NZ614185B2 - Skin collagen production promoter - Google Patents
Skin collagen production promoter Download PDFInfo
- Publication number
- NZ614185B2 NZ614185B2 NZ614185A NZ61418512A NZ614185B2 NZ 614185 B2 NZ614185 B2 NZ 614185B2 NZ 614185 A NZ614185 A NZ 614185A NZ 61418512 A NZ61418512 A NZ 61418512A NZ 614185 B2 NZ614185 B2 NZ 614185B2
- Authority
- NZ
- New Zealand
- Prior art keywords
- tgf
- skin
- collagen production
- degradation product
- product
- Prior art date
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Classifications
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- A61K38/17—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- A61K38/18—Growth factors; Growth regulators
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- A61K8/18—Cosmetics or similar toiletry preparations characterised by the composition
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- A61Q19/08—Anti-ageing preparations
Abstract
Disclosed is the use of a TGF-? and/or a TGF-? degradation product in the preparation of a medicament or a food or drink product for the prevention and/or treatment of wrinkles, sagging, dryness, or roughness of the skin, wherein wrinkles, sagging, dryness, or roughness of the skin is prevented or treated by oral ingestion of the medicament or food or drink product by a subject in need thereof. reated by oral ingestion of the medicament or food or drink product by a subject in need thereof.
Description
DESCRIPTION
TITLE OF THE INVENTION: SKIN COLLAGEN PRODUCTION PROMOTER
TECHNICAL FIELD
The present invention relates to a skin collagen production-promoting agent, a
skin collagen production-promoting food or drink product, and a skin collagen
production-promoting cosmetic product useful for preventing skin deterioration such as
roughening, wrinkles, and the loss of elasticity in the skin. Particularly, the present
invention relates to a skin collagen production-promoting agent comprising transforming
growth factor-beta (TGF-P) and/or a TGF-[3 degradation product acquired by degrading
TGF-P with a protease as an active ingredient.
BACKGROUND ART
As a result of recent advancement in researches on the mechanism of skin
deterioration, it has been confirmed that, macroscopically speaking, the feeling of skin
dryness and the roughening of the skin are not only caused by the decline of metabolism
due to aging but also intricately involved with the effect of factors such as sunlight
(ultraviolet), drying, and oxidation. It has been revealed that collagen fibers, which are
the most primal matrix components of the dermis, are significantly reduced by the effect
of these factors. Wrinkles and sagging of the skin are increased if the machinery for
retaining the tension of the skin, such as resilience and elasticity, supported by the
collagen fibers is destroyed due to the effect of the factors such as ultraviolet. Since
collagen can hold water in molecules thereof and thereby helps to keep the skin
moisturized, if collagen is destroyed by an external factor, the skin is dried and roughened.
From the above, a skin collagen production-promoting agent is desired that can prevent
wrinkles and sagging of the skin by promoting the biosynthesis of collagen, which is one
of the major components of the dermic layer, without safety problems.
Transforming growth factor beta (TGF-P) is one of the growth factors present in
the milk of mammals. T he TGF-P family includes five subtypes, which are proteins
forming a dimer of about 25 kDa by disulfide bonds. The TGF-P family has a function
of regulating the promotion/inhibition of cell proliferation, biosynthesis, differentiation,
and apoptosis. The effect of inducing differentiation in animal cells has been confirmed
as a useful effect of TGF-p (Patent Document 1). TGF-P is also reported as a growth
factor of fibroblast cells in the skin (Non-Patent Literature 1).
CITATION LIST
PATENT LITERATURE
Patent Document 1: Japanese Laid-Open Patent Publication No. 2004-254674
NON PATENT LITERATURE
Non-Patent Literature 1: J. Dermatol. Sci., Vol. 24 (Supple), p.70, 2000
SUMMARY OF INVENTION
TECHNICAL PROBLEM
One aspect of the present invention is to provide a skin collagen
production-promoting agent without safety problems. Another aspect of the present
invention is to provide a skin collagen production-promoting food or drink product and a
skin collagen production-promoting cosmetic product containing such a substance.
