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| United States Patent Application |
20080260662
|
| Kind Code
|
A1
|
|
Johnsen; Geir
; et al.
|
October 23, 2008
|
Sunscreen Compositions Comprising Carotenoids
Abstract
The invention concerns methods of treating or preventing the effects of
irradiation in a human or non-human animal using carotenoid compounds,
preferably diadinoxanthin, diatoxanthin and/or fucoxanthin as well as
photoprotective compositions and their use to prepare photoprotective or
photoprotected products.
| Inventors: |
Johnsen; Geir; (Trondheim, NO)
; Lysaa; Per Age; (Oslo, NO)
; Aamodt; Kristin; (Oslo, NO)
|
| Correspondence Address:
|
SCHWEGMAN, LUNDBERG & WOESSNER, P.A.
P.O. BOX 2938
MINNEAPOLIS
MN
55402
US
|
| Family ID:
|
34259517
|
| Appl. No.:
|
11/795668
|
| Filed:
|
January 23, 2006 |
| PCT Filed:
|
January 23, 2006 |
| PCT NO:
|
PCT/GB2006/000220 |
| 371 Date:
|
April 15, 2008 |
| Current U.S. Class: |
424/59 ; 424/70.9; 549/541; 568/825 |
| Current CPC Class: |
A61K 8/33 20130101; A61K 8/34 20130101; A61K 8/975 20130101; A61Q 19/08 20130101; A61Q 5/06 20130101; A61Q 17/04 20130101; A61Q 19/00 20130101; A61Q 5/02 20130101 |
| Class at Publication: |
424/59 ; 424/70.9; 568/825; 549/541 |
| International Class: |
A61K 8/34 20060101 A61K008/34; A61Q 17/04 20060101 A61Q017/04; A61K 8/49 20060101 A61K008/49; C07C 29/74 20060101 C07C029/74; C07D 301/32 20060101 C07D301/32 |
Foreign Application Data
| Date | Code | Application Number |
|---|
| Jan 21, 2005 | GB | 0501365.1 |
Claims
1-28. (canceled)
29. A method of treating or protecting against the effects of irradiation
in a human or non-human animal wherein a photoprotective composition
comprising a carotenoid compound with the formula:
R.sub.3--CR.sub.4a--CR.sub.4b--CR.sub.4c--CR.sub.4d--CR.sub.4e--CR.sub.4f-
--CR.sub.4g--CR.sub.4h--CR.sub.4i--CR.sub.4j--CR.sub.4k--CR.sub.4l--CR.sub-
.4m--CR.sub.4n--CR.sub.4o--CR.sub.4p--C.ident.C--R.sub.6; wherein R.sub.3
and R.sub.6, which may be the same or different, are each a cyclic group
selected from: ##STR00004## each of R.sub.4a to R.sub.4p is an
optionally substituted alkyl group, a hydrogen atom, an oxygen atom or a
hydroxy group, wherein if R.sub.4 is an oxygen atom the adjacent carbon
atom carries two R.sub.4 groups, or a pharmaceutically acceptable
derivative or salt thereof, together with one or more pharmaceutically
acceptable excipients and/or diluents, is administered to said human or
non-human animal.
30. A method as claimed in claim 29 wherein R.sub.4a, R.sub.4b, R.sub.4d,
R.sub.4e, R.sub.4f, R.sub.4h, R.sub.4i, R.sub.4j, R.sub.4k, R.sub.4m,
R.sub.4n, R.sub.4o are hydrogen atoms and R.sub.4c, R.sub.4g, R.sub.4l,
R.sub.4p are methyl groups.
31. A method as claimed in claim 29 wherein R.sub.6 is cyclic group I.
32. A method as claimed in claim 29 wherein said carotenoid compound is
5,6-epoxy-7',8'-didehydro-5,6,dihydro-.beta.,.beta.-carotene-3-3'-diol or
7',8'-didehydro-.beta.,.beta.-caroten-3,3'-diol or a pharmaceutically
acceptable derivative or salt thereof.
33. A method as claimed in claim 29 wherein said carotenoid compound is
diadinoxanthin or diatoxanthin or a pharmaceutically acceptable
derivative or salt thereof.
34. A method as claimed in claim 29 wherein said pharmaceutically
acceptable derivatives are cis- and trans-isomers, naturally occurring
seco-, apo- and nor-carotenoid derivatives, epoxide derivatives,
degradation products and dehydration derivatives, or pro-drugs.
35. A method as claimed in claim 34 wherein said degradation product is
diadinochrome.
36. A method as claimed in claim 29 wherein said carotenoid compound used
in said composition is purified to a degree of purity of more than 30%.
37. A method as claimed in claim 29 wherein said carotenoid compounds are
obtained or derived from naturally occurring sources.
38. A method as claimed in claim 29 wherein said carotenoid compounds are
isolated from microalgae belonging to the phytoplankton classes Diatoms,
Dinoflagellates, Prymnesiophytes, Euglenophytes and Chrysophytes.
39. A method as claimed in claim 29 wherein said carotenoid compounds are
generated synthetically.
40. A method as claimed in claim 29 wherein said carotenoid compound is
combined in the composition with additional sunscreen compounds.
41. A method as claimed in claim 40 wherein said composition contains two
or more carotenoid compounds.
42. A method as claimed in claim 29 wherein said composition is in the
form of a solution, suspension, gel, emulsion, ointment or cream.
43. A method as claimed in claim 29 wherein said composition optionally
comprises additional sunscreen compounds wherein said composition is in
the form of a gel, emulsion, ointment or cream.
44. A method as claimed in claim 29 wherein said composition is suitable
for topical administration.
45. A method as claimed in claim 29 wherein said composition is
formulated in a make-up product, a body product or a hair product and
optionally comprises additional sunscreen compounds.
46. A method as claimed in claim 29 wherein said composition is
administered in combination with one or more active ingredients which are
effective in treating or preventing the effects of radiation.
47. A method as claimed in claim 29 wherein said composition is topically
administered to the skin or hair of a human.
48. A method as claimed in claim 29 wherein said composition is
photoprotective against light irradiation with a wavelength of 400-500
nm.
49. A photoprotective composition comprising a carotenoid compound with
the formula:
R.sub.3--CR.sub.4a--CR.sub.4b--CR.sub.4c--CR.sub.4d--CR.sub.4e--CR.sub.4f-
--CR.sub.4g--CR.sub.4h--CR.sub.4i--CR.sub.4j--CR.sub.4k--CR.sub.4l--CR.sub-
.4m--CR.sub.4n--CR.sub.4o--CR.sub.4p--C.ident.C--R.sub.6; wherein R.sub.3
and R.sub.6, which may be the same or different, are each a cyclic group
selected from: ##STR00005## each of R.sub.4a to R.sub.4p is an
optionally substituted alkyl group, a hydrogen atom, an oxygen atom or a
hydroxy group, wherein if R.sub.4 is an oxygen atom the adjacent carbon
atom carries two R.sub.4 groups, or a pharmaceutically acceptable
derivative or salt thereof, together with one or more pharmaceutically
acceptable excipients and/or diluents.
50. A photoprotective composition as claimed in claim 49 for use as a
medicament.
51. A method of treating or protecting against the effects of irradiation
in a human or non-human animal comprising administering to the human or
non-human animal the photoprotective composition as defined in claim 49.
52. A method of preparing a photoprotective or photoprotected product
comprising incorporating the photoprotective composition defined in claim
49 into said product, or impregnating said product with said compound or
composition.
53. A photoprotective or photoprotected product obtainable by the method
of claim 52.
54. A method of purifying a carotenoid as defined in the composition of
claim 49 from algae comprising the steps of (i) mixing algae with water
adjusted to a pH of 8 to 12, (ii) adding alcohol to a final water:alcohol
ratio of 0.2 to 1.5:1.0, (iii) extracting said alcohol-water mixture
(aqueous phase) with a liquid organic solvent (organic phase) at a
water-alcohol:organic solvent ratio of 0.75 to 1.5:1.0, (iv) optionally
cooling said organic phase at less than 10.degree. C. for more than 5
minutes; and (v) collecting the aqueous and/or organic phase and
purifying the carotenoid therefrom.
55. A method as claimed in claim 54 wherein said alcohol is ethanol and
said organic solvent is heptane.
Description
[0001] The present invention relates to compositions comprising
algae-derived compounds diadinoxanthin, diatoxanthin, fucoxanthin and
related compounds. Preferably the compositions are pharmaceutical or
cosmetic compositions, particularly compositions with photoprotective
properties, such as sunscreens for preventing damage resulting from
exposure of body coverings or surfaces such as skin and hair to the UV--
and visible range of the solar spectrum.
