COMPOSITIONS BASED ON ACTIVE PRINCIPLES OF PLANT ORIGIN HAVING EYE PROTECTION ACTION

The present invention relates to nutraceutical or pharmaceutical compositions based on a combination of cyanidin-3-O-glucoside and verbascoside, or extracts of plant origin enriched in the two active ingredients, with a protective action on eyesight.

In recent years, polyphenolic compounds of plant origin have been of particular interest due to their capacity of acting as protectors with respect to sight disorders due to aging and in the treatment and/or prevention of visual pathologies. Among these, numerous studies relate to anthocyanoside compounds, pigmented substances present in various plants in nature ((bilberries, mulberries, blackberries, oranges, black potatoes, black corn, etc.).

Between the '60s and '80s, various scientific studies were conducted on the beneficial effects produced by the intake of food rich in anthocyanins on the wellbeing of sight (Kalt W. et al., 2010).

The results obtained so far, even if sometimes controversial, have shown how these substances can act on some molecular biochemical mechanisms involved in vision and in different visual degenerations.

In the in vitro study carried out by Matsumoto H. et al. (Matsumoto H. et al., 2003), anthocyanoside compounds, having different chemical structures, were evaluated in the regeneration of rhodopsin, a photosensitive protein present in the rods which, on undergoing a conformational variation from the 11-cis-retinal form to the 11-trans-retinal form, activates a cascade of biochemical events and mediators responsible for visual nerve impulses. From the results obtained by Matsumoto H. et al., it has been observed that among the various anthocyanoside compounds, giucosylated forms, such as cyanidin-3-O-glucoside, induce a greater increase in rhodopsin regeneration kinetics, resulting in improved visual ability and adaptation in the dark (Nakaishi H. et al., 2000). Furthermore, numerous in vitro studies conducted using cell models have demonstrated the strong protective effect of anthocyanoside compounds, obtained from various food sources, from damage induced by oxidative stress on retinal pigment epithelial cells (Wang Y. et al., 2015; Liu Y. et al., 2012; Sun M. et al., 2015).

It is known, in fact, that the retinal pigment epithelium (RPE) exerts functions essential for the retinal activity and is particularly sensitive to the damage induced by the radical species of oxygen produced in ocular tissues, with consequences that can cause various eye diseases such as senile degenerative maculopathies, retinal detachment or retinal dystrophies.

The effect produced by anthocyanoside compounds and, in particular, cyanidin-3-O-glucoside on the prevention and treatment of ocular degenerations, also seems to be correlated to the protective action exerted by these compounds on another important ocular tissue, retinal ganglion cells.

The in vitro and in vivo study carried out by Tanaka et al. (Tanaka J. et al., 2013) showed that treatment with an anthocyanoside extract from black rice containing cyanidin-3-O-glucoside, is able to inhibit the overproduction of cellular radical species induced by tunicamycin treatment, and increase cell viability by inhibition of the caspase-3 activation process, with a consequent reduction in potential cell death due to various ocular pathologies such as glaucoma, diabetic retinopathy, retinal ischemia (Kalt W. et al., 2010).

There are studies, however, that report conflicting data in literature. The effect of anthocyanosides on vision, in fact, seems to be dose dependent.

According to Levy Y. & Glovinsky Y. in a study on 16 healthy volunteers, the administration of tablets at a dosage of 12, 24 and 36 mg of anthocyanosides extracted from blueberry berries did not show any effects on improving the central vision of the mesopic or scotopic visual field. Analogously, in a study on 18 healthy volunteers, Zadok D. et al. confirmed that the administration of 12 mg and 24 mg of anthocyanosides of blueberry did not result in visual improvements. The lack of effect was also confirmed by Muth E. R. et al. in a double-blind study on contrast sensitivity and night vision after administration of anthocyanosides (160 mg of blueberry extract titrated at 25%).

Verbascoside is a polyphenolic compound, belonging to the family of phenipropanoids, present in various plant species, such as mullein and olive trees, with known anti-inflammatory, antioxidant, antimicrobial, antiviral activities, etc.

Recently, only a few in vivo and clinical studies have evaluated the potential protective actions of this bioactive compound on vision. The results obtained have shown that this compound is capable, after oral administration, to protect the tissues and ocular fluids from natural oxidative processes and, moreover, topically to promote the cicatrization of lesions induced on guinea pig corneal epithelia (Mosca M. et al., 2014; Ambrosone L. et al., 2014). The authors of the present invention have now identified a surprising synergistic action between cyanidin-3-O-glucoside and verbascoside in terms of protective action and increased cell viability of retinal epithelial cells.

An object of the present invention relates to nutraceutical or pharmaceutical compositions comprising cyanidin-3-O-glucoside and verbascoside or plant extracts, each enriched in cyanidin-3-O-glucoside and verbascoside as active ingredients together with physiologically acceptable adjuvants and/or excipients, for use in the prevention and/or treatment of sight disorders or pathologies affecting the retina.

The two active ingredients or their enriched plant extracts present in the compositions or in the combinations according to the invention, are in a mutual weight ratio verbascoside:cyanidin 3-O-glucoside ranging from 1:1 to 1:20, preferably in a mutual weight ratio ranging from 1:4 to 1:10.

A further object of the present invention relates to a combination of cyanidin-3-O-glucoside and verbascoside or plant extracts enriched in cyanidin-3-O-glucoside and verbascoside for simultaneous, sequential or separate use in the prevention and treatment of sight disorders or diseases affecting the retina.

The invention relates in particular to a combination of cyanidin-3-O-glucoside and verbascoside, wherein the two active ingredients or two enriched plant extracts are administered in combination maintaining a mutual weight ratio ranging from 1:1 to 1:20, preferably in a mutual weight ratio ranging from 1:4 to 1:10.

The plant extracts enriched in cyanidin-3-O-glucoside are preferably selected from extracts of black rice (Oryza sativa L.), red orange (Citrus sinensis L. Osbeck), black mulberry (Moms nigra L.), blackberry (Rubus ulmifolius S.) and black corn (Zea mays L.) or another plant source containing anthocyanoside substances.

According to the present invention, hybrid varieties of black rice can also be used.

According to the present invention, a plant extract enriched in cyanidin-3-O-glucoside refers to a extract having a content of cyanidin-3-O-glucoside ranging from 2-30% parts by weight (w/w).

