FORMULATIONS CONTAININGASTRAGALUSEXTRACTS AND USES THEREOF
Field of the Invention
The present invention relates to formulations containing plant extracts, and in
particular to formulations containing Astragalus extracts, and their use in skin
conditioning, in protecting the skin from UV damage, and in inducing telomerase activity
in cells.
Background of the Invention and References
Astragalus Extracts
Herbal extracts of Astragalus species have been used as a traditional Chinese
medicine. The extracted material is typically taken orally, as a nutritional supplement or a
tea preparations. References relating to Astragalus species and extracts thereof include:
Abdallah, R. M. et al.,"Astragalosides from Egyptian Astragalus spiraosus Vahl", Die
Pharmazie (Germany) 48 (6): 452-4 (Jun 1993).
Bedir, E. et al.,"Cycloartane triterpene glycosides from the roots ofAstragalus
brachypterus and Astragalus microcephalus", J. Natural Products 61 (12): 1469-72 (Dec
1998).
Bedir, E. et al.,"Trojanosides I-K : new cycloartane-type glycosides from the aerial
parts of Astragalus trojanus", Chem. Pharm. Bull. (Japan) 49 (11): 1482-6 (Nov 2001).
Ber, L. G., U. S. Patent No. 5,786, 343 (Jul 1998).
Calis, I. et al.,"Cycloartane triterpene glycosides from the roots ofAstragalus
melanophrurius", Planta medica (Germany) 63 (2): 183-6 (Apr 1997).
Calis, I. et al.,"Four novel cycloartane glycosides from Astragalus oleifolius", J.
Natural Products 59 (11): 1019-23 (Nov 1996).
Calis, I. et al.,"Secondary metabolites from the roots ofAstragalus zahlbruckneri",
J. Natural Products 64 (9): 1179-82 (Sep 2001).
Chang, T. S. , U. S. patent 5,942, 233 (Aug 1999).
Chu, D. T. et al.,"Fractionated extract of Astragalus membranaceus, a Chinese
medicinal herb, potentiates LAK cell cytotoxicity generated by a low dose of recombinant
interleukin-2", Journal of clinical & laboratory immunology 26 (4): 183-7 (Aug 1988).
Chu, D. T. et al.,"Immunotherapy with Chinese medicinal herbs. II. Reversal of
cyclophosphamide-induced immune suppression by administration of fractionated
Astragalus membranaceus in vivo", Journal of clinical & laboratory immunology
25 (3): 125-9 (Mar 1988).
Dagarag, M. et al.,"Differential impairment of lytic and cytokine functions in
senescent human immunodeficiency virus type 1-specific cytotoxic T lymphocytes", J
Virol 77 (5): 3077-83 (Mar 2003).
Hasenoehrl, E. J. etal., U. S. patent 6,190, 678 (Feb 2001).
Gariboldi, P. et al.,"Cycloartane triterpene glycosides from Astragalus trigonus",
Phytochemistry 40 (6): 1755-60 (Dec 1995).
Huang, Y. et al.,"Selected non-timber forest products with medicinal applications
from Jilin Province in China", Conference Title: Forest communities in the third
millennium: Linking research, business, and policy toward a sustainable non-timber forest
product sector; Kenora, Ontario, Canada, 1-4 October, 1999; General Technical Report-
North Central Research Station, USDA Forest Service (No. NC-217): p. 93-101 (2000).
Pistelli, L., et al.,"Antimicrobial and antifungal activity of crude extracts and isolated
saponins from Astragalus verrucosus", Fitoterapia 73 (4): 336-339 (2002).
Raman, A. et al., U. S. Patent No. 6,346, 539 (Feb 2002).
Semmar, N. et al.,"Two new glycosides from Astragalus caprinus", J. Natural
Products 64 (5): 656-8 (May 2001).
Sinclair, S. ,"Chinese herbs: a clinical review of Astragalus, Ligusticum, and
Schizandrae", Alternative medicine review : ajournal of clinical therapeutic 3 (5): 338-44
(Oct 1998).
Verotta, L. et al.,"Cycloartane saponins from Astragalus peregrinus as modulators
of lymphocyte proliferation", Fitoterapia (Netherlands) 72 (8): 894-905 (Dec 2001).
Watanabe, K. et al.,"Cycloartane glycosides from the rhizomes of Cimicifuga
racemosa and their cytotoxic activities", Chem. Pharm. Bull. (Japan) 50 (1) : 121-5 (Jan
2002).
Zhang, Q. W. et al.,"A new cycloartane saponin from Cimicifuga acerina", Journal
ofAsian Nat. Prod. Res. 2 (1) : 45-9 (1999).
Zhang, Q. W. et al.,"Cycloartane glycosides from Cimicifuga dahurica", Chem.
Pharm. Bull. (Japan) 49 (11): 1468-70 (Nov 2001).
Zhao, K. S. et al.,"Enhancement of the immune response in mice by Astragalus
membranaceus extracts", Immunopharmacology 20 (3): 225-33 (Nov-Dec 1990).
Zheng, Z. et al.,"Studies on chemical constituents and immunological function
activity of hairy root of Astragales nieinbranaceus", Chinesejournal of biotechnology
14 (2): 93-7 (1998).
Zhu, N. et al.,"Cycloartane triterpene saponins from the roots of Cimicifuga
foetida", J. Natural Products 64 (5): 627-9 (May 2001).
Telomerase
Telomerase is a ribonucleoprotein that catalyzes the addition of telomeric repeats to
the ends of telomeres. Telomeres are long stretches of repeated sequences that cap the
ends of chromosomes and are believed to stabilize the chromosome. In humans,
telomeres are typically 7-10 kb in length and comprise multiple repeats of the sequence
TTAGGG. Telomerase is not expressed in most adult cells, and telomere length
decreases with successive rounds of replication. After a certain number of rounds of
replication, the progressive shortening of the telomeres results in the cells entering a
telomeric crisis stage, which in turn leads to cellular senescence.
Certain diseases are associated with rapid telomeric loss, resulting in premature cell
senescence. Expression of the gene encoding the human telomerase protein in human
cells has been shown to confer an immortal phenotype, presumably though bypassing the
cells'natural senescence pathway. In addition, expression of the telomerase gene in aging
cells with short telomeres has been shown to produce an increase in telomere length and
restore a phenotype typically associated with younger cells.
References discussing these and other characteristics of telomerase include:
Allsopp, R. C. et al.,"Telomere shortening is associated with cell division in vitro and
in vivo", Exp. Cell Res. 220 (1) : 194-200 (Sep 1995).
Bodnar, A. G. et al.,"Extension of life-span by introduction of telomerase into normal
human cells", Science 279 (5349): 349-52 (Jan 16 1998).
Bodnar, A. G. et al.,"Extension of life-span by introduction of telomerase into normal
human cells"Science 279 (5349): 349-52 (Jan 16 1998).
Cech, T. et al., U. S. Patent No. 6,261, 836 (Jul 2001).
Chiu, C. P. et al.,"Replicative senescence and cell immortality: the role of telomeres
and telomerase"Proc. Soc. Exp. Biol. Med. 214 (2): 99-106 (Feb 1997).
Dagarag, M. et al.,"Differential impairment of lytic and cytokine functions in
senescent human immunodeficiency virus type 1-specific cytotox T lymphocytes", J.,
Virol. 77 (5) : 3077-83 (Mar 2003).
Farwell, D. G. et al.,"Genetic and epigenetic changes in human epithelial cells
immortalized by telomerase", American Journal of Pathology 156 (5) : 1537-47 (May
2000).
Fujimoto, R. et al.,"Expression of telomerase components in oral keratinocytes and
squamous cell carcinomas", Oral Oncology 37 (2): 132-40 (Feb 2001).
Funk, Walter D. et al.,"Telomerase expression restores dermal integrity to in vitro-
aged fibroblasts in a reconstituted skin model", JOURNAL : Experin7ental Cell Research
258 (2): 270-278 (Aug 1,2000).
Harle-Bachor, C. et al.,"Telomerase activity in the regenerative basal layer of the
epidermis inhuman skin and in immortal and carcinoma-derived skin keratinocytes", Proc.
Natl. Acad. Sci. USA 93 (13): 6476-81 (Jun 25 1996).
Harley, C. B. et al.,"Telomerase and cancer", ImportafitAdv. Oncol. 57-67 (1996).
Harley, C. B. et al.,"Telomerase, cell immortality, and cancer", Cold Spring Harb.
Snap. Quant. Biol. 59: 307-15 (1994).
Harley, C. B. et al.,"Telomeres and telomerase in aging and cancer", Curr. Opin
Genet. Dev. 5 (2): 249-55 (Apr 1995).
Harley, C. B. et al.,"Telomeres shorten during ageing of human fibroblasts"Nature
345 (6274): 458-60 (May31, 1990).
Harley, C. B. ,"Human ageing and telomeres", Ciba Found. Syinp. 211: 129-39
(1997).
Harley, C. B. ,"Telomerase is not an oncogene", Oncogene 21: 494-502 (2002).
Henderson, S. et al.,"In situ analysis of changes in telomere size during replicative
aging and cell transformation", J. Cell Biol. 134 (1) : 1-12 (Jul 1996).
Jiang, X. et al., PCT Pubn. No. WO 02/91999.
Jiang, X. R. et al.,"Telomerase expression in human somatic cells does not induce
changes associated with a transformed phenotype", Nature Genetics 21 (1) : 111-4 (Jan
1999).
Kang, M. K. et al.,"Replicative senescence of normal human oral keratinocytes is
associated with the loss of telomerase activity without shortening of telomeres", Cell
Growth &Differentiation 9 (1) : 85-95 (Jan 1998).