[0002] Sunlight is composed of a continuous spectrum of electromagnetic
radiation that is divided into three main regions of wavelengths:
ultraviolet (UV), visible, and infrared. UV radiation comprises the
wavelengths from 200 to 400 nm, while visible light ranges from 400 to
700 nm. The ultraviolet spectrum is further divided into three sections,
each of which has distinct biological effects: UVA (320-400 nm), UVB
(280-320 nm), and UVC (200-280 nm).
[0003] The damaging effects of sunlight on skin are well documented, and
the multiple deleterious effects include burns, premature aging and
wrinkling of the skin (dermatoheliosis), development of pre-malignant
lesions (solar keratoses) and various malignant tumours.
[0004] While the UVC rays are effectively blocked from reaching the
Earth's surface by the stratospheric ozone layer, UVA and UVB radiation
both reach the Earth's surface in amounts sufficient to have important
biological consequences to the skin and eyes. Of the UV radiation that
reaches the surface of the earth, 90-99% is comprised of UVA and 1-10% is
comprised of UVB. The damaging effects of UVB have been widely
documented. The short term effects of these high intensity rays include
erythema and burns. In the longer term the risk of skin cancer is
significant as UV radiation from 245 to 290 nm is absorbed maximally by
DNA, and is able to directly induce mutagenic photoproducts or lesions in
DNA among adjacent pyrimidines in the form of dimers.
[0005] UVA rays are not directly absorbed by DNA, but can have indirect
harmful effects by forming radical oxygen species that can react with
cellular proteins and DNA. The UVA rays are lower in intensity; they
penetrate below the skin surface and cause long-term damage such as
premature wrinkling and photoaging, and are believed to be carcinogenic.
Skin cancer is the most common type of cancer, in the US about 800 000
cases occur each year. Most skin cancers are either basal cell or
squamous type and tend to grow and spread slowly. Malignant melanoma is a
much more serious form of skin cancer and is now increasing by about 4%
per year.
[0006] The exact wavelength of radiation in the solar spectrum which
induces melanoma is not known, but the limited data that are available
suggest that the UVR spectrum is most important, particularly UVB but
possibly also UVA and visible blue light. With the growing awareness that
UVA damage exacerbates the risk of melanoma and other tumours, the need
for broad spectrum protection has become obvious. The classical means of
measuring sunscreen efficiency is the sun protection factor (SPF) number,
which is defined as the prolonged exposure to UVB rays the skin can
endure before getting burned, compared to untreated skin. Several studies
speak of the potentially dangerous false sense of security the SPF factor
gives with regards to damage induced by UVA and visible blue light.
[0007] In view of their convenience of use, sunscreens have assumed a
major component of protection against sun rays. Sunscreens work by
absorbing, reflecting or scattering the sunrays, and thereby either
shielding the skin from the sun's rays or transforming the light energy
to a harmless energy form. Sun protecting agents can roughly be divided
into chemical and physical filters. The physical sunscreens are inorganic
microparticles that act as broad spectrum photoprotectors by reflecting
or scattering the sunrays. Extensively used physical barriers include
zinc oxide and titanium dioxide. They are known to provide good
photoprotection but are less appealing cosmetically; they are not
absorbed by the skin and tend to stay as a white layer on the skin
surface.
[0008] Chemical sunscreens are absorbed by the skin, and exert their
sunscreen activity by absorbing the rays emitted by the sun and
re-emitting this light energy as vibrational energy (heat). Common
chemical sunscreen agents include PABA (para-amino benzoic acid) and its
derivatives, cinnamates, salicylates, anthranilates, camphor derivatives,
benzimidazole, triazones, octocrylene, urocanic acid, bisimidazylate and
anisotriazine.
[0009] Consumer safety is a major concern with regards to sunscreen
compounds. Available research establishes that some sunscreen compounds
are potentially photo allergenic; for example PABAs, that are known to
induce photo allergenic reactions in 1-2% of the population (Kimbrough,
1997, J. Chem. Ed., 74(1), p51-53). Although generally regarded as good
photo protectors, the safety of the physical sunscreen has also been
discussed, as in vitro studies with human fibroblasts has shown formation
of hydroxyl radicals upon the combination of sun exposure and titanium
dioxide, which led to strand breakage in the DNA (Dunforda et al, 1997,
FEBS Lett., 418, p87-90). In addition, all of these chemicals photo
decompose into unknown compounds and the long-range safety effects have
not been studied.
[0010] There is particularly a need for a good means for rating UVA
protection, as no such standard exist today. Despite increasing awareness
of the importance of broad spectrum protection, studies show that
commercially available sunscreens claiming to have good UVA protection do
not protect sufficiently against UVA rays (Haywood et al, 2003, J.
Invest. Derm., 121(4), p862). Particularly, in the longer wavelength UVA
radiation (370-400 nm) the available sun filters provide poor protection
and particularly poor or no protection against wavelengths above 400 nm.
[0011] Most of the commercially available UV-- and sun protecting
compounds in skin creams are synthetic, and the search for natural
compounds with equal or greater efficiency is becoming more significant
because of the consumer's preference for natural products.
[0012] The UV-absorbing properties of various organisms and natural
extracts have been studied among higher plants, corals, cyanobacteria and
phytoplankton, but commercialization of natural sunscreen compounds is
still limited. There remains a need for naturally derived sun-absorbing
or sunscreen agents that are efficient filters of sun in the UV-- and
visible range of the solar spectrum.
[0013] Surprisingly a discrete family of carotenoids in the xanthophyll
group have been identified which are effective UV and visible light
filters (particularly for use on the skin of animals, especially humans),
are antioxidants, have a golden yellow colour, are oil soluble and
stable. This family are embodied by the carotenoids diadinoxanthin,
diatoxanthin, fucoxanthin and their derivatives.
[0014] Diadinoxanthin, diatoxanthin and fucoxanthin are carotenoids in the
xanthophyll group, found in 50' of the 10 world wide important
bloom-forming phytoplankton classes: Diatoms, Dinoflagellates,
Prymnesiophytes, Euglenophytes, Chrysophytes. Fucoxanthin is also present
in abundance in other organisms, e.g. seaweed, raphidocytes and brown
algae (macroalgae) such as Fucus vesiculosus.
[0015] Diatoms, dinoflagellates and Prymnesiophytes are characterized by
having the ability to synthesize significant amounts of diadinoxanthin
and diatoxanthin under high-light conditions in spring and summertime,
while staying in shallow brackish top layers in fjords, coastal areas and
along the ice edge.
[0016] These organisms have developed efficient photoprotective mechanisms
in order to minimize photoinhibition that could result from their
periodic exposure to excess light intensities. Among the short-term
defenses that are activated by a sudden increase in light intensity, the
photoprotective radiative dissipation of excess absorbed light energy is
known as an important mechanism. In this mechanism the xanthophylls
diadinoxanthin and diatoxanthin are involved, in a process referred to as
non-photochemical quenching (NPQ). Diadinoxanthin is localized in a major
light harvesting pigment-protein complex (LHC), where it normally
receives light energy and sends it to reaction centres in photosystem II
(PS II). In NPQ diadinoxanthin is de-epoxydized to diatoxanthin, which
has an active role in dissipating excess light energy instead of sending
it to the reaction centre.
[0017] The present inventors have found that diadinoxanthin, diatoxanthin,
fucoxanthin and related compounds have particularly useful properties as
sunscreens, particularly when applied to living organisms.
[0018] The compounds have not previously been identified as having any
utility as sun-absorbing compounds. Diadinoxanthin and diatoxanthin in
particular are rare carotenoids, and were considered difficult to isolate
and of poor stability. Particularly when diadinoxanthin and fucoxanthin
occur together in a biological system, a method of isolating both
compounds simultaneously has been assumed to be particularly difficult.
The inventors have now isolated the compounds in stable form and
investigated their properties. These carotenoids have surprisingly been
found to be useful in absorbing irradiation, particularly in the
previously overlooked blue light range and thus have utility in
applications reliant on sun-absorbing properties, e.g. as sunscreens.
[0019] In a first aspect, the present invention provides a composition
comprising a carotenoid, preferably a xanthophyll, a hydroxy carotenoid
(particularly a di-hydroxy-carotenoid) or epoxy carotenoid, wherein said
carotenoid contains an optionally substituted, linear unsaturated alkyl
chain comprising conjugated double bonds, substituted at each end of the
chain by a cyclic alkyl group and wherein said alkyl chain contains at
least one --C.sub.3R.sub.1R.sub.2-- group, wherein R.sub.1 and R.sub.2
may be the same or different and are each a hydrogen atom, a hydroxy
group or an alkyl group or together with the carbon atom to which it is
attached may form part or all of one of said cyclic alkyl groups or a
pharmaceutically acceptable derivative or salt thereof.