The plant extracts enriched in verbascoside are preferably but not limitedly selected from extracts of mullein (Verbascum L.), Olive tree (Olea europaea L.) or another plant source containing verbascoside. According to the present invention, a plant extract enriched in verbascoside refers to an extract having a verbascoside content ranging from 0.2-20% parts by weight (w/w). The enrichment of plant extracts in the respective active ingredients is preferably effected by means of nano-ultrafiltration techniques or with the use of adsorbing resins.

The plant extracts enriched in verbascoside or cyanidin-3-O-glucoside according to the invention can be in liquid or powder form. (i.e. dried or freeze-dried).

Said sight disorders affecting the retina can be selected from the group consisting of alterations in night vision, glare, retinal photosensitivity, whereas said visual pathologies affecting the retina can be selected from the group consisting of maculopathies, retinopathies, retinal degenerations due to aging and dystrophies. Said visual pathologies are preferably retinitis pigmentosa, diabetic retinopathy or senile degenerative maculopathy. The combinations or compositions according to the invention can obviously be used as adjuvants for the treatment of said visual pathologies in association with ad hoc drug therapies.

Said compositions or combinations are preferably suitable for oral administration, even more preferably in the form of oral solutions, oral emulsions, oral suspensions, capsules, tablets or powder. For oral administration, the preferred total concentration range of the two extracts can vary from 10% to 90% by weight of the final composition.

The active ingredients present in the compositions or combinations according to the invention can be administered orally within the following daily dosage ranges in one or more administrations:

cyanidin-3-O-glucoside: from 30 mg/day to 500 mg/day, preferably 100 mg/day

verbascoside: from 10 mg/day to 500 mg/day, preferably 25 mg/day.

The present invention is now described for illustrative but non-limiting purposes according to some preferred embodiments with particular reference to the attached figure, in which:

FIG. 1 shows the histogram relating to the percentages of cell viability (MTT assay) of retinal pigment epithelial cells after treatment with H₂O₂and in the presence of cyanidin-3-O-glucoside extract, verbascoside extract, alone and combined with each other.

By way of example, but not limitative of the present invention, some examples of the compositions according to the invention and their uses are provided hereunder.

EXAMPLE 1
Preparation of Extracts Enriched in Cyanidin-3-O-Glucoside and Verbascoside

An exemplary extractive process is described hereunder for obtaining an anthocyanoside plant extract enriched in cyanidin-3-O-glucoside:

Step a: (extraction from black rice or black corn): maceration of the whole grain of rice or corn or pigmented pericarp alone obtained by abrasion of the outer surface of the grain with an aqueous or hydroalcoholic solution (10-60%) at acid pH with hydrochloric acid (0.1% HCl), at room temperature. The maceration process can also be effected with the aid of a Soxhlet extraction system.

Step b: (extraction from black rice or black corn): second extraction on the same vegetable matrix with a new extraction solvent, to favour the recovery of the active substances present.

Step c: recovery and concentration under vacuum of the extracts obtained at a temperature not higher than 50-60° C. until the complete elimination of the organic solvent.

Step d: (purification of anthocyanoside substances from red orange juice or blackberry juice or mulberry juice or extract obtained from step c from black rice or black corn): purification of the anthocyanoside compounds by passing the juice or liquid product obtained from step c on an ultrafiltration system (optimal cut off 10,000 daltons) and subsequent concentration by passage on a nanofiltration system (suggested cut off 200 daltons).

Step e: isolation of the anthocyanoside substances by passage of the product obtained from step don macroporous adsorbent resin Amberlite XAD-7 or another similar adsorbent resin, by elution with an aqueous or hydroalcoholic solution (50-90%) at acid pH with hydrochloric acid (0.1% HCl).

Step f: subsequent drying by spray-drying or freeze-drying using maltodextrin or another technological support.

The anthocyanoside extract obtained has a content of cyanidin-3-O-glucoside, its main constituent, ranging from 2-30% w/w.

An exemplary extraction process is described hereunder for obtaining a polyphenolic plant extract enriched in verbascoside:

Step a: (extraction from vegetable matrix): maceration of the fresh or dried matrix with an aqueous or hydroalcoholic solution (10-60%), acid with a pH value of around 4-5, at a temperature of 40-60° C. The maceration process can also be effected with the aid of a Soxhlet extraction system.

Step b: second extraction on the same vegetable matrix with a new extraction solvent, to favour the recovery of the active substances present.

Step c: recovery and concentration under vacuum of the extracts obtained at a temperature not higher than 50-60° C. until the complete elimination of the organic solvent.

Step d: purification of the flavonoid compounds by passage of the liquid product obtained on macroporous adsorbent resin Amberlite XAD-7 or another similar adsorbent resin, by elution with an aqueous or hydroalcoholic solution (30-70%) at acid pH with hydrochloric acid (0.1% HCl).

Step e: concentration under vacuum of the extracts obtained at a temperature not higher than 50-60° C. until the complete elimination of the organic solvent and subsequent drying by spray-drying or freeze-drying, with the use of a suitable technological support, e.g. maltodextrin.

The polyphenolic extract obtained has a consent of verbascoside, its main constituent, ranging from 0.2-20% w/w.

EXAMPLE 2

Formulation Examples

Different formulations for oral use (tablets, capsules, powders) are exemplified hereunder, comprising the combination of the anthocyanoside extract (cyanidin-3-O-glucoside) and polyphenolic extract (verbascoside) with a different mutual weight ratio.

I) Formulation Examples for Oral Use

- CAPSULES (ratio between verbascoside:cyanidin-3-O-glucoside extracts 1:4)

COMPONENTS
% w/w

Polyphenolic extract (verbascoside)
2.5%

Anthocyanoside extract (cyanidin-3-O-
10%

glucoside)

Lactose
Up to 100 g

Preparation Method

Mixing the extracts with lactose, according to the rule of geometric dilutions and then proceeding with distribution in capsules.

COMPONENTS
% w/w

Polyphenolic extract (verbascoside)
43.7%

Anthocyanoside extract (cyanidin-3-O-glucoside)
43.7%

Vegetable magnesium stearate
0.9%

Silicon dioxide
1.6%

Talc
0.9%

Arabic gum
0.9%

Citric acid
1.0%

Coating agents:

Modified pregelatinized starch
3.5%

Talc
2.2%

Lacquer rubber
0.9%

Glycerol
0.7%

Preparation Method

Mixing the anthocyanoside and polyphenolic extracts and proceeding, according to the art, with fluid-bed granulation, using a granulating solution acidified with citric acid and Arabic guru. Mixing the granulate with anti-caking agents (talc, silicon dioxide, magnesium stearate); subjecting the mixture to compression with the use of a tablet press. Applying a first coating of the tablets with lacquer rubber and talc and a subsequent coating with modified pregelatinized starch, glycerol and talc.

