Validation of the Explorer® 2.0 test coupled to e-Reader® for the screening of antimicrobials in muscle from different animal species

The Explorer^® 2.0 tube test is a microbial inhibition test for the screening of antimicrobial residues in food samples. The new e-Reader^® device coupled to Explorer^® 2.0 operates by incubation at a selected temperature, determination of the endpoint of the assay and interpretation to generate results. This system was validated for muscle samples according to the European Commission Decision 2002/657/EC. Sensitivity towards 25 substances from several groups of antimicrobials was investigated in a first step. Detection capabilities for six substances representing the six major antimicrobial groups were also determined in bovine muscle. The detection capabilities for amoxicillin (10 µg l^?1), cefalexin (200 µg l^?1), doxycyclin (100 µg l^?1), sulfamethazine (100 µg l^?1), tylosin (100 µg l^?1) and neomycin (200 µg l^?1) were in all cases at or below the maximum residue limit (MRL). Specificity and applicability of the test were demonstrated with muscle samples from four animal species (bovine, porcine, ovine and poultry) and results were found to be satisfactory. Ruggedness was evaluated on negative and spiked samples with sulfamethazine as a representative antimicrobial. Neither false-positives nor false-negatives were detected when varying the sample volume, the time of pre-incubation, the temperature of incubation and the batch of the test. These results prove that Explorer^® 2.0 coupled to e-Reader^® is a valuable tool for the screening of a broad range of antimicrobials in muscle. This new methodology simplifies the analysis and increases the accuracy of interpretation of the test results since the endpoint of the assay is automatically determined and results are interpreted objectively.     

Selective Determination of Selenium in Garlic, Mushroom and Water Samples by Chemically Modified Mesoporous Silica Solid Phase Coupled with ICP-OES

A selective sorbent for solid phase extraction (SPE), based on a chemically modified mesoporous silica (SBA-15), followed by inductively coupled plasma-optical emission spectrometry was used for extraction, preconcentration, and determination of selenium in water and food samples. The main parameters of SPE including pH, amount of mesoporous (solid phase), concentration of the eluent (desorption solvent), and equilibrium time were optimized by using a fractional central composite design (f-CCD). The optimum conditions were found to be 3.2 for pH, 21 mg for amount of the mesoporous, 1 mol l^?1 for eluent concentration, and 9 min for equilibrium time. Under the optimal conditions, the limit of detection (LOD) was 2.56 μg l^?1. The linear dynamic range (LDR) was 5–1,000 μg l^?1 with determination coefficient (R ²) of 0.999. Relative standard deviation (C?=?400 μg l^?1, n?=?5) was 3.84 %. The enrichment factor was 20. The maximum sorption capacity of the modified SBA-15 was 15 mg g^?1. The sorbent presented good stability, reusability, high adsorption capacity, and fast rate of equilibrium for sorption/desorption of selenium (IV) ions.     

Effects of post-harvest stigmasterol treatment on quality-related parameters and antioxidant enzymes of green asparagus (Asparagus officinalis L.)

The effects of immersion of green asparagus spears in stigmasterol solution (0, 0.5 and 1.0 g l^?1, 15 min, 25°C) on weight loss, surface colour, enzyme activities and content of malondialdehyde, total phenol, lignin and chlorophyll were investigated during 40 days of storage at 4 ± 0.5°C. Of the concentrations tested, 0.5 g l^?1 treatment was most effective. Stigmasterol (0.5 g l^?1) treatment significantly reduced colour changes and losses of fresh weight and chlorophyll content. Superoxide dismutase (SOD) and catalase (CAT) activities were maintained higher in stigmasterol-treated (0.5 g l^?1) asparagus, whereas the activity of peroxidase (POD) was significantly reduced. Stigmasterol treatment (0.5 g l^?1) also significantly decreased the content of malondialdehyde (MDA) and increased total phenol content. Accumulation of lignin was positively correlated to activity of guaiacol-POD (r = 0.960, p < 0.01) in stigmasterol-treated (0.5 g l^?1) asparagus. The polyphenol oxidase (PPO) activity decreased and showed a significant negative correlation with the chroma L* value (r = –0.899, p < 0.01) in stigmasterol-treated (0.5 g l^?1) asparagus. It was concluded that stigmasterol treatment (0.5 g l^?1) could inhibit the senescence of green asparagus, and therefore prolong its shelf-life, maintaining the quality of post-harvest green asparagus.     

