Chili and Sweet Pepper Seed Oil Used as a Natural Antioxidant to Improve the Thermo-Oxidative Stability of Sunflower Oil

Cocan, Ileana; Negrea, Monica; Cozma, Antoanela; Alexa, Ersilia; Poiana, Mariana-Atena; Raba, Diana; Danciu, Corina; Popescu, Iuliana; Cadariu, Andreea I.; Obistioiu, Diana; Radulov, Isidora

doi:10.3390/agronomy11122579

Open AccessArticle

Chili and Sweet Pepper Seed Oil Used as a Natural Antioxidant to Improve the Thermo-Oxidative Stability of Sunflower Oil

by

Ileana Cocan

^1,†

,

Monica Negrea

^1,*

,

Antoanela Cozma

^2,*,

Ersilia Alexa

^1,†

,

Mariana-Atena Poiana

¹

,

Diana Raba

³,

Corina Danciu

⁴,

Iuliana Popescu

²,

Andreea I. Cadariu

¹,

Diana Obistioiu

⁵

and

Isidora Radulov

²

¹

Faculty of Food Engineering, Banat’s University of Agricultural Sciences and Veterinary Medicine “King Michael I of Romania” from Timisoara, Calea Aradului No. 119, 300645 Timisoara, Romania

²

Faculty of Agriculture, Banat‘s University of Agricultural Sciences and Veterinary Medicine “King Michael I of Romania” from Timisoara, Calea Aradului No. 119, 300645 Timisoara, Romania

³

Faculty of Management and Rural Tourism, Banat’s University of Agricultural Sciences and Veterinary Medicine “King Michael I of Romania” from Timisoara, Calea Aradului No. 119, 300645 Timisoara, Romania

⁴

Faculty of Pharmacy, University of Medicine and Pharmacy “Victor Babes” Timisoara, Eftimie Murgu Square No. 2, 300041 Timisoara, Romania

⁵

Faculty of Veterinary Medicine, Banat’s University of Agricultural Sciences and Veterinary Medicine “King Michael I of Romania” from Timisoara, Calea Aradului No. 119, 300645 Timisoara, Romania

^*

Authors to whom correspondence should be addressed.

^†

The two authors contributed equally to the work.

Agronomy 2021, 11(12), 2579; https://doi.org/10.3390/agronomy11122579

Submission received: 30 November 2021 / Revised: 16 December 2021 / Accepted: 17 December 2021 / Published: 18 December 2021

(This article belongs to the Special Issue Agricultural Products: Nutritional Value and Functional Properties)

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Abstract

:

The main purpose of this work was to assess the potential of chili pepper seed oil (CPSO) and sweet pepper seed oil (SPSO) to inhibit or retard the thermo-oxidative processes undergoing in sunflower oil (SFO) when subjected to high-temperature heating for 4 and 8 h in simulated frying conditions. The effects of high-temperature treatment for 4 and 8 h on the fatty acid composition and the lipid oxidation degree of the investigated oil samples were evaluated using the peroxide value (PV), the p-anisidine value (p-AV) and the thiobarbituric acid test (TBA). All determinations were performed before and after sample heating in order to evaluate the changes in lipid oxidation as well as in the chemical composition. In all studied samples, both after 4 h and 8 h of high-temperature heating, there was an increase of the saturated fatty acid content. This increase is lower in the case of SFO samples supplemented with CPSO and SPSO when compared with SFO. A 41.67% increase was recorded for the SFO sample supplemented with 300 ppm CPSO, and a 36.76% increase was recorded for the SFO supplemented with 300 ppm SPSO, compared to the 44.97% increase recorded for the SFO. Heating the samples supplemented with CPSO and SPSO with a concentration of 300 ppm for 8 h led to the much lower values of the investigated parameters in relation to the control sample, as follows: PV (12.95 ± 0.17 meq/kg oil for SFO + 300 ppm CPSO and 13.45 ± 0.32 meq/kg oil for SFO + 300 ppm SPSO, compared with 16.4 + 0.17 meq/kg oil for SFO), p-AV (63.445 ± 1.259 ppm oil for SFO + 300 ppm CPSO and 64.122 ± 1.208 ppm oil for SFO + 300 ppm SPSO, compared with 72.493 + 1.340 ppm oil for SFO), CD (45%; 30%), TOTOX (88.374 for SFO + 300 ppm CPSO and 101.366 for SFO + 300 ppm SPSO compared with 105.347 ppm for SFO) and TBA (98.92 ± 2.49 µg MDA/g oil for SFO + 300 ppm CPSO and 114.24 ± 3.51 µg MDA/g oil for SFO + 300 ppm SPSO, compared with 180.08 + 5.82 µg MDA/g oil for SFO). Regarding the lipid oxidation process occurring during the heat treatment, we observed the reduction of lipid oxidation by the addition of CPSO and SPSO and recommend these seed oils as potential natural antioxidants in order to improve the oxidative stability of SFO during heat treatment.

Keywords:

sweet pepper seed oil; chili pepper seed oil; thermo-oxidative stability; sunflower oil

1. Introduction

Food lipids are components subjected to heat treatment at medium and high temperatures, which, in the presence of oxygen, suffer from various processes such as thermo-oxidation, polymerization and hydrolysis. These processes lead to the decomposition of the chemical composition, producing an unpleasant odor and decreasing the nutritional value of the fried product [1].

Oxidation processes are one of the main damage sources that occur during the processing, storage, distribution and final processing of food products. Lipid oxidation products are ubiquitous in food, but the problem of lipid oxidation severely compromises the quality of some foods and limits the shelf life of others [2].

The oxidation degree (rancidity) of edible vegetable oils is an indicator of their freshness, with major implications for food quality and safety [3].Vegetable oils are preferred for consumption due to their low cholesterol level, but they are more exposed to oxidation due to the high level of unsaturated fatty acids compared to animal lipids, which contain saturated fatty acids and therefore do not react with other chemicals, especially oxygen [4]. Recently, new natural preservative discoveries that provide better thermal stability of edible oils during frying were discussed [5]. The addition of synthetic antioxidants to increase the oxidative stability of edible oils is not recommended [6]; however, lately there has been growing interest in identifying natural sources of antioxidants [7,8,9], with a particular emphasis on byproducts [1]. Recent studies have pointed out that, due their toxicity and carcinogenic effects in animals and humans, the use of synthetic antioxidants is restricted [10]. Currently, the US Food and Drug Administration (FDA) and the European Food Safety Authority (EFSA) have established legal limits with regard to the allowed amounts of synthetic antioxidants [11].