- POWDER FOR ORAL USE (ratio between verbascoside:cyanidin-3-O-glucoside extracts 1:20)

COMPONENTS
% w/w

Polyphenolic extract (verbascoside)
1%

Anthocyanoside extract (cyanidin-3-O-
20%

glucoside)

Silicon dioxide
0.67%

Sucralose
0.17%

Maltodextrin
Up to 100 g

Preparation Method

Mixing the extracts with maltodextrin, according to the rule of geometric dilutions and then proceeding with distribution in sachets or bags.

EXAMPLE 3
Study on the Protective Activity of Anthocvanoside Extracts (Cyanidin-3-O-Glucoside) and Polyphenolic Extracts (Verbascoside) using an In Vitro Cell Model

The objective of the study was the in vitro evaluation of the protective action exerted by anthocyanoside plant extracts (cyanidin-3-O-glucoside) and polyphenolic extracts (verbascoside) individually and combined with each other on retinal pigment epithelial cells.

The experimental protocol provided for the use of an in vitro cell model capable of evaluating the protective action exerted by the extracts on retinal epithelial cells subjected to a state of oxidative stress.

Materials and Methods

The retinal pigment epithelium (RPE) consists of a layer of pigmented cells, firmly attached to the underlying choroid and to the overlying visual retinal cells, with various functions essential for maintaining the physiological anatomical-functional conditions of the retina.

Various visual pathologies, such as retinitis pigmentosa, retinal degenerations due to the physiological aging process, maculopathies and dystrophies, derive and can originate from an altered function of the retinal pigment epithelium.

The ARPE-19 cell line (ATCC CRL-2302) is a line of human retinal pigment epithelium (RPE) cells used as an in vitro study model.

These cells were cultured in a 5% CO₂atmosphere at 37° C., in Dulbecco's Modified Eagle's Medium (DMEM)-HAM F12, with the addition of 10% (v/v) of Fetal Bovine Serum (FBS) and 1% (v/v) of penicillin/streptomycin antibiotics.

Cell Viability Assay

The RPE cells were trypsinized, counted in a hemocytometer, plated on wells for the MTT assays and, after 24 hours of incubation in a 5% CO₂atmosphere at 37° C., they were treated for 1 hour with each extract used individually or in a combination, according to what is indicated in Table 1 hereunder. 0.3 mM of H₂O₂were subsequently added for 24 hours at 37° C.

TABLE 1

Sample
Composition
Concentration

C
Cyanidin-3-O-glucoside extract
100 μg/ml

V
Verbascoside extract
25 μg/ml

A/V
Cyanidin-3-O-glucoside/verbascoside
125 μg/ml

extract

A: Cyanidin-3-O-glucoside extract;

V: verbascoside extract;

C/V: combination of the two extracts

The cell viability was measured, after treatment with H₂O₂, by the colorimetric assay of tetrazolium salts, which evaluates the capacity of the cells of reducing, by means of mitochondrial succinate dehydrogenase, the bromide of 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium (MTT). The MTT enters the cells and passes into the mitochondria where it is reduced to a colored and insoluble product, formazan. To make the color visible, the coloured formazan granules are solubilized by the addition of DMSO. The MTT-cleavage reaction requires the complete integrity of the cell and is proportional to the degree of metabolic activity of the same. The assay provides that after incubation of the cells for three hours, in 5% CO₂at 37° C., with 20 μl of the solution of the tetrazolium salt, solubilized in medium (5 mg/ml), and 180 μl of medium, the supernatant be removed and 100 μl of DMSO added. The optical density (O.D.) was subsequently measured at a wavelength of 570 nm with a microplate spectrophotometer (Titertek Multiscan, Flow Laboratories). The cell viability was expressed as percentage of optical density with respect to the non-treated control. The experiment was carried out in triplicate for each sample.

Results

The data obtained from the MTT assays showed that both the anthocyanoside extract (cyanidin-3-O-glucoside) (C) and the polyphenol extract (verbascoside) (V) are able to protect, when used individually, the viability of human retinal pigment epithelial (RPE) cells from the damage induced by treatment with H₂O₂(Table 1).

The treatment of RPE cells with both extracts used in combination (C/V), causes a significant increase in the cell viability, with a synergic-type effect (see FIG. 1 and Table 1). Table 2 hereunder shows the average cell proliferation values (MTT) expressed as cell viability percentage with respect to the control (CTRL) and cell viability percentage (RPE) vs treatment with H₂O₂.

TABLE 2

cell viability %

vs control

RPE cells
(viability % vs H₂O₂)

Treatment with H₂O₂
45.47 ± 3.74

Cyanidin-3-O-glucoside extract (C)
63.47 ± 2.91

(18 ± 1.35)

Verbascoside extract (V)
55.03 ± 2.70

(9.6 ± 4.03)

Cyanidin-3-O-glucoside/verbascoside
87.13 ± 3.18*

extract (C/V)
(41.7 ± 6.7)*

*p < 0.05 vs C and V

EXAMPLE 4
Clinical Study on Healthy Volunteers

In the present double-blind randomized study, the in vivo results are illustrated, obtained after oral administration of a preparation containing purified cyanidin 100 mg and verbascoside 25 mg to verify the improvement in sight, the retinal sensitivity and contrast vision.

Patients

50 healthy volunteers were enrolled, emmetropes (spherical equivalent 0.50 dioptres) between the ages of 30 and 40, 20 men and 20 women (average age 36 years) selected after ascertaining the absence of eye diseases with the following tests:

- Slit lamp examination of the anterior segment and of the fundus
- Applanation tonometry
- Refraction in miosis and cycloplegia
- Natural visual acuity at 6 meters with Sbisá computerized optotype with a brightness of 400 lux
- Contrast visual acuity at 6 meters with Pelli-Robson charts Sbisá computerized optotype with a brightness of 400 lux.

The patients were divided into two groups: 20 men and 20 women. The 20 women patients were respectively divided into two randomized groups, group A and group B.

The 20 patients of group A were used as control and were therefore treated with a capsule preparation containing lactose (inert substance) for 4 weeks.

The 20 patients of group B were treated for 4 weeks with a capsule preparation containing cyanidin-3-O-glucoside (100 mg) and verbascoside (25 mg).

Materials and Methods

The two groups of patients were subjected to three groups of tests.