English translation of
SOLUTION TO PROBLEM
As a result of extensive search for a substance producing a skin collagen
production-promoting effect contained in various food materials in order to solve the
problems, the inventers found that TGF-P or a TGF-[3 degradation product acquired by
degrading TGF-P increases collagen content in the skin, thereby completing the present
invention.
The present invention includes the following embodiments.
(1) A skin collagen production-promoting agent comprising TGF-p and/or a
TGF-P degradation product as an active ingredient.
(2) The skin collagen production-promoting agent of (1), wherein the TGF-P
degradation product is acquired by degrading TGF-P with a protease.
(3) The skin collagen production-promoting agent of (2), wherein the protease is
one or more selected from trypsin, pancreatin, chymotrypsin, pepsin, papain, kallikrein,
cathepsin, thermolysin, and Y8 protease.
(4) The skin collagen production-promoting agent of any one of (1) to (3),
wherein the TGF-P degradation product has an average molecular weight of 500 or more
and 8,000 or less.
(5) A skin collagen production-promoting food or drink product comprising the
TGF-p and/or the TGF-P degradation product of any one of (1) to (4).
(6) A skin collagen production-promoting cosmetic product comprising the
TGF-P and/or the TGF-P degradation product of any one of (1) to (4).
(7) A method of improving skin quality by oral ingestion of or application of
TGF-P and/or a TGF-P degradation product.
(8) A method of improving skin quality by oral ingestion of 10 |xg per day or
English translation of
more of TGF-P and/or a TGF-(3 degradation product or application thereof at 0.001 to 2
wt%.
(9) A method of promoting production of collagen in the skin comprising
administering TGF-P and/or a TGF-P degradation product.
(10) The method of promoting production of collagen in the skin of (9), wherein
the TGF-P degradation product is acquired by degrading TGF-p with a protease.
(11) The method of promoting production of collagen in the skin of (10),
wherein the protease is one or more selected from trypsin, pancreatin, chymotrypsin,
pepsin, papain, kallikrein, cathepsin, thermolysin, and V8 protease.
(12) The method of promoting production of collagen in the skin of any one of
(9) to (11), wherein the TGF-P degradation product has an average molecular weight of
500 or more and 8,000 or less.
(13) A method of preventing or improving skin deterioration comprising
administering TGF-P and/or a TGF-P degradation product.
(14) The method of preventing or improving skin deterioration of (13), wherein
the TGF-P degradation product is acquired by degrading TGF-P with a protease.
(15) The method of preventing or improving skin deterioration of (14), wherein
the protease is one or more selected from trypsin, pancreatin, chymotrypsin, pepsin,
papain, kallikrein, cathepsin, thermolysin, and V8 protease.
(16) The method of preventing or improving skin deterioration of any one of (13)
to (15), wherein the TGF-P degradation product has an average molecular weight of 500
or more and 8,000 or less.
(17) A skin deterioration-preventing or -improving agent comprising TGF-P
and/or a TGF-P degradation product as an active ingredient.
(18) The skin deterioration-preventing or -improving agent of (17), wherein the
TGF-P degradation product is acquired by degrading TGF-P with a protease.
(19) The skin deterioration-preventing or -improving agent of (18), wherein the
protease is one or more selected from trypsin, pancreatin, chymotrypsin, pepsin, papain,
kallikrein, cathepsin, thermolysin, and Y8 protease.
(20) The skin deterioration-preventing or -improving agent of any one of (17) to
(19), wherein the TGF-P degradation product has an average molecular weight of 500 or
more and 8,000 or less.
(21) A skin deterioration-preventing or -improving food or drink product
comprising the TGF-|3 and/or the TGF-P degradation product of any one of (17) to (20).
(22) A skin deterioration-preventing or -improving cosmetic product comprising
the TGF-P and/or the TGF-P degradation product of any one of (17) to (20).