Fluoride content of soft drinks,nectars, juices,juice drinks,concentrates, teas and infusions marketed in Portugal

A potentiometric method using a fluoride combination ion-selective electrode was validated and used to analyse 183 samples, including soft drinks, juices, nectars, juice drinks, concentrates, teas and infusions marketed in Portugal. The fluoride levels were higher in extract-based soft drinks, juice drinks and juice, with fluoride values of 0.86 ± 0.35, 0.40 ± 0.24 and 0.37 ± 0.11 mg l^?1, respectively. The lowest fluoride concentration was found in infusion samples (0.12 ± 0.01 mg l^?1), followed by teas and carbonated soft drinks with fluoride concentrations of 0.16 ± 0.12 and 0.18 ± 0.07 mg l^?1, respectively. Nectars, concentrates and juice-based drinks had similar fluoride concentrations of 0.33 ± 0.16, 0.29 ± 0.12 and 0.25 ± 0.14 mg l^?1, respectively. The fluoride concentrations in all these samples would only contribute intakes below the acceptable daily intake (ADI = 0.05 mg kg^?1 body weight day^?1), indicating that, individually, these beverages cannot induce fluoride toxicity in the population group of children.     

Chemical Composition, Antioxidant Capacity, and Sensory Quality of Pomegranate (Punica granatum L.) Arils and Rind as Affected by Drying Method

The objective of this study was to evaluate the application of: (1) freeze drying, (2) convective drying (50, 60, or 70 °C), (3) vacuum–microwave drying (240, 360, or 480 W), and (4) a combined method of convective pre-drying and vacuum–microwave finish drying in the processing of pomegranate arils and rind. The quality parameters under study included sugars and organic acids, punicalagins and ellagic acid, total polyphenols, total antioxidant activity, and sensory quality. In general, drying led to a reduction in all studied parameters; however, the behavior of arils and rind was different. Vacuum–microwave drying at 240 or 360 W was the best drying treatment for arils, while rind required freeze drying or soft conditions of convective drying (50 °C). Further research is needed to obtain proper results with convective pre-drying and vacuum–microwave finish drying of arils and rind. With proper selection of the drying protocol, high-quality dried arils will be available for consumers; these arils will be characterized by high contents of fructose (25 g 100 g^?1), phytic acid (2.2 g 100 g^?1), punicalagins (0.57 mg g^?1), total polyphenols (1.6 mg eq gallic acid g^?1), high antioxidant capacity (0.6 mg eq Trolox g^?1), and high intensities of garnet color, sweetness, sourness, and fresh pomegranate aroma. Besides, dried rind with very high contents of active compounds (123 mg g^?1 of punicalagins and 108 mg eq gallic acid g^?1) and high antioxidant capacity (26 mg eq Trolox g^?1) will be also available as functional material.     

Tissue distribution and residue depletion of metronidazole in rainbow trout (Oncorhynchus mykiss)

Tissue distribution and residue depletion of metronidazole (MNZ) was studied in rainbow trout (Oncorhynchus mykiss) following oral administration of MNZ in feed at the average dose of 25 mg kg^?1 body weight day^?1 for 7 days at 11 ± 2°C. The MNZ concentration in feed was 0.25% while daily feed intake was 1% of body weight. The concentrations of MNZ and its main metabolite, hydroxymetronidazole (MNZOH), in fish tissues were determined by LC-MS/MS. The drug was well distributed in tissues with maximum concentrations on day 1 post-administration. At this time, the mean MNZ concentrations in muscle, skin, kidney, liver and gill were 14 999, 20 269, 15 070, 10 102 and 16 467 µg kg^?1 respectively. MNZ was converted into MNZOH with the ratio of MNZOH:MNZ up to 7% in all fish tissues throughout the withdrawal period. This shows that MNZ itself is the main residue in rainbow trout. MNZ was detected at the level close to the decision limit (0.20 µg kg^?1) in muscle, skin and muscle with adhering skin up to 42 days, while in kidney, liver and gill it was up to 28 days post-administration. MNZOH was eliminated more rapidly from fish tissues and it was present in muscle alone up to 21 days. The elimination half-lives of MNZ and MNZOH in rainbow trout tissues were 1.83–2.53 and 1.24–2.12 days, respectively. When muscle without skin was analysed, higher MNZ and MNZOH concentrations were detected, and for a longer period of time, than in muscle with adhering skin. Thus muscle alone could be more appropriate for the effective residue control of MNZ in rainbow trout. For the same reason, it is also essential to ensure direct cooling immediately after sampling, since MNZ and its metabolite degrade in fish muscle and skin stored in non-freezing conditions.     