Kirs, N. W. etal., U. S. Patent No. 5,629, 154 (May 1997).
Mattson, M. P. ,"Emerging neuroprotective strategies for Alzheimer's disease: dietary
restriction, telomerase activation, and stem cell therapy", Exp Gerontol. 35 (4): 489-502
(Jul 2000).
Morales, C. P. et al.,"Absence of cancer-associated changes in human fibroblasts
immortalized with telomerase", Nature Genetics 21 (1) : 115-8 (Jan 1999).
Oh, H. and Schneider, M. D. ,"The emerging role of telomerase in cardiac muscle cell
growth and survival", JMol Cell Cardiol 34 (7): 717-24 (Jul 2002).
Simonsen, J. L. et al.,"Telomerase expression extends the proliferative life-span and
maintains the osteogenic potential of human bone marrow stromal cells", Nat Biotechnol
20 (6): 592-6 (Jun 2002).
Villeponteau, B. et al., U. S. Patent No. 5, 583, 016 (Dec 1996).
Yang, J. et al.,"Human endothelial cell life extension by telomerase expression",
Journal of Biological Chemistry 274 (37): 26141-8 (Sep 10 1999).
Yang, J. et al.,"Telomerized human microvasculature is functional in vivo", Nature
Biotechnology (United States) 19 (3): 219-24 (Mar 2001).
Yang, J., et al.,"Human endothelial cell life extension by telomerase expression", J.
Biol. Chem. 274 (37): 26141-8 (Sep 10 1999).
Summary of the Invention
The invention described herein is generally related to the discovery of the ability of
extracts of certain plant species, e. g. Astragales or Cimicifuga species, to activate
telomerase in cells. In particular embodiments, the plant is an Astragalus species, and in
further embodiments the plant is Astragalus membranaceus. Aspects of the invention
include formulations of such plant extracts for use in cosmetic, nutraceutical and
pharmaceutical applications, in particular in applications where increasing telomerase
activity in cells is desired.
Methods of using the plant extracts and formulations thereof for such applications are
also provided, as are methods for formulating the plant extract, and methods of applying
such formulations after the need for, or advantage of, increasing telomerase activity in
cells or tissues has been determined.
The extract used in the formulation and methods of the invention is preferably
obtained by extracting the plant material with a polar solvent selected from the group
consisting of water, lower alcohols, lower alkyl esters, lower alkyl ketones, chloroform,
and combinations thereof, preferably selected from water, lower alcohols, and
combinations thereof. An exemplary solvent is one containing at least 75% ethanol and
the remainder water, for example, 95% aqueous ethanol.
An extract ofAstragalus membranaceus root may be obtained, for example, in an
aqueous ethanolic solution, by a process that comprises:
(a) heating a mixture containing Astragalus membraslaceus root in a solvent of 95%
aqueous ethanol, preferably at reflux;
(b) filtering the solid from the resulting mixture;
(c) repeating steps (a)- (b) with the solid of step (b) and fresh solvent; and
(d) combining the filtrates from steps (b).
The extract may also be obtained as a solid, by removing the solvent from the combined
filtrates. In step (a) of the process, the mixture preferably includes about 0. Ig to 2. 5g of
root per 5 ml of solvent, e. g. about lg/5 ml. Preferably, the mixture is kept at room
temperature for about 0.5 to 1 hour prior to refluxing, and is refluxed for about 2 hours.
The concentration of the extract (based on weight of solid extract, exclusive of any
solvent) in the formulation is preferably in the range of 0. 1 to 100% (w/v). The extract
may also be, provided directly in solid form, without a vehicle or excipients. In this case,
the extract is typically provided as a dry powder or in pressed form as a pill or tablet.
In further embodiments, the concentration is in the range of 0. 1 to about 75% (w/v);
e. g. 1 to 50,5 to 25, or 10 to 15% (w/v). The extract is thus formulated in a vehicle that
is appropriate for the relevant application, whether it be a cosmetic for topical use,
nutraceutical for ingestion, or pharmaceutical for administration by a variety of routes
including topical, oral or injection. By way of example, a cosmetic formulation will
typically include the plant extract and one or more additional ingredients such as
emulsifiers, thickeners, and skin emollients. In selected embodiments, the cosmetic
formulation comprises an emulsifier and/or a skin emollient; in further embodiments, it
comprises at least a skin emollient. The emulsifier, thickener, and/or skin emollient is one
that is conventionally used in cosmetic formulations, as described further below.
In one aspect, the invention provides compositions and methods for conditioning the
skin. Such methods comprise applying topically to the skin a formulation comprising an
extract of an Astragalus or Cimicifuga species, preferably an extract of an Astragalus
species, e. g an Astragalus membranaceus extract, in a cosmetic formulation or vehicle.
In another aspect, the invention provides a method of increasing telomerase activity
in a cell or tissue, comprising contacting the cell or tissue with a formulation comprising
an extract of an Astragalus species, as described above. The biological activity of the
subject extract is such that, when formulated in a solvent at a concentration of 25 p. g/ml
or less, it is effective to produce a level of telomerase activity in keratinocytes or
fibroblasts, as measured in a TRAP assay, at least 50% greater than the level in said cells
treated with said solvent, as measured in a TRAP assay as described herein. In further
preferred embodiments, the extract is effective to produce a level of telomerase activity in
keratinocytes or fibroblasts, as measured in a TRAP assay, at least 100% greater than the
level in said cells treated with said solvent, as measured in a TRAP assay as described
herein. The assay, which is described in detail below, comprises applying a composition
to cells, typically keratinocytes or fibroblasts, and subsequently measuring telomerase
activity in the cells.
Also described herein is a"scratch assay"in which the ability of a composition to
increase the rate of closure of a scratch"wound"applied to a layer of cells, such as
keratinocytes, is determined. The biological activity of the subject extract is preferably
such that it is able to produce, at a concentration of 25, ug/ml or less, an amount of
wound closure (wound healing activity) in a scratch assay of keratinocytes or fibroblasts,
as described below, which is at least 25% greater than that seen in untreated or control
cells. Even more potent activities may be appropriate for some applications, such as
extracts that produce, at a concentration of 1 Ag/ml or less, an amount of wound closure
in a scratch assay of keratinocytes or fibroblasts which is at least about 50% or 100%
greater than that seen in untreated or control cells.
The methods of the invention that are directed to enhancing telomerase activity in a
cell or tissue, by contacting the cell or tissue with the extract or formulation, may further
comprise a prior step of identifying a cell or tissue in which induction of telomerase is
desired. This identification may entail, for example, diagnosing in a subject the presence
of a condition associated with telomerase deficiency, or subject to treatment by increasing
telomerase activity in cells or tissue of the subject. In a related aspect, the invention
provides the use of a composition comprising an extract of an Astragalus or Cimicifuga
species as described above, including the preferred embodiments described above, for the
manufacture of a medicament for treating a condition subject to treatment by increasing
telomerase activity in a cell or tissue.
The range of beneficial effects that may be achieved by telomerase activation include,
for example: more rapid wound healing; the slowing of telomere loss occurring during
aging of cells; postponing or reversing cellular senescence in disease conditions associated
with cellular senescence; treating a disease condition associated with cells having a higher
rate of cell division than normal cells of that cell type; treating a disease condition in
which one or more cell types are limiting; and reducing telomere repeat loss while
expanding cell number ex vivo, e. g. for use in cell-based therapies. Disease conditions
subject to treatment by an increase in telomerase activity include HIV infection and
degenerative disease, such as neurodegenerative disease, degenerative disease of the
bones or joints, macular degeneration, atherosclerosis, and anemia, as discussed further
below, as well as wounds or other acute or chronic condition of the epidermis. Also
included are explant cells obtained from a patient, where the contacting is done ex vivo.
In a further aspect, the invention provides a cosmetic composition comprising an
extract of an Astragalus species, as described above, present at a concentration (based on
weight of solid extract, exclusive of solvent) of at least about 2.5% (w/v), up to about
75%, preferably up to about 50% (w/v), in a cosmetic formulation or vehicle. Preferably,
the species is Astragalus membranaceus, and the extract is obtained from the root of the
plant. The extract may be obtained by the processes described above and preferably has
activity in a telomerase activation assay or wound closure assay as described above. The
cosmetic formulation or vehicle will typically include at least one ingredient selected from
the group consisting of an emulsifier, a thickener, and a skin emollient. The amount of
the extract in the cosmetic composition is preferably at least about 5% (w/v), e. g. about 5
to 50% or 5 to 25% (w/v). In other embodiments the amount of the extract in the
cosmetic composition may be at least about 10% (w/v), e. g. about 10 to 50% or about 10
to 25% (w/v).
In a further aspect, the invention provides a method of selecting an extract which is
effective to increase telomerase activity in cells, by assaying a plant extract (preferably an
extract of a flowering vascular plant, such as an herb) in a TRAP assay of keratinocytes or
fibroblasts, as described further below, and selecting the extract if it produces a level of
telomerase activity in the cells, at a concentration of 25, ug/ml, that is at least 50% greater
than the level measured in a solvent control. The active extract can then be formulated in
a pharmaceutical or cosmetic vehicle.
These and other objects and features of the invention will become more fully apparent
when the following detailed description of the invention is read in conjunction with the
accompanying drawings.