(23) A method of improving skin quality for purely cosmetic purposes by oral
ingestion of or application of TGF-P and/or a TGF-P degradation product.
(24) A method of improving skin quality for purely cosmetic purposes by oral
ingestion of 10 jj,g per day or more of TGF-P and/or a TGF-P degradation product or
application thereof at 0.001 to 2 wt%.
(25) Use of TFG-P and/or a TFG-P degradation product in the preparation of a
medicament or food or drink product for the prevention and/or treatment of wrinkles,
sagging, dryness, or roughness of the skin, wherein wrinkles, sagging, dryness, or
roughness of the skin is prevented or treated by oral ingestion of the medicament or food
or drink product by a subject in need thereof.
ADVANTAGEOUS EFFECTS OF INVENTION
The present invention provides a skin collagen production-promoting agent, a
skin collagen production-promoting food or drink product, and a skin collagen
production-promoting cosmetic product containing TGF-0 and/or a TGF-P degradation
product as an active ingredient. The skin collagen production-promoting agent, the skin
collagen production-promoting food or drink product, and the skin collagen
production-promoting cosmetic product have an effect of promoting collagen production
in the skin and are useful for the prevention and treatment of wrinkles, sagging, feeling of
dryness, and roughening of the skin.
DESCRIPTION OF EMBODIMENTS
English translation of
A feature of the skin collagen production-promoting agent of the present
invention is that TGF-P and/or a TGF-P degradation product acquired by degrading
TGF-P with a protease is contained as an active ingredient. TGF-P of any origin is
usable in the present invention. For example, human- and bovine-derived TGF-Ps have
gene sequences already revealed and can be produced with gene recombination, and
TGF-P produced with a genetic engineering technique is usable in the present invention.
TGF-P is contained in a relatively large amount in bovine colostrum and may be collected
from the milk. T GF-P is also collectable from the medium of cell culture and such
cell-derived TGF-P is also usable. F or example, milk-derived TGF-P is producible in
accordance with a known method (see, e.g., J. Protein Chem., Vol. 10, pp. 565-575, 1991),
and TGF-P can be acquired from raw milk, powdered milk, skim milk, reconstituted milk,
or other processed milk by heat treatment, salting treatment, ethanol treatment, various
chromatographic processes such as ion exchange chromatography and gel filtration
chromatography, and an ultrafiltration process in a combined manner as needed.
For the TGF-P degradation product, a peptide mixture is usable that is acquired
by limited proteolysis of TGF-P with a protease such as trypsin, pancreatin, chymotrypsin,
pepsin, papain, kallikrein, cathepsin, thermolysin, and V8 protease to an average
molecular weight of 8,000 or less. Meanwhile, the lower limit of the average molecular
weight is preferably equal to or greater than 500. For example, the average molecular
weight of the TGF-P degradation product is 500 or more and 8000 or less, 1500 or more
and 8000 or less, 2500 or more and 8000 or less, 3500 or more and 8000 or less, 4500 or
more and 8000 or less, 5500 or more and 8000 or less, 6500 or more and 8000 or less,
7500 or more and 8000 or less, 500 or more and 7500 or less, 1500 or more and 7500 or
less, 2500 or more and 7500 or less, 3500 or more and 7500 or less, 4500 or more and
7500 or less, 5500 or more and 7500 or less, 6500 or more and 7500 or less, 500 or more
English translation of
and 6500 or less, 1500 or more and 6500 or less, 2500 or more and 6500 or less, 3500 or
more and 6500 or less, 4500 or more and 6500 or less, 5500 or more and 6500 or less,
500 or more and 5500 or less, 1500 or more and 5500 or less, 2500 or more and 5500 or
less, 3500 or more and 5500 or less, 4500 or more and 5500 or less, 500 or more and
4500 or less, 1500 or more and 4500 or less, 2500 or more and 4500 or less, 3500 or more
and 4500 or less, 500 or more and 3500 or less, 1500 or more and 3500 or less, 2500 or
more and 3500 or less, 500 or more and 2500 or less, 1500 or more and 2500 or less, or
500 or more and 1500 or less.