Sunflower oil (SFO) is one of the main edible vegetable oils, with high levels of polyunsaturated fatty acids, especially linoleic acid. It is added to various food products, contributing to the increase of the essential fatty acid content in their composition [12].

The sweet pepper and chili seeds are a cheap raw material and a source of fat with high value oils due to their high antioxidant content. The processing of peppers in the canning industry results in a significant amount of seeds, whose recovery is currently limited. Pepper seed oil has a high content of linoleic acid, about 70%, and is rich in vitamin C and capsaicin, which is the main active component of hot peppers, thereby generating an antioxidant effect [12,13]. The antioxidant mechanism of capsaicin has been reported by Kogure et al. [14], which showed that capsaicin delayed the lipid oxidation of soybean oil during the frying process at 200 °C [15] and 140 °C [5] but is not so effective at 100 °C [16]. However, data regarding the antioxidant effect of pepper seed oil in the case of sunflower oil have not been reported in the literature.

Given that lately there is an increasing emphasis regarding the concept of circular economy and promoting the sustainability of alternative resources, capitalizing on byproducts resulting from vegetable processing is a topical approach with a positive economic, social and environmental impact. In this context, the aim of this study was to determine the fatty acid content as well as the antioxidant effect of the oil obtained from pepper seeds, and the potential uses as a sustainable food matrix.

In this paper, we evaluated the potential of chili pepper seed oil (CPSO) and sweet pepper seed oil (SPSO) as a source of natural antioxidants that could increase the shelf life of SFO. Primarily, we evaluated the changes in fatty acids in the sample composition concerning the degree of oxidation of the lipids. Moreover, the peroxide value (PV), the p-anisidine value (p-AV) and the thiobarbituric acid test (TBA) analysis were determined. The total oxidation value (TOTOX) was calculated using the PV and p-AV values. The antioxidative activity of CPSO and SPSO in the sunflower oil was evaluated during, before and after thermal treatment, and was compared with the antioxidative activity of the commercially available antioxidant BHT.

2. Materials and Methods

2.1. Oil Samples

SFO, CPSO and SPSO were purchased from the Solaris, Bucharest, Romania, who produces cold-pressed vegetal oils, natural, 100%, without the addition of any additives. The reagents used were of analytical grade and were purchased from Sigma-Aldrich Chemie GmbH, München, Germany.

2.2. Application of CPSO and SPSO to SFO

A total of 8 samples were weighed in 50 mL of SFO oil free of synthetic antioxidants. In one, 200 ppm of BHT (maximum legal admissible dose) was added; in six were added CPSO and SPSO at three levels of concentrations (100 ppm, 200 ppm and 300 ppm). Moreover, a SFO sample without any antioxidant was used as a control. The obtained oil mixtures were stirred using a mechanical stirrer for complete homogenization.

2.3. Heating Processes

To examine the heating effect on the sunflower oil supplemented with CPSO, SPSO and BHT, the individual samples were subjected to the heat treatment in a conventional furnace (Esmach, Esmach Ali Group S.r.l., Grisignano, Italy; 1200 W, 50 Hz) to a temperature of 180 °C, similar to the conditions specific to the food industry, for 8 h of frying. After each heating period, the samples were removed from the furnace, cooled and analyzed.

The experimental process of heating was developed in agreement with previous studies [1,3]. Preliminary tests have been carried out to establish the heat regime for this treatment. The samples were heated separately for 4 to 8 h.

The studied oil sample temperature was determined immediately after each heating period with the help of a calibrated chromel-alumel thermocouple (HI 935009, Hanna Instruments, New York, NY, USA). The internal temperatures of the oil sample heated in a conventional oven are shown in Table 1.

The samples were removed from the oven, cooled rapidly and stored at −18 °C until they were analyzed. Separate samples were used for each heating period.

2.4. Determination of Fatty Acid Composition by GC-MS

Fatty acids were analyzed as fatty acid methyl esters (FAME). The fatty acids contained in 0.1 g lipids were derivatized with 3 mL of 3% boron trifluoride 20% (Sigma-Aldrich Chemie GmbH, München, Germany). The derivatization was performed for 1 h at 80 °C in an ultrasonic bath (FALC Instruments, Treviglio, Italy). After cooling, 2.5 mL of 10% NaCl solution was added, and FAME was extracted in 2 mL of hexane (Sigma-Aldrich Chemie GmbH, München, Germany). The organic layer was separated by centrifugation at 3000 rpm for 15 min (Centrifuge Hermle Labortechnik, Wehingen, Germany). The FAMEs were analyzed using Shimadzu GCMS-QP2010PLUS (Kyoto, Japan) equipment with AT-WAX column (30 m, 0.32 mm i.d., 1 µm). The temperature program was 140 °C for 10 min, then the temperature was raised by 7 °C/min up to 250 °C, with this temperature being maintained for 10 min. The partition ratio was 1:10. The injection port temperature was set at 250 °C, the source temperature was 210 °C and ionic interface temperature was 255 °C. For FAME determination, hexane was used as a solvent, and helium was used as a carrier gas, with a flow rate of 1.00 mL/min and a linear velocity of 37.8 cm/s. FAME peaks were identified using NIST05 library and quantified by area normalization method. The percentage of compounds was determined by reporting the peak area corresponding to a specific compound to the total peak area (for all identified components) [17].

Saturated fatty acids (SFA) were calculated based on the sum of C16:0 and C18:0, monounsaturated fatty acids (MUFA) were calculated as sum of C18:1 and C22:1 and polyunsaturated fatty acids (PUFA) were represented by C18:2.

In this section, the decreases/increases registered for SFA, MUFA and PUFA after 4 and 8 h of heat treatment were also calculated, these being expressed as a percentage.

2.5. Determination of Peroxide Value

The peroxide (PV) value was determined by the iodometric method according to the standard method for oil analysis, and the results were expressed in meq/kg oil [18].