[0020] Preferably said --C.sub.3R.sub.1R.sub.2-- group is selected from
one of the following groups:
[0021] --CR.sub.1.dbd.C.dbd.CR.sub.2--, --C.ident.C--CR.sub.1R.sub.2-- and
--CR.sub.1R.sub.2--C.ident.C-- wherein preferably R.sub.1 or R.sub.2 is
hydrogen and the other R group (or both R.sub.1 and R.sub.2) together
with the carbon atom to which it is attached is part or all of a terminal
cyclic alkyl group.
[0022] Alternatively described the carotenoid comprises --CRCCR.sub.2-- or
--CR.sub.3CCR.sub.2-- wherein only one of the optional bonds is present,
and R.sub.1 or R.sub.2 may be absent or present together on a terminal
carbon atom depending on the bonds which are present.
[0023] In a particularly preferred feature, the carotenoid has the
formula:
R.sub.3--[C.sub.3R.sub.1R.sub.2].sub.a--[CR.sub.4].sub.b--[C.sub.3R.sub.-
1R.sub.2].sub.c--R.sub.5
wherein a and c are each an integer from 0 to 2 wherein a+c is .gtoreq.1,
preferably=1; b is an integer from 6 to 25, especially preferably 11, 13,
14, 16, 17 or 19; R.sub.1 and R.sub.2 are as defined hereinbefore;
R.sub.3 and R.sub.5, may be the same or different and are each a cyclic
alkyl group or a portion of a cyclic alkyl group and the remainder of
said cyclic group is provided by R.sub.1, R.sub.2 or R.sub.4 (or R.sub.1
and R.sub.2), together with the carbon atom to which it is attached; and
R.sub.4 is an optionally substituted alkyl group, a hydrogen atom, an
oxygen atom or hydroxy group or together with the carbon atom to which it
is attached may form part or all of one of said cyclic alkyl groups,
wherein if R.sub.4 is an oxygen atom and thereby provides a carbonyl
group, the adjacent carbon atom carries two R.sub.4 groups, preferably
hydrogen atoms.
[0024] Such compounds may therefore take the formula:
##STR00001##
wherein relative to the preceding formula, R.sub.4 is represented by
R.sub.4a to R.sub.4s, (wherein optionally .dbd.CR.sub.4r--CR.sub.4s-- may
be absent), a is 0, b is 17 or 19, c is 1, R.sub.3 together with R.sub.4a
and the carbon atom to which they are attached forms a cyclic group, and
R.sub.5 together with R.sub.2 and the carbon atom to which they are
attached forms a cyclic group. (In an alternative embodiment, the group
--CR.sub.1CCR.sub.2R.sub.5 in the formula above, may be replaced with the
group --C.ident.C--CR.sub.1R.sub.2R.sub.5.)
[0025] Optionally a --CR.sub.4CR.sub.4-- group may be replaced with a
--CR.sub.4R.sub.4CO-- group as described hereinbefore. In a preferred
feature said --CR.sub.4CR.sub.4-- group is --CR.sub.4bCR.sub.4c--. One or
more of R.sub.4a to R.sub.4s is preferably an alkyl group, especially
preferably R.sub.4d, R.sub.4h, R.sub.4m and R.sub.4q are alkyl groups,
preferably methyl groups.
[0026] Preferred cyclic groups (which may be the same or different at
either end of the hydrocarbon chain) are optionally substituted aromatic
or non-aromatic hydrocarbons, preferably hexyl groups. The cyclic group
is preferably a substituted cyclohexyl, cyclohexenyl group (e.g.
1-cyclopenten-1-yl) or the cyclohexane bivalent radical cyclohexylidene,
wherein such groups are preferably substituted at one or more of the ring
carbons by an alkyl group, epoxy group, hydroxy group or carbonyl group,
which themselves may be further substituted.
[0027] In a particularly preferred feature, the cyclic group is a
cyclohexyl group and C2 of the hexyl group is substituted with a hydroxy
group or an alkyl group (preferably a methyl group) (and/or C1 and C2
carry an epoxide group), C4 is substituted with an alkyl group
(preferably a methyl group), and/or a hydroxy group (which itself may be
substituted by a carbonyl group, e.g. to give an acetoxy group) and C6 is
bi-substituted with alkyl groups, preferably methyl groups.
[0028] As referred to herein alkyl groups may be mono- or polyunsaturated
and include both alkenyl and alkynyl groups. Such groups may contain up
to 40 carbon atoms.
[0029] The alkyl chain is preferably C15-C25, e.g. C19-C23. Substituent
alkyl groups are preferably shorter, e.g. preferably alkyl groups contain
up to 10, e.g. from 1 to 5 carbon atoms. In particular straight-chained
saturated hydrocarbons, e.g. with 1, 2 or 3 carbon atoms are preferred.
Substituted alkyl groups may be mono or poly-substituted, e.g. they may
be alkoxyalkyl, hydroxyalkoxyalkyl, polyhydroxyalkyl, hydroxy poly
alkyleneoxyalkyl, oxyalkyl, polyoxaalkyl and the like.
[0030] Cyclic groups may thus be selected from the group comprising:
##STR00002##
which reflect commonly found cyclic groups in carotenoids, wherein the
indicated R group corresponds to the rest of the molecule and C16, C17
and/or C18 may be replaced with an alkyl or oxygen-containing group as
described above and where appropriate the cyclohexenyl ring converted
into a cyclohexyl ring and/or C3 may be substituted with an alkyl or
oxygen-containing group as described above. Preferred cyclic groups
according to the invention are:
##STR00003##
[0031] The preferred compounds are thus carotenoids containing one or more
alkadienylene or alkynylene groups (preferably one or more propdienylene
or ethynylene groups) in the hydrocarbon chain, wherein the alkadienylene
or alkynylene group may include a carbon which is part of a terminal
cyclic group.
[0032] Carotenoids of the invention are based on the carotene structure
with optionally substituted .beta., .epsilon., .gamma., .kappa., .phi. or
.lamda. cyclic groups, as described hereinbefore. Such carotenoids have
at least one didehydro group, preferably at one or more of the positions
corresponding to the position selected from: a) 6,7; b) 6',7'; c) 7,8;
and d) 7',8' on the carotene structure. Especially preferably, a
didehydro group is present at positions 6',7' and/or 7',8'.
[0033] Preferably the above described family does not encompass naturally
occurring carotenoids, other than specifically mentioned carotenoids
described herein in accordance with the invention, e.g. fucoxanthin,
diatoxanthin and diadinoxanthin and preferably also their naturally
occurring derivatives such as their seco-, apo- or nor-carotenoid
derivatives or degradation products. In a preferred feature the above
described family does not extend to alloxanthin, neoxanthin, crocoxanthin
or vaucheriaxanthin, especially preferably neoxanthin.
[0034] Especially preferably the carotenoid is:
5,6-epoxy-3,3',5'-trihydroxy-6',7'-didehydro-5,6,7,8,5',6'-hexahydro-.bet-
a.,.beta.-caroten-8-one 3'-acetate (preferably 3S,5R,6S,3'S,5'R,6'R);
5,6-epoxy-7',8''-didehydro-5,6,dihydro-.beta.,.beta.-carotene-3,3'-diol
(preferably 3S,5R,6S) or 7',8'-didehydro-.beta.,.beta.-caroten-3,3'-diol
(preferably 3R,3'R).
[0035] Especially preferably said compound is diadinoxanthin, diatoxanthin
or fucoxanthin which have the structures shown in FIG. 1.
[0036] In a particularly preferred aspect, the carotenoid has the formula:
R.sub.3--CR.sub.4a--CR.sub.4b--CR.sub.4c--CR.sub.4d--CR.sub.4e--CR.sub.4-
f--CR.sub.4g--CR.sub.4h--CR.sub.4i--CR.sub.4j--CR.sub.4k--CR.sub.4l--CR.su-
b.4m--CR.sub.4n--CR.sub.4o--CR.sub.4p--C.sub.3--R.sub.1R.sub.2-R.sub.5
wherein R.sub.1 is a hydrogen atom when --C.sub.3R.sub.1R.sub.2-- is
--CR.sub.1.dbd.C.dbd.CR.sub.2-- or forms part of a cyclic group together
with R.sub.2 and R.sub.5, when --C.sub.3R.sub.1R.sub.2-- is
--C.ident.C--CR.sub.1R.sub.2--; R.sub.3 is a cyclic group selected from
cyclic groups I, II and III (as defined hereinbefore); each of R.sub.4a
to R.sub.4p is an optionally substituted alkyl group, a hydrogen atom, an
oxygen atom or a hydroxy group, wherein if R.sub.4 is an oxygen atom the
adjacent carbon atom carries two R.sub.4 groups, preferably R.sub.4a,
R.sub.4b, R.sub.4d, R.sub.4e, R.sub.4f, R.sub.4h, R.sub.4i, R.sub.4j,
R.sub.4k, R.sub.4m, R.sub.4n, R.sub.4o are hydrogen atoms and R.sub.4c,
R.sub.4g, R.sub.4l, R.sub.4p are methyl groups or
--CR.sub.4a--CR.sub.4b-- is the group --CH.sub.2--CO--; R.sub.5 is a
portion of a cyclic group which cyclic group may be the same as or
different to R.sub.3 and the remainder of said cyclic group is provided
by R.sub.2 and the carbon to which it is attached when
--C.sub.3R.sub.1R.sub.2-- is --CR.sub.1.dbd.C.dbd.CR.sub.2-- or is
provided by R.sub.1 and R.sub.2 together with the carbon atom to which
they are attached when --C.sub.3R.sub.1R.sub.2-- is
--C.ident.C--CR.sub.1R.sub.2--, or a pharmaceutically acceptable
derivative or salt thereof.