Brief Description of the Drawings
Figure 1 shows the results of a TRAP assay of telomerase activity of an Astragalus
niembratiaceus root extract, designated GRN139925, in young neonatal keratinocytes;
Figure 2 shows the results of a similar assay in aging adult keratinocytes;
Figure 3 shows the results of a similar assay in young neonatal fibroblasts;
Figures 4A-D and 5A-D show the results of screening Astragalus membranaceus
root extracts, obtained using various solvents, for effectiveness in increasing telomerase
activity;
Figure 6 is a series of computer-generated images showing wound healing activity of
anAsíragalus membranaceus root extract, as measured in a"scratch assay"in aging adult
keratinocytes;
Figure 7 is a series of computer-generated images showing wound healing activity of
an Astragalus membranaceus root extract, as measured in a"scratch assay"in late
passage neonatal keratinocytes;
Figure 8 is a series of computer-generated images showing wound healing activity of
an Astragalus menabranaceus root extract in aging adult keratinocytes, as compared to
PDGF (platelet derived growth factor);
Figure 9 is a graph showing the result of an assay such as shown in Fig. 7, run in the
presence of mitomycin C, with data expressed as the percent of the"wound"area created
by the scratch which remains (that is, is not covered by cells);
Figure 10 is a graph showing the wound healing activity of an Astragalus
membi, anaceus root extract in aging neonatal keratinocytes, in the presence or absence of
a telomerase inhibitor, and in comparison to PDGF; and
Figures 11-12 show the results of short term (Fig. 11) and long term (Fig. 12) assays
evaluating the protection of adult keratinocytes from cell death by an astragales
membranaceus root extract and by AdhTERT (adenovirus human telomerase protein
component).
Detailed Description of the Invention
I. Definitions
The following terms have the meanings given below, unless indicated otherwise.
"Conditioning the skin"includes such effects as improving the appearance, elasticity,
thickness, or smoothness of skin, protecting skin from UV radiation, healing
photodamaged skin, and/or reducing signs of skin aging, such as excessive dryness or
wrinkling. Such signs of aging may be macroscopic, i. e. visually or tactilely apparent skin
features, or they may be on a more microscopic or cellular level, such as cellular
senescence of skin cells.
A"cosmetic vehicle"or"cosmetic formulation"or"cosmetically acceptable vehicle"
refers to a composition formulated in a manner that is suitable for application to the skin,
e. g. as a cream, gel, lotion, or ointment, and containing one or more components such as
emulsifiers, surfactants, thickeners, emollients, and lubricants. Such a vehicle is not
intended or necessarily suitable for internal consumption.
A"safe and effective amount"refers to an amount sufficient to induce a significant
benefit, but to minimize undesired side effects ; i. e. to provide a reasonable risk to benefit
ratio.
By"effective to increase telomerase activity in a cell", with reference to an extract as
described herein, is meant that a composition containing the extract at a concentration of
25 Ag/ml or less (based on solid weight) is effective to produce a level of telomerase
activity in a keratinocyte or fibroblast cell, as measured in a TRAP assay as described
herein, which is greater, by a factor of at least 1. 5 (i. e. at least 50% greater), than the
level produced by a similar formulation not containing the extract, as measured in a TRAP
assay in said cells. In preferred embodiments, the extract is effective, at a concentration
of 25 p. g/ml or less, to produce a level of telomerase activity in such a cell, as measured in
a TRAP assay as described herein, which is greater by a factor of at least 2 (i. e. at least
100% greater) than the level produced by a similar formulation not containing the extract.
In reference to administration of an extract to a patient, an"effective amount"refers
to an amount of extract effective to increase telomerase activity in the cells or tissue of
the patient, such that a desired therapeutic result is achieved. In reference to treatment of
cells in vitro or ex vivo, an"effective amount"refers to an amount effective to increase
telomerase activity in the cells, thereby increasing the replicative capacity and/or life span
of the cells.
In concentrations expressed herein as % (w/v), 100% (w/v) corresponds to 1 g
extract (solids)/ml vehicle. Concentrations present in formulations refer to weight of solid
extract, exclusive of solvent.
A"vascular plant"refers to a plant which possesses a system of conducting tissue to
transport water, mineral salts and sugars.
An"herb"refers to a plant whose stem does not produce woody, persistent tissue
and generally dies back at the end of each growing season.
A plant"extract", as used herein, refers to the material resulting from exposing a
plant part to a solvent and removing the solvent. When the solvent used for extraction is
retained rather than removed, an extract solution is obtained. The material may also
undergo further purification, e. g. chromatographic separation into fractions.
"Lower alkyl"refers to an alkyl group having one to four carbon atoms, and, in
selected embodiments, 1-2 carbon atoms (methyl or ethyl).
A"lower alcohol"is an alkanol having one to four carbon atoms; e. g., methanol,
ethanol, isopropanol, or butanol. In selected embodiments, the lower alcohol is ethanol.
II. Telomerase Activating Extracts
A. Plant Sources
In one embodiment, the species extracted is Astragalus membranaceus, also referred
to as Radix astragali, and also known by names such as Chinese Astragalus, Chinese
milkvetch, Huang Qi, membranous milkvetch, and yellow vetch. However, extracts of
other plant species, particularly other Astragalus species and species of Cimicifuga,
having the desired properties may also be used. Indices of species of the Astragalus and
Cimicifuga genus are available from various taxonomic reference sources, such as
textbooks or online sources. For example, the Integrated Taxonomic Information System
(IT IS) of the USDA maintains a searchable website, and a search of the genus Astragalus
produced a list containing 619"accepted"and 296"not accepted"species. The website
"GardenWeb"also includes a searchable database of various plant species, and a search of
the genus Astragalus yielded information on 647 species. The genus Cimicifuga is much
smaller, having about 15 species reported by these two sources.
Such species include, but are not limited to, species reported to contain components
similar to components ofA. rzembranaceus, such as A. trojans (Bedir, 2001) ; A.
zahlbruckneri (Calis, 2001); A. brachypterus, A. microcephalus (Bedir, 1998); A.
peregrinus (Verotta, 2001); A. caprinus (Semmar, 2001); A. melarzophrurius (Calis,
1997); A. oleifolius (Calis, 1996); A. trigonus (Gariboldi, 1995); A. spit7osus (Abdallah,
1993); A. verrucosus (Pistelli, 2002); C. racemosa (Watanabe, 2002); C. dal7urica
(Zhang, 2001); C. foetida (Zhu, 2001); and C. acerina (Zhang, 1999), all cited above.
B. Extraction Methods
An exemplary procedure for extracting the plant material, which is not intended to be
limiting, is as follows. In a preferred embodiment, the root of the plant is extracted;
however, other plant parts, such as stems, leaves, or flowers, may also be employed.
A mixture containing the plant material, e. g. Astragalus memb7 anaceus root
segments, is heated in a polar solvent selected from the group consisting of water, lower
alcohols, lower alkyl esters, lower alkyl ketones, chloroform, and combinations thereof.
Preferably, the solvent is selected from the group consisting of water, lower alcohols, and
combinations thereof. Exemplary solvents include 75% and 95% aqueous ethanol. The
ratio of plant material to solvent is typically about 1-5 g or less for every 5 ml of solvent,
more typically 1 g or less for every 5 ml of solvent. Heating the mixture generally
comprises refluxing the solvent for about 0.5 to 3 hours, e. g. about 2 hours. The solid is
then filtered from the mixture, and is preferably extracted again, in a similar manner, with
fresh solvent. Again, the solid is filtered from the mixture, and the combined filtrates
(solvent components) are concentrated to obtain the extract. In some cases, some or all
of the extraction solvent may be retained, if its presence in the final formulation is
acceptable.
An exemplary extraction procedure used to prepare an Astragalus membranaceus
root extract, designated GRN925, is provided in Example 1.
llI. Biological Activity
The extracts disclosed herein as active ingredients of the subject compositions are
active in inducing telomerase activity in normal cells. Telomerase is a species-specific
ribonucleoprotein that catalyzes the addition of oligonucleotide repeats (telomeres) onto
the ends of chromosomal DNAs, to compensate for losses that occur with each round of
DNA replication. Somatic cells, in contrast to tumor cells and certain stem cells, have
little or no telomerase activity and stop dividing when the telomeric ends of at least some
chromosomes have been shortened to a critical length, leading to programmed cellular
senescence (cell death). Accordingly, an increase in telomerase activity is expected to
inhibit cell death, and to promote cell proliferation.
A. TRAP Assay Protocol
The ability of a substance to increase telomerase activity in a cell can be determined
using the TRAP (Telomeric Repeat Amplification Protocol) assay, which is known in the
art (e. g. Kim et al., U. S. Patent No. 5,629, 154; Harley et al., U. S. Patent No. 5,891, 639).
As used herein, "telomerase activity as measured in a TRAP assay"refers to telomerase
activity as measured in keratinocytes or fibroblasts according to the following protocol.
The activity is typically compared to the activity similarly measured in a control assay of
such cells (e. g., a telomerase activity 50% greater than observed in a solvent control).
Cell lines suitable for use in the assay, preferably normal human fibroblasts (NHF) or
normal human keratinocytes (NHK), can be obtained from commercial sources, such as
Cascade Biologics, Portland, OR or 4C Biotech, Seneffe, Belgium, or from the ATCC
(American Type Culture Collection). ATCC normal human fibroblast cell lines, which
can be located on the ATCC web site, include, for example, CCL135, CCL137, and
CCL151.
Cells are plated at approx. 5000 cells/well, in growth medium (e. g. Epi-Life Medium
+ Keratinocyte Growth Factor Supplement + 60 mM CaCl2, supplied by Cascade
Biologics, Inc. ) for two days. Test compositions in a suitable solvent, such as 95%
ethanol or DMSO, are added to selected wells in a range of concentrations and incubated
for 16-24 hours. For the data reported herein, the solvent used was DMSO.
Cell lysing solution is prepared by addition of 3. 0 mL Nonidetd3 P40,1. 0 mL CHAPS
lysis buffer (see below), and 1.0 mL 10X TRAP buffer (see below) to 5.0 mL DNase-,
RNase-free H2O. (DNase-, RNase-free water may be generated by DEPC
(diethylpyrocarbonate) treatment or purchased from vendors such as Sigma.)