- 1) visual tests. Natural and contrast visual acuity before and after treatment to assess possible changes in visual acuity.
- 2) test for resistance to visual stress. Measurement of glare time and recovery time after glare to evaluate the retinal capacity of adaptation to visual stress.
- 3) retinal sensitivity test. Examination of the central visual field with white and blue-yellow stimulus.

Test for Resistance to Visual Stress

In order to evaluate their visual capacity after light stress, the patients were subjected to the glare test and recovery test after glare provided by the Ministry of Health for the issue of driving licenses.

The following tests were performed 4 weeks before and after the administration of the composition according to the invention:

- glare test with a standardized Sbisá optotype
- recovery test after glare with a standardized Sbisá optotype.

The visual acuity tests were performed with standardized computerized Sbisá optotype at a distance of 6 meters with a Snellen Chart with brightness of 400 lux at 50 cm from the screen.

Glare Test with Standardized Sbisá Optotype

Two lamps placed at the sides of the optotype with 900 lumen light emission (obtained with two 20 watt lamps), to allow additional illumination to that of the 400-500 Lux optotype measured at 50 centimeters.

After switching on the two lamps, the subject is asked, in binocular vision, to recognize at least 50% of the letters present from 1/10 onwards.

Recovery Test after Glare with Standardized Sbisá Optotype

The following were used for performing the test: Sbisá computerized optometry with illumination of 300 lux at 50 centimeters. Light source producing an illuminance of 200 lux at 20 cm when in an orthogonal position with respect to the luxmeter sensor (i.e. appropriate light pen).

The test is conducted monocularly on the two eyes with the possible correction of the ametropia and the best result is taken into consideration for the assessment. After adaptation to the dark for a maximum time of one minute, one eye is covered and the light source is placed at 3 cm from the contralateral eye for ten seconds, inviting the subject to stare at it. Once the high beam source has been removed, the lights are turned on again and the subject is asked to instantly read the line corresponding to 4/10, in a maximum time of 30 seconds, the line is considered read if 50% of the letters are recognized in the time established. If the relative line is not read in the maximum time provided, the procedure is repeated in the same way on the other eye.

The eye that has achieved the best result in a time not exceeding 30 seconds, is considered (specific licenses group 2, Ministry of Health). Table B indicates the time necessary for reading the line corresponding to 4/10 measured with a stopwatch and expressed in seconds from the beginning of the test.

Retinal Sensitivity Test

In order to assess possible changes in the retinal sensitivity before and after 4 weeks of treatment, the following visual field tests were also performed (Octopus 311 TOP G32 strategy, 30 degrees central).

- white light field of vision
- blue-yellow field of vision

In both types of field of vision, only the MS (mean sensitivity) was analyzed, which is the arithmetic mean of the differences between the sensitivity values measured in the various points of the visual field and the normal values corrected for age.

It was decided to perform both visual fields in order to evaluate the different responses of the photoreceptors to the white and blue-yellow stimulus. The use of the blue-yellow perimetry derives from the fact that numerous studies have shown that the S cones, specific for blue, are those affected earlier in glaucoma. The white light, in fact, saturates the responses of all the cones: the defect in response of a single cone system can be compensated by that of the others. The blue-yellow field of vision, viceversa, offers an isolation of 15 dB, the blue yellow ganglion system must therefore lose 15 dB of sensitivity before other cell types intervene in response to the blue stimulus.

Using this method it is possible to evaluate a possible increase in the activity of retinal ganglion cells to support and amplify the luminous message of the photoreceptors.

Method for Examining the Visual Field

The examination was carried out with Octopus 311 before administration of the composition according to the invention and after 4 weeks of treatment. The examination was effected after a 5-minute adaptation in the dark. In order to avoid false positives, the initial white light test was repeated twice and only the retinal sensitivity indexes of the second field of vision were considered. Subsequently, after a rest period of 30 minutes in normal light and a new adaptation in the dark of 5 minutes, a blue-yellow field of vision was performed which is universally used to test the functionality of retinal ganglion cells. Also in this case, the examination was carried out twice at 10-minute intervals and the retinal sensitivity indices obtained with the second examination were used.

At the end of the 4 weeks of treatment, all patients (group A and group B) were re-examined using the slit lamp of the anterior segment and fundus to ascertain the onset of possible pathologies or side-effects.

Results

The results obtained are summarized in the following tables.

The patients of group A to whom placebo was administered were compared with the patients of group B treated with the composition according to the invention for 4 weeks.

The results were assessed at the end of the month of administration. During the weeks of administration, no general or ocular side-effects were observed, either in the placebo group or in the group B treated with the composition according to the invention. All the patients completed the month of treatment.

Table 3 summarizes the changes in the natural and contrast visual acuity, before and after the treatment.

Table 4 summarizes the visual stress resistance data measured with the glare test and recovery after glare test before and after treatment.

Table 5 shows the changes in the retinal sensitivity before and after treatment.

In the three tables, the results obtained in group A of patients who took placebo for 4 weeks are always juxtaposed.

Statistical Analysis

The results obtained in the two groups were analyzed statistically with standard deviation and Student's T.