Characterization of starch and cell walls from mature-green ambarella (Spondias cytherea Sonnerat) and their enzymatic hydrolysis

Juice from mature-green ambarella contains starch, a characteristic detrimental to its visual appearance due to the white sediment formed upon storage. The purpose of this work was to evaluate the effects of starch and cell wall degrading enzymes on juice residual starch and content in soluble sugars. Starch and cell walls from mature-green ambarella fruits were purified and characterized. Starch was found to contain 21.0% amylose, 78.1% amylopectin and 0.9% other minors compounds. Its average granule size was 20 μm. Its thermal characteristics were: temperatures of onset (T _o = 57.8 °C), peak (T _p = 65.6 °C), and conclusion (T _c = 72.6 °C) of gelatinization and the endothermic enthalpy (ΔH _{gelatinisation} = 12.4 J g^?1). Cell walls represented 2.8% of the edible fresh matter and were mainly constituted of highly methylated (HM) pectic substances and cellulose. The amylolytic preparations we tested, AMG^® 300 L and Hazyme^® C, showed similar behaviours in terms of starch hydrolysis and profit of Brix degree obtained. With 200 μg g^?1 of AMG^® 300 L or Hazyme^® C, the degree of amylolysis of coarse ambarella puree was close to 50% and its increased up to 70% with enzymes concentrations higher than 1,000 μg g^?1 (gelatinization at 75 ± 5 °C for 15 min followed by starch amylolysis at 60 ± 5 °C for 15 min). Total hydrolysis of ambarella starch is possible when pectinolysis occurred before amylolysis treatment, probably because of the fluidification of the medium by the pectocellulolytic enzymes. Pectinex^® Ultra SP-L was the most efficient preparation to degrade the ambarella pectins (～80% of cell wall uronides liberated from 120 mg g^?1 of purified cell walls within 1 h at 30 °C, pH 2.7).     

Physicochemical and sensory characteristics of red wines from the rediscovered autochthonous Tintilia grapevine grown in the Molise region (Italy)

Tintilia is an autochthonous grapevine of the Italian Molise region which risked to disappear. However, recently, the production of Tintilia red wines is resuming and in the year 2011 the protected designation origin ‘Tintilia del Molise’ was officially registered. In this work, an analytical characterization of representative red wines from Tintilia grape is reported. A total of 36 different physicochemical variables were determined and discussed, considering those with an estimated coefficient of variation <25 % as more characterizing. These were found to be (mean): density (0.9949); dry extract (34.4 g L^?1) and ashes (3.8 g L^?1); ethyl alcohol (14.2 mL 100 mL^?1), glycerol (9.2 g L^?1) and total higher alcohols (1.7 g L^?1); pH (3.65); the titratable (5.9 g L^?1), fixed (5.4 g L^?1), and salified (2.5 g L^?1) acidity; buffering capacity (52.6 mM/L/pH); total phenols (2,341 mg mL^?1); total flavonols (223 mg mL^?1) and epicathechin (75.0 mg mL^?1); %Red (49.1 %) and %Yellow (43.6 %). Sensory analysis was also performed by professional wine tasters. Finally, the Tintilia results were compared with those of Montepulciano wines. Findings of this analytical study describe the Tintilia red wine as a full-bodied wine; alcoholic; with feeble, but stable acidic profile; rich of phenols, especially flavonols; and finally, with a color balanced between red and yellow pigments.     