The morphology of treated cells is first observed under a microscope, to verify that
there are no visual signs of irregular growth. Media is removed from the wells, and the
cells are rinsed twice in PBS (Ca and Mg free). The dishes are chilled, preferably on ice,
and cell lysis buffer (see below) is added (approx. 100 Al per well) and triturated by
pipetting up and down several times. The cells are the incubated on ice for 1 hour.
CHAPS Lysis Buffer
Stock For 1 mL Final concn.
1 M Tris-HCl pH 7.5 10 ut 10 mu
1 MMgCl2 1 µl 1 mM
0. 5MEGTA 2ul ImM
100 mM AEBSF 1 pl 0.1 mM
10% CHAPS'50 ul 0.5%
BSA 1 mg 1 mg/ml
100% Glycerol 100 ul 10%
DNase-, Rase-free H20 936 ul (to lmL)
"The CHAPS detergent should be added just before use of the lysis buffer. In addition, AEBSF (4-
(2-aminoethyl)-benzenesulfonyl fluoride hydrochloride) should be added to the lysis buffer just
prior to performing the extraction step.
10X TRAP Buffer
Stock For 5 ml Final concn.
1M Tris-HCl, pH 8. 3 1 ml 200 mM
1M MgCl2 75 µl 15 mM
1M KCl 3. 15 ml 630 mM
Tween 20 (Boehringer Mannheim) 25 Rl 0. 5%
0. 1M EGTA 500 µl
20 mg/ml BSA 250 µl 1 mg/ml
The following materials are combined to generate a master PCR Mix.
Stock Per Reaction (40 Fl) Final concn. a
1 OX TRAP Buffer 5.0 ul ix
2. 5 mM dNTPs 1.0 Ill 50 uM
Cy5-TS Primer (0.1 mg/ml) 0.2 1ll 0.4 ng/ml
ACX Primer (0. 1 mg/ml) 1. 0 µl 2 ng/ml
TSU2 Int. Std. (1 pg/ml) 1. 0 µl 20 fg/ml
U2 Primer (0. 1 mg/ml) 1. 0p1 2ng/ml
Taq Polymerase (5U/1ll) 0.4 µl 2 units
DNase-, RNase-free H20 30.4 µl (to 40 l total)
aBased on final volume of 40 il PCR mix plus 10 jj. l cell lysate = 50 jj. l.
The PCR mix includes the following components: Cy5-TS primer, a 5'-Cy5 labeled
oligonucleotide having the sequence 5'-AAT CCG TCG AGC AGA GTT-3' (SEQ ID
NO : 1), is a telomerase substrate. Depending on the telomerase activity of the medium,
telomer repeats (having the sequence.. AGGGTT..) will be added to the substrate, to
form telomerase extended products, also referred to as telomerase products or TRAP
products. The ACX primer, having the sequence 5'-GCG CGG CTT ACC CTT ACC
CTT ACC CTA ACC-3' (SEQ ID NO: 2), is an anchored return primer that hybridizes
to the telomerase extended products.
The TSU2 internal standard, an oligonucleotide having the sequence 5'-AAT CCG
TCG AGC AGA GTT AAA AGG CCG AGA AGC GAT-3' ; SEQ ID NO : 3), an
extension of the TS primer sequence, is added in a small controlled quantity for
quantitation purposes. The U2 primer, having the sequence 5'-ATC GCT TCT CGG
CCT TTT (SEQ ID NO : 4), is a return primer designed to hybridize to the 3'region of the
internal standard.
A sample of cell lysate (10 pL) is added to 40 µL of this PCR mix in a reaction tube,
and the mixture is incubated at room temperature (30°C) for 30 minutes. PCR is carried
out by incubating the mixture at the following temperatures for the times indicated:
94°C/30 sec, 60°C/30 sec, and 72°C/30 sec; repeating this three-step cycle to conduct 20-
30, preferably 31 cycles.
Loading dye containing e. g. bromophenol blue and xylene cyanol is added, and the
samples are subjected to 10-15% non-denaturing PAGE in 0.6x TBE, until the
bromophenol blue runs off the gel. Product formation is observed, e. g. by using a
fluoroimager for detection of CY5-labeled telomerase products (maximal excitation at
650 nm ; maximal emission at 670 nm).
The final amount of TSU2 internal standard after amplification is generally 5-10 amol
per 50 ul reaction mixture. This internal control gives a specific 36-mer PCR
amplification product that appears as a distinct band on the gel below the first telomer
addition product (that is, the product of one telomer addition to the TS oligonucleotide,
followed by amplification with the ACX return primer). This internal control band can be
used to normalize the PCR amplifications from different samples.
The relative number of telomerase product molecules (TM) generated in the assay is
determined according to the formula below:
TM = (TTRAP ProductsTBKD1)/ (TlNt StdTBKD2)
where: TTRAP products is the total intensity measured on the gel for all telomerase products,
TBKD1 is the background intensity measured in a blank lane for an area equivalent in size to
that encompassed by the telomerase products, Tnt std is the intensity for the internal
standard band, and TBKD2 is the background intensity measured in a blank lane for an area
equivalent in size to that encompassed by the internal standard band. The resulting
number is the number of molecules of telomerase products generated for a given
incubation time, which, for the purposes of determining TM, is designated herein as 30
minutes.
The activity of the subject extract is preferably such that, at a concentration of 25
, Lg/ml or less, it is able to produce a telomerase activity at least about 25% greater than
that measured for a solvent control, and more preferably at least about 50% greater than
that measured for a solvent control, as measured in a TRAP assay.
B. Exemplary TRAP Assay Results
Cell lines used in these experiments were obtained from Cascade Biologics, Inc.
Neonatal keratinocytes (HEKneo-P) were obtained from a pool generated from three
donors, designated HEKn (12), PD 8.46 ; HEKn (15), PD 9.3 ; and HEKn (16), PD 5.16.
Adult keratinocytes were obtained from a single donor, designated HEKa (18). The terms
"neonatal"and"adult"refer to the age of the donor, while the terms"young"and"aging"
or"late passage"refer to the age of the cell culture, and correspond to the number of
population doublings (indicated as PD no.).
Activation of telomerase was evaluated for compositions containing a 95% aqueous
ethanol extract of Astragalus membranaceus root, prepared according to the procedure
described in Example 1, and designated herein as GRN925. Various formulations of the
extract GRN925 were assayed for telomerase activation in young (PD8) neonatal
keratinocytes (Fig. 1), aging (PD34) adult keratinocytes (Fig. 2) and young (PD10)
neonatal fibroblasts (Fig. 3), using a TRAP (telomerase repeat amplification protocol)
assay, as described above.
Data is presented in Figs. 1 and 3 as telomerase activity relative to control, and in
Fig. 2 as TPG, or"total product generated", determined as described in U. S. Patent No.
5,891, 639. As can be seen from the Figures, telomerase activity was significantly greater
than in the control in assays of compositions containing the extract at concentrations of
25 pg/ml or higher. For example, the composition of Fig. 1 containing 25 pg/ml of
extract produced a telomerase activity at 170% of control.
The extract was shown not to increase telomerase activity in KB carcinoma cells,
where such activity is already expected to be high (leading to abnormal proliferation). In
this assay, telomerase activity was in fact lower in GRN925-treated cells (12 u. g/ml and
25 tg/rnl) than in the untreated cells.
Screening assays were also conducted on compositions containing extracts obtained
using several different solvents (pet ether, n-hexane, chloroform, ethyl acetate, acetone,
70% aqueous ethanol, 95% aqueous ethanol, and water) and fractionated by HPLC. As
shown in Figs. 4A-D and 5A-D, TRAP assays employing numerous fractions showed
telomerase activity more than 100% greater than seen in control cells, with activity
generally increasing in extracts from more polar solvents.
C. Wound Healing Assay Protocol
Wound healing activity of compositions containing the extracts can be evaluated,
preferably in keratinocytes or fibroblasts, via a"scratch assay", carried out as follows:
Cells are plated in flasks (5 x 105 cells per flask) and cultured for two days in a
humidified chamber at 5% C02, 37°C. To create the"wound", a 2 ml plastic pipette is
gently dragged to"scratch"the cell surface. The ideal wound is approximately 2-3 mm
wide and 50 mm long (along the long axis of the tissue culture flask). The cells are
retreated with medium containing either vehicle (DMSO; control sample) or test
compositions at multiple concentrations. A wound area is identified, the flask marked,
and the appearance of the cells documented photographically over 3-4 days continued
culturing of the cells.
Amount of wound closure is determined by measuring the width of the wound over
time for extract-treated samples relative to vehicle-treated or other control cells.
Measurements are made from the photographs taken for each of the samples on days 1
(immediately after scratching), 2,3, and 4. Percentage of wound healing is calculated by
the following formula:
WH=100- [100xWn/Wo],
where Wn is the width of the wound on day n and Wo is the width of the wound on day
one (immediately after scratching).
The activity of the subject extract is preferably such that it is able to produce, at a
concentration of 25 u, g/ml or less, an amount of wound closure (wound healing activity)
in a scratch assay of keratinocytes or fibroblasts which is at least 25% greater than that
seen in untreated or control cells. Even more potent activities may be appropriate for
some applications, such as extracts that produce, at a concentration of 1, ug/ml or less, an
amount of wound closure in a scratch assay of keratinocytes or fibroblasts which is at
least about 50% or 100% greater than that seen in untreated or control cells.
D. Exemplary Scratch Assay Results
Results of typical scratch assays are shown in Figs. 6-7, where the top row of images
shows control cells, and the bottom row shows cells treated with 25 ßg/ml GRN925. Fig.
