Abstract

A novel, simple, and more sensitive spectrophotometric procedure has been developed for the determination of brilliant blue FCF in water and food samples by an aqueous two-phase system (ATPS). In this method, adequate amount of polyethylene glycol/ sodium carbonate (PEG-4000/) was added to aqueous solution for formation of a homogeneous solution. To the mixture solution, suitable amount of was added, the mixture solution was shaken until the salt was dissolved, and then it was separated into two clear phases easily and rapidly. The target analyte in the water sample was extracted into the polyethylene glycol phase. After extraction, measuring the absorbance at 634 nm was done. The effects of different parameters such as polyethylene glycol (type and concentration), pH, salt (type and amount), centrifuge time, and temperature on the ATPS of dye was investigated and optimum conditions were established. Linear calibration curves were obtained in the range of 0.25–750 ng/mL for brilliant blue FCF under optimum conditions. Detection limit based on three times the standard deviation of the blank () was 0.12 ng/mL. The relative standard deviation (RSD) for 400 ng/mL was 3.14%. The method was successfully applied to the determination of brilliant blue FCF in spiked samples with satisfactory results. The relative recovery was between 96.0 and 102.2%.

1. Introduction

The goal of this work was to determine the optimal conditions for separating brilliant blue FCF by liquid-liquid extraction with PEG/salt aqueous tow-phases system.

Food dyes including Tartrazine, Quinoline Yellow, Sunset Yellow, Carmoisine, and Brilliant Blue FCF have been widely used to optimize food color, appearance, flavor, taste, and texture of many industrial food products [1, 2]. Food dyes classified into natural and synthetic [3]. These additives attribute a wide range of colors such as yellow, orange, red, green, blue, purple, and brown [4]. Many of them are having enormous application in the food, pharmaceutical, tanning, paper, rubber, plastics, cosmetics, cosmetic, textile and leather industries [57]. However, the excess use of these substances may cause significant problems for human healthy such as cancer and others diseases [8, 9]. Therefore, it is necessary to have efficient methodologies to control the amount of colorants in foods.

There are a lot of analytical procedures to carry out the determination of dyes in foods, such as chromatographic methods [10], high-performance liquid chromatography [11], differential pulse polarography [12], photoacoustic spectroscopy [13], and voltametric [14]. However, most of these methods are time consuming, needing a great deal of hazardous organic solvents and high cost instrumentation.

The procedures described here provide a more sensitive, fast, and simple spectrophotometry method for determination of Brilliant Blue in different food samples using an aqueous two-phase system (ATPs). Aqueous two-phase extraction has been widely used for recovery and purification of many compounds such as protein, DNA, and some cations from different matrices [1517]. ATPS is usually composed of two or more polymer-polymer ATPS or a polymer-salt system. This selection is often ruled by economic considerations [18]. Polyethylene glycol (PEG)-potassium phosphate, and PEG and magnesium sulfate are among the most frequently used polymer-salt systems [19]. ATPSs have advantages over the conventional extraction systems using organic solvents (e.g., short processing time, low energy consumption, relative reliability in scaleup, and a biocompatible environment [20].

2. Experimental

2.1. Reagents and Instruments

PEG with molecular weight of 4000, sodium sulfate, sodium carbonate, potassium phosphate and ammonium sulfate were obtained from Merck (Darmstadt, Germany). Other reagents were of analytical grade and were purchased from Merck (Darmstadt, Germany). A stock standard solution of brilliant blue FCF(For Coloring Food) purchased from Merck (Germany) at a concentration of 0.04 mg/L was prepared. The working solutions of brilliant blue FCF were prepared by appropriate dilutions of the stock solution immediately prior to their use. All aqueous solutions were prepared with double-distilled water.

The spectrophotometer UV-Vis (model 6705, Jenway, England) was used for all the absorbance measurements with a 10 mm quartz cell. pH measurements were made with a 827 pH meter (Metrohm, Switzerland) and equipped with a combined glass electrode. The centurion scientific centrifuge (K280R, UK) was used for centrifuging.

2.2. Experimental Method

At the beginning of the experiments, a 2 mL portion of the standard solution containing the brilliant blue FCF at concentration level of 40 ng/mL was placed into a 20 mL glass tube and adjusted pH to 5.5 with 9 mL of acetic acid/acetate buffer solution with the concentration of 0.05 mol/L. Then, 4 g (20% w/w) of PEG 4000 and 2.5 g (12.5% w/w) of sodium carbonate were added to it and diluted to the mark with doubled-distilled water. The mixture was shaken for 3 min at 35°C in bath water for formation of a homogeneous solution. After the mixture was centrifuged at 3500 rpm for 10 min. The upper phase was completely transferred to a quartz cell using a syringe. Finally, the absorbance of brilliant blue FCF extracted into the upper PEG-rich phase was measured at 634 nm versus reagent blank.

2.3. Sample Pretreatment Procedure

Appropriate amounts of strawberry jelly (Tehran, Iran), fruity candy (ben ben, Iran), smarties (morvarid, Iran), and smarties (mino Co, Iran) samples were dissolved in water, filtered if necessary, and diluted to 25 mL in a volumetric flask. An aliquot of the above solutions was treated under the general procedure for ATPS and subsequent determination of brilliant blue FCF.

3. Results and Discussion

In order to obtain high extraction efficiency, the effect of different parameters on extraction conditions such as salt (type and amount), polyethylene glycol (type and concentration), temperature, and pH of sample solution were evaluated and optimized. The optimization process was carried out using one variable at a time method for simplifying the optimization procedure.

3.1. Effect of pH and Volume of Buffer

The pH is evaluated as a critical parameter for regulating the partitioning of the analyte in the PEG-rich phase which seems to control the extraction efficiency. Therefore, the effect of pH on ATPA of brilliant blue FCF from water samples was investigated. The absorbance of brilliant blue FCF was measured at 634 nm, respectively, after performing ATPS in the pH range of 2.4–11.3. The pH of the solution was adjusted to the desired value by the addition of hydrochloric acid and sodium hydroxide and using a pH meter. As the results shown in Figure 1, the signal increased with the increase in pH from 2.4 to 5.5, and then declined with pH higher than 5.5. Therefore, pH 5.5 was selected for further study. The effect of volume of the buffer on the extraction process was examined in the range of 1–12 mL. The result of Figure 2 verified that an optimum volume of buffer with pH 5.5 has been obtained 9 mL.

3.2. Effect of Type and Amount of PEG

We concluded the brilliant blue FCF partitioning behavior was very sensitive to changes in the PEG molecular mass. We had observed that brilliant blue FCF showed a decrease in their partition coefficient value as the PEG molecular weight increased due to an increase in the polymer hydrophobic character which agrees with a general rule observed for most ATPSs [21]. Figure 3 has shown the effect of PEG with different molecular weight of 4000, 6000, 8000, and 10000. The result demonstrated that PEG-4000 higher absorption signal obtained.

The effect of the amount of PEG-4000 on the absorption was studied using various amount of the reagent ranging from 3 g to 6 g, and the results were shown in Figure 4. It was found that by increasing the amount of PEG-4000, the analytical signal increased, reaching a maximum value at 4 g, and then decreased. According to this result, all further experiments were carried out at the amount of 4 g of PEG 4000 (20% w/w).

3.3. Effect of Type of Salt and Amount of Salt

The influence of the ionic strength was also investigated in many techniques of liquid-liquid extraction. The electrolytes play an important role on the ATPS of nonionic surfactant systems. When small amounts of inorganic salts are added to the system, a decrease in the ATPS of PEG phase is noted. This fact indicates that it is necessary to consider the secondary effect of the electrolytes, that is, salting-out. For investigating the influence of ionic strength on performance of ATPS, various experiments were performed by adding different salt such as sodium sulfate, sodium carbonate, potassium phosphate, and ammonium sulfate. The results demonstrated that sodium carbonate provided the higher signal absorption than other salts. Hence, sodium carbonate was chosen as the most appropriate salt for subsequent experiments (see Figure 5). Effect of amount of sodium carbonate on the extraction of brilliant blue FCF was investigated in the range of 1–3 g. The differences observed in the signals at various amount of sodium carbonate are shown in Figure 6. According to this result, all further experiments were carried out at the optimum amount of 2.5 g (12.5% w/w) of sodium carbonate.

3.4. Effect of Temperature

Temperature affects the mass transfer process and the extraction efficiency. To determine the influence of the extraction temperature, 20 mL aqueous solution containing 4 ng/mL of brilliant blue FCF was extracted at different temperatures ranging from 30°C to 50°C. The absorption scales are almost decreased Figure 7 shows the absorbance of brilliant blue FCF as a function of temperature. Accordingly with these results, the temperature that gave the best results for the majority of the target analyte was 35°C.

3.5. Centrifuging Time

Centrifugation controls the phase separation and is a crucial step in aqueous two phase system method, and the final performance would benefit from a full phase separation. After centrifugation, the volume of PEG-4000 was very small when the centrifuging time was too short, and longer centrifuging time resulted in heat generation, leading to the dissolving of parts of the PEG-4000 phase and to the loss of sensitivity. As can be seen from Figure 8, 10 min was the optimal centrifuging time. the centrifuging time was increase partition coefficient, purification factor, efficiency and signal.

3.6. Effect of Coexisting Ions

Interferences were studied in the presence of a constant concentration of brilliant blue FCF (4 ng/mL) and different amounts of foreign cations and anions under the recommended conditions. The tolerance limits of a foreign species are shown in Table 1. The tolerance level was defined as the maximum concentration of the foreign ion causing a change in the analytical signal no higher than 5%, when compared with the signal of 4 ng/mL brilliant blue FCF alone. As it is observed most of the ions tested do not have significant effect on the determination of brilliant blue FCF.

3.7. Analytical Figures of Merit

Important parameters such as the linear range, calibration graph, precision, detection limit, and recoveries were determined to evaluate the method performance. Under the above-optimized conditions, the calibration graph was linear in the range of 0.25–750 ng/mL with a correlation coefficient () of 0.9995 () of brilliant blue FCF. The relative standard deviation (RSD) for eight replicates of 400 ng/mL brilliant blue FCF was 3.14%.

The lower limit of detection for brilliant blue FCF is defined as the concentration of analyte which gives a signal above the mean blank signal (where is the standard deviation of the blank signal). The LLOD for brilliant blue FCF was found to be 0.12 ng/mL.

3.8. Application of Real Samples

To validate the proposed method, brilliant blue FCF contents in water and food samples were analyzed. Table 2 summarizes the average recovery of brilliant blue FCF in the fortified samples. Water and food samples were spiked with 10 and 40 ng/mL of standard solution of brilliant blue FCF. As can be seen in Table 2, recoveries were more than 96.0%. The result indicated that the proposed method was applicable for quantitative determination of brilliant blue FCF in real samples.

Characteristics of the proposed method have been also compared with other methods which were used for the determination of brilliant blue FCF. Table 3 compares the lower limit of detection (LLOD), relative standard deviation (RSD), linear range (LR), recovery and correlation coefficient of this work with cloud point extraction [3], microemulsion-modified-zeolit [8], flow injection method [8], light-emitting diode [12], and reversed-phase high-performance liquid chromatography (RP-HPLC) [16]. As can be seen, the proposed method provides similar quantification extraction efficiency, with advantages such as good linearity and correlation coefficient than many of the mentioned techniques. Detection limit of ATPS is lower than other mentioned method.

4. Conclusion

The development of techniques and methods for the separation and purification of brilliant blue FCF has been an important prerequisite for many of the advancements made in the industrial food products. In our work, liquid-liquid partitioning with PEG/Na2CO3 aqueous tow-phase system was used to selectively extract brilliant blue FCF.

In this study, a fast, simple, sensitive, and selective method named aqueous two-phase system was proposed for determination of brilliant blue FCF in water and food samples in the range of 0.25–750 ng/mL. The developed ATPS was successfully applied to real system such as water and food samples analysis, indicating that the proposed method was suitable for the extraction and determination of effective component in water and food samples.

Acknowledgment

This work has been supported by the Research Council of Payam Noor University of Ilam.