TABLE 3

Visual
Visual
Visual
Visual

acuity
acuity
acuity
acuity
Contrast
Contrast
Contrast
Contrast

pre
pre
post
post
pre
pre
post
post

Patient
Group A
Group B
Group A
Group B
Group A
Group B
Group A
Group B

1
1.0
1.0
1.0
1.0
0.8
0.8
0.8
0.9

2
1.0
1.0
1.0
1.0
0.8
0.8
0.8
0.9

3
1.0
1.0
1.0
1.0
0.9
0.8
0.9
0.9

4
1.0
1.0
1.0
1.0
0.8
0.8
0.9
0.9

5
1.0
1.0
1.0
1.0
0.8
0.9
0.8
0.9

6
1.0
1.0
1.0
1.0
0.8
0.9
0.8
0.9

7
1.0
1.0
1.0
1.0
0.8
0.9
0.8
0.9

8
1.0
1.0
1.0
1.0
0.8
0.8
0.8
0.8

9
1.0
1.0
1.0
1.0
0.8
0.8
0.9
0.8

10
1.0
1.0
1.0
1.0
0.9
0.8
0.8
0.9

11
1.0
1.0
1.0
1.0
0.8
0.8
0.9
0.9

12
1.0
1.0
1.0
1.0
0.8
0.8
0.9
0.9

13
1.0
1.0
1.0
1.0
0.8
0.8
0.8
0.9

14
1.0
1.0
1.0
1.0
0.8
0.8
0.9
0.8

15
1.0
1.0
1.0
1.0
0.9
0.8
1.0
0.8

16
1.0
1.0
1.0
1.0
0.9
0.8
0.9
0.9

17
1.0
1.0
1.0
1.0
0.9
0.8
0.9
0.9

18
1.0
1.0
1.0
1.0
0.8
0.8
0.8
0.9

19
1.0
1.0
1.0
1.0
0.9
0.8
0.9
0.9

20
1.0
1.0
1.0
1.0
0.9
0.8
0.9
0.9

Mean
1.0
1.0
1.0
1.0
0.83
0.81
0.86
0.88*

± DS
0
0
0
0
0.05
0.04
0.06
0.04

*p <0,05 vs pre-treated group

Legend: Contr. = contrast

The visual acuity tests substantially showed that the treatment with the composition according to the invention does not improve the central visual acuity beyond ten tenths (1.0), even if with this study it cannot be excluded that the improvement in the visual acuity can occur below ten tenths. Viceversa, the contrast visual acuity improves after 4 weeks of treatment with respect to the pre-treatment measurements.

TABLE 4

(1)Glare
(1)Glare
Rec.
Rec.

Patient
Group A
Group B
Group A
Group B

1
0.3
0.4
29
18

2
0.1
0.2
27
22

3
0.2
0.3
28
23

4
0.2
0.3
30
26

5
0.1
0.3
30
28

6
0.1
0.3
30
26

7
0.1
0.2
25
24

8
0.1
0.2
26
25

9
0.1
0.2
28
26

10
0.1
0.2
28
24

11
0.1
0.2
30
24

12
0.1
0.2
28
24

13
0.1
0.2
30
26

14
0.1
0.2
27
24

15
0.1
0.2
25
24

16
0.1
0.2
27
22

17
0.1
0.2
28
23

18
0.1
0.2
26
24

19
0.1
0.3
30
25

20
0.2
0.2
36
27

Mean
0.12
0.23*
28.40
24.25*

±DS
0.06
0.06
2.46
2.15

*p < 0.05 vs placebo (group A)

Legend: Glare = glare test group A and group B visual acuity in tenths; Rec. = recovery testafter glare group A and group B in tenths necessary for viewing the line of 4/10 (1) Natural visual acuity before glare group A and group B, see table A.

The glare and recovery after glare tests show that group B treated with the composition according to the invention has a greater recovery rate of the visual acuity with respect to the control group A.

TABLE 5

MS pre
MS pre
MS post
MS post
MS pre
MS pre
MS post
MS post

b/b
b/b
b/b
b/b
b/g
b/g
b/g
b/g

Patient
Group A
Group B
Group A
Group B
Group A
Group B
Group A
Group B

1
27.5
27.4
27.6
27.5
21.4
21.4
21.4
21.5

2
27.4
27.4
27.5
27.5
21.4
21.4
21.4
21.5

3
27.4
27.4
27.4
27.6
21.4
21.3
21.4
21.4

4
27.4
27.4
27.4
27.5
21.3
21.3
21.3
21.3

5
27.5
27.5
27.5
27.5
21.4
21.3
21.4
21.4

6
27.6
27.5
27.6
27.5
21.2
21.2
21.3
21.3

7
27.3
27.7
27.3
27.7
21.3
21.3
21.3
21.3

8
27.5
27.7
27.5
27.7
21.2
21.3
21.2
21.3

9
27.4
27.3
27.4
27.5
21.4
21.4
21.3
21.5

10
27.5
27.5
27.5
27.6
21.4
21.4
21.4
21.5

11
27.5
27.5
27.5
27.6
21.3
21.3
21.3
21.3

12
27.5
27.5
27.5
27.6
21.3
21.3
21.3
21.4

13
27.6
27.6
27.5
27.6
21.3
21.3
21.2
21.3

14
27.4
27.5
27.4
27.5
21.3
21.3
21.3
21.3

15
27.4
27.5
27.5
27.5
21.3
21.3
21.3
21.4

16
27.4
27.5
27.3
27.5
21.4
21.4
21.4
21.5

17
27.4
27.4
27.3
27.6
21.3
21.3
21.3
21.4

18
27.6
27.3
27.6
27.5
21.2
21.3
21.3
21.3

19
27.6
27.5
27.6
27.5
21.2
21.3
21.3
21.4

20
27.5
27.3
27.5
27.6
21.3
21.2
21.3
21.3

Mean
27.47
27.47
27.47
27.55*
21.31
21.31
21.32
21.38*

± DS
0.09
0.11
0.10
0.07
0.07
0.06
0.06
0.08

*p <0.05 vs pre-treated group

Legend: MS = mean sensitivity;

b/b = visual field with white light stimulus;

big = visual field with blue-yellow light stimulus.

In both the white and blue-yellow light fields of vision, group B treated with the composition according to the invention showed an improvement in the retinal sensitivity (MS=mean sensitivity) with respect to the control group A.

Statistics

In conclusion, the visual tests showed an improvement in the contrast vision, starting from a sample of perfectly healthy subjects and with a normal visual acuity of ten tenths. The best perception of contrast visual acuity is a clear indication of improvement in the retinal sensitivity threshold. The subjects treated are able to perceive higher contrast shades than those treated with placebo.

The glare and recovery after glare tests showed that the retinal ability to withstand light stress significantly improves after treatment with cyanidin and verbascoside. This improvement is explained by a higher regeneration rate of rhodopsin after treatment with the compositions according to the invention.

The retinal sensitivity tests showed an improvement in the blue-yellow sensitivity of the rods thanks to a better functioning of the retinal ganglion cells. This datum should be considered together with the improvement in the contrast vision.

In both cases, the effect is mainly due to the increase in the activity of the retinal ganglion cells which amplify the signal of the rods with an increase in the blue-yellow light sensitivity and with an increase in the sensitivity of the cones with an improvement in the contrast vision.

EXAMPLE 5
Clinical Study on Patents with Eye Diseases

Macular oedema is a multifactorial disease due to an alteration in the permeability of macular capillaries. Vascular damage may be due to systemic diseases such as diabetes, renal failure and blood disorders.

In general, all wet macular degenerations are associated with macular oedema especially when damage of the retinal pigment epithelium and Bruch lamina occurs, which anatomically separates the pigmented epithelium and the retinal layers overlying the layer called capillary chorion. This vascular layer in the absence of protection of the bruch lamina spreads the blood inside the retinal layers, dissecting them and separating them from each other until there is a severe reduction in the visual acuity.