6 shows an assay employing aging (PD34) adult keratinocytes, and Fig. 7 shows an assay
employing late passage (PD40) neonatal keratinocytes. In both cases, the treated cells
were nearly confluent at day 3 and fully confluent at day 4, in contrast to the control cells,
in which a sizable"wound"remained at day 4.
The activity of the extract in promoting healing was similar to that of PDGF (platelet
derived growth factor), as shown in Fig. 8 (aging adult keratinocytes). Both treatments
(second and third row of images) restored the cells to a confluent or near-confluent state
by day 4, in contrast to the control cells (top row of images).
The following table shows WHcntrl and WHtest values for the compositions employed
in the scratch assays shown in Figs. 6-8, based on the results of those assays, using the
formula shown above.
Approx. wound width (arbitrary units) WHcntrl WHtest
Dayl Day4 Dayl Day4
cntl cntl test test
Fig. 6 18 8 14 0 55. 6 100. 0
Fig. 7 22 9 19 0 59.1 100.0
Fig. 8 22 11 17 4 50.0 76.5
A similar assay was run in the presence of 10 pM : GRN163, a telomerase inhibitor.
(GRN163 is an oligonucleotide that targets the template region of the telomerase RNA
component. Specifically, GRN163 is a specific 13-mer N3'OP5'thiophosphoramidate
oligonucleotide; it is described in detail in PCT Pubn. No. WO 01/18015.) The results
demonstrated that the wound healing activity of the extract composition is telomerase-
dependent, as there was no apparent difference between the treated and the control cells
in this assay.
The wound healing activity of the extract composition was also reduced by the
presence of an antiproliferative agent, mitomycin C, as shown in Fig. 9 (aging adult
keratinocytes), demonstrating that the activity is both migration and proliferation
dependent. A significant level of activity was retained under these conditions, providing
evidence that telomerase activation can benefit non-dividing cells.
The wound healing activity of the extract composition, in the presence or absence of
a telomerase inhibitor, and in comparison to PDGF (platelet derived growth factor), is
shown graphically in Fig. 10 (aging neonatal keratinocytes). As shown, both the extract
composition and PDGF produced complete or near-complete wound closure after four
days, in contrast to control cells (about 50% closure) and cells treated with the extract
and the telomerase inhibitor GRN163 (about 45% closure).
E. Inhibition of UV-Induced Cell Death
Protection of adult keratinocytes from cell death by the extract was comparable to
that of AdhTERT (adenovirus human telomerase protein component), as shown in Figs.
11-12. Both short term (Fig. 11) and long term (Fig. 12) photoaging was studied,
according to the protocol described in Example 2.
As shown in Figs. 11 and 12, minor differences in levels of apoptosis were observed
between treated and untreated cells which were not exposed to UVB radiation. However,
for cells exposed to 7. 5- 10 Mj/cm2UVB radiation, significant differences were observed,
particularly in the long-term assay (Fig. 12). For example, in cells exposed to 7.5 mJ/cm2
UVB, about 32% apoptosis was observed for untreated cells, but only about 13%
apoptosis was observed for cells treated with 25 jj. g/ml GRN925.
IV. Cosmetic Compositions and Methods
In one aspect, the invention provides a method for conditioning the skin, regulating
signs of skin aging, and/or protecting the skin from UV radiation. In accordance with the
method, a formulation comprising, as an active ingredient, an extract of an Astragalus
species, in a cosmetic vehicle, as defined further below, is applied topically to the skin.
Also part of the invention is a cosmetic composition containing such an extract in a
cosmetic vehicle. As demonstrated below, the composition is effective to induce
telomerase activity in cells and to protect the cells from UV-induced apoptosis. Benefits
of such activity are manifested in protection of skin from radiation, suppression of signs of
aging in the skin, and promotion of healing.
The active ingredient (i. e. a telomerase inducing plant extract) can be present at
various levels, i. e. about 0.1 to about 25% (w/v) or more in the cosmetic formulation,
preferably up to about 75% (w/v), more preferably up to about 50% (w/v). In selected
embodiments, the formulation contains about 1-10,2. 5-25,5-10, 5-15, 5-25, 5-50,10-15,
10-25, or 15-25% (w/v) of the extract. In other embodiments, the extract is present at at
least 5%, at least 10%, at least 15%, at least 20%, or at least 25% (w/v) of the
formulation.
The formulation contains other ingredients conventional to cosmetic formulations, as
described further below.
A. Cosmetic Vehicle
Al. Product Forms
The subject compositions may include a wide variety of product forms, including, for
example, lotions, creams, gels, ointments, sticks, sprays, or pastes. These product forms
may comprise several types of carriers, including, but not limited to, solutions, aerosols,
emulsions, gels, solids, and liposomes. The carrier is frequently formulated as an
emulsion, as described further below.
When the composition is formulated as an ointment, it may comprise a simple carrier
base of animal or vegetable oils or semi-solid hydrocarbons, or an absorption ointment
base which absorbs water to form an emulsion. Aerosols can be formed by adding a
propellant, such as halogenated hydrocarbons known in the art, to a solution of the
subject composition in a carrier such as described above. Aerosols are typically applied to
the skin as a spray-on product.
The compositions of the present invention comprise a dermatologically acceptable
carrier, within which the active ingredient and other components are incorporated, to
allow these components to be delivered to the skin at an appropriate concentration. The
carrier may contain one or more dermatologically acceptable solid, semi-solid or liquid
fillers, diluents, solvents, extenders and the like. The carrier may be solid, semi-solid or
liquid; preferred carriers are substantially liquid. The carrier should be physically and
chemically compatible with the active ingredient and other components described herein.
Preferred carriers contain a dermatologically acceptable, hydrophilic diluent; e. ., water,
lower monovalent alcohols, low molecular weight glycols and polyols, such as propylene
glycol, polyethylene glycol, polypropylene glycol, glycerol, butylene glycol, 1,2, 4-
butanetriol, sorbitol esters, 1,2, 6-hexanetriol, and butanediol, ethoxylated ethers,
propoxylated ethers, and combinations thereof. Water is a preferred diluent. The
composition preferably comprises from about 60% to about 99% of the hydrophilic
diluent.
In one embodiment, the formulation comprises an emulsion containing a hydrophilic
phase, e. g., water or other hydrophilic diluent, and a hydrophobic phase, e. g., a lipid, oil
or oily material, where one phase is dispersed in the other, continuous, phase. Examples
are oil-in-water emulsions, water in oil emulsions, and water-in-silicone emulsions.
Generally, the emulsion contains about 1% to 98% of the hydrophilic phase and about 1%
to 50% of the hydrophobic phase. The emulsion may also comprise a gel network or a
multiphase emulsion.
Preferred emulsions have an apparent viscosity at room temperature of from about
5,000 to about 200,000 centipoise (cps), depending on the physical form of the
formulation. For example, a lotion may have an apparent viscosity of from about 10,000
to about 40,000 cps, and a cream may have an apparent viscosity of from about 60,000 to
about 160,000 cps.
Suitable hydrophobic components employed in emulsions include, for example,
vegetable oils, e. g. safflower oil, coconut oil, cottonseed oil, palm oil, soybean oil, and the
like, which may be hydrogenated; animal fats and oils, such as lanolin; mineral oil;
petrolatum, or petroleum jelly; or C7 to C40 hydrocarbons, e. g. such as dodecane,
squalane, cholestanes, hydrogenated polyisobutylene, docosane, and various isoparaffins
(branched hydrocarbons). Also suitable are esters of Cl-C30 carboxylic acids and of C2-
C30 dicarboxylic acids, where the alcohol component is derived from C1-C30 alcohols,
glycols, or glycerols. Examples include, but are by no means limited to, isopropyl
myristate, methyl palmitate, myristyl propionate, cetyl palmitate, dioctyl maleate, dioctyl
sebacate, caprylic/capric triglyceride, PEG-8 caprylic/capric triglyceride, and ethylene
glycol distearate; as well as propoxylated and ethoxylated derivatives thereof.
C1-C30 mono-and polyesters of sugars or other polyol moieties may also be used, as
is known in the art, and include, for example, liquid materials such as glucose tetraoleate,
glucose and mannose tetraesters of soybean oil fatty acids, galactose tetraesters of oleic
acid, sorbitol hexaesters of unsaturated soybean oil fatty acids, and sucrose octaoleate.
Solid materials include, for example, a sucrose polyester in which the degree of
esterification is 7-8, and in which the fatty acid moieties are C 18 mono-and/or di-
unsaturated and behenic. Esters suitable for use in cosmetic emulsions are further
described in, for example, U. S. Patent. Nos. 4,005, 196,5, 306,516, 4,797, 300, and
4,518, 772. Also useful are C4-C20 alkyl ethers of polypropylene glycols, e. g PPG-14
butyl ether, PPG-15 stearyl ether, dioctyl ether, dodecyl octyl ether, and mixtures thereof.
The hydrophobic component employed in an emulsion may also be an
organopolysiloxane oil, such as disclosed in U. S. Patent No. 5,069, 897 (Orr). Examples
of suitable organopolysiloxane oils include polyalkylsiloxanes, cyclic polyalkylsiloxanes,
and polyalkylarylsiloxanes. Commercially available polyalkylsiloxanes include the
polydimethylsiloxanes, which are also known as dimethicones, examples of which include
the Vicasiff series (General Electric) and the Dow Corning 200 series. Examples of
alkyl-substituted dimethicones include cetyl dimethicone and lauryl dimethicone.
