Broiler production

Three hundred and twenty Ross 308 broilers were raised from 1 to 42 days of age, given feed supplemented with ASO or CSO and 100 mg kg^-1 oregano oil (80 broilers by treatment) and without oregano oil (80 broilers). Broilers were randomly distributed into four treatments with four replications of 20 birds (20 birds × 4 replications × 4 treatments = 320 birds). Diet was formulated according National Research Council (¹⁹⁹⁴); Starter ASO as % (corn 65.55, soybean meal 29.10, ASO 1.17, L-Lysine HCL 0.30) and starter CSO as % (corn 65.61, soybean meal 29.22, CSO 1, LLysine HCL 0.29), for both: calcium bicarbonate (38%) 1.64, dicalcium phosphate (18/21) 1.49, salt 0.30, mineral and vitamin 0.11, DL Methionine 0.30 and coccidiostate 0.05. Grower-finisher ASO as % (corn 71.36, soybean meal 22.19, ASO 2.22, calcium bicarbonate (38%) 1.51, L-Lysine HCL 0.18) and CSO as % (corn 71.79, soybean meal 22.11, CSO 1.85, calcium bicarbonate (38%) 1.52, L-Lysine HCL 0.19, for both: dicalcium phosphate (18/21) 1.30, salt 0.30, mineral and vitamin 0.11, xantophyls 0.60 and coccidiostate 0.05. Experimental diets and water, were provided ad libitum during entire grow-out period. Data of broiler production variables were not reported.

Broiler processing

At the end of growing period, 42 d, four broilers per replication were randomly selected for slaughter according to Mexican Official Standard NOM-033-ZOO-1995 (Diario Oficial de la Federación [DOF], ²⁰¹² (Humane slaughter of domestic and wild animals). Broilers were not fed for a period of 8 h and slaughtered by severing jugular vein and carotid artery, bleeding for 3 min., scalding during 45 s in hot water (45 s, ~64 ºC), defeathering, and manually eviscerating them. Carcasses were chilled in ice-water for 1 h, kept them in coolers with ice, and at 6 h postmortem breast meat was deboned. Skin and visible fat were removed from Longissimus dorsi and then meat was vacuum-packed and stored frozen (-20 °C) for ~1 month. One samples of eight chicken breast meat were obtained from each treatment. Meat was thawed (4 °C) for 24 h, then mixed and ground it (Mill, Model DPA 139, Moulinex, Mexico).

Reagents and standard solutions

Thymol (99.5%) and carvacrol (98%) standards (Catalog T0501 and W224502, Sigma-Aldrich, Mexico, Toluca); methylene chloride 99.9% (Catalog PQ06235, CH₂Cl₂, Fermont, Mexico), sodium chloride (Catalog 3624-01, NaCl, J. T. Baker, State of México, Toluca) and magnesium sulfate (Catalog M7506, MgSO4, Sigma-Aldrich, Japan).

Two solutions, one of thymol and one of carvacrol were prepared (965 μg mL^-1 and 976 μg mL^-1, respectively). Thymol was weighed on an analytical balance (Model AP210S, Ohaus®, Switzerland), and carvacrol was measured with a micro pipette (Hamilton®, USA, Reno Nevada). From these solutions, 100 μL were taken to 1 mL with CH2Cl2 (Kimax®, USA) and from them, 80 μL, 50 μL, 20 μL, 10 μL, 5 μL and 2 μL were also taken with CH₂Cl₂ to 100 μL, these solutions were used to obtain standard curves.

Meat thymol and carvacrol extraction

Meat was ground in a mill (Model DPA139, Moulinex, GSEB Mexican, State of Mexico) for a period of 20 s and mixed by gloved hands for 5 min; 10 g of meat were placed in a polypropylene tube with 10 mL of CH₂Cl₂. Solution was mixed for 2 min and allowed to stand for 30 min. Then, 1.5 g of MgSO₄ and 1 g of NaCl were added. Sample was shaken vigorously and centrifuged (Mod. 5804, Eppendorf®, USA, New York) at 4083 relative centrifugal force (rcf), for a period of 5 min. From the upper layer of sample, 6 mL were taken, then 0.9 g of MgSO₄ was added and solution was again centrifuged (4083 rcf). One mL of the upper layer was concentrated to 100 μL by nitrogen flow, and finally 1 μL was injected into gas chromatograph (GC).

Determination of thymol and carvacrol

To identify and determine thymol and carvacrol amount, a gas chromatograph was used (GC, Hewlett Packard P-6890, USA, California) coupled with a mass spectrometer (MS; Hewlett Packard 7953, USA, California) containing a capillary column Hewlett Packard 5ms® (30 m length, 0.25 mm internal diameter and 0.25 μm film thickness, USA., California) was used as well. Temperature of GC injection port was 150 °C, initial temperature of oven was 60 °C during 5 min, and was increased 20 °C per m to reach 200 °C. Helium was used as a carrier gas (Helio, Infra S.A. de C.V., and State of Mexico, Mexico). MS was operated in scan mode (range m/z: 30 - 550) electron ionization (70 eV). Temperatures of quadrupole, ion source and interface were 150 °C, 230 °C y 220 °C, respectively. One μL of sample was injected into GC by using splitless mode, and mass spectrum obtained were compared to NIST 2.0 (^{National Institute of Standards and Technology, USA}) database. Ions were identified, as well as their retention times and their relative abundance.

