ID 1333 - Hydroksytyrozol, oleuropeina

PL: Hydroksytyrozol, oleuropeina
EN: Hydroxytyrosol simple phenol; oleuropein complex polyphenol belonging to ai secoiridoids
Pdf: polyphenols in olive

Oświadczenie (4)

Oświadczenie (2)

1. Charakterystyka żywności / składnika

The food constituent that is the subject of the health claims is polyphenols (e.g. hydroxytyrosol and oleuropein complex) in olive (olive fruit, olive mill waste waters or olive oil, Olea europaea L. extract and leaf).
The conditions of use specify 200 mg/day of polyphenols (ID 1638, 1882, 2865), 2-15 mg per day of hydroxytyrosyl or oleuropein complex (ID 1638, 1639, 1696), and 250-500 mg of an Olea europaea L. extract standardised to 4-23% oleuropein (ID 3467, 3468, 3779, 3781).
Polyphenols comprise a very wide group (several thousands of compounds) of plant secondary metabolites including flavonoids, isoflavonoids, phenolic acids, proanthocyanidins and other tannins, and lignans with different biological activities. The major polyphenols in olive oil are phenolic acids (e.g. hydroxytyrosol and tyrosol), secoiridoids (e.g. oleuropein) and lignans (e.g. pinoresinol). Table olives typically contain hydroxytyrosol, tyrosol, caffeoylquinic acid, verbacoside, luteolin and rutin. Hydroxytyrosol, a major polyphenol typically present in olives, is also present in olive mill waste water. In nature, hydroxytyrosol is found in olives in the form of its elenolic acid ester, oleuropein. These polyphenolic compounds can be measured in foods by established methods.
Total polyphenols are usually expressed as gallic acid equivalents (GAE), but other phenolic compounds such as catechin/epicatechin or caffeic acid have also been used for standardisation. This standardisation refers to the traditional spectrophotometrical measurement of total polyphenols using the Folin-Ciocalteau method (Singleton and Rossi, 1965), which is based on reducing capacity. The method is not specific for polyphenols because other reducing compounds such as ascorbic acid, sugars and proteins will also be included in the quantification, thus leading to an overestimation of the actual polyphenol content. The total polyphenol content assessed with this method is not suitable for characterisation of polyphenols in foods.
The Panel considers that polyphenols (e.g. hydroxytyrosol and oleuropein complex) in olive (olive fruit, olive mill waste waters or olive oil, Olea europaea L. extract and leaf) can be characterised by their content of hydroxytyrosol and its derivatives (e.g. oleuropein complex).
The Panel considers that the food constituent, polyphenols in olive (olive fruit, olive mill waste waters or olive oil, Olea europaea L. extract and leaf) standardised by their content of hydroxytyrosol and its derivatives (e.g. oleuropein complex), which is the subject of the health claims, is sufficiently characterised in relation to the claimed effects.

2.1. Ochrona cząsteczek LDL przed uszkodzeniem oksydacyjnym (ID 1333, 1638, 1639, 1696, 2865)

The claimed effects are “reduces oxidative stress”, “antioxidant properties”, “lipid metabolism”, “antioxidant activity, they protect body cells and LDL from oxidative damages”, and “antioxidant properties”. The Panel assumes that the target population is the general population.
In the context of the proposed wordings, the Panel assumes that the claimed effects refer to the protection of low-density lipoprotein (LDL) particles from oxidative damage.
Reactive oxygen species (ROS) including several kinds of radicals are generated in biochemical processes (e.g. respiratory chain) and as a consequence of exposure to exogenous factors (e.g. radiation and pollutants). These reactive intermediates can damage molecules such as DNA, proteins and lipids if they are not intercepted by the antioxidant network which includes free radical scavengers such as antioxidant nutrients.
The Panel considers that protection of LDL particles from oxidative damage may be a beneficial physiological effect.