2.6. p-Anisidine Value (p-AV)

To determine the p-AV, a spectrophotometric analysis method was used by measuring the absorbance at 350 nm, according to the official method (AOCS Official Method Cd 18–90), [19]. For the p-AV measurement, 2 g of oil sample was dissolved in 25 mL of isooctane (Sigma-Aldrich Chemie GmbH, München, Germany). The absorbance of the obtained solutions was measured against a blank isooctane sample at 350 nm using a double-beam UV-Vis spectrophotometer (Specord 205; Analytik Jena AG, Jena, Germany). A total of 5 mL of the obtained solutions were transferred to individual tubes, as well as 5 mL of the isooctane solvent used as a control and 1 mL of the p-anisidine/glacial acetic acid solution (0.25%, w/v) (Sigma-Aldrich Chemie GmbH, München, Germany) was added. After 10 min, the absorbance of the oil solutions in the tubes was measured at 350 nm compared to the solution containing isooctane and p-anisidine. The p-AV was calculated based on the relationship shown in Equation (1):

p - AV = 25 \times \frac{1.2 \times A_{2} - A_{1}}{W}

(1)

where A₁—the absorbance of 2 g oil sample in 25 mL isooctane measured against a blank of isooctane; A₂—the absorbance of 2 g oil sample in 25 mL isooctane with 1 mL p-anisidine solution measured against a sample of isooctane containing p-anisidine solution; W—the sunflower oil sample weight (g).

2.7. Total Oxidation Value (TOTOX)

PV and p-AV were converted to the total oxidation value (TOTOX) by using Equation (2).

Totox value = 2·PV + AV

(2)

2.8. Assessing the Lipid Oxidation Degree of Oil Samples by TBA Test

This method represents one of the most commonly used methods to evaluate the lipid oxidation degree of oil samples and is based on measuring the absorbance of the TBA-malonaldehyde complex at 532–535 nm [2]. Malondialdehyde (MDA) is a three-carbon dialdehyde, being one of the oxidation products of the unsaturated acid intermediates. Literature data has shown that malondialdehyde can be dosed by a treatment with thiobarbituric acid, the reaction of which forms red condensation products that absorb at 532–535 nm with a molar absorptivity of 27.5 absorbance units/mmol [20].

Determination of antioxidant activity by the thiobarbituric acid method (TBA) was performed according to the method of Singh et al. [21], Kikuzaki and Nakatani [22] and Tarladgis et al. [23], with small changes. The TBA was expressed as µg of malonaldehyde per g sample.

A total of 2 g of oil of each type was weighed, to which 5 mL of benzene and 4 mL of thiobarbituric acid (0.67% aqueous solution) (Sigma-Aldrich Chemie GmbH, München, Germany) were added. The samples prepared were shaken for 30 min using a mechanical stirrer (Heidolph, Illinois, IL, USA) and maintained at rest for 10 min to separate the phases. The supernatant was taken into the tubes and then heated on the water bath at 80 °C for 45 min.

After cooling, absorbance of the supernatant was measured at 540 nm using the Specord 210 Analytik Jena spectrophotometer against an oil-free control sample. The calibration curve of the thiobarbituric acid test was performed by measuring the extinctions of some samples with known concentrations of malonaldehyde. The amount of malonaldehyde in the samples was calculated based on the calibration line, depending on the extinctions read and the sample weight taken into work.

2.9. Statistical Analysis

All determinations were carried out in triplicates and values were presented as mean values ± SD. Values p < 0.05 were considered statistically significant. One-way ANOVA and two-sample t-test assuming equal variances were applied to evaluate the statistical significance. Statistical processing data was performed using Microsoft Excel 2010.

3. Results

3.1. Fatty Acids Composition

The effects of the high-temperature treatment for 4 and 8 h on the fatty acid composition of the investigated oil samples are shown in Table 2 (p < 0.05).

In the untreated oil samples, polyunsaturated fatty acids (PUFA) represented the largest amounts of identified fatty acids, namely linoleic acid (C18:2) followed by monounsaturated (MUFA), respectively, oleic acid (C18:1) and erucic acid (C22:1), identified only in SPSO and the samples containing SPSO. Saturated fatty acids (SFA) such as palmitic acid (C16:0) and stearic acid (C18:0) were identified in smaller quantities (p < 0.05).

Regarding the variation of the fatty acid content in the oil samples before thermal treatment, the results are as follows:

The highest content of palmitic acid (C16:0) was found in CPSO (13.90%) and the lowest in SFO + BHT (8.51%);
The highest content of stearic acid was found in SPSO (4.82%) and the lowest in SFO (3.33%);
The highest content of oleic acid was identified in SFO (30.76%) and the lowest in CPSO (11.42%);
The largest amounts of linoleic acid were registered in CPSO (70.41%) and the smallest in SFO + BHT (56.83%).

Erucic acid was identified in small quantities only in SPSO and the samples containing SPSO.

For all the samples studied, after the heat treatment application, both at 4 and at 8 h, there was a significant decrease in the proportion of PUFA (Table 3) due to the oxidation reaction produced during the heating process, this decrease being inversely proportional to the duration of the thermal process.

In the case of samples supplemented with CPSO and SPSO after 4 h of heat treatment, the lowest decrease in PUFA (%) was recorded for SFO + 300 ppm CPSO (9.99%) and SFA + 300 ppm SPSO (9.87%). The decrease of PUFA (%) in the SFO control sample was 13.69% compared to SFO + BHT, which decreased with 3.41% (Figure 1). Within 4–8 h of the heat treatment, a slowdown in the oxidation process was recorded, with a smaller decrease in the proportion of PUFA (%). However, the lowest decrease in PUFA (%) compared to the 4-h values was found in the case of SFO + 300 ppm CPSO (2.71%) and SFA + 300 ppm SPSO (2.55%), compared to the SFO control sample that recorded a decrease of 3.18% and SFO + BHT, which recorded a decrease of 1.82%.

In all the samples studied, both after 4 h and after 8 h of heat treatment, there was an increase in the content of saturated fatty acids (SFA), this increase being directly proportional to the duration of the heat treatment. The highest increase was registered for SFO + 100 ppm CPSO (41.16%) and SFO + 100 ppm SPSO (41.73%), compared to the SFO control sample which registered an increase of 44.90% and the SFO + BHT test with an increase of 12.55% (Figure 1). PUFA growth was slower in the 4–8 h heat treatment period than in the first 4 h (Figure 1).