[0037] Especially preferably R.sub.3 is cyclic group I or III and R.sub.5
(together with R.sub.2 or R.sub.1 and R.sub.2) is cyclic group I or II,
preferably I and preferably --C.sub.3R.sub.1R.sub.2-- is
--C.ident.C--CR.sub.1R.sub.2--.
[0038] In an especially preferred aspect, the carotenoid has the formula:
R.sub.3--CR.sub.4a--CR.sub.4b--CR.sub.4c--CR.sub.4d--CR.sub.4e--CR.sub.4-
f--CR.sub.4g--CR.sub.4h--CR.sub.4i--CR.sub.4j--CR.sub.4k--CR.sub.4l--CR.su-
b.4m--CR.sub.4n--CR.sub.4o--CR.sub.4p--C.ident.C--R.sub.6
wherein R.sub.3 and R.sub.6, which may be the same or different, are each
a cyclic group selected from cyclic groups I and III (as defined
hereinbefore); each of R.sub.4a to R.sub.4p is an optionally substituted
alkyl group, a hydrogen atom, an oxygen atom or a hydroxy group, wherein
if R.sub.4 is an oxygen atom the adjacent carbon atom carries two R.sub.4
groups, preferably R.sub.4a, R.sub.4b, R.sub.4d, R.sub.4e, R.sub.4f,
R.sub.4h, R.sub.4i, R.sub.4j, R.sub.4k, R.sub.4m, R.sub.4n, R.sub.4o are
hydrogen atoms and R.sub.4c, R.sub.4g, R.sub.4l, R.sub.4p are methyl
groups, or a pharmaceutically acceptable derivative or salt thereof.
[0039] Preferably R.sub.6 is cyclic group I. (When R.sub.3 and R.sub.6 is
cyclic group I the compound is diatoxanthin and when R.sub.3 is cyclic
group III and R.sub.6 is cyclic group I the compound is diadinoxanthin.)
[0040] Pharmaceutically acceptable derivatives, which are described in
more detail hereinafter, include degradation products such as
diadinochrome in which relative to the formula above
R.sub.3--CR.sub.4a--CR.sub.4b-is a fused heterocyclic group in which the
oxygen of the epoxide group of cyclic group III forms a bond with the
alkyl chain comprising conjugated double bonds to form a 5-membered
heterocyclic group comprising an oxygen atom, CR.sub.4a--CR.sub.4b from
the alkyl chain and 2 carbon atoms from cyclic group III.
[0041] In an alternative preferred aspect, the carotenoid has the formula:
R.sub.3--CR.sub.4a--CR.sub.4b--CR.sub.4c--CR.sub.4d--CR.sub.4e--CR.sub.4-
f--CR.sub.4g--CR.sub.4h--CR.sub.4i--CR.sub.4j--CR.sub.4k--CR.sub.4l--CR.su-
b.4m--CR.sub.4n--CR.sub.4o--CR.sub.4p--CH.dbd.C.dbd.R.sub.7;
wherein R.sub.3 and R.sub.7, which may be the same or different, are each
a cyclic group selected from cyclic groups II and III (as defined
hereinbefore); --CR.sub.4a--CR.sub.4b-- is the group --CH.sub.2--CO--;
each of R.sub.4c to R.sub.4p is an optionally substituted alkyl group, a
hydrogen atom, an oxygen atom or a hydroxy group, wherein if R.sub.4 is
an oxygen atom the adjacent carbon atom carries two R.sub.4 groups,
preferably R.sub.4d, R.sub.4e, R.sub.4f, R.sub.4h, R.sub.4i, R.sub.4j,
R.sub.4k, R.sub.4m, R.sub.4f, R.sub.4o are hydrogen atoms and R.sub.4c,
R.sub.4g, R.sub.4l, R.sub.4p are methyl groups, or a pharmaceutically
acceptable derivative or salt thereof.
[0042] Preferably R.sub.3 is cyclic group III and preferably R.sub.7 is
cyclic group II.
[0043] By "pharmaceutically acceptable" or "physiologically acceptable" is
meant that the ingredient must be compatible with other ingredients in
the composition as well as physiologically acceptable to the recipient.
[0044] Pharmaceutically acceptable derivatives (which have the same or
similar functional properties to the compounds described above), include
isomers ranging from all trans to a mixture of cis-trans to all cis
isomers and includes optical isomers (e.g. 3S, 5S, 6R, 3'R and 3S, 5R,
6S, 3'R for diadinoxanthin). Derivatives further include molecules which
have been modified by e.g. modification of the hydrocarbon backbone, e.g.
by substitution with one or more alkyl groups or modification of either
or both of the cyclic groups (e.g. as described hereinbefore), providing
such modifications do not alter the functional properties of the
compounds as described herein. For example, derivatives extend to esters,
e.g. the carotenoids may be esterified with fatty acids.
[0045] Derivatives also extend to derivatives, which may occur naturally,
such as seco-, apo- and nor-carotenoid derivatives. Seco-carotenoids
refers to carotenoid derivatives which have undergone oxidative fission
without the loss of any carbon atoms. Apo-carotenoids are derivatives in
which the carbon skeleton is shortened during oxidative fission and
nor-carotenoids are derivatives in which carbon atoms have been removed
by processes other than cleavage of carbon-carbon bonds. Derivatives thus
extend to truncated carotenoids, e.g. in which one or more isoprene units
are removed from the isoprene polymer chain.
[0046] Derivatives also include epoxide derivatives and their 5,8 epoxide
isomers. Degradation products, e.g. in which the carbonyl group of
fucoxanthin is reacted e.g. with sodium borohydride in ethanol are also
included. As mentioned above, the compound product diadinochrome is a
representative degradation product of diadinoxanthin. Dehydration
derivatives, e.g. generated after treatment of the compounds described
hereinbefore with hydrogen chloride in chloroform, are also included.
[0047] Derivatives may also be generated to modify compounds of the
invention for their use in cosmetic and pharmaceutical applications, e.g.
by the addition of targeting or functional groups, e.g. to improve
lipophilicity, aid cellular transport, solubility and/or stability. Thus
oligosaccharides, fatty acids, fatty alcohols, amino acids, peptides or
proteins may be conjugated to the aforementioned compounds. Derivatives
may be in the form of "pro-drugs" such that the added component may be
removed by cleavage once administered, e.g. by cleavage of a substituent
added through esterification which may be removed by the action of
esterases.
[0048] Derivatives which retain functional activity may be tested to
establish if they retain the desired properties by the test described
herein e.g. to determine photoprotective properties.
[0049] The active ingredient for administration may be appropriately
modified for use in a pharmaceutical composition. For example the
compounds used in accordance with the invention may be stabilized against
degradation by the use of derivatives as described above.
[0050] The active ingredient may also be stabilized in the compositions
for example by the use of appropriate additives such as salts or
non-electrolytes, acetate, SDS, EDTA, citrate or acetate buffers,
mannitol, glycine, HSA or polysorbate.
[0051] Pharmaceutically acceptable salts are preferably acid addition
salts with physiologically acceptable organic or inorganic acids.
Suitable acids include, for example, hydrochloric, hydrobromic,
sulphuric, phosphoric, acetic, lactic, citric, tartaric, succinic,
maleic, fumaric and ascorbic acids. Hydrophobic salts may also
conveniently be produced by for example precipitation. Appropriate salts
include for example acetate, bromide, chloride, citrate, hydrochloride,
maleate, mesylate, nitrate, phosphate, sulfate, tartrate, oleate,
stearate, tosylate, calcium, meglumine, potassium and sodium salts.
Procedures for salt formation are conventional in the art.
