Drop Electrode for Differential Pulse Adsorptive Stripping Voltammetric Analysis of a Diquat Herbicide

An imprinted polymer modified hanging mercury drop electrode (HMDE) in Model 303A system in conjunction with a PAR Model 264A Polarographic Analyzer/Stripping Voltammeter has been used for the selective analysis of a diquat herbicide viz., 5,6‐dihydropyrazino[1,2,3,4‐[lmn]‐1,10‐phenanthrolinium dichlorides in differential pulse cathodic stripping voltammetry mode. Complex aqueous samples (drinking water and agricultural soil suspension), spiked with a diquat herbicide, were directly analyzed by the adsorptive accumulation of the analyte over the working electrode (accumulation potential ?0.8 V (vs. Ag/AgCl), accumulation time 120 s, pH 7.0, supporting electrolyte 0.1 M KCl, scan rate 10 mV s^?1, pulse amplitude 25 mV). The limit of detection for diquat herbicide was found to be 0.34 nmol L^?1 (0.1 ppb, RSD 2%, S/N=2).     

2,2‐Bis(3‐Amino‐4‐hydroxyphenyl)hexafluoropropane Modified Glassy Carbon Electrodes as Selective and Sensitive Voltammetric Sensors. Selective Detection of Dopamine and Uric Acid

2,2‐bis(3‐Amino‐4‐hydroxyphenyl)hexafluoropropane (BAHHFP) was electro‐polymerized oxidatively on glassy carbon by cyclic voltammetry. The activity of the modified electrode towards ascorbic acid (AA), uric acid (UA) and dopamine (DA) was characterized with cyclic voltammetry and differential puls voltammetry (DPV). The findings showed that the electrode modification drastically suppresses the response of AA and shifts it towards more negative potentials. Simultaneously an enhancement of reaction reversibility is seen for DA and UA. Unusual, selective preconcentration features are observed for DA when the polymer‐modified electrode is polarized at negative potential. In a ternary mixture containing the three analytes studied, three baseline resolved peaks are observed in DPV mode. At physiological pH 7.4, after 5 min preconcentration at ?300 mV, peaks positions were ?0.073, 0.131 and 0.280 V (vs. Ag/AgCl) for AA, DA and UA, respectively. Relative selectivities DA/AA and UA/AA were over 4000 : 1 and 700 : 1, respectively. DA response was linear in the range 0.05–3 μM with sensitivity of 138 μA μM^?1 cm^?2 and detection limit (3σ) of 5 nM. Sensitive quantification of UA was possible in acidic solution (pH 1.8). Under such conditions a very sharp peak appeared at 630 mV (DPV). The response was linear in the range 0.5–100 μM with sensitivity of 4.67 μA μM^?1 cm^?2 and detection limit (3σ) of 0.1 μM. Practical utility was illustrated by selective determination of UA in human urine.     

Covalently Anchored p‐Aminobenzene Sulfonate Multilayer on a Graphite Pencil Lead Electrode: A Highly Selective Electrochemical Sensor for Dopamine

An electrochemical sensor for dopamine (DA) has been developed based on the electrografting of 4‐aminobenzene sulfonic acid (4‐ABSA) onto the graphite pencil lead electrode (GPLE). The process of covalent anchoring and presence of 4‐ABSA on the GPLE was studied using cyclic voltammetry and electrochemical impedance spectroscopy. Electrochemical behaviour of the sensor towards DA, ascorbic acid (AA), and uric acid (UA) was studied in detail in phosphate buffer of pH 7. After optimizing the various parameters that influence the differential pulse voltammetric (DPV) signal for DA, the sensor exhibited a linear response over the 0.5 – 10 μmol⋅L^‐1concentration range with a limit of detection, 0.095 μmol⋅L^‐1 (at an S/N of 3). The sensor can selectively quantify DA even in the presence of 1 mmol⋅L^‐1 AA. Distinct DPV signals were obtained for DA (at 0.191 mV vs. Ag/AgCl) and for UA (at 0.343 mV vs. Ag/AgCl). The sensor is highly selective, sensitive and stable. It was applied to the quantification of DA in injections and urine. Recovery studies were done by spiking both the real samples with a known quantity of DA.     

