3.1. Classification of Hams According to Meat Type and Processing, Using Color-Measurement, FT-IR Spectra-Interpretation, and Textural-Image Analysis Methods
Color is a significant indicator of meat quality, because it is one of the most important features influencing the evaluation of meat by the consumer [
2,
15]. In the food industry, the most popular numerical color space system is the CIE L*, a* and b*.
Results of color measurement are shown in
Table 1. Regarding turkey hams, the smoking process led to a reduction (
p < 0.05) of lightness (L*) and of total color change (DE*) values and an increase of hue (h) value. The smoking treatment, however, did not affect yellowness (b*) (
p > 0.05).
Concerning pork hams, color measurements on the surface of boiled and smoked ones revealed no statistical differences (p > 0.05) between the average color values L*, C*, h, ΔE*, a* and b*. In contrast, roasted process led to an increase (p < 0.05) of chroma (relative saturation, C*) of redness (a*), of yellowness (b*) and of total color change (DE*) values.
Color values L*, h, a* and b* showed significant differences (
p < 0.05) between pork- and turkey-ham samples of the same processing. Specifically, turkey-ham slices revealed almost double b* values and nearly half a* values compared to pork hams. Dvorak et al. [
16] reported that redness is the most important color parameter in assessing the quality of pork ham. Moreover, Garcia-Esteban et al. [
17] reported that a* is the most sensitive parameter, featuring the red color and color stability of meat products. Furthermore, turkey-ham slices were characterized by significantly higher (
p < 0.05) lightness (L*) and hue (h) values compared to pork ones, with turkey fillets having almost twice the hue value (h) of the pork.
Pattern-recognition methods were employed using textural features from the hams’ images, in order to highlight an initial grouping of the samples, depending on meat type (pork and turkey) and processing (boiled, smoked, or roasted), and to gain suitable information for the selection of the most appropriate features for the potential separation among groups.
A scatter diagram (
Figure 2a) showed that boiled turkey hams were separated from smoked ones with 95.5% overall discrimination accuracy, via the features of standard deviation (SD), a* and gray-level nonuniformity (GLNU). SD is computed from the image histogram and it quantifies textural inhomogeneity. Feature a* is a color feature and it quantifies image redness/greenness. GLNU is a second-order statistic [
13,
18] and it quantifies unevenness in the distribution of image structures throughout the grey levels. This three-feature combination was used in the design of a high-performance pattern-recognition system that correctly classified 32 out of 34 boiled turkey slices (two slices were wrongly assigned to the smoked-turkey class), and 31 out of 32 smoked turkey slices (one slice was wrongly classified to the boiled-turkey class). As shown in
Figure 2a, smoked-turkey slices, in comparison with boiled-turkey slices, had higher GLNU but lower a* and SD values.
As shown in the scatter diagram of
Figure 2b, the three types of pork hams were separated with 98% overall precision. This was realized employing three features, one feature from the color attributes, chroma (C*), and two textural features, angular second moment (ASM) from the co-occurrence matrix, and long-run emphasis (LRE) from the run-length matrix. This three-feature combination provided a high-precision pattern-recognition system that correctly classified all but one boiled-pork slice. ASM quantifies image homogeneity, and LRE indicates the presence of large structures in the image. ASM was higher in boiled-pork slices, LRE was higher in smoked-pork-ham slices, and chroma C* was higher in roasted-pork slices.
Concerning the meat type, the scatter diagrams of
Figure 3a,b showed the adequate separation between boiled turkey and pork hams, as well as between smoked turkey and pork hams via hue (h) and redness (a*) values, with 100% overall precision. Therefore, these results suggest that the meat type altered the color parameters, allowing for clear distinction.
Ham slices were further analyzed using FT-IR spectroscopy in the midinfrared region (4000–500 cm
−1). All spectra (
Figure 4) showed characteristic absorption bands associated with proteins, triglycerides, fatty acids, and carbohydrates. Characteristic bands of the spectra have been evaluated based on the literature data [
9,
10,
11,
12,
19,
20].