The skin collagen production-promoting agent of the present invention is orally
administered or applied to produce the skin collagen production-promoting effect.
When the skin collagen production-promoting agent of the present invention is orally
administered, the active ingredient, i.e., TGF-P or a TGF-P degradation product may
directly be used or may be formulated in a usual manner and used as an oral agent such as
powders, granules, tablets, capsules, and drinkable preparations. In the present
invention, for example, oral agents such as powders, granules, tablets, and capsules are
formulated in a usual manner by using excipients such as starch, lactose, sucrose,
mannitol, carboxymethylcellulose, corn starch, and inorganic salts. This kind of
formulation can be achieved by using the excipients as well as pharmaceutical additives
such as binders, disintegrating agents, surfactants, lubricants, fluidity promoters, coloring
agents, and flavors as needed. More specifically, binding agents include, for example,
starch, dextrin, gum arabic, gelatin, hydroxypropyl starch, sodium carboxymethyl
cellulose, methylcellulose, crystalline cellulose, ethyl cellulose, and polyvinyl pyrrolidone.
Disintegrating agents include, for example, starch, hydroxypropyl starch, carboxymethyl
cellulose, sodium carboxymethyl cellulose, cross-linked sodium carboxymethyl cellulose,
and crystalline cellulose.
Surfactants include soybean lecithin, sucrose fatty acid ester,
etc.; lubricants include talc, wax, sucrose fatty acid ester, hydrogenated vegetable oil, etc.;
; English translation of
I and fluidity promoters include anhydrous silicic acid, dried aluminum hydroxide,
| magnesium silicate, etc.
] TGF-P or a TGF-P degradation product may be combined with nutrients, food or
I drink etc., directly or after formulated into preparations. If TGF-P or a TGF-P
degradation product is contained together with a component conventionally considered to
| be effective in collagen production, such as vitamin C, a further skin collagen
I production-promoting effect can be expected. Since TGF-P or a TGF-P degradation
| product is relatively stable to heat, raw materials containing TGF-P or a TGF-P
I degradation product can be heat-sterilized under the normally used conditions,
j [0013]
When the skin collagen production-promoting agent of the present invention is
applied, the skin collagen production-promoting agent can be combined with known
I normally used components depending on the purpose of use and prepared as various
j dosage forms such as liquid formulation, solid formulation, and semisolid formulation
; and preferable compositions include ointment, gel, cream, spray, patches, lotion, powder,
i etc. For example, the skin collagen production-promoting agent of the present invention
I can be mixed with hydrocarbons such as vaseline, stearyl alcohol, higher fatty acid lower
I alkyl ester such as isopropyl myristate, animal oil and fat such as lanolin, polyhydric
I alcohol such as glycerin, glycerin fatty acid ester, mono-stearic acid, surfactants such as
j polyethylene glycol, inorganic salt, wax, resin, water, and, if needed, preservatives such
! as methyl parahydroxybenzoate and butyl parahydroxybenzoate, so as to produce skin
j collagen production-promoting cosmetics and pharmaceutical agents.
| [0014]
Although an effective oral administration dose of the skin collagen
I production-promoting agent of the present invention is not constant and is prescribed as
I needed depending on the drug formulation, the administration method, the purpose of use,
and the age, body weight, and disease condition of the patient to which the promoter is
English translation of
administered, it was found as a result of animal experiments using rats that the skin
collagen production-promoting effect can be expected to be produced by ingesting 10 |a.g
per one kilogram of rat body weight or more of TGF-|3 and/or a TGF-P degradation
product. Therefore, according to the extrapolation method, the effect can be expected by
ingesting 10 (xg per adult human or more of TGF~p and/or a TGF-(3 degradation product
daily and, thus, TGF-p and/or a TGF-P degradation product may be combined with food
or drink or administered as a medical drug so that this required amount can be ensured.