Commercially available cyclic polyalkylsiloxanes include the cyclomethicones. Also useful
are materials such as trimethylsiloxysilicate, such as that sold as a mixture with
dimethicone as Dow Corning 593 fluid, and polyalkylaryl siloxanes.
A2. Components
Formulations of the present invention, particularly emulsions, preferably include one
or more components selected from emulsifiers, surfactants, structuring agents, thickeners,
and emollients, as described below.
A2 (a). Emulsifiers and Surfactants
An emulsifier and/or surfactant is employed to disperse and suspend the
discontinuous phase within the continuous phase. The surfactant should be hydrophilic
enough to disperse in the hydrophilic phase; preferred surfactants are those having an
HLB of at least about 8. The choice of surfactant will also depend upon the pH of the
composition and the other components present.
Preferred hydrophilic surfactants are selected from nonionic surfactants, including
those broadly defined as condensation products of long chain alcohols, e. g. C8-30
alcohols, with sugar or starch polymers, i. e. , glycosides. Commercially available examples
include decyl polyglucoside (available as APG 325 CS from Henkel) and lauryl
polyglucoside (available as APG 600 CS and 625 CS from Henkel). Other useful
nonionic surfactants include alkylene oxide esters and diesters of fatty acids, and alkylene
oxide ethers of fatty alcohols, as well as the condensation products of alkylene oxides
with both fatty acids and fatty alcohols. Nonlimiting examples of alkylene oxide-derived
nonionic surfactants include ceteth-12, ceteareth-10, steareth-12, PEG-10 stearate, PEG-
100 stearate, PEG-20 glyceryl stearate, PEG-80 glyceryl tallowate, PEG-30 glyceryl
cocoate, PEG-200 glyceryl tallowate, PEG-8 dilaurate, PEG-10 distearate, and mixtures
thereof. Still other useful nonionic surfactants include polyhydroxy fatty acid amides,
such as coconut alkyl N-methyl glucoside amide.
The hydrophilic surfactants useful herein can also include any of a wide variety of
cationic, anionic, zwitterionic, and amphoteric surfactants such as are known in the art.
See, e. g., McCutcheon's, Detergents and Emulsifiers, North American Edition (1986),
published by Allured Publishing Corporation; or U. S. Patent No. 5,011, 681 (Ciotti et al.).
Cationic surfactants include, for example, cationic ammonium salts, such as quaternary
ammonium salts, and amino-amides. Anionic surfactants include the alkoyl isethionates
(e. g., C12-C30), alkyl and alkyl ether sulfates and phosphates, alkyl methyl taurates, and
alkali metal salts of fatty acids. Examples of amphoteric and zwitterionic surfactants
include derivatives of aliphatic secondary and tertiary amines in which one aliphatic
substituent contains from about 8 to about 22 carbon atoms and one contains an anionic
water solubilizing group, e. g., carboxy, sulfonate, sulfate, phosphate, or phosphonate.
Examples are alkyl imino acetates, iminodialkanoates and aminoalkanoates, imidazolinium
and ammonium derivatives. Other suitable amphoteric and zwitterionic surfactants include
betaines, sultaines, hydroxysultaines, alkyl sarcosinates (e. g., C12-C30), and alkanoyl
sarcosinates.
Silicone containing emulsifiers or surfactants include dimethicone copolyols, i. e.
polydimethyl siloxanes having polyether side chains, as well as dimethicone copolyols
modified with pendant alkyl, cationic, anionic, amphoteric, and zwitterionic moieties.
Dimethicone copolyol emulsifiers useful herein are described, for example, in U. S. Patent
No. 4,960, 764 (Figueroa, Jr. et aL) ; G. H. Dahms etal., Cosmetics & Toiletries, vol. 110,
pp. 91-100,1995 ; M. E. Carlotti et al., J. Dispersion Science & Technology, 13 (3), 315-
336 (1992); P. Hameyer, HAPPI 28 (4), pp. 88-128 (1991); J. Smid-Korbar et al., Intl
Journal of Cosmetic Science, 12, 135-139 (1990); and D. G. Krzysik et al., Drug and
Cosmetic Industry, vol. 146 (4) pp. 28-81 (1990).
A2 (b). Structuring Agents
The subject formulations, particular when in the form of an oil-in-water emulsion,
may contain a structuring agent, preferably at a level of about 2% to about 9%. Preferred
structuring agents are those having an HLB (hydrophile-lipophile balance) of about 1-8
and a melting point of at least about 45°C. Suitable structuring agents include, for
example, saturated C14 to C30 fatty alcohols or amines, which may contain 1 to about 5
moles of ethylene oxide; saturated C 16 to C30 diols; saturated C 16 to C30 monoglycerol
ethers; C14 to C30 saturated fatty acids, which may be hydroxylated or ethoxylated; C14
to C30 saturated glyceryl monoesters having a monoglyceride content of about 40% or
more; C14 to C30 saturated polyglycerol esters having from about 1 to about 3 alkyl
groups and from about 2 to about 3 saturated glycerol units; C14 to C30 glyceryl
monoethers; C14 to C30 sorbitan mono/diesters or saturated methyl glucoside esters,
which may be ethoxylated and/or contain 1 to about 5 moles of ethylene oxide; C14 to
C30 saturated sucrose mono/diesters ; C14 to C30 saturated polyglucosides having an
average of 1 to 2 glucose units, and mixtures thereof. In selected embodiments, the
structuring agent includes stearyl alcohol, cetyl alcohol, behenyl alcohol, a polyethylene
glycol ether of stearyl or cetyl alcohol having an average of about 2 ethylene oxide units,
and mixtures thereof.
A2 (c). Thickeners and Gelling Agents
The compositions of the present invention can also comprise a thickening or gelling
agent, preferably in a level of about 0.1% to about 5%, more preferably from about 0.1%
to about 3%, and most preferably from about 0.25% to about 2%. Nonlimiting classes of
thickening agents include, for example, crosslinked polymers of acrylic acid, substituted
acrylic acids, such as methacrylic acid, and salts and esters thereof, where the crosslinking
agent is typically derived from a polyhydric alcohol. Preferred crosslinkers include allyl
ethers of sucrose or of pentaerythritol. Also included are copolymers with acrylate esters,
e. g. one short chain (C1-C4) and one long chain (C8-C40) acrylate ester. See, for
example, U. S. Patent No. 5,087, 445 (Haffey et al.) or U. S. Patent No. 4,509, 949 (Huang
et al.), as well as the CTFA International Cosmetic Ingredient Dictionary, fourth edition,
1991, pp. 12 and 80. Commercially available polymers of this type include the carbomers,
which are homopolymers of acrylic acid crosslinked with allyl ethers of sucrose or
pentaerytritol, e. g. the Carbopol Tm 900 series (B. F. Goodrich), and acrylates/C10-30 alkyl
acrylate crosspolymers, e. g. Carbopol Tm 1342 and 1382 (B. F. Goodrich).
Crosslinked polyacrylate polymers are also used as thickeners or gelling agents, and
include both cationic and nonionic polymers, with the cationic polymers being generally
preferred. See, for example, U. S. Patent Nos. 5,100, 660 (Hawe etal.), 4,849, 484
(Heard) 4,835, 206 (Farrar et al.) 4,628, 078 (Glover et al.), and 4,599, 379 (Flesher et
al.). In general, these materials are high molecular weight copolymers of a
dialkylaminoalkyl acrylate monomer and a dialkylaminoalkyl methacrylate monomer, or
their quaternary ammonium or acid addition salts, and may also incorporate any of a
variety of unsaturated third monomers, such as ethylene, propylene, butylene, isobutylene,
eicosene, maleic anhydride, acrylamide, methacrylamide, maleic acid, acrolein,
cyclohexene, ethyl vinyl ether, and methyl vinyl ether. The alkyl portions of the acrylate
monomers are preferably short chain alkyls such as C1-C8. Crosslinking agents, generally
included to increase the viscoifying effect of the polymer, include
methylenebisacrylamides, diallyldialkyl ammonium halides, polyalkenyl polyethers of
polyhydric alcohols, allyl acrylates, vinyloxyalkylacrylates, and polyfunctional vinylidenes.
Examples of such cationic polymers include Salcare SC92 and SC95 (Allied Colloids
Ltd. , Norfolk Va. ), both provided as mineral oil dispersions.
Also useful as thickeners are polymers such as high molecular weight
polyacrylamides, including block copolymers of acrylamides and substituted acrylamides
with acrylic acids and substituted acrylic acids, e. g. Hypan SR150H, SS500V,
SS500W, and SSSA1OOH (Lipo Chemicals, Inc. , Patterson, N. J. ) ; polysaccharides, e. g.
cellulose, carboxymethyl hydroxyethylcellulose, hydroxypropylcellulose, sodium cellulose
sulfate, and the like, as well as alkyl substituted celluloses, such as cetyl
hydroxyethylcellulose; crosslinked vinyl ether/maleic anhydride copolymers; and
crosslinked poly (N-vinylpyrrolidones), as described, for example, in U. S. Patent Nos.
5,139, 770 (Shih et al.). Commercially available examples include ACP-1120,-1179, and
- 1180 (International Specialty Products, Wayne, N. J.).
Thickening and gelling agents may also include materials derived from natural
sources, such as acacia, agar, algin, amylopectin, carrageenan, carnitine, dextrin, gelatin,
gellan gum, guar gum, hectorite, hyaluroinic acid, hydrated silica, chitosan, kelp, locust
bean gum, natto gum, tragacanth gum, xanthan gum, derivatives thereof, and mixtures
thereof.