In eye diseases, the vascular damage due to diabetes or hypertension causes an increase in the permeabilization of the vessel and consequently the leakage of plasma from the vessel wall.

This anomaly is easily visible in ophthalmology with retinal fluorangiography. With this examination, the retinal blood circulation is photographed after injection of contrast medium (fluorescein).

The damage to the vascular wall continues with a weakening of the capillary structure which, due to the blood pressure, is reduced by creating a microaneurysm.

In diabetic retinopathy, exudates and microaneurysms are always present both in the initial and late phases where other vascular alterations arise.

In this study, the capillary protection activity was evaluated of cyanidin alone and in combination with the anti-inflammatory, anti-oedema activity and inhibition of metalloproteinases of mullein in the following eye diseases:

- Macular oedema
- Diabetic retinopathy
- Dry macular degeneration
- Wet macular degeneration

Materials and Methods

A randomized double-blind study was conducted on 4 groups of 50 patients each, having the same age.

In order to assess the effectiveness of cyanidin and cyanidin-mullein combination, voluntary patients without other eye diseases and general vascular pathologies, were enrolled.

To avoid vascular pharmacological interactions, the 160 patients were not treated with vaso-protector or antiplatelet drugs for at least three months. Diabetic patients were all treated with oral hypoglycemic agents and with fasting blood sugar not exceeding 200 mg/dl for at least three months.

Groups of Patients

The 4 groups of 40 patients each were divided as follows:

Group A: multifactorial macular oedema: average age 58.2 years (15 males and 25 females) affected by chronic macular oedema diagnosed at least 6 months before, due to the following diseases:

10 patients with post-surgical macular oedema

20 patients with macular oedema from diabetic retinopathy

10 patients with macular oedema due to retinal vein occlusion

Group B: 40 patients with non-proliferating diabetic retinopathy: average age 59.9 years (17 males and 23 females)

Group C: 40 patients with dry macular degeneration: a age 65.2 (20 males and 20 females)

Group D: 40 patients with wet macular degeneration: average age 65.4 (18 males and 22 females)

The patients were previously selected for pathology and diagnosis and underwent the following eye exams:

- Slit lamp examination (CSO)
- OCT (OCT-SLO Optos)
- Fluorangiography (Kowa SW50 degrees)
- Natural and corrected visual acuity test (Standardized Computerized Sbisá optotype)

Protocol

Unbeknown to the examiner and patients, each group of 40 patients was divided into:

20 patients treated with placebo tablets containing only excipients

20 patients treated with cyanidin-mullein tablets (400 mg cyanidin and 100 mg of verbascoside divided into two tablets—1 tablet containing 200 mg of cyanidin and 50 mg of verbascoside).

One tablet was given for lunch and one for dinner, continuously for three months. Every seven days, the patients were periodically contacted by telephone to ensure the correct implementation of the therapy.

The following clinical parameters were assessed in the 4 groups:

- best correct visual acuity (RSCA) with visual acuity measured in decimals from 0.1 to 1.0
- maximum thickness of the macular retinal oedema (SM) with OCT macular topography
- fundus variations (OCT and flurangiography).

This evaluation was made by comparing OCT and flurangiography before treatment and at the end of treatment.

Possible variations in a positive sense were evaluated with a subjective scale from 1 to 5 (+ sign) and in a negative sense with a scale from 1 to 5 (− sign). Not only was the trend of the visual acuity evaluated, but also the appearance of the retina before and after treatment. In particular, in the group of patients with diabetic retinopathy, possible reductions in the number and size of retinal exudates and microaneurysms and intraretinal microhemorrhages from capillary fragility, were observed and evaluated, and finally, in fluorangiography, the diffusion of dye from the retinal vessels 3 minutes after the injection of fluorescein and any capillary amputations, indication of retinal ischemic inducing proliferative retinopathy, was evaluated.

Statistical Analysis

The results of the groups treated were compared to the placebo groups, comparing the delta of the BCVA (best correct visual acuity) values and the macular thickness (SM) before and after treatment.

The deltas obtained from the pre- and post-treatment differences of each group (placebo and treated) were statistically analyzed with standard deviation and Student's T.

Results

The results illustrated in the following Tables 6 and 7 show a clear activity of the cyanidin+verbascoside combination in the improvement of macular oedema in the treated group A compared to the placebo group.

TABLE 6

Placebo

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after 3

Patient
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.1
0.2
4
385
381
4
+

2
0.1
0.2
3
397
394
3
+

3
0.1
0.1
6
405
399
6
+

4
0.1
0.2
1
403
402
1
+

5
0.1
0.3
−8
389
397
−8
+

6
0.2
0.3
16
383
367
16
+

7
0.2
0.2
−18
370
388
−18
+

8
0.2
0.2
−8
449
457
−8
−

9
0.2
0.3
−19
447
466
−19
−

10
0.2
0.3
10
456
446
10
+

11
0.1
0.1
−15
400
415
−15
−

12
0.1
0.1
2
380
378
2
−

13
0.2
0.1
−5
454
459
−5
−

14
0.2
0.2
−14
356
370
−14
−

15
0.2
0.2
−9
421
430
−9
−

16
0.3
0.3
7
349
342
7
+

17
0.2
0.2
−3
299
302
−3
−

18
0.1
0.1
−10
340
350
−10
−

19
0.2
0.2
−10
356
366
−10
−

20
0.1
0.2
3
321
318
3
+

Mean
0.16
0.20
−3.35
388.00
391.35
−3.35

DS
0.06
0.07
−1.47
43.96
45.43
−1.47

TABLE 7

Group A

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after 3

Patient
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.1
0.6
0.5
426
221
205
+++++