Selective Electrochemical Determination of Dopamine with Molecularly Imprinted Poly(Carbazole‐co‐Aniline) Electrode Decorated with Gold Nanoparticles

Dopamine (DA) is a significant neurotransmitter in the central nervous system, coexisting with uric acid (UA) and ascorbic acid (AA). UA and AA are easily oxidizable compounds having potentials close to that of DA for electrochemical analysis, resulting in overlapping voltammetric response. In this work, a novel molecularly imprinted (MI) electrochemical sensor was proposed for selective determination of DA (in the presence of up to 80‐fold excess of UA and AA), relying on gold nanoparticles (Au_nano)‐decorated glassy carbon (GC) electrode coated with poly(carbazole (Cz)‐co‐aniline (ANI)) copolymer film incorporating DA as template (DA imprinted‐GC/P(Cz‐co‐ANI)‐Au_nano electrode, DA‐MIP‐Au_nano electrode). The DA recognizing sensor electrode showed great electroactivity for analyte oxidation in 0.2 mol L^?1 pH 7 phosphate buffer. Square wave voltammetry (SWV) was performed within 10^?4–10^?5 mol L^?1 of DA, of which the oxidation peak potential was observed at 0.16 V. The limit of detection (LOD) and limit of quantification (LOQ) were 2.0×10^?6 and 6.7×10^?6 mol L^?1, respectively. Binary and ternary synthetic mixtures of DA‐UA, DA‐AA and DA‐UA‐AA yielded excellent recoveries for DA. Additionally, DA was quantitatively recovered from a real sample of bovine serum spiked with DA, and determined in concentrated dopamine injection solution. The developed SWV method was statistically validated against a literature potentiodynamic method using a caffeic acid modified‐GC electrode.     

Detection of Uric Acid in the Presence of Dopamine and High Concentration of Ascorbic Acid Using PDDA Modified Graphite Electrode

The properties of graphite electrode (Gr) modified with poly(diallyl dimethyl ammonium chloride) (PDDA) for the detection of uric acid (UA) in the presence of dopamine (DA) and high concentration of ascorbic acid (AA) have been investigated by cyclic voltammetry, differential pulse voltammetry and chronoamperometry. The polymer modified graphite electrode was prepared by a very simple method just by immersing the graphite electrode in PDDA solution for 20 minutes. The PDDA/Gr modified electrode displayed excellent electrocatalytic activity towards the oxidation of UA, DA and AA compared to that at the bare graphite electrode. The electrochemical oxidation signals of UA, DA and AA are well resolved into three distinct peaks with peak potential separations of 220 mV, 168 mV and 387 mV between AA‐DA, DA‐UA and AA‐UA respectively in cyclic voltammetry studies and the corresponding peak potential separations are 230 mV, 130 mV and 354 mV respectively in differential pulse voltammetry. The lowest detection limits obtained for UA, DA and AA were 1×10^?7 M, 2×10^?7 M and 800×10^?9 M respectively. The PDDA/Gr electrode efficiently eliminated the interference of DA and a high concentration of AA in the determination of UA with good selectivity, sensitivity and reproducibility. The modified electrode was also successfully applied for simultaneous determination of UA, DA and AA in their ternary mixture.     

Simultaneous Determination of Nickel and Cadmium by Adsorptive Stripping Voltammetry

A sensitive and fast method for the simultaneous determination of trace amounts of nickel and cadmium in real samples has been described using differential pulse adsorptive stripping voltammetry (DPASV) by adsorptive accumulation of the N,N′‐bis(salicylaldehydo)4‐carboxyphenylenediamine (BSCPDA)–complex on the hanging mercury drop electrode (HMDE). As supporting electrolyte 0.02 mol L^?1 ammonia buffers containing ligand has been used. Optimal analytical conditions were found to be: BSCPDA concentration of 42 μM, pH 9.6 and adsorption potential at ?50 mV versus Ag/AgCl. With an accumulation time of 20 s, the peaks current are proportional to the concentration of nickel and cadmium over the 1–180, and 0.5–200 ng mL^?1 with detection limits of 0.06 and 0.03 ng mL^?1 respectively. The sensitivity of method for determination of nickel and cadmium were obtained 0.54 and 0.98 nA mL ng^?1, respectively. The procedure was applied to simultaneous determination of nickel and cadmium in some real and synthetic artificial samples with satisfactory results.     