It is worth mentioning that the ratio of saturated and polyunsaturated fatty acids increased proportionally with the concentration of CPSO and SPSO, and the MUFA ratio decreased inversely proportional with the concentrations of CPSO and SPSO used.

3.2. Peroxide Value

The data presented in Table 4 express the PV changes recorded during heating in response to the addition of BHT, CPSO and SPSO to the oil. The peroxide value was in the range of 1.29–15.66 meq/kg for the oil samples with additions of CPSO and SPSO, while for the control sample (SFO) values were determined between 1.58–16.40 meq/kg, and between 1.59–12.37 meq/kg for SFO + BHT. Both after 4 h and after 8 h of heat treatment, the highest PV was observed for the control sample (SFO) followed by SFO + 100 ppm SPSO, SFO + 100 ppm CPSO, SFO + 200 ppm SPSO, SFO + 200 ppm CPSO, SFO + 300 ppm SPSO, SFO + 300 ppm CPSO and SFO–BHT, respectively. The CPSO and SPSO samples recorded the lowest PV values both before and after the heat treatment.

After 8 h of heat treatment, there was a regular pattern of PV growth for all samples. The values recorded for SFO–BHT (12.37 ± 0.26 meq/kg oil) may be comparable to those recorded for SFO + 300 ppm CPSO (12.95 ± 0.17 meq/kg oil) and SFO + 300 ppm SPSO (13.45 ± 0.32 meq/kg oil), suggesting that both CPSO and SPSO may provide oxidative stability to sunflower oil during heat treatment.

3.3. p-Anisidine Value (p-AV)

The data shown in Table 5 express the p-AV recorded during the heating process in response to the addition of BHT, CPSO and SPSO.

Analyzing the results obtained for the samples of sunflower oil with BHT and different doses of CPSO and SPSO added, it can be seen that, with the increase of the heat treatment duration, the p-AV value also increases (p < 0.05) (Table 5). This increase in p-AV is attributed to the formation of secondary oxidation products.

After 4 h of heat treatment, the increase in p-AV was very fast in all samples and continued to increase with the heat treatment period, but at a slower rate.

The p-AV value ranged from 0.673–70.222 ppm in the oil samples with the addition of CPSO and SPSO and 1.861–165.397 ppm in the SFO + BHT samples, while for the control sample (SFO), values between 1.873–65.397 ppm were recorded.

Both after 4 h and after 8 h of heat treatment, the highest p-AV was observed for the control sample (SFO), followed by SFO + 100 ppm SPSO, SFO + 100 ppm CPSO, SFO + 200 ppm SPSO, SFO + 200 ppm CPSO, SFO + 300 ppm SPSO, SFO + 300 ppm CPSO and SFO–BHT, respectively. CPSO and SPSO samples recorded the lowest p-AV values both before and after heat treatment.

3.4. Total Oxidation Value (TOTOX Value)

The TOTOX values for the analyzed oil samples increased significantly with the heating time (Figure 2).

The TOTOX values for the samples mixed with BHT, CPSO and SPSO were significantly lower than the values recorded for the control sample.

After 4 h of convective heating, the addition of oil with different doses of CPSO and SPSO led to a decrease in the TOTOX value in the range of 65.178–72.673 compared to the control (74.579), while the sample supplemented with BHT recorded a value of 43.334.

Heating for 8 h decreased the TOTOX value to 90.934–101.366 compared to 105.347 for the control, while the sample supplemented with BHT recorded a value of 53.358. The best inhibitory effect against oil oxidation during heating was recorded in the SFO + 300 ppm CPSO test. In both stages of the heat treatment, the lowest TOTOX values were recorded when supplementing the sunflower oil with 300 ppm CPSO and SPSO, with these concentrations approaching the level of inhibition recorded when using BHT.

3.5. Assessing the Lipid Oxidation Degree of Oil Samples by TBA Test

The data presented in the Table 6 represent changes in the TBA value content during the heating process as a result of BHT, CPSO and SPSO supplementation (p < 0.05).

In all samples a progressive increase of TBA value is observed during the heat treatment period. In the case of the control sample, the increase was the most significant, almost up to 10 times higher at the end of the thermal process compared to the initial value. The smallest increase was recorded for CPSO and SPSO, with the final value of TBA being up to 5 times higher than the original one.

The TBA values recorded for CPSO and SPSO were significantly lower than for SFO both before and after the heat treatment, due to the fact that the number of polyunsaturated fatty acids decreased less in the case of CPSO and SPSO than in the case of SFOs.

After the application of thermal treatment for 4 h and 8 h, the TBA values in the SFO with addition of CPSO and SPSO were significantly lower compared to the control sample, with the best results being recorded in the case of the SFO + 300 ppm CPSO sample, which is even smaller than in the case of the SFO sample with a synthetic antioxidant.

CPSO and SPSO at a 200 ppm use a rate of lipid oxidation inhibition in a similar manner to the synthetic antioxidant.

In the case of the samples in the form of SFO and CPSO or SPSO mixtures, the TBA value was dependent to the dose; therefore, the lipid oxidation degree was inversely proportional to the percentage of the CPSO and the SPSO added. Thus, the lowest TBA values were obtained for SFO + 300 ppm CPSO and SFO + 300 ppm SPSO, and the highest for SFO + 100 ppm CPSO and SFO + 100 ppm SPSO, for both 4 and 8 h. Moreover, good results were recorded in samples of SFO with the addition of CPSO compared with those with SPSO.

Thus, the results obtained in the present study suggest that the lipid oxidation process occurring during heat treatment can be reduced by the addition of CPSO and SPSO, and as such may be used as potential natural antioxidants in order to improve the oxidative stability of SFO during heat treatment.

4. Discussion

Increased consumption of edible oils worldwide is limited by several factors, including the content of trans fatty acids and rancid properties. Edible oils are highly susceptible to lipid oxidation and the loss of flavor that occurs during the frying process, depending on the fatty acid composition, shelf life and processing temperature [5]. It also affects numerous interactions between food constituents, which lead to both desirable and unwanted products.