2
0.1
0.7
0.6
455
201
254
+++++

3
0.1
0.7
0.6
458
199
259
+++++

4
0.1
0.7
0.6
405
196
209
+++++

5
0.1
0.7
0.6
406
203
203
+++++

6
0.1
0.8
0.7
433
186
247
+++++

7
0.2
0.8
0.6
402
188
214
+++++

8
0.2
0.7
0.5
344
189
155
+++++

9
0.2
0.7
0.5
352
192
160
+++++

10
0.2
0.8
0.6
333
189
144
+++++

11
0.2
0.8
0.6
321
188
133
+++++

12
0.2
0.8
0.6
367
178
189
+++++

13
0.2
0.8
0.6
378
177
201
+++++

14
0.2
0.7
0.5
375
178
197
+++++

15
0.3
0.9
0.6
322
180
142
+++++

16
0.3
0.9
0.6
303
178
125
+++++

17
0.3
0.8
0.5
389
179
210
+++++

18
0.3
0.9
0.6
296
188
108
+++++

19
0.3
0.9
0.6
300
177
123
+++++

20
0.3
0.8
0.5
344
176
168
+++++

Mean
0.20
0.78*
0.58**
370.45
188.15*
182.30**

DS
0.08
0.09
0.01
50.62
11.52
39.10

*p <0.05 vs pre-treatment of the same group

**P <0.05 vs placebo

The action of capillary protection and repair of the basement membrane of the capillary, characteristic of cyanidin together with the anti-inflammatory and anti-oedema action of mullein, justifies the reduction of the oedema. The improvement in the visual acuity is also justified by the further action of cyanidin in facilitating the metabolism of the retinal photoreceptors through an acceleration of the rhodopsin cycle. The comparative results between the group treated with the cyanidin-mullein combination and the placebo show a clear effectiveness of the combination of the two substances.

Data Statistical Analysis

The statistical analysis of the data obtained in group A shows a significant difference between the BCVA and MS data obtained before and after the treatment (p<0.05), a condition which is not observed in the placebo. Furthermore, the variation in BCVA and MS expressed as delta BCVA and delta MS in the treated group is significantly different from that obtained in the non-treated group (placebo) (p<0.05).

The results illustrated in the following Tables 8 and 9 show a clear activity of the cyanidin+verbascoside combination in the improvement of non-proliferating diabetic retinopathy in the treated group B compared to the placebo group.

TABLE 8

Placebo

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after 3

Patient
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.5
0.5
0.00
203
223
−20
−

2
0.5
0.4
−0.10
197
242
−45
−−

3
0.5
0.5
0.00
199
221
−22
−

4
0.4
0.4
0.00
204
201
3
−

5
0.4
0.4
0.00
200
226
−26
−

6
0.4
0.3
−0.10
199
233
−34
−−

7
0.5
0.2
−0.30
197
222
−25
−−−−

8
0.5
0.2
−0.30
198
231
−33
−−−

9
0.5
0.3
−0.20
201
235
−34
−−−

10
0.5
0.3
−0.20
203
241
−38
−−−

11
0.3
0.3
0.00
230
240
−10
−−

12
0.4
0.3
−0.10
241
256
−15
−−

13
0.4
0.4
0.00
221
231
−10
−−

14
0.3
0.4
0.10
189
197
−8
+

15
0.2
0.2
0.00
227
231
−4
−

16
0.3
0.3
0.00
267
288
−21
−

17
0.4
0.4
0.00
236
256
−20
−

18
0.4
0.4
0.00
278
276
2
+

19
0.5
0.5
0.00
268
300
−32
−

20
0.3
0.3
0.00
296
292
4
+

Mean
0.41
0.35*
−0.06
222.70
242.10*
−19.40

DS
0.09
0.09
0.00
31.90
28.27
3.62

*p <0.05 vs pre-treatment of the same group

TABLE 9

Treated

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after 3

Pat.
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.2
0.6
0.4
277
221
56
+++++

2
0.3
0.7
0.4
235
201
34
+++++

3
0.3
0.7
0.4
245
199
46
+++++

4
0.3
0.7
0.4
255
196
59
+++++

5
0.3
0.7
0.4
278
203
75
+++++

6
0.2
0.8
0.6
223
186
37
+++++

7
0.3
0.8
0.5
235
188
47
+++++

8
0.3
0.7
0.4
234
189
45
+++++

9
0.3
0.7
0.4
257
192
65
+++++

10
0.4
0.8
0.4
267
189
78
+++++

11
0.4
0.8
0.4
289
188
101
+++++

12
0.4
0.8
0.4
267
178
89
+++++

13
0.6
0.8
0.2
277
177
100
+++++

14
0.6
0.7
0.1
274
178
96
+++++

15
0.7
0.9
0.2
210
180
30
+++++

16
0.7
0.9
0.2
222
178
44
+++++

17
0.4
0.8
0.4
231
179
52
+++++

18
0.4
0.9
0.5
221
173
48
+++++

19
0.6
0.9
0.3
189
170
19
+++++

20
0.5
0.8
0.3
194
176
18
+++++

Mean
0.41
0.78*
0.37**
244.00
187.05*
56.95**

DS
0.16
0.09
−0.07
29.18
12.42
16.76

*p <0.05 vs pre-treatment of the same group

**p <0.05 vs placebo

The improvements are perceived both as an increase in the visual acuity and as a reduction in the number of exudates, microhemorrhages and microaneurysms, before and after treatment. The reduction, in fact, of vascular permeability obtained thanks to cyanidin reduces the formation of exudates that are consequent to the diffusion of plasma through the capillary and the synergy with verbascoside also reduces the retinal oedema typical of diabetic retinopathy. In addition to the improvements in the visual acuity, the action of cyanidin and verbascoside causes an overall improvement the framework of the retinopathy confirmed by the statistical analysis effected on the judgment of the examiner.

Also in this group, the sample subjected to placebo did not show any significant improvements, but rather, due to the progression of the retinopathy, there were cases of a reduction in the visual acuity (negative delta values). The statistical data show how, in the treated group, the BVCA and MS values are significantly improved after treatment (p<0.05 post-treatment vs pre-treatment) and this improvement is significantly different from what was observed in the placebo (delta BCVA and delta MV treated vs delta BCVA and delta MS placebo with p<0.05).

The results shown in Tables 10 and 11 indicate a clear activity of the cyanidin+verbascoside combination in the improvement of the dry macular degeneration in the treated group C with respect to the placebo.

This retinal pathology, which currently represents the most frequent cause of hypovision in the Western world, is caused by a series of action mechanisms at present partially unknown.

The improvement in the visual acuity obtained in three months with the combination of cyanidin+verbascoside is probably due to an improvement in the metabolism of the retinal photoreceptors. The powerful capillary-protection and inhibition of retinal proliferation factors (anti-VEGF) demonstrated with verbascoside, however, certainly plays a beneficial role in the long-term treatment of this disabling eye disease.