Adsorptive Stripping Differential Pulse Voltammetry for Determination of Trace Amounts of Noscapine in Human Plasma

A new adsorptive anodic differential pulse stripping voltammetry method for the direct determination of noscapine at trace levels in human plasma of addicts is proposed. The procedure involves an adsorptive accumulation of noscapine on a hanging mercury drop electrode (HMDE), followed by oxidation of adsorbed noscapine by voltammetry scan using differential pulse modulation. The optimum conditions for the analysis of noscapine are pH = 8.5 using Britton‐Robinson (B‐R) buffer, accumulation potential of ?100 mV (vs. Ag/AgCl), and accumulation time of 150 s. The peak current is proportional to the concentration of noscapine, and a linear calibration graph is obtained at 0.015–2.75 μg mL^?1. A relative standard deviation of 1.28% (n = 5) was obtained, and the limit of detection was 7 ng mL^?1. The capability of the method for the analysis of real samples was evaluated by determination of noscapine in spiked human plasma and addicts, human plasma with satisfactory results.     

A Selective Voltammetric Method for Uric Acid Detection at a Glassy Carbon Electrode Modified with Electrodeposited Film Containing DNA and Pt‐Fe(III) Nanocomposites

A novel biosensor by electrochemical codeposited Pt‐Fe(III) nanocomposites and DNA film was constructed and applied to the detection of uric acid (UA) in the presence of high concentration of ascorbic acid (AA). Based on its strong catalytic activity toward the oxidation of UA and AA, the modified electrode resolved the overlapping voltammetric response of UA and AA into two well‐defined peaks with a large anodic peak difference (ΔE_pa) of about 380mV. The catalytic peak current obtained from differential pulse voltammetry (DPV) was linearly dependent on the UA concentration from 3.8×10^?6 to 1.6×10^?4 M (r=0.9967) with coexistence of 5.0×10^?4 M AA. The detection limit was 1.8×10^?6 M (S/N=3) and the presence of 20 times higher concentration of AA did not interfere with the determination. The modified electrode shows good sensitivity, selectivity and stability.     

Silver Doped Poly(L‐valine) Modified Glassy Carbon Electrode for the Simultaneous Determination of Uric Acid,Ascorbic Acid and Dopamine

In this paper, a silver doped poly(L ‐valine) (Ag‐PLV) modified glassy carbon electrode (GCE) was fabricated through electrochemical immobilization and was used to electrochemically detect uric acid (UA), dopamine (DA) and ascorbic acid (AA) by linear sweep voltammetry. In pH 4.0 PBS, at a scan rate of 100 mV/s, the modified electrode gave three separated oxidation peaks at 591 mV, 399 mV and 161 mV for UA, DA and AA, respectively. The peak potential differences were 238 mV and 192 mV. The electrochemical behaviors of them at the modified electrode were explored in detail with cyclic voltammetry. Under the optimum conditions, the linear ranges were 3.0×10^?7 to 1.0×10^?5 M for UA, 5.0×10^?7 to 1.0×10^?5 M for DA and 1.0×10^?5 to 1.0×10^?3 M for AA, respectively. The method was successfully applied for simultaneous determination of UA, DA and AA in human urine samples.     

Simultaneous Detection of Dopamine and Uric Acid under Coexistence of Ascorbic Acid with DNA/Pt Nanocluster Modified Electrode

A novel biosensor by electrochemically codeposited Pt nanoclusters and DNA film was constructed and applied to detection of dopamine (DA) and uric acid (UA) in the presence of high concentration ascorbic acid (AA). Scanning electron microscopy and X‐ray photoelectron spectroscopy were used for characterization. This electrode was successfully used to resolve the overlapping voltammetric response of DA, UA and AA into three well‐defined peaks with a large anodic peak difference (ΔE_pa) of about 184 mV for DA and 324 mV for UA. The catalytic peak current obtained from differential pulse voltammetry was linearly dependent on the DA concentration from 1.1× 10^?7 to 3.8×10^?5 mol·L^?1 with a detection limit of 3.6×10^?8 mol·L^?1 (S/N=3) and on the UA concentration from 3.0×10^?7 to 5.7×10^?5 mol·L^?1 with a detection limit of 1.0×10^?7 mol·L^?1 with coexistence of 1.0×10^?3 mol·L^?1 AA. The modified electrode shows good sensitivity and selectivity.     