The administration can be performed several times per day in a divided manner as
needed.
Although an effective application dose of the skin collagen
production-promoting agent of the present invention varies depending on the dosage form,
TGF-P and/or a TGF-P degradation product may preferably be contained to be 0.001 to 2
wt% based on the total dosage of the composition to be applied. However, if the
composition is diluted upon use as in the case of bath additives, the contained amount
may further be increased.
EXAMPLES
The present invention will hereinafter be described in detail with reference to
examples and test examples; however, these examples only exemplarily illustrate
embodiments of the present invention and the present invention is not limited by these
examples.
EXAMPLE 1
After a column packed with 3,000 gram of S-Sepharose was sufficiently washed
English translation of
with deionized water and 10,000 liter of skim milk was allowed to flow therethrough, the
column was sufficiently washed with deionized water before elution with a linear
concentration gradient of 0.1 to 1.0 M sodium chloride. An elution fraction containing
TGF-p was fractionated again with phenyl-S Sepharose hydrophobic column
chromatography. This fraction was further sequentially processed by C4 and C8 reverse
phase chromatography and gel filtration chromatography in an HPLC system to acquire
412 mg of TGF-P (fraction A). T GF-|3 acquired in this manner is directly usable as the
skin collagen production-promoting agent.
EXAMPLE 2
After 25 mg of the fraction A acquired in Example 1 was suspended in 100 ml of
water, pancreatin was added at the final concentration of 1 % to perform enzyme
treatment at 37 °C for 5 minutes to 6 hours. After heat treatment was performed at
90 °C for 5 minutes to inactivate the enzyme, 24 mg of TGF-P degradation products
(fractions B, C, and D) was acquired by lyophilization. The average molecular weights
of the TGF-P degradation products B, C, and D acquired in this manner were about 8,000,
about 500, and about 300, respectively. The fractions B and C are directly usable as the
skin collagen production-promoting agent.
[Test Example 1]
The collagen production-promoting effects of the fraction A acquired in
Example 1 and the fractions B to D acquired in Example 2 were examined by animal
experiments using rats. Seven-week-old Wistar male rats were divided into nine test
groups (n=6) consisting of a group administered saline (control group), a group
administered 10 |j,g per one kilogram of rat body weight of the fraction A acquired in
Example 1 (A-l group), a group administered 100 |a,g per one kilogram of rat body weight
English translation of
of the fraction A acquired in Example 1 (A-2 group), groups administered 10 |ig per one
kilogram of rat body weight of the fractions B to D acquired in Example 2 (B-l to D-l
groups), and groups administered 100 (j,g per one kilogram of rat body weight of the
fractions B to D acquired in Example 2 (B-2 to D-2 groups), and each of the rats received
oral administration once a day with a probe and was fed for 10 days. With regard to the
collagen content in the skin, after treating the dermis of the rats in accordance with the
method of Nimni etal., (see Arch. Biochem. Biophys., p. 292, 1967), hydroxyproline
content in the soluble fraction was measured. Since hydroxyproline is a specific amino
acid contained only in collagen and accounts for about 10 % of the total amino acid
constituting collagen, collagen content can be estimated (see Ryuji Asano et al., Bio
Industory, p. 12, 2001). The results are shown in Table 1.
[Table 1]
Hydroxyproline content (U g/ml)
Control group 0.3 ± 0.1
A-1 group 0. 7 ± 0.1 *
A-2 group 1. 1 ± 0.2*
B-1 group 0.6 ± 0.1*
C-1 group 0.7
± 0.2*
D-1 group 0.5 0.1 *
B-2 group 1.0 ±
0. 3 *
C-2 group
1. 1 ± 0.2*
D-2 group 0. 6 0.2*
Each numerical value is a mean ± standard deviation (n-6).
* A significant difference exists as compared to the control group (p<0.05).