Determination of Eugenol in Aquatic Products by Dispersive Solid-Phase Extraction and Ultra-High-Performance Liquid Chromatography-Tandem Mass Spectrometry

A novel procedure, dispersive solid-phase extraction coupled with ultra-high-performance liquid chromatography-tandem mass spectrometry (UHPLC-MS/MS), was developed for the determination of eugenol in aquatic products (shrimp, crab, and carp). Aquatic products were extracted with acetonitrile and primarily purified by dispersive solid-phase extraction with graphitized carbon black as absorbent. The pretreated acetonitrile extract was detected by UHPLC-MS/MS. UHPLC was carried out on Dikma Endeavorsil C₁₈ (30 mm × 2.1 mm, 1.8 μm) column eluted by methanol and water (80:20 v/v) at a rate of 0.30 mL min^?1. Tandem mass spectrometry was performed by electrospray ionization in negative ion mode to identify and quantify eugenol during multiple reaction monitoring. Under optimized analytical conditions, the matrix-matched spiked calibration sample demonstrates good linearity between 5.0 and 500.0 μg kg^?1 with a linear regression coefficient of 0.9996. The average recovery of eugenol from aquatic products is 95.3–103.4% at spiked levels between 5 and 50 μg kg^?1 with a relative standard deviation (n = 6) less than 5.4%. The limits of detection and quantification for eugenol were calculated to be 1.47 and 4.91 μg kg^?1, respectively. In comparison with those reported, the proposed method has advantages in low detection limit, high recovery, and short analysis time, meeting the requirements for the determination of trace eugenol residue in aquatic products.     

Assessment of the dietary intake of propylene glycol in the Korean population

An improved method for the analysis of propylene glycol (PG) in foods using a gas chromatography-flame ionisation detector (GC-FID), with confirmation by GC-MS, was validated by measuring several analytical parameters. The PG concentrations in 1073 products available in Korean markets were determined. PG was detected in 74.1% of the samples, in a concentration range from the limit of detection (n.d., 0.39 μg ml^?1) to 12,819.9 mg kg^?1. The Korea National Health and Nutrition Examination Survey (KNHANES) 2011–2013 reported the mean intake levels of PG from all sources by the general population and consumers were 26.3 mg day^?1 (0.52 mg kg^?1 day^?1) and 34.3 mg day^?1 (0.67 mg kg^?1 day^?1), respectively. The 95th percentile intake levels of the general population and consumers were 123.6 mg day^?1 (2.39 mg kg^?1 day^?1) and 146.3 mg day^?1 (2.86 mg kg^?1 day^?1), respectively. In all groups of the general population, breads were the main contributors to the total PG intake. These reports provide a current perspective on the daily intake of PG in the Korean population.     

Characterization and transformation of the <Emphasis Type="Italic">Opuntia ficus indica</Emphasis> fruits

Opuntia ficus indica fruits have been associated with health effects, due to their protective actions against oxidation. Nevertheless, few studies about processing of Opuntia fruits are available’; therefore, we studied the pulp characteristics and processing of a local variety, for producing beverage nectars. The pulp had an average pH of 5.64, 13.47 °Brix, with total sugars (106 g L^?1), K (1180 mg L^?1), 503.3 µg L^?1 of β carotene, 120 mg L^?1 of total phenolic compounds, 4.9 mg and 46.9 mg L^?1 respectively for betacyanins and betaxanthins and 243.4 mg L^?1 of vitamin C. The formulated nectars with 35% of pulp (N35) and 45% of pulp (N45) had respectively 14 and 15 °Brix. Minor components represent 1109 and 1112 mg L^?1 of K for N35 and N45 respectively, β carotene (318.6 µg and 362.8 µg L^?1), and vitamin C 227 and 231 mg L^?1. We confirmed the stability and acceptability of these beverages after a month of storage, after stability and panel tests. Therefore, we suggest that the pulp processing can be used as a new form of agro industrial utilization of this underutilized fruit.     