3.1. Ochrona cząsteczek LDL przed uszkodzeniem oksydacyjnym (ID 1333, 1638, 1639, 1696, 2865)

The vast majority of the references provided for the scientific substantiation of this claim included narrative reviews, human intervention studies, animal studies and in vitro experiments on food/food constituents other than olive polyphenols, and/or on effects other than protection of lipids, including LDL particles, against oxidative damage. The latter include references on blood pressure, vasodilation, allergenicity, inflammation, immunotherapy, antimicrobial properties, renal disorders, gut disorders, postprandial absorption, carbohydrate and lipid metabolism, obesity, diabetes, and oxidative damage to molecules (e.g. DNA and proteins) other than LDL particles. The Panel considers that no conclusions can be drawn from these references for the scientific substantiation of the claimed effect.
In a randomised, single-blind, cross-over trial, 25 healthy male and female smokers consumed olive oil with low (3 mg/day) or high (21.6 mg/day) phenolic content for three weeks (Moschandreas et al.,
2002). Total plasma resistance to oxidation, and the ferric reducing ability of plasma, as markers of the antioxidant capacity of plasma, concentrations of protein carbonyl as a marker of protein oxidation, and malondialdehyde (MDA) and lipid hydroperoxides measured with a kit assay as markers of lipid peroxidation, were assessed. The Panel notes that no valid markers of lipid (or LDL) peroxidation were used in this study, and considers that no conclusions can be drawn from this study for the scientific substantiation of the claimed effect.
In a randomised, sequential cross-over acute study, 21 hypercholesterolaemic volunteers (16 female) received two breakfasts with olive oil (phenolic content 400 mg/kg olive oil, i.e. 14 mg/day or 80 mg/kg olive oil, i.e. 2.8 mg/day) (Ruano et al., 2005). Postprandial plasma concentrations of lipoperoxides (LPO, colorimetric assay) and 8-epi-prostaglandin-F2α (immunoenzymatic assay) were obtained at baseline and 2 hours after consumption of the meal. The Panel notes that this was an acute study, that the phenolic composition of the olive oils used is not sufficiently characterised, that LPO measured by a colorimetric assay is not a reliable marker of lipid peroxidation, and that no markers of peroxidation of LDL particles were assessed. The Panel considers that no conclusions can be drawn from this study for the scientific substantiation of the claimed effect.
In a multicentre (six centres in Finland, Denmark, Germany, Italy and Spain), randomised, cross-over, controlled human intervention study, olive oils with high (366 mg/kg olive oil, i.e. 8.0 mg/day; hydroxytyrosol content 63.5 mg/L, tyrosol 24.4 mg/L, and oleuropein derivatives 327.2 mg/L as measured by HPLC) moderate (164 mg/kg olive oil, i.e. 3.6 mg/day, hydroxytyrosol content approx. 28.5 mg/L), and low (2.7 mg/kg olive oil, i.e. 0.1 mg/day, no hydroxytyrosol) phenolic content were consumed (25 mL/day) by 200 male subjects for three weeks (Covas et al., 2006b). The phenolic composition and content of the olive oils used in this study are reported by de la Torre-Carbot et al. (2010). Oxidative damage to lipids was assessed by measuring plasma-circulating oxidised LDL (oxLDL, immunoenzymatic assay), plasma total F2α-isoprostanes (HPLC, stable isotope-dilution and MS), plasma C18 hydroxy fatty acids (GC-MS) and serum LDL cholesterol un-induced conjugated dienes. Hydroxytyrosol and tyrosol excretion in urine were measured to assess compliance. A significant linear decrease in biomarkers of lipid peroxidation (conjugated dienes, hydroxy fatty acids and oxLDL) was observed in association with the increasing phenolic content of the olive oils. oxLDL significantly increased with the low phenolic-containing olive oil, and significantly decreased with the medium and high phenolic-containing olive oils (p<0.014). No consistent change was observed in plasma total F2α-isoprostanes. The Panel notes the large sample size of this multicentre study, the sufficient characterisation of polyphenols in the olive oils used, the use of valid biomarkers to assess lipid peroxidation, and in particular the peroxidation of LDL particles, and the dose-dependent response observed between the intake of polyphenols in olive oil and the decrease in LDL peroxidation.