A2 (d). Emollient
The subject formulations may also include a dermatologically acceptable emollient,
e. g. at a level of about 2% to about 50%, depending on the physical form of the
formulation. For example, lotions typically comprise about 5% to 10% emollient and
about 60% to 80% water. A cream typically comprises about 10% to 20% emollient and
about 50% to 75% water. An ointment may comprise about 2% to 10% emollient and
about 0.1% to 2% of a thickening agent as described below. Generally, the emollient is
present at a level of about 5% to about 25%.
Emollients are typically water-immiscible, oily or waxy materials which serve to
lubricate the skin. An emollient may be selected from one or more of the following
classes: triglyceride esters, which include, for example, vegetable and animal fats and oils;
acetylated or ethoxylated glycerides; alkyl or alkyenyl esters of fatty acids, e. g. methyl
palmitate, isopropyl isostearate, diisohexyl adipate, cetyl lactate, oleyl stearate, and the
like; long chain fatty acids or alcohols such as myristic, palmitic, stearic, oleic, behenic,
hydroxystearyl, and the like; lanolin and lanolin derivatives; polyhydric alcohol esters, e. g.
mono and di-fatty acid esters of ethylene glycol, diethylene glycol, polyethylene glycol
(200-6000), propylene glycol, and polypropylene glycol, and sorbitan, which may be
ethoxylated; wax esters such as beeswax, spermaceti, and ethoxylated derivatives thereof ;
vegetable waxes such as carnauba and candelilla waxes; phospholipids such as lecithin and
derivatives thereof ; sterols, such as cholesterol and its fatty acid esters; and fatty acid
amides.
Additional types of conditioning compounds include polyhydric alcohols and their
derivatives, such as, for example, polypropylene glycol, hydroxypropyl sorbitol,
pentaerythritol, xylitol, ethoxylated glycerol, soluble collagen, dibutyl phthalate, or
gelatin. Also useful are ammonium and quaternary alkyl ammonium glycolates and
lactates; aloe vera gel; and hyaluronic acid and derivatives thereof.
A2 (e). Other Components
The formulations of the present invention may comprise a wide variety of additional
components, as known in the art, including but not limited to anticaking agents,
antimicrobial agents, astringents, opacifying agents, fragrances, pigments, preservatives,
propellants, reducing agents, skin penetration enhancing agents, waxes, sunscreens,
antioxidants and/or radical scavengers, chelating agents, sequestrants, anti-inflammatory
agents, and vitamins. See, for example, Harry's Cosmeticology, 7th Ed. , Harry &
Wilkinson (Hill Publishers, London 1982); Pharmaceutical Dosage Forms-Disperse
Systems; Lieberman, Rieger & Banker, Vols. 1 (1988) & 2 (1989); Marcel Decker, Inc.;
The Chemistry and Manufacture of Cosmetics, 2nd. Ed., deNavarre (Van Nostrand 1962-
1965); and The Handbook of Cosmetic Science and Technology, 1st Ed. Knowlton &
Pearce (Elsevier 1993).
Such additional components should be physically and chemically compatible with the
vehicle and active components described herein, and not unduly impair stability, efficacy
or other use benefits associated with the compositions of the present invention.
The compositions of the present invention are preferably formulated to have a pH of
10.5 or below,, more preferably from about 3-8, and most preferably from about 5-8.
B. Methods of Application
A formulation of a biologically active extract as described above, in a cosmetic
vehicle such as described above, is applied in an amount and frequency effective to obtain
the desired effects, which include, for example, diminishing roughness and dryness of the
skin, diminishing or preventing wrinkling, and preventing or alleviating damage of skin by
UV radiation. The formulation is also beneficial in healing of superficial wounds or
abrasions of the skin.
Quantities of the present compositions applied per application can vary, but are
typically from about 0.1 to about 10 mg/cm2 of skin surface. In one embodiment, the
formulation is applied daily, to areas such as the face, hands, arms, or feet; however,
application rates can vary from about once per week up to about three times per day or
more. The compositions may also be applied, generally in the form of a skin lotion or
cream, to be left on the skin for an extended period such as one or more hours, for some
aesthetic, prophylactic, therapeutic or other benefit (i. e. , a"leave-on"composition).
V. Therapeutic Compositions and Methods
A. Formulations and Methods of Administration
Pharmaceutical formulations containing the telomerase activating extracts described
herein may take the form of solid, semi-solid, lyophilized powder, or liquid dosage forms, such
as, for example, tablets, capsules, powders, sustained-release formulations, solutions,
suspensions, emulsions, suppositories, creams, ointments, lotions, aerosols, or the like,
preferably in unit dosage forms suitable for simple administration of precise dosages.
The compositions typically include a conventional pharmaceutical carrier or excipient and
may additionally include other medicinal agents, carriers, adjuvants, and the like. Typically, the
composition will contain about 0.1% to 100% (w/v), preferably 0.5% to 50% (w/v), more
preferably 2.5 to 25% (w/v), of a telomerase inducing extract as described herein, with the
remainder consisting of suitable pharmaceutical excipients. As noted above, the extract may
also be provided without a vehicle or excipients, e. g. as a dry powder or in pressed pill or
tablet form, for oral administration.
Further exemplary concentrations of the extract in a formulation are in the range of
0.5 to 75,1 to 50,5 to 25,10 to 25,10 to 50,20 to 75,20 to 50, and 20 to 25% (w/v).
Choice of a suitable concentration depends on factors such as the desired dose, frequency
and method of delivery of the active agent.
For oral administration in solid form, or for preparation of a nutraceutical formulation,
suitable excipients, when present, can include pharmaceutical grades of carriers such as
mannitol, lactose, glucose, sucrose, starch, cellulose, gelatin, magnesium stearate, sodium
saccharine, and/or magnesium carbonate. For use in oral liquid preparation, the composition
may be prepared as a solution, suspension, emulsion, or syrup, being supplied either in solid or
liquid form suitable for hydration in an aqueous carrier, such as, for example, aqueous saline,
aqueous dextrose, glycerol, or ethanol, preferably water or normal saline. If desired, the
composition may also contain minor amounts of non-toxic auxiliary substances such as wetting
agents, emulsifying agents, or buffers.
The composition may be administered to a subject by a variety of known routes, e. g.
orally or parenterally ; that is, by intravenous, intrathecal, subcutaneous, intraperitoneal, or
intramuscular injection; by inhalation, topically, or transdermally.
For parenteral administration, an injectable composition typically contains a formulation
of a telomerase activating extract in a suitable IV solution, such as sterile physiological salt
solution. The composition may also formulated as a suspension in a lipid or phospholipid, in a
liposomal suspension, or in an aqueous emulsion.
The extract compositions may also be delivered transdermally, typically by the use of a
transdermal patch which allows for continuous slow delivery to a selected skin region. It may
be desirable to include permeation enhancing substances, such as fat soluble substances (e. g.,
aliphatic carboxylic acids, aliphatic alcohols), or water soluble substances (e. g., alkane polyols
such as ethylene glycol, 1,3-propanediol, glycerol, propylene glycol, and the like).
Methods for preparing such dosage forms are known or will be apparent to those skilled
in the art; for example, see Remington's Pharmaceutical Sciences (19th Ed., Williams &
Wilkins, 1995). The composition to be administered will contain a quantity of the extract in a
pharmaceutically safe and effective amount for effecting telomerase induction in the target cells
or tissue.
For therapeutic treatment of a subject or patient, such as a mammal or a human
patient, dosage levels of telomerase activating extract are determined based on factors
such as the weight and overall health of the subject, the condition treated, severity of
symptoms, etc., but are typically in the range of about 1 to 50 g/day or more for a human
patient, typically about 4 to 40g/day.
For administration as a nutraceutical, e. g. a dietary supplement, dosages are typically
in the range of 20 mg-lg/day, typically 20-200 mg/day, for a human subject.
B. Therapeutic Indications
The present invention provides methods for increasing telomerase activity in a cell, by
contacting a cell or tissue with an extract as described herein, in an amount effective to
increase telomerase activity in the cell. The method may include the preliminary step of
identifying a cell or tissue in which an increase in telomerase activity is desired. The cell
may be in culture, i. e. in vitro or ex vivo, or within a subject or patient in vivo.
Benefits to be realized from an increase in telomerase activity in a cell or tissue
include, for example, enhancement of the replicative capacity and/or life span of the
contacted cells. The method may further comprise diagnosing a condition in a subject or
patient wherein an increase in telomerase activity in cells or tissue of the patient is desired;
e. g., diagnosing a disease subject to treatment by an increase in telomerase activity in cells
or tissue. Accordingly, the invention provides methods of treating a condition in a
patient, by increasing telomerase activity in cells or tissue of said patient, the method
comprising administering to a subject in need of such treatment an effective amount of an
extract as described herein. An"effective amount"refers to an amount effective to
increase telomerase activity in the cells or tissue of the patient, such that a therapeutic
result is achieved.
Such conditions may include, for example, conditions associated with cellular
senescence or with an increased rate of proliferation of a cell in the absence of telomerase,
which leads to accelerated telomere repeat loss. By"increased rate of proliferation"is
meant a higher rate of cell division compared to normal cells of that cell type, or
compared to normal cells within other individuals of that cell type. The senescence of
those groups of cells at an abnormally early age can eventually lead to disease (see West
et al., U. S. Patent No. 6,007, 989).
Various disease states exist in which an increase in telomerase activity in certain cell
types can be beneficial. Accordingly, the invention provides methods of treating in a
patient a condition selected from the following, by increasing telomerase activity in the
cells of the patient, comprising administering to a subject in need of such treatment, an
effective amount of an extract as described herein. In some cases, the condition may also
be subject to treatment by ex vivo cell therapy, as described further below, employing the
associated cell types (indicated in parenthesis).