The fatty acid composition of the SFO, SPSO and CPSO analyzed in this study is consistent with data reported in the literature [12,24,25]. Jarret et al. [26] obtained for CPSO the following values: 13.38% (C16:0), 3.61% (C18:0), 6.55% (C18:1), 76.1% (C18:2), and for SPSO: 13.85% (C16.0), 3.23% (C18:0), 7.51% (C18:1) and 73.92% (C18:2).

Silva et al. [27] reported a higher content of palmitic acid (23.16%) and stearic acid (18.25%), and lower for oleic acid (2.66%) and linoleic (38.31%), for sweet pepper oil.

The results obtained after the thermal treatment are consistent with other studies. Thus, Aladedunye and Przybylski [24] analyzed sunflower oil samples supplemented with different levels of linoleic acid subjected to heating at 140 °C for 14 days. The obtained results highlighted a decrease of PUFA content and an increase of SFA proportional with the duration of the heat treatment, in accord with the data reported in our study.

Medina-Juárez and Gámez-Meza [28] have found a decrease in PUFA content and an increase in SFA content after keeping sunflower oil at a frying temperature for 80 h. Budryn et al. [12] have noticed a decrease of PUFA content and an increase of SFA content in a sunflower oil sample with the addition of green coffee extract exposed to heating at 110 and 180 °C for 60 min, and further stored for 3 months. PV and p-AV together provide a complete overview of the oil oxidation process. PV is the measure of primary oxidation degree of oils and fats. The determination of peroxides can be used as an oxidation index for the early stages of lipid oxidation. The p-AV is a measure of the secondary oxidation of oils and fats [1]. A continuous increase of PV with heating time was observed for all the samples (p < 0.05). This increase is attributed to the formation of hydroperoxides, i.e., primary oxidation products. After 4 h of heat treatment, the PV increases very fast in all the analyzed samples, while between 4–8 h a slower rate was recorded.

The PV values recorded in our study for the samples of oil with the addition of CPSO and SPSO was in the range between 1.29–5.66 meq/kg oil.

Previous results highlighted the effect of byproducts enriched in antioxidant compounds on oil stability. Iqbal et al. [4] studied the antioxidant effect of pomegranate peel extract in the stabilization of sunflower oil, with the values obtained for the PV being between the range of 64.21–147.34 meq/kg depending on the concentration of pomegranate peel extract used. Singh et al. [20] studied the antioxidant potential of Foeniculum vulgare volatile oil on sunflower oil and found that it is significantly more effective than butylated hydroxy toluene. Poiană [1] investigated the effectiveness of grape seed extract compared to butylated hydroxy toluene on retarding the lipid oxidation of sunflower oil subjected to convection heating up to 240 min under simulated frying conditions, with the values recorded being between 1.77–9.81 meq/kg oil, which are values comparable to those obtained in the present study.

In our study, the sample of oil with the addition of CPSO and SPSO registered values between 1.713–64.122 ppm. The results obtained in this study regarding the antioxidant effects of pepper seed oil and its role in stabilizing the thermo-oxidative effect of sunflower oil are in line with those reported in the literature. The effectiveness of grape seed extract compared to butylated hydroxytoluene on the delayed lipid oxidation of sunflower oil subjected to heating under simulated frying was studied by Poiana [1], who showed that after convective heating, the p-AV of the samples with the addition of grape seed extract records a decrease in the p-AV depending on the dose; thus, 45.25 ppm for a concentration of 200 ppm grape seed extract to 35.75 ppm for 1000 ppm grape seed extract. Moreover, the effectiveness of blueberry processing byproducts compared to butylated hydroxy toluene on retarding the lipid oxidation of sunflower oil subjected to convection heating up to 240 min under simulated frying conditions was reported [29], with the p-AV value in this case also being dependent on the dose of blueberry byproduct extracts added (63.67 ppm for 200 ppm blueberry byproduct extracts and 57.81 ppm for 800 ppm blueberry byproduct extracts). Other studies have reported the antioxidant effect of spearmint or pomegranate essential oils in the stabilization of sunflower oil [30]. The TOTOX value is a mathematical prediction of oxidative stability and is used as an indicator of the overall oxidative stability being correlated with the degree of oil damage [1]. The values of TOTOX recorded in our study (between 4.088–101.366) for all the samples are comparable to those reported in other studies. Poiana [1] obtained, for samples of oil supplemented with grape seed oil, TOTOX values in the range of 5.82–92.27, while Ungureanu et al. [29] concluded that the addition of other oils or extracts with a high antioxidant activity may limit or reduce the lipid oxidation of sunflower oil during heating. The values reported by Ungureanu et al. [29] were between the range 51.19–81.27 for the sample supplemented with blueberry byproduct extracts, which are values comparable to those obtained in the present study. The oxidation degree of the vegetable oils subjected to thermal treatment was evaluated on the basis of the thiobarbituric acid test (TBA). The malondialdehyde amount generated in response to the oxidation processes undergoing in the oil samples has been quantified on the basis of the calibration curve. The thiobarbituric acid test gives satisfactory results, with the amount of malondialdehyde formed increasing with the evolution of the oxidation process. After the tests were carried out, an increase of malondialdehyde content was found due to oxidation which occurred after the heat treatment.

In our study, the TBA value varied from 18.70–114.24 µgMDA/mL oil. Similar observations were also reported by Yang et al. [5], who studied the thermal oxidative stability of red pepper seed oil in which different proportions of capsaicin or tocopherol were added as antioxidants during heating up to 140 ± 5 °C for 48 h. Similar results were also reported by Iqbal et al. [4], who studied the antioxidant effect of pomegranate peel extract in the stabilization of sunflower oil, and observed that pomegranate peel extract at concentrations of 800–850 ppm has a stabilization efficiency comparable to conventional synthetic antioxidants, i.e., butylated hydroxy toluene at its legal limit. Moreover, Ungureanu et al. [29] investigated the effectiveness of blueberry byproduct extracts compared to butylated hydroxy toluene on retarding the lipid oxidation of sunflower oil subjected to convection heating up to 240 min under simulated frying conditions, obtaining values between 5.16–51.58 µg MDA/mL oil, which are values comparable to those obtained in the present study.

Wang et al. [31] studied the influence of spearmint essential oil on sunflower oil during deep frying, demonstrating the antioxidant effect of M. spicata in sunflower oil.