TABLE 10

Placebo

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after 3

Patient
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.5
0.5
0.00
203
223
−20
−

2
0.5
0.4
−0.10
197
220
−23
−−

3
0.5
0.5
0.00
199
203
−4
−

4
0.4
0.4
0.00
204
201
3
−

5
0.4
0.4
0.00
200
202
−2
−

6
0.4
0.3
−0.10
199
198
1
−−

7
0.5
0.2
−0.30
197
204
−7
−−−−

8
0.5
0.2
−0.30
198
202
−4
−−−

9
0.5
0.3
−0.20
201
212
−11
−−−

10
0.5
0.3
−0.20
203
199
4
−−−

11
0.4
0.4
0.00
188
185
3
+

12
0.4
0.3
−0.10
185
185
0
−

13
0.5
0.4
−0.10
178
179
−1
−

14
0.6
0.6
0.00
189
177
12
+

15
0.6
0.5
−0.10
178
179
−1
−

16
0.5
0.5
0.00
183
189
−6
−

17
0.4
0.3
−0.10
178
167
11
−

18
0.5
0.4
−0.10
168
166
2
−

19
0.7
0.6
−0.10
170
174
−4
−

20
0.7
0.7
0.00
178
179
−1
+

Mean
0.50
0.41*
−0.09
189.80
192.20
−2.40

DS
0.09
0.13
0.04
11.74
16.61
−4.87

*p <0.05 vs pre-treatment of the same group

TABLE 11

Treated

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after 3

Patient
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.2
0.3
0.1
232
221
11
++++

2
0.3
0.4
0.1
231
201
30
++++

3
0.3
0.4
0.1
242
199
43
++++

4
0.3
0.4
0.1
236
196
40
++++

5
0.3
0.4
0.1
233
203
30
++++

6
0.2
0.4
0.2
198
186
12
+++++

7
0.3
0.5
0.2
199
188
11
+++++

8
0.3
0.4
0.1
194
189
5
++++

9
0.3
0.4
0.1
231
192
39
++++

10
0.4
0.5
0.1
237
189
48
++++

11
0.4
0.5
0.1
194
188
6
++++

12
0.4
0.5
0.1
196
178
18
++++

13
0.6
0.6
0
193
177
16
+

14
0.6
0.6
0
192
178
14
+

15
0.7
0.8
0.1
199
180
19
+++

16
0.7
0.8
0.1
198
178
20
+++

17
0.4
0.5
0.1
193
179
14
++++

18
0.4
0.6
0.2
197
173
24
+++++

19
0.6
0.7
0.1
196
170
26
++++

20
0.5
0.6
0.1
199
176
23
++++

Mean
0.41
0.52*
0.11**
209.50
187.05*
22.45**

DS
0.16
0.14
−0.02
19.12
12.42
6.70

*p <0.05 vs pre-treatment of the same group

**p <0.05 vs placebo

The treated group shows a significant variation in the BCVA and SM values with respect to the initial values (pre-treatment) and a superior pre-post treatment improvement in a statistically significant manner, with respect to the placebo (delta BCVA and delta MS values). The results indicated in the following Tables 12 and 13 show a clear activity of the cyanidin+verbascoside combination in the improvement of the most disabling form of macular degeneration, the wet form.

The wet form can be found in about 25% of the patients suffering from macular degeneration. The formation of new subretinal vessels, typical of the wet form, causes a total disruption of the delicate macular retinal structure, accelerating the destruction process of the retinal photoreceptors.

TABLE 12

Placebo

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after 3

Patient
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.5
0.5
0.00
203
200
3
+

2
0.5
0.4
−0.10
197
199
−2
−

3
0.5
0.5
0.00
199
200
−1
−

4
0.4
0.4
0.00
204
201
3
+

5
0.4
0.4
0.00
200
200
0
+

6
0.4
0.3
−0.10
199
202
−3
−

7
0.5
0.4
−0.10
197
203
−6
−

8
0.5
0.4
−0.10
198
201
−3
−

9
0.5
0.4
−0.10
201
204
−3
−

10
0.5
0.4
−0.10
203
205
−2
−

11
0.3
0.2
−0.10
189
197
−8
−

12
0.3
0.2
−0.10
199
203
−4
−−

13
0.3
0.1
−0.20
197
234
−37
−−−

14
0.3
0.3
0.00
188
186
2
−

15
0.2
0.2
0.00
234
264
−30
−

16
0.2
0.2
0.00
313
326
−13
−

17
0.3
0.2
−0.10
278
279
−1
−

18
0.3
0.2
−0.10
306
312
−6
−

19
0.3
0.2
−0.10
295
299
−4
−

20
0.3
0.3
0.00
222
225
−3
−

Mean
0.38
0.31
−0.06
221.10
227.00
−5.90

DS
0.11
0.12
0.01
41.16
43.55
−2.39

TABLE 13

Treated

Evaluation

Pre
Post
DELTA
Pre
Post
DELTA
after three

Patient
BCVA
BCVA
BCVA
SM
SM
SM
months

1
0.2
0.3
0.1
236
222
14
++

2
0.3
0.3
0
231
201
30
+

3
0.3
0.4
0.1
242
199
43
++

4
0.3
0.4
0.1
246
198
48
+++

5
0.3
0.4
0.1
243
200
43
++++

6
0.2
0.4
0.2
228
187
41
+++++

7
0.3
0.4
0.1
399
188
211
++++

8
0.3
0.3
0
394
189
205
+

9
0.3
0.3
0
243
192
51
+

10
0.4
0.4
0
277
189
88
+

11
0.4
0.5
0.1
197
188
9
++

12
0.4
0.5
0.1
198
178
20
+++

13
0.3
0.5
0.2
196
177
19
+++

14
0.4
0.7
0.3
197
178
19
++++

15
0.3
0.3
0
199
180
19
++

16
0.3
0.4
0.1
198
182
16
++

17
0.2
0.3
0.1
198
180
18
++

18
0.2
0.3
0.1
191
178
13
++

19
0.2
0.3
0.1
295
183
112
++

20
0.2
0.3
0.1
285
180
105
++

Mean
0.29
0.39*
0.10**
244.65
188.45*
56.20**

DS
0.07
0.10
0.03
60.82
11.19
49.63

*p <0.05 vs pre-treatment of the same group

**p <0.05 vs placebo

Statistical Analysis of the Data

The statistical analysis of the data shows how no significant improvement is observed in the placebo group before and after the treatment, whereas a significantly different variation between pre- and post-treatment is obtained for the BCVA and SM parameters in the group treated with the combination in question (p<0.05). Also in this case, in fact, the values of delta BCVA and delta SM obtained in the treated group prove to be significantly different from those obtained in the placebo (p<0.05).

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COMPOSITIONS BASED ON ACTIVE PRINCIPLES OF PLANT ORIGIN HAVING EYE PROTECTION ACTION

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