Specifically, the wide absorption band at 3500–3200 cm
−1 is due to O-H and N-H symmetric stretching vibration of alcohols and amide/proteins, respectively. The band from 3100 to 3020 cm
−1 is related to the vinyl C-H stretching vibrations of lipids. The strong absorption bands at 2950–2920 and 2852 cm
−1 corresponds to methyl and methylene groups’ asymmetric and symmetric stretching vibrations of lipids, respectively. The characteristic band at 1744 cm
−1 is assigned to C=O stretching of carbonyl group of triglycerides’ ester bond. Moreover, the strong absorption band at 1627 cm
−1 is ascribed to C=O stretching vibration of amides, whereas the band at 1541 cm
−1 to the combined vibration of the amino group (N-H) bending with the C-N stretching of proteins. According to Yu [
21], the bands in the 1600–1700 and 1500–1560 cm
−1 regions represent the protein primary features and are characterized as amide I and amide II, respectively. The weak absorbance band at 1530 cm
−1 is related to the COO– asymmetric stretching vibration of fatty acids and proteins. The band at 1467 cm
−1 is due to C-H bending of alkyl chain methylene of lipid moieties. The weak bands at 1450 and 1395 cm
−1 correspond to C-H asymmetric and symmetric stretching vibrations, respectively, of protein moieties. The strong band from 1170 to 1154 cm
−1 is attributed to C-O stretching of proteins and triglycerides. Phospholipids and nucleic acids are characterized by P=O asymmetric and symmetric stretching vibrations at 1240 and 1083 cm
−1, respectively. The medium band at 1117 cm
−1 is ascribed to C-H bending and deformation of fatty acids. The bands from 1040 to 1020 cm
−1 are assigned to carbohydrate moieties and, in the case of meat products, it might indicate the presence of glycogen. The medium bands at 966 and 870 cm
−1 are attributed to the out-of-plane deformation of CH=CH
trans double bond and para-disubstituted aromatic derivatives, respectively.
From the interpretation of the FT-IR spectra of the ham samples (
Table 2) (boiled turkey, smoked turkey, boiled pork, smoked pork, and roasted pork), the most interesting findings concerning the type of meat and processing are summarized below.
The spectra of pork samples, irrespective of processing type, showed absorbance bands of higher (
p < 0.05) intensities at 2950–2920, 2852, and 1744 cm
−1 than the spectra of the turkey samples. Therefore, it seems that pork hams have a higher (
p < 0.05) lipid content compared to turkey hams. Moreover, since the band at 3100–3020 cm
−1 was associated with the vibration of the olefin group, it could be estimated that turkey hams were characterized by higher content of unsaturated fatty acids than the pork hams. An important indication confirming the above finding was the presence of the band at 717 cm
−1 only in the turkey-ham samples, which is associated with the out-of-plane bending vibration of the –CH=CH– group in unsaturated fatty acids [
22]. Furthermore, pork hams have higher (
p < 0.05) protein content compared to turkey hams, as the spectra of pork hams exhibited higher (
p < 0.05) intensities at 1450, 1395, and 1170–1154 cm
−1 than the ones of the turkey samples. In this sense, the adsorption bands at 1627 and 1541 cm
−1, which are characteristics of the protein presence, showed a higher (
p < 0.05) signal in the spectra of pork hams than in those of the turkey ones. Furthermore, according to Yu [
21], if the amide I adsorption band, which characterizes the protein secondary structure, is located in the region, 1648–1658 and 1620–1640 cm
−1 are associated with the α-helix and the β-sheet protein structure, respectively. Therefore, the major protein-structure content of pork- and turkey-ham samples is β-sheet. The spectra of the turkey hams presented significantly (
p < 0.05) higher intensities at 1040–1020 cm
−1 compared to the pork hams, which is indicative of higher carbohydrate content.
According to the findings of Wong et al. [
23], when the ratio of C=O absorption at 1740 cm
−1 to the P=O absorption at 1240 cm
−1 is between 1.9 and 2.3, then the P=O bond is attributed to phospholipids, while outside this ratio to nucleic acids. In the spectra of all samples studied, the ratio was found to be approximately 1.3–1.4, which proves, on the basis of the above, that the P=O bond is attributed to nucleic acids.