Determination of Small Phenolic Compounds in Tequila by Liquid Chromatography with Ion Trap Mass Spectrometry Detection

Tequila is elaborated from Agave tequilana Weber blue variety and it is commercialized at different stages of aging. Chemical composition of this product has often been addressed; however, data on phenolic compounds are scarce. In this work, a high-performance liquid chromatography–electrospray ionization-ion trap mass spectrometry (HPLC–ESI-ITMS) procedure has been established for the determination of 34 small phenolic compounds. The combination of suitable separation conditions with extraction of chromatograms at individual m/z values has enabled for total analysis run of 17 min (11 min separation plus 6 min column cleaning/equilibration) with the detection limits in the range 1.28–75.0 μg l^?1 (0.07–6.1 pmol on-column). Commercial tequilas analyzed included 6 white, 12 rested, and 4 aged. The following acids were found and quantified: gallic, procatechuic, 4-hydroxybenzoic, vanillic, syringic, homovanillic, 3-hydroxybenzoic, ferulic, salicylic, and benzoic. The white tequilas contained fewer compounds and lower total phenolics concentrations (range 36–408 μg l^?1) as compared to the rested and aged liquors (515–4,296 and 2,048–3,249 μg l^?1, respectively). In the latter products, syringic, vanillic, procatechuic, and gallic acids were the most abundant, which indicates that maturation in wooden barrels is the main source of small phenolics in tequila. On the other part, homovanillic acid was found in all tequila types (medians for white, rested, and aged products 82, 153, and 162 μg l^?1, respectively), suggesting that some phenolics may originate from the raw material or might be formed during liquor elaboration.     

Use of 4-chloro-3, 5-dinitrobenzotrifluoride (CNBF) Derivatization and Ultrahigh-performance Liquid Chromatography Tandem Mass Spectrometry for the Determination of 20 Free Amino Acids in Chinese Jujube Date

Ultrahigh-performance liquid chromatography tandem mass spectrometry with 4-chloro-3,5-dinitrobenzotrifluoride (CNBF) derivatization was developed for simultaneous determination of 20 free amino acids in Chinese jujube date. The MS/MS conditions, choice of mobile phase, the extraction process, and matrix effects were studied with a view to a method of optimization. The limits of detection for measurement of the amino acids ranged from 0.8 to 600.0 μg L^?1. The correlation coefficients (r²?≥?0.9947) indicated good correlation between the concentrations of amino acids and the peak areas for the CNBF-derivatives. Recoveries for samples spiked at 25.0, 50.0, and 100.0 mg kg^?1 ranged from 66.3 to 106.6 % (except tryptophan spiked at 25.0 and 50.0 mg kg^?1, which provided recoveries of 61.2 and 60.4 %, and tyrosine spiked at three different concentrations, which provided recoveries of 54.8–58.6 %), with relative standard deviation values of less than 9.1 %.     

Investigation of the presence of prednisolone in bovine urine

Over the past two years low levels of prednisolone have been reported in bovine urine by a number of laboratories in European Union member states. Concentrations vary, but are reported to be below approximately 3 µg l^–1. Forty per cent of bovine urine samples from the Dutch national control plan had concentrations of prednisolone between 0.11 and 2.04 µg l^–1. In this study the mechanism of formation of prednisolone was investigated. In vitro conversion of cortisol by bacteria from faeces and soil, bovine liver enzymes and stability at elevated temperatures were studied. In vitro bovine liver S9 incubation experiments showed a significant 20% decrease of cortisol within 6 h, and formation of prednisolone was observed from 0.2 g l^–1 at t = 0 to 0.5 g l^–1 at t = 6. Under the influence of faeces, the stability of cortisol in urine is reduced and cortisol breaks down within 50 h. Prednisolone is formed up to 4 µg l^–1 at 70°C after 15 h. However, this decreases again to zero after 50 h. With soil bacteria, a slower decrease of cortisol was observed, but slightly higher overall formation of prednisolone, up to 7 µg l^–1 at 20°C. As opposed to incurred urine, in fortified urine incubated with faeces or soil bacteria no prednisolone was detected. This difference may be explained by the presence of natural corticosteroids in the incurred sample. With UPLC-QToF-MS experiments, in urine and water samples incubated with faeces, metabolites known from the literature could be (tentatively) identified as 20β-hydroxy-prednisolone, cortisol-21-sulfate, oxydianiline, tetrahydrocortisone-3-glucuronide and cortexolone, but for all compounds except 20β-hydroxy-prednisolone no standards were available for confirmation. Based on the results of this study and literature data, for regulatory purposes a threshold of 5 µg l^–1 for prednisolone in bovine urine is proposed. Findings of prednisolone in concentrations up to 5 µg l^–1 in bovine urine can, most likely, originate from other sources than illegal treatment with growth promoters.     

Determination and surveillance of hydrocortisone and progesterone in livestock products by liquid chromatography-tandem mass spectrometry

A simple analytical method for the determination of hydrocortisone and progesterone in bovine, swine, and chicken muscle and eggs was developed. Hydrocortisone and progesterone were extracted with acetonitrile and subsequently cleaned-up using an Oasis^® HLB mini-cartridge. The method was validated in accordance with Japanese guidelines and exhibited trueness from 86.6% to 104.3% and precision (relative standard deviations (RSDs) of repeatability and within reproducibility were under 8.7% and 11.7%, respectively). The method was applied to 103 bovine muscle, 137 swine muscle, 69 chicken muscle and 52 egg samples that were commercially available in Tokyo, Japan. The hydrocortisone concentration was 0.9–41.2 µg kg^?1 in all bovine muscle samples, with an average of 7.7 µg kg^?1 and a median of 6.2 µg kg^?1. The progesterone concentration in 50 samples exceeded the limit of quantification (LOQ) and reached a maximum of 95.4 µg kg^?1. Hydrocortisone was also detected in all swine muscle samples at concentrations of 2.0–56.0 µg kg^?1. Its average and median concentrations amounted to 13.1 and 11.3 µg kg^?1, respectively. Twenty-three samples contained progesterone levels surpassing the LOQ, with a maximum concentration of 107.0 µg kg^?1. No chicken muscle samples contained any of the analytes. The progesterone concentration was 15.5–200.0 µg kg^?1 in all egg samples, with an average of 95.4 µg kg^?1 and a median of 90.5 µg kg^?1.     

Analysis of Ochratoxin A in Wine by High-Resolution UHPLC-MS

A method for determination of ochratoxin A (OTA) in wines using a new-solid phase extraction clean-up procedure followed with ultra performance liquid chromatography (UHPLC)-Orbitrap MS based on two scan events (full-scan Fourier transform mass spectrometer [FTMS] and higher energy-induced collision dissociation[HCD] data-dependent MS/MS) in positive ionization mode has been developed. The limit of detection (LOD) was estimated at 0.46 μg l^?1 for white wine, 0.53 and 0.54 μg l^?1 for rosé and red wines, respectively. The limit of quantification (LOQ) was estimated at 1.57 μg l^?1 in white wine, 1.77 and 1.81 μg l^?1 in rosé and red wines. Recovery experiments were carried out with spiked samples at three concentration levels (2, 5 and 10 μg l^?1). The OTA recoveries in spiked white wine samples varied from 69.6 % to 99.8 %, while the recoveries for rosé and red wine samples were in the range of 63.0–110.2 % and 63.6–103.2 %, respectively. Finally, based on the results, it is concluded that the combination of C18 cartridge with conventional particle packed columns and UHPLC LTQ-Orbitrap XL is an appropriate procedure for OTA analysis in wines.     

Biogenic amines in commercially produced Yulu,a Chinese fermented fish sauce

Seven biogenic amines were determined in 35 commercially produced Yulu samples from three provinces of China by pre-column derivatisation with dansyl chloride (Dns-Cl) and high-performance liquid chromatography with fluorescence detection (HPLC-FLD). Putrescine, cadaverine, histamine and tyramine were the major biogenic amines (more than 100 mg kg^?1), while tryptamine, spermidine and spermine were regarded as minor biogenic amines (less than 25 mg kg^?1). Twenty samples contained more than 50 mg kg^?1 histamine (the limit for histamine in seafood products as suggested by the Food and Drug Administration). Twenty-one samples contained more than 100 mg kg^?1 tyramine and 10 contained more than 1000 mg kg^?1 total biogenic amines. This study provided data on biogenic amine levels in Chinese fermented fish sauce. The results suggested that biogenic amine content should be monitored in commercially produced Yulu.     

Mathematical quantification of total carotenoids in Sioma<Superscript>®</Superscript> oil using color coordinates and multiple linear regression during deep-frying simulations

Sioma^® is a variety of red palm oil produced in Ecuador; it is mainly unsaturated, has no flavor, odor, nor cholesterol, and it is GMO-free and free of trans fatty acids. The main objectives of this study were: (a) to study changes in fatty acids, color coordinates, total carotenoids and carotenoid composition during deep-frying simulations; (b) to develop a mathematical model that allows quantification of total carotenoids (antioxidant compounds) using routine color measurements. Two different deep-frying temperatures were assayed 180 and 240 °C. The main fatty acids and carotenoids found in this oil were: (a) oleic, palmitic, and linoleic acids, and (b) α-, β-, and δ-carotenes. During these deep-frying simulations, Sioma^® oil became lighter and more yellowish (L* and b* values increased) and more greenish (a* values decreased); these changes were more evident for higher temperatures. At 180 °C, total carotenoids decreased linearly, from almost 500 mg L^?1, at a rate of 5 mg /kg¹ min^?1; however, at 240 °C the degradation of carotenoids was almost complete after 40 min. Finally, the mathematical models developed using multiple linear regressions allowed an easy and fast quantification of total carotenoids using color measurements.     

Bisphenol A contamination in soft drinks as a risk for children’s health in Italy

Bisphenol A (BPA) was determined in sugary carbonated, non-carbonated and milk-based beverages, through HLPC-fluorescence detection and confirmed by LC-MS/MS, in a selection of brands that are mostly consumed by Italian children. The daily intake was determined through the WHO budget method (BM). BPA was found at detectable levels in 57% of carbonated beverages, in 50% of non-carbonated and in 100% of milk-based beverages. The median concentrations were 1.24 µg l^–1 (range = < LOD–4.98 µg l^–1) in canned carbonated beverages and 0.18 µg l^–1 (< LOD–1.78 µg l^–1) in non-canned carbonated beverages. In non-carbonated beverages, median concentrations were 0.80 µg l^–1 (< LOD–2.79 µg l^–1) and 0.18 µg l^–1 (< LOD–3.58 µg l^–1), respectively, for canned and non-canned beverages; in milk-based products the BPA median concentration was 3.60 µg l^–1 (1.00–17.65 µg l^–1). BPA daily intake from sugary drink consumption in children ranged from 0.008 to 1.765 µg kg^–1 bw day^–1. The median exposure values for the ‘best’ and ‘worst’ cases were 0.16% and 0.47% respectively of the EFSA t-TDI for BPA (4 µg kg^–1 bw day^–1), and 10.59% and 35.30% of the t-TDI when the maximum levels were considered.     

Improvement of wine aromatic quality using mixtures of lysozyme and dimethyl dicarbonate,with low SO2 concentration

The use of sulphur dioxide (SO₂) in the treatment of foodstuffs presents some problems as it could lead to pseudo-allergies in some people. The aim of this research work was to study the addition of different preservative mixtures and their influence on the concentration of volatile compounds and sensorial quality in wine. To do so, vinifications were carried out using Garnacha must to which lysozyme, dimethyl dicarbonate (DMDC) and mixtures of these with SO₂ were added at different doses (25 and 50 mg l^?1). The results were compared with a control sample to which only SO₂ had been added (50 mg l^?1). In general, mixtures of SO₂ with lysozyme and DMDC favoured the formation of volatile compounds in the wines. Wines obtained from the mixtures of lysozyme and DMDC with 25 mg l^?1 of SO₂ had better sensorial quality than the wines obtained with 50 mg l^?1 as the only preservative used.