[0052] Preferably the compounds used in compositions and uses of the
invention are obtained or derived from naturally occurring sources. They
may however be generated entirely or partially synthetically (e.g. from
commercially available carotenoids such as .beta.-carotene, astaxanthin,
lutein or zeaxanthin), or derivatized after purification. Preferably the
compounds are isolated from natural sources, preferably macro or
microalgae, particularly microalgae belonging to the phytoplankton
classes Diatoms, Dinoflagellates, Prymnesiophytes, Euglenophytes,
Chrysophytes, especially preferably from the diatoms Phaeodactulym
tricornutum or Procentrum minimum or the microalgae Prymnesium parvum.
[0053] Fucoxanthin may additionally be isolated from various other
sources, such as any seaweed (Kingdom: Protists, Divison: Phaeophyta)
e.g. including Fucus vesiculosus as mentioned hereinbefore, Fucos
serratus and Laminaria Hyperborea. Other sources include: Undaria
pinnitifida, Sargassum muticum, Macrocystis pyrifera, Macrocystis
angustifolia, Padina boryana, Ecklonia maxima, Laminaria pallida,
Ecklonia biruncinata, Pelagophycus porra, Turbinaria ornata, Bifurcaria
brassicaeformis and Splachnidium rugosum.
[0054] Compounds of the invention may be isolated from natural sources or
isolated from natural sources which have been modified to allow
production of the carotenoids used in the invention, e.g. by
transformation of microbiological organisms to produce the required
synthetic enzymes and isolation of the compounds from those organisms.
[0055] Conveniently such compounds are isolated by techniques known in the
art such as by partition and chromatography (see Haugan & Liaaen-Jensen,
1989, Phytochemistry, 28(10), p2797-2798) or HPLC (Zapata et al., 2000,
MEPS, 195, p29-45). The Britten method may also be used for isolation,
e.g. of fucoxanthin (Britton et al. and Schiedt & Liaaen-Jensen, 1995, in
"Carotenoids, Volume 1A: Isolation and Analysis", Eds. Britton et al.,
Birkhauser Verlag, Base1, p13-16 and p81-108, respectively). The
compounds may also be isolated by supercritical CO.sub.2 extraction which
has been used for carotenoid isolation (Mendes et al., 2003, Inorganica
Chimica Acta, Vol. 356, p328-334; Valderrama et al., 2003, J. Chem. Eng.
Data, 48, p827-830).
[0056] Compounds for use in compositions of the invention may also be
isolated in accordance with the protocols described in the Examples. Such
methods and the products of such methods form further aspects of the
invention. Thus in a further aspect the present invention provides a
method of purifying a carotenoid from algae comprising the steps of
[0057] (i) mixing algae with water adjusted to a pH of 8 to 12 (preferably
pH 8-10, e.g. pH 8.3),
[0058] (ii) adding alcohol, preferably ethanol (or alternatively
methanol), to a final water:alcohol ratio of 0.2 to 1.5:1.0 (preferably
0.3 to 1.0:1, e.g. 0.3:1),
[0059] (iii) extracting said alcohol-water mixture (aqueous phase) with a
liquid organic solvent (organic phase), preferably heptane (or
alternatively hexane), at a water-alcohol:organic solvent ratio of 0.75
to 1.5:1.0 (preferably 1-1.4:1, e.g. 1.3:1),
[0060] (iv) optionally cooling said organic phase e.g. at less than
10.degree. C., e.g. .ltoreq.5, 0, -5, -10 or -20.degree. C. (e.g.
5-10.degree. C.) for more than 5 minutes, e.g. 15-60 minutes, or for
longer, e.g. for 12-26 hours, e.g. 24 hours; and
[0061] (v) collecting the aqueous and/or organic phase and purifying the
carotenoid therefrom.
[0062] In the above described method, the order in which the water,
alcohol and organic solvent is added is not crucial. Thus the alcohol and
water may be added to one another and then the organic solvent may be
added, or the alcohol and organic solvent may be mixed, followed by the
addition of the water.
[0063] Preferably said method is used for isolation of diadinoxanthin,
diatoxanthin and/or fucoxanthin wherein diadinoxanthin and diatoxanthin
is isolated from the organic phase and fucoxanthin is isolated from the
aqueous phase. Step (iii) is preferably performed by mixing for 30-90
minutes, e.g. 1 hour at ambient temperature, e.g. 15-25.degree. C., e.g.
around 20.degree. C. Specific variations of the general method are
described in the Examples.
[0064] The alcohol for use in the method is liquid at room temperature and
is soluble in water, but not heptane and is preferably ethanol or
methanol, though other alcohols such as propanol may be used. Organic
solvents are substantially immiscible in water and are preferably liquid
at -20.degree. C., e.g. heptane, hexane or pentane.
[0065] Compounds thus isolated are preferably substantially free of any
contaminating components derived from the source material or materials
used in the isolation procedure. Especially preferably the compound is
purified to a degree of purity of more than 50 or 60%, e.g. >70, 80 or
90%, preferably more than 95 or 99% purity as assessed w/w (dry weight).
Such purity levels correspond to the specific compound of interest, but
including its isomers and optionally its degradation products. Where
appropriate, enriched preparations may be used which have lower purity,
e.g. contain more than 1, 2, 5 or 10% of the compound of interest, e.g.
more than 20 or 30%.
[0066] Conveniently the level of purity may be assessed by analysis, e.g.
using UV/visible spectrophotometry, HPLC analysis or mass spectrometry.
Synthetically generated or modified compounds should be similarly free
from contaminating components.
[0067] Carotenoids used in accordance with the invention may be generated
synthetically based, for example, on a synthetic carbon skeleton. Such
skeletons may be generated using techniques known in the art, such as
Witting type reactions, Grignard and Nef reactions, enol ether
condensations, Reformatsky reactions, Robinson's Mannic base synthesis,
reductive or oxidative dimerizations and Wurtz reactions (see e.g.
Haugan, Dr. Ing. thesis, University of Trondheim, NTH, 1994, from p155
and Mayer & Isler, 1971, in "Carotenoids", Ed. Isler, Birkhauser, Base1,
p325).
[0068] The carbon skeleton may then be modified accordingly to generate
the carotenoid of interest using techniques known in the art. For
example, fucoxanthin may be synthesized as described (Ito et al., 1994,
Pure & Appl. Chem., 66(5), p939-946) in which a C10 carbon skeleton
portion was condensed with molecules providing the cyclic end groups. The
synthesis of diatoxanthin is described in Haugan et al., 1994, supra,
p165-205. Diadinoxanthin may be prepared for example, from diatoxanthin
by the introduction of an epoxy group at the 5'-6' or 5-6 double bond of
diatoxanthin. Derivatives of these synthetically prepared carotenoids may
be made as described above using techniques known in the art.
[0069] The carotenoid compound may be present in said compositions as the
sole active ingredient or may be combined with other ingredients,
particularly other active ingredients, e.g. to increase the range over
which light protection may be offered and/or to change the physical or
chemical characteristics of the product or to make it appealing to the
consumer. Thus for example one or more additional sunscreen compounds may
be included in the composition or co-administered with the composition.
Chemical or physical sunscreen agents may be used, e.g. as described
hereinbefore which are able to absorb/quench radiation, particularly
solar radiation, particularly in the UVB and shorter UVA range or
infrared region of the spectrum. Compounds which may be used include
UVB/UVA2 filters (which filter in the range 290-340 nm) such as octyl
methoxy-cinnamate, oxybenzone, octyl salicylate, homosalate, octocrylene,
padimate O, menthyl anthranilate and 2-phenylbenzimadazole-5-sulfonic
acid. UVA1 filters (filtering in the range 340-400 nm) include
avobenzone, zinc oxide and titanium dioxide. Preferably however,
compounds are used which are found naturally, e.g. other carotenoids,
(e.g. as described herein), mycosporine-like amino acids or scytonemin.
[0070] Carotenoids as described herein may be used in combination. Thus
for example preferred compositions in accordance with the invention may
include two or more carotenoids as described herein, e.g. two or more
compounds selected from diadinoxanthin, diatoxanthin, diadinochrome and
fucoxanthin, especially preferably diadinoxanthin and fucoxanthin.
[0071] The composition of the invention may be used in various biological
and non-biological applications. Thus the compositions may be used in any
non-biological material in which photoprotective (or colouring)
properties are desirable, e.g. in plastics, paints, waxes, windows (of
buildings or vehicles), solar panels, windshields, stains or lacquers,
glass, contact lenses, synthetic lenses to avoid photodamage or sun
damage (e.g. bleaching) to the product to which they are applied, or to
the biological entity to which sunprotection is to be offered. The
compounds of the invention may be applied to such materials or
impregnated into those materials.
[0072] The invention thus further extends to a method of preparing a
photoprotective or photoprotected product comprising applying a compound
or composition of the invention to said product, or impregnating said
product with said compound or composition. The use of compounds or
composition of the invention to prepare such products is also considered
an object of the invention. Photoprotected or photoprotective products
thus formed form further aspects of the invention.
[0073] Preferably the compositions of the invention are pharmaceutical
compositions comprising a compound as described hereinbefore and one or
more pharmaceutically acceptable excipients and/or diluents as described
hereinafter.
[0074] The compounds described herein have photoprotective, colouring and
antioxidant properties.
[0075] The compositions as described herein may thus be used in cosmetic
or medical applications. The pharmaceutical composition described herein
may therefore be a cosmetic composition, an antioxidant composition or a
light protection filter or sunscreen. The present invention further
provides such compositions for use as a medicament.
[0076] The compounds described herein have an attractive golden colour and
therefore may be used in cosmetics which take advantage of that colouring
or add an additional property to sunscreens of the invention. Thus the
sunscreen and/or cosmetic preparations described herein preferably have 2
or more properties, selected from colouring, sunscreen and antioxidant
properties. As an alternative or complementary to this property as a
colorant the compounds may be used for their antioxidant or
photoprotective properties.
[0077] Thus in a further aspect the present invention provides
compositions as described herein as a cosmetic, sunscreen (light
protection filter) or antioxidant.
[0078] As referred to herein, a "cosmetic" refers to a composition used on
a human or non-human animal for non-medical purposes.
[0079] As used herein a "sunscreen" or "light protection filter" or
"photoprotective composition" refers to a composition which is suitable
for administration to an individual which provides protection against
light irradiation (i.e. acts as a light or sun-absorbing compound),
particularly of ultraviolet and visible light, preferably wavelength
280-700 nm, especially preferably at least 350-500 nm, e.g. 370-500 nm or
400-500 nm. Preferably at least one compound in said composition is
capable of achieving protection in these wavelength ranges. Protection
may be assessed by various techniques, including the time taken to
develop a light induced response or the severity of that response, e.g.
erythema or burns, e.g. using the currently available tests to determine
SPF ratings. When such a test is performed, preferably the composition
achieves a SPF of at least 2, preferably at least 10, 20, 30 or 50.
[0080] Conveniently however, in order to test efficacy e.g. to filter
light of wavelengths that do not significantly result in such responses
(e.g. UVA, particularly long-wavelength UVA, i.e. 340-400 nm), in vitro
tests may be conducted such as filtering of light through filters (to
simulate skin) comprising compounds of interest, or determining the
extinction coefficient, to determine the ability of those compounds to
absorb radiation. In methods which employ a filter comprising the test
compound, the efficacy of absorption may be determined directly or
indirectly by assessing the level of radiation (e.g. of a particular
wavelength) passing through the filter or by assessing the effect of that
radiation passing through a filter with or without the test compound,
e.g. on cells which are sensitive to radiation and show a response to
such radiation.
[0081] Preferably in such tests, (e.g. as described in the Examples), said
compounds prevent more than 40%, preferably more than 50 or 600
transmission at a given wave-length. Preferred compounds for use in
compositions of the invention preferably exhibit maximal absorption in
the 400-500 nm range, e.g. >1.5 to 2 times greater absorption at a
given wavelength in the 400-500 nm range compared to absorption at 350
nm.
[0082] Appropriate techniques for in vitro analysis involve the
application of a test compound to a substrate which preferably simulates
skin (e.g. a collagen substrate or a quartz plate with simulated skin
topography) which is then irradiated with radiation reflecting full solar
radiation or preferably narrower wavelength radiation, e.g. using a Xenon
arc to simulate the solar UV spectrum, e.g. 290-400 nm.
[0083] The UV absorbance of the test compound may be measured, e.g. using
a Labsphere UV-1000S UV transmitter analyzer (Labsphere Inc., North
Sutton, N.H.). The ability of the test compound to absorb UVA as assessed
by e.g. critical wavelength determination (as described by Diffey et al.,
2000, J. Am. Acad. Dermatol., 43(6), p1024-1035) provides an indication
of the efficacy of the test compound to absorb in the UV range of the
spectrum. Preferably the critical wavelength is more than 360 nm,
especially preferably >370 or 380 nm, especially in combination with
the SPF values described above.
[0084] The invention thus provides a method of treating or preventing the
effects of irradiation in a human or non-human animal wherein a
pharmaceutical compound or composition as described hereinbefore is
administered to said animal. Alternatively stated, the present invention
provides the use of a pharmaceutical compound or composition as described
herein in the preparation of a medicament for treating or preventing the
effects of irradiation of a human or non-human animal body.
[0085] In a preferred aspect the invention provides a method of treating
or preventing the effects of solar radiation on a human wherein a
pharmaceutical compound or composition as described hereinbefore is
topically administered to the skin or hair of said human. This method
serves to protect the skin or hair from the deleterious effects of said
solar radiation.
[0086] As used herein, "irradiation" refers to direct or indirect
irradiation from one or more natural or synthetic light sources,
particularly from the sun, i.e. solar radiation. Preferably said
radiation is of light in the range 280-700 nm, especially preferably at
least 350-500 nm, e.g. 400-480 nm or 400-500 nm. The "effects" of
irradiation may be damaging effects including burns, erythema, premature
aging and wrinkling of the skin (dermatoheliosis), development of
pre-malignant lesions (solar keratoses) and various malignant tumours or
other effects which are undesirable for, for example, cosmetic reasons,
e.g. melanin deposition.
[0087] As used herein, "treating" refers to the reduction, alleviation or
elimination, preferably to normal non-irradiated levels, of one or more
of the symptoms or effects of said irradiation e.g. presence or extent of
burning or pigmentation, relative to the symptoms or effects present on a
different part of the body of said individual not subject to irradiation
or in a corresponding individual not subject to irradiation. "Preventing"
refers to absolute prevention, or reduction or alleviation of the extent
or timing (e.g. delaying) of the onset of that symptom or effect.
[0088] The method of treatment or prevention according to the invention
may advantageously be combined with administration of one or more active
ingredients which are effective in treating or preventing the effects of
irradiation. Preferably such additional active ingredients include
sunscreen agents (as described herein and as known in the art),
antioxidants, vitamins and other ingredients conventionally employed in
sunscreen and cosmetic preparations of the art.
[0089] Thus, pharmaceutical compositions of the invention may additionally
contain one or more of such active ingredients.
[0090] According to a yet further aspect of the invention we provide
products containing one or more compounds as herein defined and one or
more additional active ingredients as a combined preparation for
simultaneous, separate or sequential use in human or animal therapy.
[0091] The compositions of the invention may be formulated in conventional
manner with one or more physiologically acceptable carriers, excipients
and/or diluents, according to techniques well known in the art using
readily available ingredients. Where appropriate compositions according
to the invention are sterilized, e.g. by .gamma.-irradiation, autoclaving
or heat sterilization, before or after the addition of a carrier or
excipient where that is present, to provide sterile formulations.
[0092] Thus, the active ingredient may be incorporated, optionally
together with other active substances as a combined preparation, with one
or more conventional carriers, diluents and/or excipients, to produce
conventional galenic preparations such as tablets, pills, powders,
lozenges, sachets, cachets, elixirs, suspensions (as injection or
infusion fluids), emulsions, solutions, syrups, aerosols (as a solid or
in a liquid medium), ointments, soft and hard gelatin capsules,
suppositories, sterile injectable solutions, sterile packaged powders,
and the like. Biodegradable polymers (such as polyesters, polyanhydrides,
polylactic acid, or polyglycolic acid) may also be used for solid
implants. The compositions may be stabilized by use of freeze-drying,
undercooling or Permazyme.
[0093] Suitable excipients, carriers or diluents are lactose, dextrose,
sucrose, sorbitol, mannitol, starches, gum acacia, calcium phosphate,
calcium carbonate, calcium lactose, corn starch, alginates, tragacanth,
gelatin, calcium silicate, microcrystalline cellulose,
polyvinylpyrrolidone, cellulose, water syrup, water, water/ethanol,
water/glycol, water/polyethylene, glycol, propylene glycol, methyl
cellulose, methylhydroxybenzoates, propyl hydroxybenzoates, talc,
magnesium stearate, mineral oil or fatty substances such as hard fat or
suitable mixtures thereof. Agents for obtaining sustained release
formulations, such as carboxypolymethylene, carboxymethyl cellulose,
cellulose acetate phthalate, or polyvinylacetate may also be used.
[0094] The compositions may additionally include lubricating agents,
wetting agents, emulsifying agents, viscosity increasing agents,
granulating agents, disintegrating agents, binding agents, osmotic active
agents, suspending agents, preserving agents, sweetening agents,
flavouring agents, adsorption enhancers (e.g. surface penetrating agents
or for nasal delivery, e.g. bile salts, lecithins, surfactants, fatty
acids, chelators), browning agents, organic solvent, antioxidant,
stabilizing agents, emollients, silicone, alpha-hydroxy acid, demulcent,
anti-foaming agent, moisturizing agent, vitamin, fragrance, ionic or
non-ionic thickeners, surfactants, filler, ionic or non-ionic thickener,
sequestrate, polymer, propellant, alkalinizing or acidifying agent,
opacifier, colouring agents and fatty compounds and the like.