(a) Alzheimer's disease, Parkinson's disease, Huntington's disease, and stroke (cells
of the central nervous system, including neurons, glial cells, e. g. astrocytes, endothelial
cells, fibroblasts),
(b) age-related diseases of the skin, such as dermal atrophy and thinning, elastolysis
and skin wrinkling, sebaceous gland hyperplasia or hypoplasia, senile lentigo and other
pigmentation abnormalities, graying of hair and hair loss or thinning, or chronic skin
ulcers (fibroblasts, sebaceous gland cells, melanocytes, keratinocytes, Langerhan's cells,
microvascular endothelial cells, hair follicle cells),
(c) degenerative joint disease (cells of the articular cartilage, such as chondrocytes
and lacunal and synovial fibroblasts),
(d) osteoporosis and other degenerative conditions of the skeletal system (cells of
the skeletal system, such as osteoblasts, bone marrow stromal or mesenchymal cells,
osteoprogenitor cells),
(e) age-and stress-related diseases of the vascular system including atherosclerosis,
calcification, thrombosis, and aneurysms (cells of the heart and vascular system, including
endothelial cells, smooth muscle cells, and adventitial fibroblasts),
(f) age-related macular degeneration (cells of the eye, such as pigmented epithelium
and vascular endothelial cells),
(g) AIDS (HIV-restricted CD8+ cells); and
(h) age-and stress-related immune system impairment, including impairment of
tissue turnover, which occurs with natural aging, cancer, cancer therapy, acute or chronic
infections, or with genetic disorders causing accelerated cell turnover, and related anemias
and other degenerative conditions (other cells of the immune system, including cells in the
lymphoid, myeloid, and erythroid lineages, such as B and T lymphocytes, monocytes,
circulating and specialized tissue macrophages, neutrophils, eosinophils, basophils, NK
cells, and their respective progenitors).
In addition to the cell types noted above, further cell types in which an increase in
telomerase activity can be therapeutically beneficial include, but are not limited to, cells of
the liver, endocrine and exocrine glands, smooth musculature, or skeletal musculature.
As an example, in the case of HIV-infected individuals, CD8+ cell turnover is
increased as these cells attempt to control the level of HIV-infected CD4+ cells. In AIDS
(item (g) above), disease is believed to be caused by the early senescence of HIV-
restricted CD8+ cells. The aging of such cells is attributed not simply to abnormal amount
of loss of telomere sequences per cell doubling, but, in addition, to the increased
replicative rate of the cells, such that telomere attrition is greater than normal for that
group of cells. The invention thus provides methods of treating an HIV infected subject,
and more particularly of reducing early senescence of HIV-restricted CD8+ cells in an
HIV infected subject, by administering to a subject in need of such treatment an effective
amount of an extract as described herein.
An increase in telomerase activity can benefit non-dividing cells as well as
proliferating cells, e. g. in conditions associated with increased susceptibility to cell death
due to stress, such as ischemia in heart failure or in stroke (see e. g. Oh and Schneider, J
Mol Cell Cardiol 34 (7): 717-24; Mattson, Exp Gerontol. 35 (4): 489-502). The invention
thus provides methods of reducing stress-or DNA-damage-induced cell death in a
subject, such as a subject experiencing ischemic conditions in tissue due to heart failure or
stroke, by increasing telomerase activity in cells of the subject, comprising administering
to a subject in need of such treatment an effective amount of an extract as described
herein. As noted above, the method may include the preliminary step of diagnosing in the
subject the indicated condition.
In another aspect, the compositions may be used for the treatment of individuals in
which one or more cell types are limiting in that patient, and whose life can be extended
by extending the ability of those cells to continue replication or resist stress-induced cell
death. One example of such a group of cells is lymphocytes present in Down's Syndrome
patients. The invention thus provides a method of enhancing replicative capacity and/or
life span of lymphocytes present in a Down's Syndrome patient, by increasing telomerase
activity in said cells of the patient, comprising administering to such a patient an effective
amount of an extract as described herein. The compositions may also be used to improve
resistance to stress-induced cell death occurring during normal aging.
In a further aspect of the invention, increasing telomerase activity is effective to
promote healing of wounds, burns, abrasions or other acute or chronic conditions of the
epidermis. The invention thus provides a method of treating an acute or chronic condition
of the epidermis, by administering to a patient in need of such treatment, preferably
topically to the affected area, an effective amount of an extract as described herein.
As used herein, an"acute or chronic condition of the epidermis"includes acute
conditions such as lesions suffered in trauma, burns, abrasions, surgical incisions, donor
graft sites, and lesions caused by infectious agents, and chronic conditions such as chronic
venous ulcer, diabetic ulcer, compression ulcer, pressure sores, and ulcers or sores of the
mucosal surface. Also included are skin or epithelial surface lesions caused by a persistent
inflammatory condition or infection, or by a genetic defect (such as keloid formation and
coagulation abnormalities). See, for example, PCT Pubn. No. WO 02/91999.
Desirable effects of an increase in telomerase activity in such treatment include cell
proliferation or migration at the treatment site, epithelialization of the surface, closure of a
wound if present, or restoration of normal physiological function. By"epithelialization"
or"reepithelialization"of a treatment site is meant an increase in density of epithelial cells
at the site as a result of the applied therapy.
The method may also be used to enhance growth of engrafted cells. Desirable effects
of an increase in telomerase activity in such treatment include coverage of the treatment
site, survival of engrafted cells, lack of immune rejection, closure of a wound if present,
or restoration of normal physiological function. Engrafted cells may participate in wound
closure either by participating directly in the healing process (for example, becoming part
of the healed tissue), or by covering the wound and thereby providing an environment that
promotes healing by host cells.
The invention also contemplates manipulation of the skin and repair of any perceived
defects in the skin surface for other purposes, such as cosmetic enhancement.
In a further aspect, the methods and compositions of the invention can be used to
enhance replicative capacity and/or extend life span of cells in culture, e. g. in ex vivo cell
therapy or in monoclonal antibody production, by increasing telomerase activity in the
cells. Increasing telomerase activity increases the replicative capacity of such cells by
slowing telomere repeat loss and/or improving resistance to stress-induced cell death
during cell proliferation.
In the case of ex vivo applications, an effective amount of an extract as described
herein is added to explant cells obtained from a subject. An"effective amount"refers to
an amount effective to increase telomerase activity in the cells, thereby increasing the
replicative capacity and/or life span of the cells.
The explant cells may include, for example, stem cells, such as bone marrow stem
cells (U. S. Patent No. 6,007, 989), bone marrow stromal cells (Simonsen et al., Nat
Biotechnol 20 (6): 592-6,2002), or adrenocortical cells (Thomas et al, Nat Biotechnol
18 (1) : 39-42,2000). Disease conditions such as those noted in items (a)- (h) above may
also be subject to ex vivo cell-based therapy. Examples include the use of muscle satellite
cells for treatment of muscular dystrophy, osteoblasts to treat osteoporosis, retinal
pigmented epithelial cells for age-related macular-degeneration, chondrocytes for
osteoarthritis, and so on.
For example, the recognition that functional CD8+ cells are limiting in AIDS patients
to control the expansion of infected CD4+ cells allows a therapeutic protocol to be
devised in which HIV-restricted CD8 cells are removed from an HIV-infected individual
at an early stage, when AIDS is first detected, stored in a bank, and then reintroduced into
the individual at a later stage, when that individual no longer has the required CD8 cells
available. Thus, an individual's life can be extended by a protocol involving continued
administration of that individual's limiting cells at appropriate time points. These
appropriate points can be determined by following CD8+ cell senescence, or by
determining the length of telomeres within such CD8+ cells, as an indication of when those
cells will become senescent. In accordance with the invention, the stored cells can be
expanded in number in the presence of an agent which slows telomere repeat loss, i. e. an
extract as described herein.
Accordingly, the invention provides methods of ex vivo cell based therapy, which
include obtaining a cell population from a subject, and expanding the cell population ex
vivo, wherein the cell population is treated with an extract as described herein, in an
amount effective to increase telomerase activity and thereby enhance the replicative
capacity and/or life span of the cell population. The method generally includes diagnosing
in a subject a condition subject to treatment by ex vivo cell based therapy, such as those
noted above.
In a further embodiment, the invention provides a method of stem cell proliferation,
wherein a stem cell population is treated with an extract as described herein, in an amount
effective to increase telomerase activity and thereby enhance the replicative capacity
and/or life span of the cell population.
VI. Selection of Additional Extracts Effective to Increase Telomerase Activity
The invention also provides methods of selecting a plant extract which is effective to
increase telomerase activity in cells, by screening plant extracts in accordance with the
TRAP assay described in Section III, and selecting an extract if it has a predetermined
minimum level of telomerase increasing activity. For example, the extract could be
selected if it provides, at a concentration of 25 u. g/ml or less, a level of telomerase in
keratinocytes or fibroblasts, as measured in a TRAP assay, which is at least 25% greater,
and more preferably about 50% greater, than the level observed for a solvent control.
Alternatively, or in addition, the extract, formulated in a suitable solvent medium at
one more concentrations, is assayed for wound healing activity in a scratch assay as
described above. Preferred extracts for selection include those having wound healing
activity, at a concentration of 25, ug/ml or less, which is at least 25% greater, and more
preferably at least 50% greater, than that of a solvent control.
Extracts of plant material are prepared accordingly to known methods, such as the
extraction methods described in Section IIB above and the exemplary protocol described
for Astragalus membranaceus root in Example 1. The plant material is, for example, the
root, stem, leaf or flower of a vascular plant, preferably a flowering plant, and more
preferably an herb, as defined above. In preferred embodiments, the plant is an
Astragalus or Cimicifuga species.
A selected extract can be used to formulate a pharmaceutical or cosmetic
composition, comprising a pharmaceutical or cosmetic carrier. