Supercritical CO₂ Fluid Extraction and Microencapsulation of Oil from Anchovy (Engraulis mordax) By-Products

Fish by-products

By-products from anchovy processing of a batch caught in August 2021 in FAO area 27, subarea IX Atlantic NE were used as fresh raw material for the extraction. The sample was provided by the company Balistreri Girolamo from lot No. P101, fished by Pescados Getaria S.R.L. on 31 August 2021. The fish by-products, consisting of heads and viscera, were preserved by freeze-drying (Alpha 1-4 LDplus; Martin Christ, Osterode am Harz, Germany) for 75 h at -42 °C and a vacuum of 100 Pa. Before extraction, the freeze-dried material was ground, vacuum-packed in batches of 500 g and stored at -18 °C.

Reagents

Acetone, hexane, 2,2'-azino-bis(3-ethylbenzothiazoline-6-sulfonic acid) (ABTS), potassium persulphate, 6-hydroxy-2,5,7,8-tetramethylchroman-2-carboxylic acid (Trolox), ethanol, methanol, brain heart infusion (BHI) broth, agar, resazurin sodium salt, and NaCl were purchased from Sigma-Aldrich, Merck, Darmstadt, Germany. Whey protein isolate (WPI) and casein (95 % protein) were purchased from Fonterra (Clandeboye, New Zealand).

Supercritical CO₂ fluid extraction

The SFE CO₂ extraction of the lipid phase from the fish by-products was carried out in a pilot extractor (Natex, Prozesstechnologie GesmbH, Ternitz, Austria) as described by Taati et al. (17), at pressure of 30 MPa and temperatures of 40 and 60 °C for 3 h in the presence of a co-solvent (10 % ethanol). The CO₂ mass flow rate was kept constant at max. 20 kg/h. The liquid CO₂ was cooled down to between –3 and –4 °C in the precooler, then pressurised and fed into the extractor. The extractor heating system maintained the constant temperature during extraction, thus ensuring the supercritical state of the solvent. The extracted components were fractionated with the following parameters: fraction S40 at pressure of 15 MPa and temperature of 40 °C and fraction S45 at pressure of 5 MPa and temperature of 21 °C. In each extraction batch, after depressurisation and collection of extracts, a complete recovery of the extract from the walls and the coil of the separators was achieved using a solvent mixture consisting of V(n-hexane):V(acetone)=3:1. After that the solvent was removed from the extracts by vacuum concentration at 40 °C (RVC 2-18 CD; Martin Christ). The extracts were coded according to the extraction temperatures as S40₄₀, S45₄₀, S40₆₀ and S45₆₀, respectively.

The analysis of fatty acids, phytosterols and tocopherols

The method described by Mihalcea et al. (18) was used to determine the content of fatty acids, phytosterols and tocopherols of the obtained extracts and powders. In brief, the first step was to convert the fatty acids into their respective methyl esters (FAMEs) by esterification mediated by methanolic boron trifluoride. A gas chromatographic system coupled with a mass spectrometer (GC-MS) (PerkinElmer Clarus 680), equipped with an Elite-WAX capillary column (30 m×0.25 mm i.d., 0.25 µm film thickness; PerkinElmer, Shelton, CT, USA), using helium as the carrier gas (flow of 1.5 mL/min) was used for the identification of fatty acids. The FAMEs present in the extracts were quantified in selected ion recording mode (SIR), using a 5-point calibration curve prepared from 37-component FAME Mix (Supelco, Sigma-Aldrich, Merck). The phytosterols and tocopherols were determined with GC-MS using the extracts and powders dissolved in n-hexane. The acceptability criteria were met for all the analysed compounds at a correlation coefficient R²>0.99.

Antioxidant activity

The ability of supercritical extracts to scavenge the free radicals of ABTS was assessed based by the protocol described by Lee et al. (19), with some modifications. Briefly, the fish oil was dissolved in acetone at various concentrations from 0.132 to 100 mg/mL. For the assessment of antioxidant activity of microencapsulated extracts, the microcapsules (0.25 g) were dissolved in a mixture of equal volumes of NaCl solution (10 %, m/V) and methanol. After homogenisation and ultrasonication for 30 min, 30 mL of V(hexane):V(acetone)=1:1 were added. After centrifugation (Universal 320R; Hettich, Tuttlingen, Germany) at 6000×g for 10 min at 4 °C, the supernatant was used for the antioxidant activity assay (20). A sample aliquot of 50 µL was mixed with 1.95 mL ABTS solution (λ_{734 nm}=0.70). The absorbances of the samples were determined spectrophotometrically (Libra S22; Biochrom Ltd., Cambridge, UK) after 2 h of storage in the dark. Results were expressed as mmol of Trolox equivalents (TE) per mL based on a calibration curve with Trolox:

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The evaluation of antipathogenic properties

The strains of pathogenic bacteria Escherichia coli ATCC 25922 and Staphylococcus aureus ATCC 25923 were reactivated from stock cultures in BHI broth overnight at 37 °C under aerobic conditions. The antibacterial properties of the SFE CO₂ samples were assessed as the minimum inhibitory concentration (MIC) in 96-well microplates. A volume of 100 µL of different concentrations from 0.066 to 50 mg/mL sample were mixed with 100 µL BHI in each well, then 10 µL of bacterial inoculum (10⁵ CFU/mL) and 10 µL of resazurin (0.015 %, m/V) were added. Positive (solvent with inoculum) and negative (solvent) controls were considered. The samples were incubated for 24 h at 37 °C under aerobiosis, while the microbial activity was determined by monitoring the colour change from dark blue to pink, which indicates the bacterial growth. The minimum inhibitory concentration (MIC) was established as the lowest concentration that inhibited the growth of pathogens without a colour change of the medium (21). The minimum bactericidal concentration (MBC) was determined using the concentrations that inhibited the pathogens by plating 10 µL of samples from the analysed wells on BHI agar. After 24 h of incubation at 37 °C under aerobiosis, the absence of bacterial growth at a specific concentration was defined as MBC (22).

Oxidative stability of fish oil extract using Rancimat analysis

The susceptibility of the fish oil extracts to oxidation was measured using the Rancimat equipment mod 892 (Metrohm LTD, Herisau, Switzerland) according to the manufacturer’s instructions. First, 3 g of fish oil extract were weighed directly into the reaction vessel. Then, the heating block was set at 80 °C, while the air flow through the reaction vessel was adjusted to 20 L/h. During oxidation, the effluent air containing volatile organic acids from the analysed extract samples was collected in the measuring vessel containing 60 mL of distilled water. The induction time (t_induction/h), which characterised the oxidation stability of the oil, was the time until the secondary oxidation products were detected.

Biopolymeric matrix design

In order to design the biopolymeric matrices for microencapsulation of the extracts, 2 g of WPI and 2 g of casein were dissolved in 100 mL of distilled water and allowed to hydrate at 4 °C for 24 h. The pH of the solutions was adjusted to 6.0, while the biopolymeric solutions were divided into two equal parts. One sample was subjected to crosslinking reaction by adding 1 mg of transglutaminase per mg protein. The enzymatic reaction was performed at 40 °C and 120×g for 2 h. After crosslinking, both solutions were heated at 95 °C to inactivate the enzyme and then freeze-dried (Alpha 1-4 LDplus; Martin Christ) for 48 h at -42 °C and a vacuum of 10 Pa. The powders were collected and packed in dark glass tubes. The powders were coded as C (control) and T (transglutaminase-mediated crosslinking variant). Both powders were used in the quenching and microencapsulation experiments.

Fluorescence spectroscopy quenching studies

Fractions S40₆₀ and S45₆₀ obtained from the SFE CO₂ extraction performed at 60 °C and 300 MPa were mixed in a ratio of 1:1 and further used in quenching and microencapsulation studies. The freeze-dried powders were dissolved in Tris-HCl buffer (0.1 M, pH=7.5) at a concentration of 1 mg/mL. In a typical quenching experiment, 100 µL of solution were suspended in 3 mL of Tris-HCl buffer (pH=7.5), followed by successive titration of SFE CO₂ extracts with volumes variyng from 0 up to 0.1 mL. The samples were vigorously shaken and the fluorescence emission spectrum was recorded at the excitation wavelength of 295 nm, while data for the fluorescence intensity (AU) were collected in the wavelength range of 310-420 nm. The emission and excitation slit sizes were set to 10 nm. The quenching parameters, in terms of Stern-Volmer constants, binding constants (K_a) and the number of binding sites were calculated according to Dumitraşcu et al. (23).

Microencapsulation of oil extracts of fish by-products

The biopolymeric matrices (C₀ and T₀) were used to microencapsulate the extracts of fish by-products obtained using SFE CO₂ by complex coacervation and freeze-drying. For microencapsulation, the fractioned extracts were mixed in equal parts and 2 % was added to formulated matrices, followed by homogenisation using an Ultra Turrax mixer (IKA T18 basic; IKA, Staufen, Germany) at 5000×g for 10 min to form a coarse emulsion. The samples were coded C₀ and T₀. The pH of both samples was lowered to 3.75 with 1 M HCl solution at (40±1) °C and stored at 4–6 °C overnight to enable decantation. The coacervates were freeze-dried (Alpha 1-4 LDplus; Martin Christ) at -42 °C under the pressure of 10 Pa for 48 h. The powders were then collected, packed in dark glass tubes and kept in the refrigerator at 4 °C until further analysis. The microencapsulated powders were coded as C_m and T_m.

Hyperspectral dark-field microscopy analysis

Hyperspectral dark-field microscopy (HDFM) analysis was carried out using the CytoViva hyperspectral imaging system (CytoViva Inc., Auburn, AL, USA). The microscope system (BX51; Olympus, Taunton, MA, USA) equipped with a 150 W halogen light source (Fiber-Lite, Dolan-Jenner, Boxborough, MA, USA) and a hyperspectral camera (CytoViva hyperspectral imaging system 1.4. with integrated ENVI 4.8 software) was used to generate the dark-field hyperspectral images (DF-HSI) and hyperspectral profile using 60× objective lenses. DF-HSI were processed with ENVI data analysis software (ENVI 4.8).

Statistical analysis

The reported data are average values of triplicate measurements followed by standard deviations. Statistical analysis was carried out with Minitab 19 software (24), using the analysis of variance (ANOVA) and Tukey’s post-hoc test for 95 % confidence level (p<0.05).

SFE CO₂ extraction yield

It is well known that the density of a supercritical fluid is extremely sensitive to minor changes in temperature and pressure near the critical point. Therefore, in the supercritical CO₂ fluid extraction (SFE CO₂) experiments, a direct correlation between the temperature and CO₂ density was observed, leading to the "crossing" of the solubility isotherms (25). At constant extraction pressure, the solubility of the bioactive compounds in the extracts is improved by increasing the temperature, while their diffusivity increases as the mass transfer intensifies. Consequently, a higher extraction yield of approx. 8 % was achieved at 60 °C compared to 6 % when extracted at 40 °C. Increasing the extraction temperature also has an effect on the fluidity of the lipid phase, leading to more efficient extraction (26). Rodrigues et al. (27) observed similar effects of temperature at constant pressure on extraction yield. These authors used SFE CO₂ to extract oil from sardine by-products (heads and viscera) and obtained extraction yields on dry mass basis of (21.16±0.46) and (24.36±0.53) g/100, using a temperature of 35 °C at a ρ(CO₂)=0.93 g/mL and 75 °C at a ρ(CO₂)=0.91 g/mL, respectively, as extraction parameters. Similarly, Uddin et al. (28) investigated the effects of temperature (35–45 °C) and pressure (15–25 MPa) on oil extraction from squid viscera and obtained the highest lipid phase yield (30 %) at 45 °C, 25 MPa and an extraction time of 2.5 h. Park et al. (29) used SFE CO₂ to extract the lipid phase from mackerel viscera and reported a lower yield at an extraction temperature of 35 °C and a pressure of 25 MPa, which increased from 13 to 16 % when increasing extraction temperature up to 45 °C.

Fatty acid profile of the extracts

Table 1 shows the phytochemical profile of the extracts, in terms of fatty acids, phytosterols and tocopherols. It can be seen that SFE CO₂ extraction at 40 °C allowed to obtain two fractions with a total fatty acid mass fraction on dry mass basis of (712±12) mg/g in S40₄₀ and (658.2±8.4) mg/g in S45₄₀, while at 60 °C, the two corresponding fractions had a total fatty acid mass fraction of (732±10) mg/g in S40 and (630±35) mg/g in S45. The saturated fatty acids (SFA) accounted for 56 % of total fatty acids in each fraction. An increase in the SFA content up to 59 % was observed in fraction S45₆₀. The monounsaturated fatty acids (MUFAs) and polyunsaturated fatty acids (PUFAs) accounted for 44 %, while MUFAs were represented by oleic and palmitoleic acids. Quantitatively, all extracts had significant amounts of stearic and myristic acid, which accounted for 11–13 %. It should be noted that all extracts had significant mass fractions of eicosenoic acid, increasing with the decrease of temperature, ranging between (12.7±0.6) mg/g in S45₆₀ and (24.1±0.2) mg/g in S40₄₀. The lower mass fraction of eicosapentaenoic acid was obtained in S40₄₀ (24.60±0.06), almost the same for S45₄₀ (26.4±0.2) and S40₆₀ (26.8±0.5) mg/g and the highest in S45₆₀ (28.7±1.0) (Table 1).

The representative phytosterol in all fractions was cholesterol, with mass fractions varying from (161.0±2.1) mg/g in S40₄₀ to (274.6±1.9) mg/g in the corresponding S40₆₀ fraction. It can be seen fromTable 1 that fractions S40₆₀ and S45₆₀ contain the highest mass fraction of campesterol of (0.343±0.005) and (0.303±0.006) mg/g, respectively. The same trend was observed for β-sitosterol, with concentrations of (0.610±0.002) and (0.43±0.01) mg/g in S40₆₀ and S45₆₀, respectively. Moreover, all extracts contain cholesta-3,5-dien-7-one and isofucosterol, with the highest mass fraction in S45₆₀ and S40₆₀, respectively. As for tocopherols, only α-tocopherol was detected in fraction S40₄₀ ((1.13±0.06) mg/g).

Therefore, the profile of the extracts highly depended on temperature, pressure, extraction time, solvent flow rate, particle size, water content and the use of co-solvents. However, as it can be seen inTable 1, overall, similar mass fraction of fatty acids was extracted at both tested temperatures, while the mass fraction of phytosterols was higher when extracted at 60 °C.

Karsli et al. (30) studied the fatty acid composition of 15 commercial fish oil supplements and reported that the predominant fatty acids among the SFAs in all fish oil supplements were myristic, palmitic and stearic acids, while the content of eicosapentaenoic acid ranged from 3.51 to 20.51 %. These authors found that docosahexaenoic acid content ranged from 3.28 to 52.42 %. In the fish oil fraction extracted in this study, docosahexaenoic acid was not detected.

Antioxidant activity of the extracts

The ABTS radical scavenging activity of the SFE CO₂ extracts was different based on the parameters used for the supercritical extraction. Consequently, the antioxidant potential varied between c(TE)=0.20 and 0.29 mmol/mL; the highest value was obtained in S45 fraction extracted at 60 °C (0.29 mmol/mL). In general, the antioxidant activity of fish oil is given by the mass fraction of eicosapentaenoic (EPA) and doxosahexaenoic (DHA) acids. Therefore, the increased antioxidant activity of the extracts may be due to the different mass fraction of EPA, ranging from (24.60±0.06) mg/g in S40₄₀ to (28.74±1.04) in S45₆₀. The antiradical potential increased when fish oil and shrimp oil were mixed to obtain 85 % inhibition ratio for ABTS (31).

Antimicrobial potential of the extracts

The fish oil extracts were characterised by their antipathogenic properties against strains of Escherichia coli and Staphylococcus aureus. Both inhibitory and bactericidal effects were observed at a concentration of 66 µg/mL of all analysed samples. Moreover, the SFE CO₂ parameters affected the fatty acid composition of the samples, but no difference was observed in the antibacterial properties. The experimental data are comparable to the results reported by Cardeira et al. (32), demonstrating that the antipathogenic potential of the supercritical fluid extracts of sardine by-products can vary between 70 and 1.56 mg/mL, depending on the extraction parameters. Thus, higher concentrations of the extracts of the sardine by-products were determined to have a bactericidal effect on Staphylococcus aureus ranging from 9.38 to 68.75 mg/mL, while Azmi et al. (33) combined the fish oil with lemon essential oil to suppress the growth of Escherichia coli strain at 250 mg/mL.

Huang et al. (34) reported that ω-3 PUFA showed antimicrobial activity against various oral pathogens, including S. mutans, C. albicans, A. actinomycetemcomitans, F. nucleatum and P. gingivalis. These authors suggested that linoleic acid, γ-linolenic acid, arachidonic acid, palmitoleic acid and oleic acid were responsible for this activity. Therefore, given the prevalence of palmitic, oleic and palmitoleic acids in all the extracted fractions, the antimicrobial activity of the extracts against Escherichia coli and Staphylococcus aureus may be due to the high concentration of these fatty acids, while their cumulative effect should not be excluded.

Oxidative stability of the extracts

The oil with high content of MUFA and PUFA is prone to oxidation, which consists of three successive stages, namely initiation, propagation and termination. In general, the presence of oxygen initiates the oxidative process by reacting with hydrogen atom from the double bonds found in MUFA and PUFA, which results in the formation of highly reactive free radicals with unpaired electrons. The free radicals seek to lose electrons in order to become stable, trying to form paired states with the nearby fatty acids, thus forming new radicals. The chain reaction persists until two radicals combine and thus neutralise their reactivity (35). Oxidative alterations lead to significant changes in oil, such as rancidity, generation of free fatty acids, nutrient loss, undesirable odorus and flavorus, and appearance of toxic compounds. The undesirable secondary metabolites are represented by conjugated dienes, aldehydes, peroxides and polar compounds (36).

The induction time, defined as the time corresponding to the inflection point of the conductivity vs time, was used for quantitative description of the oxidative stability of the oil extracts from fish by-products. The induction time of 3 g of fish oil extract varied from (0.010±0.001) to (0.81±0.04) h at a temperature of 80 °C and an air flow of 20 L/h (data not shown). The S45 fraction obtained at 60 °C was significantly more stable against oxidation ((0.81±0.04) h).

García-Moreno et al. (37) reported an oxidation stability index of 1.61 h, determined by the response surface method, for 6.91 g of partially purified cod liver oil at an air flow of 25 L/h and a temperature of 88.26 °C. Méndez et al. (38) suggested an induction time of 3.2 h for anchovy oil, 1.4 h for hake liver oil and 1.5 h for sardine oil at an air flow of 20 L/h and a temperature of 80 °C for 3 g of partially purified oil.

Fluorescence quenching studies

Prior to microencapsulation, the fluorescence quenching studies were used to evaluate the potential of the fatty acids to bind to the biopolymeric matrices based on WPI and casein without (C₀) and with (T₀) transglutaminase-mediated crosslinking.Fig. 1 shows the fluorescence emission spectra of the two matrices.

Fig. 1 Fluorecence emission spectra of the isolated whey protein and casein matrices without (C0) (grey dotted line) and with (T0) transglutaminase-mediated crosslinking (black dotted line)

Fig. 1 shows that the maximum emission wavelength (λ_max) for sample C₀ was recorded at 358 nm, while crosslinking led to a significant 8.5-nm redshift up to 366 nm. The redshift is due to the dipole-dipole interactions resulting from crosslinking. Consequently, the λ_max redshift implies the displacement of the hydrophobic regions in the more polar environment, which allows the molecules to unfold and to bind different ligands from the extracts. Moreover, Taheri-Kafrani et al. (39) suggested that the redshift in wavelength and the increase in the fluorescence intensity at the λ_max is due to the Trp transfer to a more hydrophilic environment and the increase in polar interactions.

In addition, the interactions between biopolymeric matrices and ligands were studied by successive titration with fractions S40₆₀ and S45₆₀, respectively, by increasing the volume of the extracts from 0 to 100 μL. The fluorescence quenching effect could be observed in both samples. Therefore, with the increased volume of the extract, the fluorescence intensity of the protein solutions gradually decreased, with a higher quenching effect in the case of crosslinked matrices (T₀). When titrating with fraction S40₆₀, the quenching effect reached a maximum of ~47 % with sample T₀ compared to ~39 % with sample C₀, while in quenching studies with S45₆₀ a maximum effect was found in sample C₀ (~43 %) compared to 41 % in sample T₀. The successive titration with the two extracts caused significant 8.5-nm redshift in sample C₀ and 2.5-nm shift in sample T₀. These results indicate a higher molecular flexibility in C₀ than structural rigidity due to the crosslinking in T₀. Therefore, the addition of the extract T₀ allowed to preserve the crosslinked structure, causing only rearrangements of the hydrophobic subdomain to which the tryptophan residues belong. The binding constants (K_a) and number of binding sites (N) were calculated for the predominant fatty acids from the extracts and are shown inTable 2.