A subsample from the study by Covas et al. (2006b) consisting of 36 males recruited from the six centres participating in the trial and consuming olive oils with high (366 mg/kg olive oil, i.e. 8.0 mg/day, hydroxytyrosol content 63.5 mg/L) or low (2.7 mg/kg olive oil, i.e. 0.1 mg/day, no hydroxytryrosol) phenolic content for three weeks (25 mL/day) were further investigated regarding the effect of specific metabolites in olive oil phenols on human LDL lipid composition and peroxidation (de la Torre-Carbot et al., 2010). The concentrations of hydroxytyrosol monosulfate and homovanillic acid sulphate (but not of tyrosol sulphate) in LDL particles significantly increased (p<0.05), whereas the concentration of circulating markers of lipid peroxidation, including LDL particles (oxLDL, conjugated dienes and hydroxy fatty acids), significantly decreased (p<0.05) after ingestion of olive oil with high phenolic content. The Panel notes the inverse relationship between the concentrations of phenolic metabolites in LDL particles and the degree of LDL peroxidation.
A controlled, double-blind, cross-over, randomised, clinical intervention using three olive oils (refined, common and virgin, 25 mL/day) with increasing phenolic concentrations (from 0 to 150 mg/kg, i.e. up to 3.3 mg/day of which 3 % tyrosol, 7 % hydroxytyrosol, 42 % oleuropein aglycones and 14 % ligstroside aglycones) was conducted in 30 healthy male volunteers for three weeks
(Marrugat et al., 2004). Urinary tyrosol and hydroxytyrosol were measured as markers of compliance. In vivo plasma oxLDL (measured by a sandwich ELISA procedure using the murine monoclonal antibody, mAb-4E6) significantly decreased (p=0.006 for linear trend), and ex vivo resistance of LDL to oxidation significantly increased (p=0.012 for linear trend) with the phenolic content of the olive oils administered. The Panel notes the use of a valid biomarker to assess LDL peroxidation (oxLDL), the inclusion of a supportive marker (ex vivo resistance of LDL to oxidation), the sufficient characterisation of polyphenols in the olive oils used, and the dose-dependent response observed between the intake of polyphenols in olive oil and the decrease in LDL peroxidation.
Twelve healthy men participated in a double-blind, randomised, cross-over study in which three olive oils with low (10 mg/kg, i.e. 0.2 mg/day), moderate (133 mg/kg, i.e. 2.9 mg/day), and high (486 mg/kg, i.e. 10.7 mg/day) phenolic content were consumed for four days (Weinbrenner et al., 2004). Percentages of individual phenolic compounds present in the olive oil were approximately 6.5 % hydroxytyrosol, 5.5 % tyrosol, 40 % oleuropein aglycones, 26 % ligstrosid aglycones, 12 % luteolin and 3 % apigenine as measured by HPLC. Consumption of olive oils significantly decreased plasma oxidised LDL (oxLDL measured by the ELISA method) and MDA in urine (HPLC-UV), and significantly increased glutathione peroxidase activity (p<0.05 for linear trend for all) in a dose- dependent manner in relation to the phenolic content of the olive oil administered, whereas plasma 8- oxo-prostaglandin F2α (HPLC and stable isotope dilution MS) was not affected. The Panel notes the use of a valid biomarker to assess LDL peroxidation (oxLDL), the sufficient characterisation of the olive oil polyphenols, and the dose-dependent response observed between the intake of polyphenols in olive oil and the decrease in LDL peroxidation.
In an acute, cross-over study design, olive oils with high (366 mg/kg, i.e. 13.2 mg/day), moderate (164 mg/kg, i.e. 5.9 mg/day), and low (2.7 mg/kg, 0.2 mg/day) phenolic content were consumed (40 mL/day) by 12 male subjects (Covas et al., 2006a). Outcome variables were assessed in blood samples at 2, 4 and 6 hours after consumption of the olive oils. Total phenolic compounds in LDL increased at postprandial state in a direct relationship to the phenolic compounds content of the olive oil ingested (p<0.05). A significant decrease in plasma oxidised LDL (oxLDL, measured by a sandwich ELISA procedure using the murine monoclonal antibody mAb-4E6) was observed at 4 and 6 hours post-prandial, in a dose-dependent manner in relation to the phenolic content of the olive oils administered (p=0.43 and p=0.28 for linear trend, respectively). No dose-response relationships were observed between the phenolic content of the olive oils and linear trends for changes in total plasma 8-iso-prostaglandin F2α (measured using HPLC-MS) at any time point. The Panel notes that this is an acute study which provides insufficient characterisation of the olive oil polyphenols. However, the Panel assumes that these oils were the same used in another study by the same authors published the same year, with exactly the same phenolic content (Covas et al., 2006b), and notes the dose-dependent response observed between the intake of polyphenols in olive oil and the decrease in LDL peroxidation.