Moreover, Hussain [32] studied the efficacy of sesame seed extracts in stabilizing the sunflower oil during storage, finding that it can be considered a very good choice as a natural antioxidant to stabilize the sunflower oil.

5. Conclusions

From the present study, we can conclude that chili pepper seed oil and sweet pepper seed oil can stabilize sunflower oil effectively at all the concentrations tested. Chili pepper seed oil and sweet pepper seed oil at concentrations of 300 ppm have better stabilization efficiency compared to conventional synthetic antioxidants, i.e., BHT at its legal limit, and improves the resistance of sunflower oil against thermal deteriorative changes. Besides this, the polyunsaturated fatty acid content is increased appreciably by creating resistance in the oil against oxidative rancidity. Therefore, through this study, chili pepper seed oils and sweet pepper seed oils can be recommended as a potent source of antioxidants for the stabilization of sunflower oils.

Author Contributions

Conceptualization, I.C., M.N., E.A. and M.-A.P.; methodology, I.C., M.N., A.C., M.-A.P., C.D., I.P., A.I.C., D.O. and I.R.; writing—original draft preparation, I.C., M.N., E.A., M.-A.P. and D.R.; writing—review and editing, I.C., M.N., E.A., M.-A.P., D.R. and C.D.; visualization, I.C., M.N., A.C., E.A., M.-A.P., D.R., C.D., I.P., A.I.C., D.O. and I.R.; supervision, I.C., E.A. and I.R.; funding acquisition, I.R. All authors have read and agreed to the published version of the manuscript.

Funding

This paper is published from the own funds of the Banat‘s University of Agricultural Sciences and Veterinary Medicine “King Michael I of Romania” from Timisoara, Romania.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

The report of the analyses performed for the samples in the paper can be found at the Interdisciplinary Research Platform (PCI) belonging to the Banat University of Agricultural Sciences and Veterinary Medicine “King Michael I of Romania” from Timisoara, being registered with number 21c/17.01.2018.

Acknowledgments

We have been able to carry out this research with the support of the Interdisciplinary Research Platform belonging to the Banat University of Agricultural Sciences and Veterinary Medicine “King Michael I of Romania” from Timisoara, where the analysis were made.

Conflicts of Interest

The authors declare no conflict of interest.

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Figure 1. Changes in fatty acid composition of oil samples in response to heat treatment versus SFO sample. (a) CPSO; (b) SPSO.

Figure 2. The impact of CPSO, SPSO and BHT on TOTOX value during heating of sunflower oil.

Table 1. Temperature evolution for sunflower oil samples during heating.

	Time
Temperature (°C)	0 h	4 h	8 h
Temperature (°C)	26.4	177.4	179.1

Table 2. The effect of heat treatment for 4 and 8 h on fatty acid composition of oil samples.

Sample	Fatty Acids (%)
	C16:0	C18:0	C18:1	C18:2	C22:1
	initial
SFO	8.54 ± 0.13 ^a	3.33 ± 0.10 ^a	30.76 ± 1.22 ^a	56.91 ± 1.11 ^a	nd
SFO + BHT	8.51 ± 0.16 ^a	3.53 ± 0.09 ^a,c	30.63 ± 1.00 ^a	56.83 ± 1.39 ^a	nd
CPSO	13.90 ± 0.45 ^b	4.26 ± 0.12 ^b	11.42 ± 0.29 ^b	70.41 ± 2.04 ^b	nd
SPSO	13.10 ± 0.47 ^b	4.82 ± 0.19 ^d	12.51 ± 0.30 ^c	69.39 ± 2.05 ^b	0.18 ± 0.03 ^a
SFO + 100 ppmCPSO	9.08 ± 0.17 ^c	3.44 ± 0.11 ^a	28.84 ± 0.97 ^a,e	58.28 ± 1.46 ^a,c	nd
SFO + 200 ppmCPSO	9.69 ± 0.20 ^d	3.52 ± 0.10 ^a,c,f	26.90 ± 0.92 ^d,e	59.66 ± 1.88 ^a,c	nd
SFO + 300 ppmCPSO	10.18 ± 0.24 ^d,e	3.62 ± 0.12 ^c,f	24.82 ± 0.89 ^d,f	60.98 ± 1.28 ^c	nd
SFO + 100 ppmSPSO	8.98 ± 0.16 ^c	3.49 ± 0.09 ^a,f	28.96 ± 0.96 ^a,e	58.19 ± 1.40 ^a,c	0.02 ± 0.01 ^b
SFO + 200 ppmSPSO	9.50 ± 0.18 ^d,f	3.63 ± 0.16 ^c,f	27.12± 0.77 ^d,e,g	59.39 ± 1.84 ^a,c	0.05 ± 0.02 ^b,d
SFO + 300 ppmSPSO	9.89 ± 0.17 ^d,f	3.75 ± 015 ^e,f	25.37 ± 0.93 ^d	60.62 ± 1.81 ^c	0.07 ± 001 ^c,d
Sample	4 h
SFO	8.21 ± 0.21 ^a	8.99 ± 0.28 ^a	33.67 ± 1.08 ^a	49.12 ± 1.04 ^a	nd
SFO + BHT	8.40 ± 0.16 ^a	5.15 ± 0.12 ^b	31.56 ± 1.06 ^a,d	54.89 ± 1.09 ^b	nd
CPSO	12.54 ± 0.51 ^b	8.21 ± 0.20 ^c	10.85 ± 0.40 ^b	68.40 ± 1.88 ^c	nd
SPSO	12.47 ± 0.37 ^b	9.49 ± 0.24 ^a,d	10.14 ± 0.26 ^b	67.43 ± 2.13 ^c	0.41 ± 0.03 ^a
SFO + 100 ppmCPSO	8.64 ± 0.34 ^a,d	8.94 ± 0.22 ^a,e	31.28 ± 0.96 ^c,d	51.05 ± 0.95 ^a,d	nd
SFO + 200 ppmCPSO	9.07 ± 0.25 ^c,d	8.85 ± 0.15 ^a,e	29.11 ± 0.97 ^c,f	52.95 ± 1.07 ^b,d	nd
SFO + 300 ppmCPSO	9.50 ± 0.35 ^c	8.75 ± 0.22 ^a,e	26.85 ± 0.99 ^e	54.89 ± 1.33 ^b	nd
SFO + 100 ppmSPSO	8.61 ± 0.22 ^a	9.04 ± 0.24 ^a	31.38 ± 1.06 ^a,d,f	50.93 ± 1.09 ^a,d	0.03 ± 0.01 ^b
SFO + 200 ppmSPSO	9.09 ± 0.20 ^c,d	9.08 ± 0.23 ^a	28.99 ± 1.02 ^e,f	52.78 ± 1.04 ^b,d	0.06 ± 0.02 ^b,c
SFO + 300 ppmSPSO	9.54 ± 0.19 ^c	9.16 ± 0.17 ^a	26.59 ± 0.92 ^e	54.64 ± 1.44 ^b	0.11 ± 0.03 ^c
Sample	8 h
SFO	8.80 ± 0.23 ^a	9.83 ± 0.29 ^a	32.81 ± 0.96 ^a	47.56 ± 1.13 ^a	nd
SFO + BHT	8.89 ± 0.38 ^a,c	6.50 ± 0.15 ^b	32.32 ± 1.10 ^a,d	53.89 ± 1.15 ^b	nd
CPSO	11.81 ± 0.41 ^b	10.49 ± 0.35 ^a	10.40 ± 0.44 ^b	67.12 ± 1.60 ^c	nd
SPSO	12.24 ± 0.46 ^b	9.96 ± 0.25 ^a	10.51 ± 0.26 ^b	66.58 ± 1.38 ^c	0.63 ± 0.12 ^a
SFO + 100 ppmCPSO	9.10 ± 0.19 ^c	9.89 ± 0.32 ^a	30.70 ± 0.98 ^a,d	49.63 ± 1.05 ^d,e	nd
SFO + 200 ppmCPSO	9.39 ± 0.39 ^c,e	9.97 ± 0.27 ^a	28.37 ± 1.03 ^c	51.49 ± 1.32 ^b,e,f	nd
SFO + 300 ppmCPSO	9.72 ± 0.37 ^c,e	10.03 ± 0.30 ^a	26.08 ± 0.98 ^e	53.40 ± 1.15 ^b	nd
SFO + 100 ppmSPSO	9.17 ± 0.29 ^c	9.85 ± 0.34 ^a	30.59 ± 0.61 ^c,d,f	49.46 ± 1.23 ^d,f,g	0.04 ± 0.01 ^b
SFO + 200 ppmSPSO	9.87 ± 0.26 ^d,e	9.86 ± 0.31 ^a	28.34 ± 1.00 ^c,g	51.38 ± 1.25 ^b,e,g	0.09 ± 0.01 ^c
SFO + 300 ppmSPSO	9.83 ± 0.38 ^d,e	9.88 ± 0.21 ^a	26.17± 0.68 ^e	53.24 ± 1.30 ^b	0.18 ± 0.04 ^d