The data inTable 2 show that palmitic, palmitoleic and oleic acids had a single class of binding sites on both C₀ and T₀. Different values of K_a were estimated for fractions S40₆₀ and S45₆₀. For example, the K_a value for the binding of palmitic acid was higher when fraction S40₆₀ was bound to C₀ ((19.2±0.2)·10³ L/mol) than when fraction S45₆₀ was bound to T₀ ((18.2±0.5)·10³ L/mol). The same trend was observed for palmitoleic acid, with higher K_a values of (40.4±0.4)·10³ L/mol and (43.6±0.4)·10³ L/mol, respectively. Given the predominance of β-lactoglobulin in WPI, Simion (Ciuciu) et al. (40) proposed the presence of two lipophilic ligand binding sites in the protein: a central hydrophobic β-barrel and a superficial pocket. It can be assumed that fatty acids bind to the superficial pocket, while other molecules bind to the calyx due to the intrinsic flexibility of the conjugates. Therefore, it can be assumed that the WPI and casein complexes act as protein-based multiligand carriers that enable the binding of small molecules.

Microencapsulation of the fish oil obtained with supercritical extraction

Table 3 shows the phytochemical profile of microencapsulated powders (C_m and T_m). It can be observed that C_m allowed the microencapsulation of a higher amount of fatty acids and phytosterols, especially palmitic, palmitoleic, myristic and stearic acids and cholesterol. Total fatty acid mass fraction of (81.2±0.9) and (68.8±0.8) mg/g was found in C_m and T_m, respectively. The main fatty acids in both powders were saturated fatty acids (SAT), representing 60 % of the total, while MUFAs and PUFAs accounted for 40 %. The sample C_m contained (11.1±0.1) mg/g PUFAs, from which ω-3 were predominant (60 %), followed by ω-6 (39 %) and ω-11 (26 %). The PUFA mass fraction in T_m was (9.6±0.6) mg/g, from which ω-3 were predominant (48 %), followed by ω-6 (31 %) and ω-11 (21 %). However, the T_m sample had a higher mass fraction of α-tocopherol.

Sànchez et al. (41) encapsulated krill oil in gum Arabic in a ratio of 1:4 and reported that the spray-dried microcapsules contained 21 % of eicosapentaenoic and docosahexaenoic acid of the total fatty acids, with low ω-6/ω-3 and SAT/unsaturated fatty acid ratios. In our study, the SAT/MUFA ratio was 1:2.38 and 1:2.41 in C_m and T_m, respectively, while SAT/PUFA ratio was 1:4.4 in C_m and 1:6.36 in T_m.

The antioxidant activity (ABTS) of the microencapsulated powders was in the range b(TE)=0.69–4.13 mmol/g, with the highest value for T_m of (4.13±0.03) mg/g. Our results confirm the findings of similar studies from the literature that involved transglutaminase, inulin and soy protein isolate to improve the microencapsulation efficiency of fish oil (42). Fan et al. (43) showed that the conjugated menhaden oil with epigallocatechin gallate, whey protein isolate and genipin improved the ABTS scavenging activity, leading to a decrease of the IC₅₀ values for ABTS, from more than 2000 µg/mL for the native whey protein isolate, up to 83.50 µg/mL for the crosslinked microcapsules.

Dark-field hyperspectral images and hyperspectral profile of the powders

The microscopic details of the microencapsulated powders are shown inFig. 2. The crosslinking reaction mediated by transglutaminase (T₀) causes aggregation/agglutination of the protein matrices (WPI and casein) so that irregular formations appear, larger than those in the control sample (C₀). The encapsulation pattern of the lipid component in the C is in the form of irregular scales with dimensions between 10 and 50 μm. Xiong et al. (44) suggested the presence of some raisin-like structures due to a low ratio between the protein shell and the lipid core. It is likely that the ratio between the lower protein content of the matrix and the temperatures near freeze-drying causes the shrinkage of the micelles and the appearance of irregular shapes. Spectral mapping showed in red all the unique elements in T_m, with the fish oil trapped in the biopolymer matrix. The mean spectral comparison of T_m vs T₀ is shown inFig. 3.

Fig. 2 Dark-field hyperspectral images (DF-HSI) of the isolated whey protein and casein matrices: a) without (C0) and b) with transglutaminase-mediated crosslinking (T0), and microencapsulated extract of anchovy by-products: c) without (Cm) and d) with transglutaminase-mediated crosslinking (Tm)

Fig. 3 Mapping of the spectral profiles of control sample (T0; white) vs microencapsulated fish oil sample (Tm; red) using CytoViva HSI optical microscopy

An inversion of the spectra is evident. If the polymer matrix generates a peak at 450 nm, the presence of fatty acids from the fish oil inverts the curve and generates an absorption maximum between 550 and 650 nm, probably due to the interactions between the components of the fish oil and the proteins during microencapsulation (44).