A few studies addressed the bioavailability of polyphenolic compounds in olive showing that the absorption of olive oil phenolics is probably larger than 55-66 mol%, and that the absorption of hydroxytyrosol is dose-dependent, suggesting that olive oil phenolics are absorbed from the intestine, that tyrosol and hydroxytyrosol are incorporated in lipoprotein fractions, and that hydroxytyrosol is excreted in urine as glucuronide conjugate (Bonanome et al., 2000; de la Torre-Carbot et al., 2010; Edgecombe et al., 2000; Miro-Casas et al., 2003; Visioli et al., 2001; Vissers et al., 2002). The incorporation of phenolic compounds from olive oil in LDL particles has been proposed as the mechanism by which olive phenolics may protect LDL particles from peroxidation.
The Panel notes that most of the human intervention studies described have been conducted in males (aged 20-60 years) using a wide range of daily doses of polyphenols in olive oil (from 0.1 to 10.7 mg/day expressed as total polyphenolic content measured spectrophotometrically), and with a content of hydroxytyrosol and its derivatives measured by HPLC up to 10 mg/day. The Panel also notes that only studies on polyphenols present in (and consumed with) olive oil have been provided for
the substantiation of the claimed effect, and that no data are available for other food matrices (e.g. leaf tea or tea extract).
The Panel notes that polyphenols naturally occurring in olive oil were shown to significantly decrease the amount of circulating oxidised LDL particles in vivo in a dose-dependent manner in one large (n=200, Covas et al., 2006b) and three small scale (12 subjects, (Weinbrenner et al., 2004), 30 subjects, (Marrugat et al., 2004), and 36 subjects, (de la Torre-Carbot et al., 2010), respectively) human intervention studies, one of which was short-term (four days, Weinbrenner et al., 2004). A dose-dependent decrease in the amount of circulating oxidised LDL particles in vivo was also found in one small scale (n=12) acute post-prandial study (Covas et al., 2006a). The lowest daily dose of hydroxytyrosol and its derivatives (measured by HPLC) in olive oil which showed a significant effect on in vivo LDL peroxidation was 5 mg (Covas et al., 2006b). A significant decrease in relation to consumption of olive oil polyphenols was also reported for serum LDL un-induced conjugated dienes (Covas et al., 2006b; de la Torre-Carbot et al., 2010) and for ex vivo resistance of LDL to oxidation (Marrugat et al., 2004), which can be considered as supportive markers to assess peroxidation of LDL particles. The Panel also notes that a significant decrease in plasma C18 hydroxy fatty acids (Covas et al., 2006b; de la Torre-Carbot et al., 2010) and urinary MDA (Weinbrenner et al., 2004) was observed following consumption of olive oil polyphenols, but that olive oil polyphenols do not appear to have an effect on F2α-isoprostanes (Covas et al., 2006a; Covas et al., 2006b; Weinbrenner et al., 2004).
In weighing the evidence, the Panel took into account that a well conducted and powered study, and two smaller-scale studies, showed a dose-dependent and significant effect of olive oil polyphenol consumption (for three weeks) on appropriate markers of LDL peroxidation (oxLDL), that these results were supported by one short-term and one acute study, and by supportive markers of LDL peroxidation (conjugated dienes, ex vivo resistance of LDL to oxidation) going in the same direction, and that evidence for a biologically plausible mechanism by which olive oil polyphenols could exert the claimed effect has been provided.
The Panel concludes that a cause and effect relationship has been established between the consumption of olive oil polyphenols (standardised by their content of hydroxytyrosol and its derivatives) and protection of LDL particles from oxidative damage.

4.1. Ochrona cząsteczek LDL przed uszkodzeniem oksydacyjnym (ID 1333, 1638, 1639, 1696, 2865)

The Panel considers that the following wording reflects the scientific evidence: “Consumption of olive oil polyphenols contributes to the protection of blood lipids from oxidative damage.”

5.1. Ochrona cząsteczek LDL przed uszkodzeniem oksydacyjnym (ID 1333, 1638, 1639, 1696, 2865)

The Panel considers that in order to bear the claim, 5 mg of hydroxytyrosol and its derivatives (e.g. oleuropein complex and tyrosol) in olive oil should be consumed daily. These amounts, if provided by moderate amounts of olive oil, can be easily consumed in the context of a balanced diet. The concentrations in some olive oils may be too low to allow the consumption of this amount of polyphenols in the context of a balanced diet. The target population is the general population.

Warunki i możliwe ograniczenia stosowania oświadczenia

Consumption of at least two soup-spoonfuls (23 g) of olive oil a day for at least three weeks, in the context of a diet low in saturated fatty acids