The values are expressed as mean values ± standard deviations of all measurements. ^a–g A t-test was used to compare the mean differences registered among samples; data within the same column sharing different superscripts are significantly different (p < 0.05); data within the same column sharing the same superscripts are not significantly different (p > 0.05).

Table 3. The changes in fatty acid profiles of the oil samples in response to heating treatment.

Fatty Acids (%)	SFO (Control)	SFO + BHT	CPSO	SPSO	SFO + 100 ppm CPSO	SFO + 200 ppm CPSO	SFO + 300 ppm CPSO	SFO + 100 ppm SPSO	SFO + 200 ppm SPSO	SFO + 300 ppm SPSO
	initial
SAT	11.87	12.03	18.16	17.92	12.52	13.20	13.80	12.46	13.13	13.64
MUFA	30.76	30.63	11.42	12.69	28.84	26.90	24.82	28.98	27.17	25.44
PUFA	56.91	56.83	70.41	69.39	58.28	59.66	60.98	58.19	59.39	60.62
	4 h
SAT	17.20	13.54	20.75	21.96	17.57	17.94	18.25	17.66	18.17	18.65
MUFA	33.67	31.56	10.85	10.56	31.28	29.11	26.85	31.41	29.05	26.70
PUFA	49.12	54.89	68.40	67.43	51.05	52.95	54.89	50.93	52.78	54.64
	8 h
SAT	18.63	15.40	22.30	22.20	18.98	19.36	19.76	19.02	19.73	19.70
MUFA	32.81	32.32	10.40	11.14	30.70	28.37	26.08	30.63	28.43	26.35
PUFA	47.56	53.89	67.12	66.58	49.63	51.50	53.40	49.46	51.38	53.24

Table 4. Peroxide value of oil samples in response to heat treatment.

Sample	PV (meq/kg Oil)
Sample	Initial	4 h	8 h
SFO	1.58 ± 0.03 ^a	11.23 ± 0.18 ^a	16.40 ± 0.17 ^a
SFO + BHT	1.59 ± 0.03 ^a	7.83 ± 0.17 ^b	12.37 ± 0.26 ^b
CPSO	0.52 ± 0.01 ^b	3.63 ± 0.16 ^c	4.88 ± 0.10 ^c
SPSO	0.66 ± 0.02 ^b	4.26 ± 0.34 ^c	5.84 ± 0.09 ^c
SFO + 100 ppm CPSO	1.48 ± 0.03 ^c	10.62 ± 0.14 ^a	15.55 ± 0.14 ^a
SFO + 200 ppm CPSO	1.37 ± 0.04 ^d	9.27 ± 0.10 ^d	14.16 ± 0.37 ^d,e
SFO + 300 ppm CPSO	1.29 ± 0.04 ^e	8.88 ± 0.11 ^d^,^e	12.95 ± 0.17 ^b
SFO + 100 ppm SPSO	1.49 ± 0.04 ^c	10.66 ± 0.12 ^a	15.66 ± 0.20 ^a
SFO + 200 ppm SPSO	1.40 ± 0.03 _d	9.72 ± 0.12 ^d,f	14.28 ± 0.24 ^d
SFO + 300 ppm SPSO	1.30 ± 0.02 ^e	9.44 ± 0.22 ^d,f	13.45 ± 0.32 ^b,e

The values are expressed as mean values ± standard deviations of all measurements. ^a–f A t-test was used to compare the mean differences registered among samples; data within the same column sharing different superscripts are significantly different (p < 0.05); data within the same column sharing the same superscripts are not significantly different (p > 0.05).

Table 5. The p-AV of oil samples in response to heat treatment.

Sample	p-AV (ppm)
Sample	Initial	4 h	8 h
SFO	1.873 ± 0.025 ^a	52.119 ± 1.372 ^a	72.496 ± 1.340 ^a
SFO + 200 ppm BHT	1.861 ± 0.027 ^a	47.121 ± 1.570 ^b	65.397 ± 1.800 ^b
CPSO	0.673 ± 0.025 ^b	32.549 ± 0.938 ^c	40.182 ± 1.353 ^c
SPSO	0.723 ± 0.023 ^b	34.814 ± 0.987 ^d	41.570 ± 0.972 ^c
SFO + 100 ppm CPSO	1.713 ± 0.022 ^c	50.666 ± 1.568 ^a,f	69.682 ± 1.141 ^d
SFO + 200 ppm CPSO	1.664 ± 0.040 ^c	48.5295 ± 1.016 ^b,g	66.553 ± 1.408 ^b,f
SFO + 300 ppm CPSO	1.488 ± 0.028 ^d	45.9195 ± 1.234 ^b,h	63.445 ± 1.259 ^b,g
SFO + 100 ppm SPSO	1.846 ± 0.032 ^a	51.3525 ± 1.592 ^a,i	70.227 ± 0.932 ^d
SFO + 200 ppm SPSO	1.769 ± 0.047 ^c	49.444 ± 1.083 ^e,f,g,i	67.818 ± 1.175 ^b,f
SFO + 300 ppm SPSO	1.687 ± 0.023 ^c	46.298 ± 1.638 ^b,h	64.122 ± 1.208 ^b,g

The values are expressed as mean values ± standard deviations of all measurements. ^a–i A t-test was used to compare the means differences registered among samples; data within the same column sharing different superscripts are significantly different (p < 0.05); data within the same column sharing the same superscripts are not significantly different (p > 0.05).

Table 6. Changes in TBA value of oil samples in response to heat treatment.

Sample	TBA (µg MDA/g)
Sample	Initial	4 h	8 h
SFO	20.26 ± 0.5 ^a	143.56 ± 4.23 ^a	180.08 ± 5.82 ^a
SFO + BHT	20.22 ± 0.47 ^a	98.13 ± 2.87 ^b	125.43 ± 3.91 ^b
CPSO	9.24 ± 0.32 ^b	28.65 ± 0.89 ^c	53.19 ± 1.88 ^c
SPSO	13.30 ± 0.37 ^c	39.05 ± 1.07 ^d	70.52 ± 2.24 ^d
SFO + 100 ppm CPSO	18.70 ± 0.51 ^d	123.25 ± 3.24 ^e	146.30 ± 4.11 ^e
SFO + 200 ppm CPSO	17.73 ± 0.42 ^e,g	100.61 ± 3.02 ^b	125.92 ± 3.10 ^b
SFO + 300 ppm CPSO	16.59 ± 0.40 ^f	85.51 ± 2.66 ^f	98.92 ± 2.49 ^e
SFO + 100 ppm SPSO	19.42 ± 0.46 ^d,h	131.19 ± 4.47 ^f	164.77 ± 5.19 ^f
SFO + 200 ppm SPSO	18.58 ± 0.47 ^d	112.81 ± 3.47 ^g	139.51 ± 4.19 ^g
SFO + 300 ppm SPSO	17.91 ± 0.41 ^d,g	96.46 ± 2.96 ^b	114.24 ± 3.51 ^h

The values are expressed as mean values ± standard deviations of all measurements. ^a–h A t-test was used to compare the means differences registered among samples; data within the same column sharing different superscripts are significantly different (p < 0.05); data within the same column sharing the same superscripts are not significantly different (p > 0.05).

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Cocan, I.; Negrea, M.; Cozma, A.; Alexa, E.; Poiana, M.-A.; Raba, D.; Danciu, C.; Popescu, I.; Cadariu, A.I.; Obistioiu, D.; et al. Chili and Sweet Pepper Seed Oil Used as a Natural Antioxidant to Improve the Thermo-Oxidative Stability of Sunflower Oil. Agronomy 2021, 11, 2579. https://doi.org/10.3390/agronomy11122579

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Cocan I, Negrea M, Cozma A, Alexa E, Poiana M-A, Raba D, Danciu C, Popescu I, Cadariu AI, Obistioiu D, et al. Chili and Sweet Pepper Seed Oil Used as a Natural Antioxidant to Improve the Thermo-Oxidative Stability of Sunflower Oil. Agronomy. 2021; 11(12):2579. https://doi.org/10.3390/agronomy11122579

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Cocan, Ileana, Monica Negrea, Antoanela Cozma, Ersilia Alexa, Mariana-Atena Poiana, Diana Raba, Corina Danciu, Iuliana Popescu, Andreea I. Cadariu, Diana Obistioiu, and et al. 2021. "Chili and Sweet Pepper Seed Oil Used as a Natural Antioxidant to Improve the Thermo-Oxidative Stability of Sunflower Oil" Agronomy 11, no. 12: 2579. https://doi.org/10.3390/agronomy11122579

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Chili and Sweet Pepper Seed Oil Used as a Natural Antioxidant to Improve the Thermo-Oxidative Stability of Sunflower Oil

Abstract

1. Introduction

2. Materials and Methods

2.1. Oil Samples

2.2. Application of CPSO and SPSO to SFO

2.3. Heating Processes

2.4. Determination of Fatty Acid Composition by GC-MS

2.5. Determination of Peroxide Value

2.6. p-Anisidine Value (p-AV)

2.7. Total Oxidation Value (TOTOX)

2.8. Assessing the Lipid Oxidation Degree of Oil Samples by TBA Test

2.9. Statistical Analysis

3. Results

3.1. Fatty Acids Composition

3.2. Peroxide Value

3.3. p-Anisidine Value (p-AV)

3.4. Total Oxidation Value (TOTOX Value)

3.5. Assessing the Lipid Oxidation Degree of Oil Samples by TBA Test

4. Discussion

5. Conclusions

Author Contributions

Funding

Institutional Review Board Statement

Informed Consent Statement

Data Availability Statement

Acknowledgments

Conflicts of Interest

References

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