[0095] The compositions of the invention may be formulated so as to
provide quick, sustained or delayed release of the active ingredient
after administration to the body by employing techniques well known in
the art.
[0096] The composition may be in any appropriate dosage form to allow
delivery or for targeting particular cells or tissues, e.g. as an
emulsion or in liposomes, niosomes, microspheres, nanoparticles or the
like with which the active ingredient may be absorbed, adsorbed,
incorporated or bound. This can effectively convert the product to an
insoluble form. These particulate forms may overcome both stability (e.g.
degradation) and delivery problems.
[0097] These particles may carry appropriate surface molecules to improve
circulation time (e.g. serum components, surfactants, polyoxamine908, PEG
etc.) or moieties for site-specific targeting, such as ligands to
particular cell borne receptors. Appropriate techniques for drug delivery
and for targeting are well known in the art and are described in
WO99/62315.
[0098] The use of solutions, suspensions, gels and emulsions are
preferred, e.g. the active ingredient may be carried in water, a gas, a
water-based liquid, an oil, a gel, an emulsion, an oil-in water or
water-in-oil emulsions a dispersion or a mixture thereof.
[0099] Compositions may be for topical (e.g. to the skin or hair), oral or
parenteral administration, e.g. by injection. Topical compositions and
administration are however preferred, and include gels, creams,
ointments, sprays, lotions, salves, sticks, soaps, powders, films,
aerosols, drops, foams, solutions, emulsions, suspensions, dispersions
e.g. non-ionic vesicle dispersions, milks and any other conventional
pharmaceutical forms in the art.
[0100] Ointments, gels and creams may, for example, be formulated with an
aqueous or oily base with the addition of suitable thickening and/or
gelling agents. Lotions may be formulated with an aqueous or oily base
and will, in general, also contain one or more emulsifying, dispersing,
suspending, thickening or colouring agents. Powders may be formed with
the aid of any suitable powder base. Drops and solutions may be
formulated with an aqueous or non-aqueous base also comprising one or
more dispersing, solubilising or suspending agents. Aerosol sprays are
conveniently delivered from pressurised packs, with the use of a suitable
propellant.
[0101] Alternatively, the compositions may be provided in a form adapted
for oral or parenteral administration. Alternative pharmaceutical forms
thus include plain or coated tablets, capsules, suspensions and solutions
containing the active component optionally together with one or more
inert conventional carriers and/or diluents, e.g. with corn starch,
lactose, sucrose, microcrystalline cellulose, magnesium stearate,
polyvinylpyrrolidone, citric acid, tartaric acid, water, water/ethanol,
water/glycerol, water/sorbitol, water/polyethylene glycol, propylene
glycol, stearyl alcohol, carboxymethylcellulose or fatty substances such
as hard fat or suitable mixtures thereof.
[0102] The concentration of active ingredient in compositions of the
invention, depends upon the nature of the compound used, the mode of
administration, the course of treatment, the age and weight of the
patient, the cosmetic or medical indication, the body or body area to be
treated and may be varied or adjusted according to choice. Generally
however, concentration ranges for the compound described herein is
0.0005, 0.001 or 0.01 to 25%, e.g. 0.01 to 10%, such as 0.1 to 5, e.g.
1-5% (w/w of the final preparation for administration, particularly for
topical administration). Said concentrations are determined by reference
to the amount of the compound itself and thus appropriate allowances
should be made to take into account the purity of the composition.
Effective single doses may lie in the range of from 1-100 mg/day,
preferably 2-10 mg/day, depending on the animal being treated, taken as a
single dose.
[0103] The administration may be by any suitable method known in the
medicinal arts, including for example oral, parenteral (e.g.
intramuscular, subcutaneous, intraperitoneal or intravenous)
percutaneous, buccal, rectal or topical administration or administration
by inhalation. The preferred administration forms will be administered
orally, or most preferably topically. As will be appreciated oral
administration has its limitations if the active ingredient is
digestible. To overcome such problems, ingredients may be stabilized as
mentioned previously.
[0104] Administration may be conducted before, during or after irradiation
to offer prevention or treatment of the effects of irradiation. Thus for
example the composition may be administered orally or applied topically
up to e.g. 1 day, but preferably less than 1 hour before irradiation, at
any time during irradiation and post-irradiation, e.g. in the 12 hours
post-irradiation.
[0105] Sunscreen formulations may be presented as topical formulations as
described hereinbefore, particularly as body, face or lip milks, foams,
sprays, lotions, gels or balms. Depending on their formulation and the
compound used in the composition, sunscreen preparations of the invention
may also have cosmetic properties, e.g. by the inclusion of additional
components or the selection of a coloured compound of the invention.
Similarly, cosmetic preparations as described herein may have sunscreen
properties.
[0106] The present invention also extends to particular cosmetic
compositions or preparations (personal care products) comprising the
compositions described hereinbefore. Such preparations may take the form
of make-up products (such as eye or face products, including eye shadow,
powder, lipstick, foundation, mascara, blush, eyeliner, nail polish,
tinted creams and foundations, sun make-up), creams, lotions or
colourants. Preferably such preparations are in the form of an anhydrous
or aqueous solid or paste. The carotenoids of the invention may be used
to impart colour, sunscreen and/or antioxidant properties to such
preparations. For sunscreen products, the compositions may be as
described hereinbefore particularly for topical administration to the
skin. For the treatment or protection of hair, the composition may be in
the form of a hair rinse, spray mist, gel, mousse, shampoo, conditioner,
lotion, emulsion or colouring product.
[0107] The invention thus further extends to a method of preparing the
above described sunscreen or cosmetic preparation comprising adding a
compound or composition as described hereinbefore to a pharmaceutically
acceptable diluent, carrier and/or excipient or base sunscreen or
cosmetic, wherein the base sunscreen or cosmetic may comprise ingredients
which impart photoprotective and/or cosmetic, e.g. colouring, properties.
The use of compounds or composition of the invention to prepare such
cosmetics/sunscreens is also considered an object of the invention.
[0108] Animals to which the compositions may be applied or administered
include mammals, reptiles, birds, insects and fish which suffer
deleterious effects from light irradiation. Preferably the animals to
which the compositions of the invention are applied are mammals,
particularly primates, domestic animals, livestock and laboratory
animals. Thus preferred animals include mice, rats, rabbits, guinea pigs,
cats, dogs, monkeys, pigs, cows, goats, sheep and horses. Especially
preferably the compositions are applied or administered to humans.
[0109] "Body coverings" or "body surfaces" to which the compositions of
the invention may be applied include body coverings such as skin, bodily
outgrowths such as hair and nails and surfaces such as mucosal membranes,
but also include equivalents in other animals such as scales or feathers.
[0110] The following Examples are given by way of illustration only in
which the Figures referred to are as follows:
[0111] FIG. 1 shows the chemical structure of diadinoxanthin (I),
diatoxanthin (II), fucoxanthin (III) and diadinochrome (IV);
[0112] FIG. 2 shows the absorption spectrum of diadinoxanthin (I),
diatoxanthin (II), fucoxanthin (III) and diadinochrome (IV) in acetone
solution;
[0113] FIG. 3 shows the transmission spectra from Integrating sphere
analysis using fucoxanthin and diadinoxanthin at different
concentrations. A commercial sunscreen SPF60 was used for comparison.
Vitro-skin+miglyol was used as the control. Curve 1: Vitro-skin+Miglyol,
2: SPF60, 3:fucoxanthin at 2.76 mg/ml, 4:fucoxanthin at 0.55 mg/ml,
5:fucoxanthin at 0.25 mg/ml, 6:diadinoxanthin at 0.64 mg/ml,
7:diadinoxanthin at 0.13 mg/ml; and
[0114] FIG. 4 shows the reduction in transmission at 454 nm as a function
of concentration for diadinoxanthin and fucoxanthin (data from
Integrating Sphere analysis). The concentrations are given as the sum of
the given compounds and their degradation products (cis-fucoxanthin and
diadinochrome). Solid lines with squares--diadinoxanthin. Solid line with
diamonds--fucoxanthin. Dashed lines illustrate a projected linear
relationship.