High positive Pearson correlations were observed among lightness (L*), hue (h), and yellowness (b*), and the intensity values at 3100–3020 cm−1 (0.915, 0.847, and 0.712, respectively; p < 0.01) as well as the intensity values at 1040–1020 cm−1 (0.913, 0.971, and 0.769, respectively; p < 0.01). This result indicates a possible relationship among the above color parameters and the presence of olefin groups and high carbohydrate content, respectively. Moreover, significant positive correlations were determined between redness (a*) and the intensity values at 1627 and 1541 cm−1 (0.957 and 0.952, respectively; p < 0.01), which characterize the protein presence.
Concerning the type of processing, minor differences were identified from the interpretation of the FT-IR spectra of the ham samples. Therefore, only the spectra of the boiled-turkey hams showed significantly (p < 0.05) higher intensities than the smoked ones at the bands relating to lipid and protein content. Moreover, smoked hams, irrespective of meat type, presented significantly (p < 0.05) higher intensities at 966 cm−1 compared to the other hams, indicating the increase of trans double bonds.
3.2. Classification of Hams According to Shelf Life Using Color Measurement, FT-IR Spectra Interpretation, and Image-Texture Analysis Methods
In order to monitor the shelf-life of the studied ham samples towards chemical deterioration at a temperature of 4–6 °C, a comparative analysis was performed during storage in refrigeration for twenty days (
Figure 5a,b and
Figure 6a–c).
The most interesting findings from the FT-IR spectra interpretation are listed below. The intensities at 1744 and 1170–1154 cm
−1, which are attributed to the C=O and the C-O stretching of carbonyl and ether bonds of triglycerides, respectively, were significantly (
p < 0.05) decreased from day 10 until day 20 of refrigerated storage in all studied samples. Moreover, the intensities at 2950–2920, 2852, and 1117 cm
−1, corresponding to the methyl and methylene groups’ stretching and deformation vibrations of fatty acids were significantly (
p < 0.05) increased during the same storage period. These results probably indicate that refrigerated storage caused the degradation of triglycerides and the increase of free fatty acids as hydrolysis products. Therefore, refrigeration storage may inhibit the activity of triglycerol acyl hydrolases that catalyze lipid hydrolysis, releasing free fatty acids, and di- and monoglycerides [
24].
The combined (p < 0.05) decrease in absorbance at 3100–3020 cm−1 with the increase in absorbance at 1117 cm−1 probably indicates the reduction of unsaturated fatty acids ratio over the saturated.
Another interesting finding was that the significant (p < 0.05) decrease of the intensities at 1627 and 1541 cm−1 was related to C=O stretching vibration and to the combined N-H bending vibration with the C-N stretching of proteins, respectively, from day 10 until day 20 of refrigerated storage in all studied samples. This result may be associated with a partial protein rupture.
Intensity at 966 cm
−1, which is related to the out-of-plane deformation of C-H of trans-olefins, was significantly (
p < 0.05) increased after 10 days of refrigerated storage in all studied samples. According to Marina et al. [
25], the absorbance at 967 cm
−1 increased as oxidation progressed, being an indicator of oxidative stability.