Simultaneous Voltammetric Determination of Uric Acid and Ascorbic Acid Using a Carbon‐Paste Electrode Modified with Multi‐Walled Carbon Nanotubes/Nafion and Cobalt(II)nitrosalophen

A composition of multiwalled carbon nanotube (MWCNT), Nafion and cobalt(II)‐5‐nitrosalophen (CoNSal) is applied for the modification of carbon‐paste electrode (CPE). The pretreated MWCNT is well dispersed in the alcoholic solution of Nafion under the ultrasonic agitation, and the resulted suspension is used as modifier (with 10% w/w) in the matrix of the paste electrode. The prepared electrode further modified by addition of 3 wt% of CoNSal. The resulted modified electrode is used as a sensitive voltammetric sensor for simultaneous determination of uric acid (UA) and ascorbic acid (AA). The electrode showed efficient electrocatalytic activity in lowering the anodic overpotentials and enhancement of the anodic currents. This electrode is able to completely resolve the voltammetric response of UA and AA. The effects of potential sweep rate and pH of the buffer solution on the response of the electrode, toward UA and AA, and the peak resolution is thoroughly investigated by cyclic and differential pulse voltammetry (CV and DPV). The best peak resolution for these compounds using the modified electrode is obtained in solutions with pH 4. The ΔE_p for UA and AA in these methods is about 315 mV, which is considerably better than previous reports for these compounds. A linear dynamic range of 1×10^?7 to 1×10^?4 M with a detection limit of 6×10^?8 M is resulted for UA in buffered solutions with pH 4.0. The voltammetric response characteristics for AA are obtained as, the linear range of 5×10^?7 to 1×10^?4 M with the detection limit of 1×10^?7 M. The voltammetric detection system was very stable and the reproducibility of the electrode response, based on the six measurements during one month, was less than 3.5% for the slope of the calibration curves of UA and AA. The prepared modified electrode is successfully applied for the determination of AA and UA in mixture samples and reasonable accuracies are resulted.     

Electrooxidation and Amperometric Detection of Ascorbic Acid at GC Electrode Modified by Electropolymerization of N,N‐Dimethylaniline

The polymer film of N,N‐dimethylaniline (DMA) is deposited on the electrochemically pretreated glassy carbon (GC) electrode by continuous electrooxidation of the monomer. This poly N,N‐dimethylaniline (PDMA) film‐coated electrode can be used as an amperometric sensor of ascorbic acid (AA). The polymer film (thickness (?): 0.3±0.02 μm) having positive charge in its backbone attracts the anionic species AA. Thus, the anodic peak potential (350 mV vs. Ag|AgCl|NaCl_(sat)) for the oxidation of AA at the bare electrode is largely shifted to the negative value (150 mV) at this electrode. The PDMA film‐coated electrode is stable in acidic, alkaline and neutral media and can sense AA at different pH's. The diffusion coefficients of AA in solution (D) and in film (D_s) were estimated by rotating disk electrode voltammetry: D=(5.5±0.1)×10^?6 cm² s^?1 and D_s=(6.3±0.2)×10^?8, (6.0±0.2)×10^?8 and (4.7±0.2)×10^?8 cm² s^?1 for 0.5, 1.5 and 3.0 mM AA, respectively. A permeability of AA through the PDMA film was found to decrease with increasing the concentration of AA in the solution. In the chronoamperometry, the current response for the oxidation of AA at different times elapsed after potential‐step application is linearly increased with the increase in AA concentration in a wide range of its concentration from 25 μM to 1.65 mM. In the hydrodynamic amperometry, a successive addition of 10 μM AA caused the successive increase in current response with equal amplitude and the sensitivity was calculated as 0.178 μA cm^?2 μM^?1. So, the fouling of the electrode surface caused by the oxidized product of AA is markedly eliminated at this PDMA film‐coated electrode. A flow injection analysis based on the present electrode was performed to estimate the concentration of vitamin C in fruit juice.     