As a result, the hydroxyproline content in the soluble fraction after 10 weeks
English translation of
indicated significantly higher values in all the test groups as compared to the control
group. Therefore, it was clarified that TGF-P and a TGF-P degradation product having
an average molecular weight of 500 or more and 8,000 or less have the skin collagen
production-promoting effect and are useful as a skin collagen production-promoting agent.
It was also clarified that the skin collagen production-promoting effect is observed when
TGF-P and a TGF-P degradation product are administered in an amount of at least 10 |ig
per one kilogram of rat body weight.
[Test Example 2]
The collagen production-promoting effects of the fraction A acquired in
Example 1 and the fraction B acquired in Example 2 were examined by experiments
using a human fibroblast cell line [CCD45SK (ATCCRL 1506) collected from the skin of
Caucasian women]. The normal human fibroblast cell line was seeded onto a 24-well
plate at 4x104 cells/well/0.4 ml by using a modified Eagle's medium (MEM, 10-101,
Dainippon Pharmaceutical Co., Ltd.) containing 10 vol% fetal bovine serum (hereinafter
abbreviated as FBS), cultured with 5 % carbon dioxide under saturated water vapor at
37 °C for 24 hours, and then replaced to a 0.6 vol% FBS-containing MEM medium.
The fraction A acquired in Example 1 and the fraction B acquired in Example 2 were
added to each well (0.1 vol% final) (n=6) and cultured for 24 hours, and
P-aminopropionitrile and tritium-L-proline were then added (50 (ig/ml and 1 |iCi/ml final,
respectively), to acquire culture medium after further culturing for 24 hours. From the
culture medium acquired in this manner, collagen fractions were fractionated in
accordance with the method of Webster et at, (see, Analytical Biochemistry, p. 220, 1979)
to measure radioactivity incorporated into the collagen fractions. The same test was
conducted as a control without adding TGF-P and the TGF-P degradation product. The
results are shown in Table 2.
English translation of
[Table 2]
Collagen production (%)
Control 100 ± 3
204 ±11*
Fraction A
215 ± 9 *
Fraction B
Each numerical value is a mean ± standard deviation (n=6).
* A significant difference exists as compared to the control group (p<0.05).
The results indicate that all the groups with TGF-P and the TGF-P degradation
product added exhibited a collagen production-promoting ability twice or more greater
than the group without the addition of TGF-P and the TGF-p degradation product
(control). Therefore, it was clarified that TGF-P and a TGF-P degradation product have
an effect on the skin fibroblast cells to promote collagen production and are useful as a
skin collagen production-promoting agent.
EXAMPLE 3
Skin collagen production-promoting drink having composition shown in Table 3
was manufactured in a usual manner. F lavor of the manufactured drink was favorable
and did not deteriorate after storage for one year at room temperature, and there was no
problem such as precipitation.
English translation of
[Table 3]
Mixed isomerized sugar 15. 0 (wt%)
Fruit juice 10. 0
Citric acid 0. 5
Fraction A (product of Example 1) 0. 1
Flavors 0. 1
Mineral mixture 0. 1
Water Added to a total amount of 100.0
EXAMPLE 4
Dough having composition shown in Table 4 was prepared, shaped, and baked in
a usual manner to manufacture skin collagen production-promoting biscuits.
[Table 4]
Flour 5 O. O (wt%)
Sugar
2 0. O
Salt
0. 5
Margarine
1 2. 5
1 2. 5
Water 3. 5
O. 8
Mineral mixture
Fraction C (product of Example 2)
0. 2
EXAMPLE 5
English translation of
Skin collagen production-promoting agent having composition shown in Table 5
was manufactured in a usual manner.
[Table 5]
9 0. 5
Dextrose monohydrate
Mineral mixture 5. O
Fraction A (product of Example 1) 3. O
Sugar ester 1 . O
Flavors O. 5
EXAMPLE 6
Skin lotion having composition shown in Table 6 was manufactured in a usual
manner.
[Table 6]
Glycerin (wt%)
3. 0
1,3-butylene glycol
3. 0
Polyoxyethylene sorbitan monooleate (20 E.O.)
0. 5
Methyl parahydroxybenzoate
0. 1 5
Citric acid
0. 1
Sodium citrate
1 . 0
Flavors
0. 0 5
Fraction B (product of Example 2)
0. 0 5
Purified water Added to a total amount of 100.0
English translation of
EXAMPLE 7
Cream having composition shown in Table 7 was manufactured in a usual
manner.
[Table 7]
Liquid paraffin 5. O
White beeswax
4. O
Cetanol 3. O
Squalane 1 0. O
Lanolin
2. O
Stearic acid
1 . O
Polyoxyethylene sorbitan monooleate (20 E.O.)
1 . 5
Glyceryl monostearate
3. O
1,3-butylene glycol 6. O
Methyl parahydroxybenzoate
1. 5
Flavors 0. 1
Fraction A (product of Example 1)
0. 5
Purified water Added to a total amount of 100.0
[Test Example 3]
The skin lotion acquired in Example 6 and the cream acquired in Example 7
were used for a practical use test. Comparison products were used that had the same
compositions as Examples 6 and 7 except that TGF-P and the TGF-P degradation product
were removed. Twenty adult women having dry skin with sagging and fine wrinkles
recognized on the facial surfaces were randomly divided into two groups of 10 each
(groups E and F) and twenty women with roughening of skin recognized on the hands
were randomly divided into two groups of 10 each (groups G and H) to apply 2 g of the
English translation of
skin lotion of the preset invention to the facial surfaces of the group E, 2 g of the skin
lotion of the comparison product to the facial surfaces of the group F, 2 g of the cream of
the preset invention to the fingers of the group G, and 2 g of the cream of the comparison
product to the fingers of the group H, twice a day in a similar manner to the normal usajge
condition for 10 days. The results are shown in Table 8.
[Table 8]
Fed^f MSB W^les Sagging
+ + + + +
Group E 4- +
Group F ± ± ± ±
+ + +
Group G ND ND
Group H
± ± ND ND
+ + : A prominent improvement effect was observed after application for 10 days.
+ : An improvement effect was observed after application for 10 days.
± : No improvement effect was observed after application for 10 days
(no change occurred from 10 days ago).
ND : Not determined
From Table 8, it was clarified that prominent improvement effects were exhibited
especially for feeling of dryness and roughening of the skin in the groups E and G using
the skin lotion of the product of Example 6 and the cream of the product of Example 7, as
compared to the groups F and H using the skin lotion and the cream of the comparison
products.
Claims (5)
1. Use of a TGF-P and/or a TGF-(3 degradation product in the preparation of a medicament or a food or drink product for the prevention and/or treatment of wrinkles, sagging, dryness, or roughness of the skin, wherein wrinkles, sagging, dryness, or roughness of the skin is prevented or treated by oral ingestion of the medicament or food or drink product by a subject in need thereof.
2. The use according to claim 1, wherein skin quality is improved by oral ingestion of 10 jag per day or more of the TGF-P and/or TGF-P degradation product
3. The use according to claim 1 or claim 2, wherein the TFG-P degradation product has an average molecular weight of between 500 and 8,000.
4. The use according to any one of claims 1 to 3, wherein the TGF-P degradation product is acquired by degrading TGF-P with a protease.
5. The use according to claim 4, wherein the protease is one or more selected from trypsin, pancreatin, chymotrypsin, pepsin, papain, kallikrein, cathepsin, thermolysin, and V8 protease.
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP2011-026446 | 2011-02-09 | ||
| JP2011026446A JP5890100B2 (en) | 2011-02-09 | 2011-02-09 | Skin collagen production promoter |
| PCT/JP2012/052690 WO2012108410A1 (en) | 2011-02-09 | 2012-02-07 | Skin collagen production promoter |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| NZ614185A NZ614185A (en) | 2014-09-26 |
| NZ614185B2 true NZ614185B2 (en) | 2015-01-06 |
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