Refrigeration storage had a significant effect on color parameters of the final products (
Table A1,
Table A2,
Table A3 and
Table A4). It is apparent that, for all samples, the L* parameter was altered significantly throughout the preservation period. More specifically, the L* parameter of turkey hams presented an initial decrease from day 3 to day 6, stabilization until day 12, and an additional decrease from day 12 to day 15. Moreover, L* values of pork hams showed a similar trend, presenting a significant decrease at 15 days of storage. The hue (h) angle, which is related to a primary color (red, yellow, green, or blue) or the combination of two of them, varied with an opposite trend during the preservation period, increasing in turkey samples and decreasing in pork ones. Therefore, even though turkey hams revealed almost double h values compared to pork ones, with refrigeration storage, they tended to acquire more similar values. Yellowness (b*) increased significantly after 9–12 days of storage for all studied samples. Redness (a*) varied depending on meat type during storage. Therefore, a* values of turkey hams showed slight or significant increase, whereas a* values of pork hams significant decrease, throughout the preservation period. Color changes could be attributed to the dehydration of meat surface and to oxygen penetration into the tissues. Based on FT-IR spectra interpretation results, the color changes of hams could be the result of the oxidative degradation of lipids. According to Leygonie et al. [
26] these color changes are undesirable and not reversible, deteriorating ham quality. An important conclusion resulting from the color measurement was that color parameters showed significant alterations after 9 days of refrigeration storage.
Nonlinear regression analysis was employed on the computed features of boiled- and smoked-ham slices of pork and turkey in order to investigate variations in image texture with storage time. In boiled-pork ham (
Figure A1), significant changes with time were observed in the kurtosis and mean-intensity features. Kurtosis values increased, while mean intensity values decreased with storage time. Kurtosis evaluates the shape of gray-level distribution. High kurtosis values indicate thin distributions around the mean with broad tails (leptokurtic), while low kurtosis values refer to distributions that are broad around the mean with light tails (platykurtic). Since kurtosis values increased with storage time, this indicates an increasing number of outlier pixels, i.e., large numbers of pixels with intensities spreading throughout the image gray-level spectrum. This redistribution of gray levels of pixels contributes to the loss of continuum of meaningful structures within the image. In boiled-pork ham, mean intensity value was found to decrease, indicating that boiled-pork-ham images turned darker with increasing storage time.
In smoked-pork ham (
Figure A2), there were four features that significantly varied with storage time: kurtosis, mean intensity, correlation, and gray-level nonuniformity. Kurtosis increased, signifying a decrease in textural continuum, and mean intensity increased, indicating smoked-pork-ham slices turned brighter. Correlation evaluates the level of linear dependencies among the gray levels of the image. The feature attained high values when there were meaningful structures present in the image. We found that correlation decreased with storage time in smoked-pork-ham slices. This indicates that structures in the smoked-pork slices broke down with storage time, losing textural continuum. Gray level nonuniformity was found to increase with storage time. The feature indicates that image structures are more unevenly distributed among the gray levels, probably due to redistribution of gray levels, resulting in the loss of structural continuum with storage time.
In boiled-turkey ham (
Figure A3), with increasing storage time, image contrast increased, while image mean intensity and correlation decreased. This indicates that, with advancing storage time, boiled-turkey-ham images attained higher local contrast, their structural continuum deteriorated, and images became darker. Three more features from the co-occurrence matrix varied significantly with storage time: difference entropy, difference variance, and inverse-difference moment. Difference entropy evaluates variation of image lack of order. It was found to increase with storage time. Difference variance quantifies variation in image heterogeneity. It was found that the feature increased with storage time. Inverse-difference moment evaluates image homogeneity. It was found that it decreased with increasing storage time. The findings from the last three features indicate that, in boiled-turkey-ham slices, texture lost its homogeneity and structural order. Three more features, emanating from the run-length matrices, i.e., gray-level nonuniformity, run-length nonuniformity, and run percentage were found to increase significantly with storage time. Increase in gray-level nonuniformity indicates that structures were more unevenly distributed in the image gray levels. Increase in run-length nonuniformity indicates that image structures were more unevenly distributed in magnitude. Increase in run percentage indicates that nonlinearity in image structures increased. These findings indicate that, in boiled-turkey-ham slices, image structures lost continuum and local linearity, gray-level composition of image structures disintegrated, and sizes of structures changed. Similar findings were observed in smoked-turkey-ham slices (
Figure A4) but for mean intensity, which seemed not to vary significantly with storage time.
Observing
Figure A1 and
Figure A2, it seems that textural-feature values of pork hams showed significant alterations after 9 days of refrigeration storage, while feature values of turkey hams presented continuous changes with storage time (
Figure A3 and
Figure A4).