Development of a Creatinine Sensor Based on a Molecularly Imprinted Polymer‐Modified Sol‐Gel Film on Graphite Electrode

An electrochemical creatinine sensor based on a molecularly imprinted polymer (MIP)‐modified sol‐gel film on graphite electrode was developed. The surface coating of MIP over sol‐gel was advantageous to obtain a porous film with outwardly exposed MIP cavities for unhindered selective rebinding of creatinine from aqueous and biological samples. A fast differential pulse, cathodic stripping voltammetric response of creatinine can be obtained after being preanodized the sensor in neutral medium containing appropriate amount of creatinine at +1.8 V versus SCE for 120 s. A linear response over creatinine concentration in the range of 1.23 to 100 μg mL^?1 was exhibited with a detection limit of 0.37 μg mL^?1 (S/N=3).     

Quantification of Sub‐Nanomolar Levels of Aluminum by Adsorptive Stripping Voltammetry Using Rubeanic Acid as a Selective Chelating Agent

A novel, sensitive and selective adsorptive stripping procedure for determination of aluminum is presented. The method is based on the adsorptive accumulation of dithiooxamide (Rubeanic acid) complex of aluminum onto a hanging mercury drop electrode, followed by reduction of adsorbed species by voltammetric scan using differential pulse modulation. The influences of control variables on the sensitivity of the proposed method for the determination of aluminum were studied. The optimum analytical conditions were found to be Rubeanic acid (RA) concentration of 8.0×10^?5 M, ammonia buffer (NH₃? NH₄Cl) pH of 6.5, and accumulation potential at ?50 mV vs. Ag/AgCl with an accumulation time of 60 s. The peak currents are proportional to the concentration of aluminum over the 0.3–70 ng mL^?1 ranges with detection limit of 0.012 ng mL^?1. The procedure was applied to the determination of aluminum in the Lab. Water, HCl of Merck and potato samples with satisfactory results.     

Simultaneous Voltammetric Determination of Lead and Tin by Adsorptive Differential Pulse Stripping Method and Orthogonal Signal Correction‐Partial Least Squares in Water Samples

An adsorptive differential pulse stripping method for the simultaneous determination of lead and tin is proposed. The procedure involves an adsorptive accumulation of lead and tin on a hanging mercury drop electrode (HMDE), followed by oxidation of adsorbed lead and tin by voltammetric scan using differential pulse modulation. The optimum experimental conditions are: 0.2 mol L^?1 HNO₃, accumulation potential of ?900 mV versus Ag/AgCl, accumulation time of 200 s, scan rate of 20 mV s^?1 and pulse height of 80 mV. Lead and tin peak currents were observed in the same potential region at about ?400 mV. The simultaneous determination of lead and tin by using voltammetry is a difficult problem in analytical chemistry, due to voltammogram interferences. The resolution of a mixture of lead and tin by the application of orthogonal signal correction‐partial least squares (OSC‐PLS) was performed. The linear dynamic ranges were 0.003‐0.35 and 0.008‐0.50 μg mL^?1 and detection limits were land 3 ng mL^?1 for lead and tin, respectively. The RMSEP for lead and tin with OSC and without OSC were 2.8737, 6.0557 and 8.0941, 9.5151, respectively. The capability of the method for the analysis of real samples was evaluated by the determination of lead and tin in water samples with satisfactory results.     

Creatinine sensor based on a molecularly imprinted polymer-modified hanging mercury drop electrode

Molecularly imprinted polymers (MIP) have been elucidated to work as artificial receptors. In our present study, a MIP was applied as a molecular recognition element to a chemical sensor. We have constructed a creatinine sensor based on a MIP layer selective for creatinine and its differential pulse, cathodic stripping voltammetric detection (DPCSV) on a hanging mercury drop electrode (HMDE). The creatinine sensor was fabricated by the drop coating of dimethylformamide (DMF) solution of a creatinine-imprinted polymer onto the surface of HMDE. The modified-HMDE, preanodised in neutral medium at +0.4 V versus Ag/AgCl for 120 s, exhibited a marked enhancement in DPCSV current in comparison to the less anodised (≤+0.3 V) HMDE. The creatinine was preconcentrated and instantaneously oxidised in MIP layer giving DPCSV response in the concentration range of 0.0025-84.0 μg mL⁻¹ [detection limit (3σ) 1.49 ng mL⁻¹]. The sensor was found to be highly selective for creatinine without any response of interferents viz., NaCl, urea, creatine, glucose, phenylalanine, tyrosine, histidine and cytosine. The non-imprinted polymer-modified electrode did not show linear response to creatinine. The imprinting factor as high as 9.4 implies that the imprinted polymer exclusively acts as a recognition element of creatinine sensor. The proposed procedure can be used to determine creatinine in human blood serum without any preliminary treatment of the sample in an accurate, rapid and simple way.     

N‐(3,4‐Dihydroxyphenethyl)‐3,5‐dinitrobenzamide‐Modified Multiwall Carbon Nanotubes Paste Electrode as a Novel Sensor for Simultaneous Determination of Penicillamine,Uric acid,and Tryptophan

N‐(3,4‐dihydroxyphenethyl)‐3,5‐dinitrobenzamide modified multiwall carbon nanotubes paste electrode was used as a voltammetric sensor for oxidation of penicillamine (PA), uric acid (UA) and tryptophan (TP). In a mixture of PA, UA and TP, those voltammograms were well separated from each other with potential differences of 300, 610, and 310 mV, respectively. The peak currents were linearly dependent on PA, UA and TP concentrations in the range of 0.05–300, 5–420, and 1.0–400 µmol L^?1, with detection limits of 0.021, 2.0, and 0.82 µmol L^?1, respectively. The modified electrode was used for the determination of those compounds in real samples.     

Trace determination of molybdenum by adsorptive cathodic stripping voltammetry

Molybdenum is determined by adsorptive cathodic stripping voltammetry in 0.15 M nitric acid solution containing 15 μM 2′,3,4′,5,7-pentahydroxyflavone (morin) as a ligand. In this medium, molybdenum is preconcentrated on a hanging mercury drop electrode and stripped cathodically in square-wave voltammetry mode, with a peak potential of -350 mV vs. Ag/AgCl (saturated KCl). The effect of various parameters (ligand concentration, supporting electrolyte composition, accumulation potential and collection time) on the sensitivity and linear range of the calibration curve are discussed. With controlled accumulation for 1 min, the detection limit (3σ) was 0.45 ng ml^?1 molybdenum and the calibration curve is linear up to 70 ng ml^?1. The procedure is applied to the determination of molybdenum in real samples with satisfactory results.     

Cathodic stripping voltammetry of 2-mercaptoethanol

The behaviour of 2-mercaptoethanol at a hanging mercury drop electrode by cathodic stripping voltammetry (c.s.v.) is studied. The stripping curves are recorded by three scanning modes: rapid-scan direct-current, differential-pulse and fundamental harmonic alternating-current polarography. Under the recommended conditions, pre-electrolysis is done at a potential of 0.0 V vs. Ag/AgCl for 3 min in a medium of pH 6.7 or 8 (Britton-Robinson buffer). Then after 1 min, stripping is done at a scan rate of 6.6 mV s^?1 preferably in the differential-pulse mode. The stripping peak at about ?0.4 V is used to determine 2-mercaptoethanol within the concentration range 3 × 10^?8/2-8 × 10^?7 mol l^?1. Calibration functions are reported; the standard additions method is preferred near the limit of detection. The interferences of several organic compounds are described.     

Determination of Ethylenethiourea (ETU) at Trace Levels in Water Samples by Cathodic Stripping Voltammetry

A stripping voltammetric method for the determination of ethylenethiourea in water samples is described based on its adsorptive deposition at the hanging mercury drop electrode (HMDE). In a borate buffer (pH 9.0) as supporting electrolyte, ETU is deposited at +100 mV (vs. Ag/AgCl) and stripped during the cathodic scan. The linear range for the measurements was from 2.0 to 100 μg L^?1, with a detection limit calculated as 1.4 μg L^?1 after a deposition time of 300 s and a RSD of 1.9% (n=5) for 50 μg L^?1 of ETU measured. The interferences of some organic compounds and metallic ions were tested. Recoveries between 93 and 110% were obtained using the standard addition method for spiked samples of natural and drinking waters. The method is rapid and applicable in the monitoring of ETU residues in water samples.