EXAMPLE 1
Formulations
[0115] Exemplary formulations in accordance with the invention are as
follows:
TABLE-US-00001
Sunscreens
Body lotions
% w/w
FORMULATION 1
Lanolin 4.5
Cocoa butter 2.0
Glyceryl stearate 3.0
Stearic acid 2.0
Octyl dimethyl PABA (UVB filter, optional) 7.0
Benzophenone-3 (UVB filter, optional) 3.0
Propylparaben 0.1
Methylparaben 0.3
Triethanolamine 1.0
Sorbitol 5.0
Carotenoid of the invention 1.0-5.0
Water qs to 100
FORMULATION 2
Phase A
Isopropyl myristate 4.0
Mineral oil 6.5
Grape seed oil 2.5
Stearyl alcohol 2.0
Petrolatum 2.0
Octyl methoxycinnamate (UVB filter - optional) 5.0
Carotenoid of the invention 1.0-5.0
Phase B
Sorbitan stearate 6.0
Disodium ricinoleamido MEA-sulfosuccinate 0.2
Glycerine 4.0
Allantoin 0.2
d-Panthenol 0.8
titanium oxide and water (optional) 15.0
Water qs to 100
(phase A&B)
Phase C
Preservative qs
[0116] Produced by separately heating phases A and B to 80.degree. C.,
then adding A to b, stirring intensively. After homogenizing the mixture
is allowed to cool to 25.degree. C. with slow agitation after which phase
C is added.
TABLE-US-00002
Hair products
% w/w
SHAMPOO
Anionic surfactant 2.5-1.5 active
Amphoteric surfactant 0-4 active
Alkanolamide 0-5
Polymeric/associative thickener 0-5
Carotenoid of the invention 1-5
UVA/B filters (e.g octyl methoxy cinnamate, 1-10
avobenzone or oxybenzone) - optional
Preservative qs
Fragrance qs
pH adjuster qs
Electrolyte qs
Water qs to 100
HAIRSPRAY
Resin plasticizer 0-2
Film forming resin 2-8
Ethanol 0-70
Alkanolamine or alternative 0-4
neutralizing agent
Carotenoid of the invention 1-5
UVA/B filters (e.g octyl methoxy cinnamate, 1-10
avobenzone or oxybenzone) - optional
Preservative qs
Fragrance qs
Hydrocarbon or alternative propellant 10-40
Water qs to 100
EXAMPLE 2
Extraction Protocols
[0117] Diadinoxanthin Extraction (from Micro Algae):
[0118] Extraction is performed in a nitrogen atmosphere in equipment
covered with aluminium foil. [0119] 1. The pH of a water suspension of
the microalgae P. tricornutum (14 g dry weight per litre of water) was
adjusted to 8.3 and ethanol was added to a final ratio of
water:ethanol=0.3:1.0. [0120] 2. The water-ethanol solution was extracted
by mixing with heptane (water-ethanol solution:heptane=1.3:1.0) for 1
hour at 20.degree. C. [0121] 3. The solution was separated into three
phases by centrifugation (10 minutes at 3222.times.g): An upper heptane
phase enriched in diadinoxanthin and fucoxanthin, a lower ethanol-water
phase enriched in chlorophylls and degradation products of chlorophylls,
and a third mid-phase with precipitated materials. The ratio of the
concentration of diadinoxanthin to fucoxanthin in the water-ethanol phase
was approximately 1:6. [0122] 4. Water was added to the water-ethanol
phase until a water:ethanol ratio of 0.7:1.0 was reached. This solution
was extracted by a similar amount of heptane and the phases separated by
centrifugation (as in step 3). Diadinoxanthin was enriched in the heptane
phase (diadinoxanthin:fucoxanthin=1:1), and fucoxanthin and
fucoxanthin-derivatives in the ethanol-water phase. [0123] 5. The heptane
phase was stored overnight at -20.degree. C. to separate fucoxanthin
which was separated by centrifugation as described above. (Alternatively,
the precipitated material may be removed with a pipette.) [0124] 6. The
heptane phase was used for further purification of diadinoxanthin by HPLC
as described hereinbefore to yield 60-70w of the diadinoxanthin found in
the starting material.
Optimization
[0125] Various parameters in the above described basic method were varied
to establish the effect of water concentration, pH and temperature on the
isolation method. The results are provided in the table below.
1. Altering the Water Concentration
[0126] The table below shows the phase distribution (in %) of the
carotenoids using different water levels. The method was performed at
room temperature without pH adjustment.
TABLE-US-00003
Extraction with
Water EtOH Heptane Phase Diadino Fuco Chla
0 1 1 water-EtOH 88 93 55
0.1 1 1 water-EtOH 7 51 0
0.2 1 1 water-EtOH 94 98 7
0.4 1 1 water-EtOH 78 97 0
0 1 1 heptane 12 7 45
0.1 1 1 heptane 93 49 100
0.2 1 1 heptane 6 2 93
0.4 1 1 heptane 22 3 100
2. Temperature/pH Effects
[0127] The table below shows the effects of temperature and pH on the
separation of diadinoxanthin from fucoxanthin by extraction of the
water:ethanol phase (1:1) with heptane after extraction of Chl a with
heptane. Values indicated are for the amount of each compound in the
indicated phase. The value in brackets indicates the % distribution
between the two phases.
TABLE-US-00004
Water-EtOH phase Heptane phase
Buffer Diadino Fuco Diadino Fuco
Phosphate, pH 11, 0 (0%) 260 (5%) 1500 (100%) 4860 (95%)
20.degree. C.
Phosphate, pH 11, 0 (0%) 135 (5%) 1470 (100%) 2745 (95%)
50.degree. C.
NaOH-buffer, 0 (0%) 0 (0%) 1440 (100%) 0 (0%)
pH 12.2, 50.degree. C.
Recovery:
TABLE-US-00005
[0128] Total present in % recovery of
both phases initial amount
Buffer Diadino Fuco Diadino Fuco
Phosphate, pH 11, 20.degree. C. 1500 5120 106% 81%
Phosphate, pH 11, 50.degree. C. 1470 2880 104% 46%
NaOH-buffer, pH 12.2, 50.degree. C. 1440 0 102% 0%
[0129] This shows that diadinoxanthin is stable under the conditions used
whereas fucoxanthin is more sensitive to extreme temperatures and pH.
3. Temperature Effects
[0130] The table below shows the effects of temperature on extraction for
200 minutes at a ratio of water:ethanol:heptane of 1:1:1 at pH 11.
TABLE-US-00006
Temp Water-EtOH phase Heptane phase
(.degree. c.) Diadino Fuco Chl a Diadino Fuco Chl a
20 170 380 0 1155 1065 3290
35 180 210 0 1260 610 3505
50 190 0 0 1310 95 4010
[0131] Diadinoxanthin is thus stable at various temperatures whereas
fucoxanthin was more sensitive to higher temperatures.
Fucoxanthin Extraction (from Macro Algae):
[0132] This method is a modification of the method (above) for
diadinoxanthin. [0133] 1. Fronds and stripes (from the algae Laminaria
hyperborea) were cut in pieces. [0134] 2. Ethanol (5 ml) and heptane (5
ml) were added to the algae material (1 g, wet weight), mixed in a
Whirl-mixer (3.times.15s) and placed at 4.degree. C., for 4 hours. (In
some protocols, at this stage the mixture was centrifuged and the
carotenoid extracted from the ethanol or heptane fraction. In other
protocols methane was in used instead of ethanol.) [0135] 3. 1.5 ml water
was added and mixed in a Whirl-mixer (3.times.15 s) and placed at
4.degree. C. for 1 hour. The solution was centrifuged (10 minutes at
3222.times.g) and the ethanol-water phase was used for further
purification of fucoxanthin. (Purification was performed by HPLC as
described hereinbefore.) [0136] 4. A yield of 800 .mu.g/g (dry weight)
was observed.
[0137] The method provides an extraction method for large scale extraction
of fucoxanthin while at the same time removing other cell constituents
that are regarded as difficult to separate from carotenoids (for example
chlorophyll a) from the sample.
EXAMPLE 3
Efficacy of Irradiation Absorption Using an In Vitro Skin Model
Method
[0138] The in vitro method of Springsteen was used (Springsteen et al.,
1999, Analytica Chimica Acta, 380, p155-164). Vitro-skin was used as the
skin simulator and Miglyol (Miglyol 812F Neutraloel CHG. 040906) was used
as the solvent. The tests were performed with a Varian Cary 300 Conc
UV-Visible Spectrophotometer (with an integrating sphere). Fucoxanthin
and diadinoxanthin (isolated as described in Example 2) were tested at
the concentrations indicated on FIG. 3.
Results
[0139] The results for diadinoxanthin and fucoxanthin (at different
concentrations) are shown in FIG. 3. The results were compared to a
conventional SPF 60 sun lotion, and demonstrates the compounds, ability
to absorb irradiation, particularly in the blue light range of the
spectrum, but also in the upper UVA area. FIG. 4 shows the transmission
in % plotted against the wavelength of the light. The dashed lines
display roughly the relation between concentration and absorption and
indicates that less than 5 mg/ml would be sufficient in the final
solution to provide sufficient protection at 454 nm (blue light).
* * * * *