Linearity and analytic interval

Four standard curves were obtained with injection of 1 μL of thymol and carvacrol at different concentrations. Two standard curves to determine amount of thymol (1.93 μg mL^-1, 4.82 μg mL^-1, 9.65 μg mL^-1, 19.30 μg mL^-1, 48.25 μg mL^-1 and 77.20 μg mL^-1) and carvacrol (1.95 μg mL^-1, 4.88 μg mL^-1, 9.76 μg mL^-1, 19.52 μg mL^-1, 48.80 μg mL^-1 y 78.08 μg mL^-1) in oregano oil, and two standard curves to determine amount of thymol (from 0.0193 μg mL^-1 to 19.3000 μg mL^-1) and carvacrol (from 0.0195 μg mL^-1 to 19.5200 μg mL^-1) in chicken breast meat were used.

Statistical analysis

Because of lack of normality, concentration of antioxidants in meat was expressed as percentage of maximum value obtained and these data were transformed with arcsine to be analyzed with Kolmogorov-Smirnov test (^{Statistical Analysis Systems, 2000}). Results indicated a trend of normality for thymol and carvacrol (p = 0.064 and p = 0.078, respectively). The main factor oregano oil was significant (p < 0.05). Then, an analysis of variance was performed to test effects of oregano oil: implemented and no; thymol and carvacrol as response variables in meat. Additionally, four treatments (CSO and ASO with and without oregano oil supplementation) were compared using test of Tukey.

RESULTS

Major ions in thymol (91, 135 and 150) and carvacrol coincide with sample and standard at NIST library ions (figure 1 y 2). Retention time was 9.93 min for thymol and 10.07 min in carvacrol, principal ion was 135 and qualifier ions were 150, 91 y 115 for thymol and 150, 91 y 136 for carvacrol (table 1).

Source: Author’s own elaboration.

Figure 1 Thymol characteristic ions #22610, adapted from the library (^{National Institute of Standards and Technology, 2002}). There was coincidence of at least three ions. RA: Relative abundance. 

Source: Author’s own elaboration.

Figure 2 Carvacrol characteristic ions #22723, adapted from the library (^{National Institute of Standards and Technology, 2002}). There was coincidence of at least three ions. RA: Relative abundance. 

Equations used to analyze carvacrol and thymol concentration in oregano oil showed linearity (areas under curve as a function of μg mL-1 of thymol and carvacrol), R2 coefficients were 0.999 and 0.994 respectively, their equations were Y = 2.16 × 10⁶ X + 2.17 × 10⁷ for carvacrol and Y = 2.92 × 10⁶ X + 1.29 × 10⁷ for thymol. Equations used to analyze oregano oil in chicken breast meat showed R2 of 0.987 for carvacrol and 0.970 for thymol, and their corresponding formula were Y = 1.31 × 10⁷ X + 5.44 × 10⁶ and Y = 1.51 × 10⁷ X + 1.04 × 10⁷, respectively. Content of thymol and carvacrol in oregano oil was 30.70 % and 9.36 % (n = 6).

Intervals of concentrations of thymol and carvacrol in chicken breast meat that received CSO were 0 μg g^-1 to 0.9526 μg g^-1 and 0 μg g^-1 to 2.0122 μg g-1, respectively. Oregano oil supplemented to CSO diet increased thymol and carvacrol levels in chicken breast meat (p < 0.05 and p < 0.075). Thymol and carvacrol increased from 0.1465^a to 0.4891^b and from 0.2002^a to 0.7340^b μg g^-1, which represent an increment of 333% and 366% respectively for each metabolite.

Intervals of thymol and carvacrol concentrations in chicken breast meat that received ASO were 0 μg g^-1 to 1.8388 μg g^-1 and 0 μg g^-1 to 1.8867 μg g^-1, respectively. Oregano oil supplemented to ASO diet increased thymol and carvacrol levels in chicken breast meat (p < 0.096 and p < 0.05). Thymol and carvacrol increased from 0.0953^a to 0.5263^b and from 0.0979^a μg g^-1 to 0.6345^b μg g^-1, which represent an increment of 552% and 648% respectively for each metabolite.

Diets with ASO showed low accumulation of thymol and carvacrol, however this accumulation increased when feed was supplemented with CSO and oregano oil (p < 0.05), respectively, compared with ASO oil without oregano oil (figure 3).

Figure 3 Means of thymol and carvacrol concentrations (μg g-1) in chicken breast meat fed on a diet based on ASO or CSO supplemented or not with OO. There was no difference in thymol (x), a, b Means with different letter on the bar graphs are statistically different (p < 0.05). Source: Author’s own elaboration. 

Considering four diets (CSO and ASO with and without oregano oil) a significant effect of CSO with oregano oil on carvacrol concentrations was observed (p < 0.05) compared ASO without oregano oil (figure 3). However, neither effect of soybean oil or interaction of soybean oil with oregano oil were detected.

Amount of thymol in broiler meat fed with CSO and oregano oil in diet was slightly lower respect to those broilers fed with ASO and oregano oil (0.4591 μg g-1 vs., 0.5263 μg g^-1). Amount of thymol in broiler meat fed with CSO without oregano oil was higher compared with those broilers fed with ASO without oregano oil (0.1765 μg g^-1 vs., 0.0953 μg g^-1). Amount of carvacrol in broiler meat fed with CSO and oregano oil in diet also was higher compared with those broilers with ASO and oregano oil (0.1765 μg g^-1, 0.3002 μg g^-1 vs., 0.0953 μg g^-1, 0.0979 μg g^-1). In general, thymol and carvacrol increase in broilers meat when they fed with oregano oil.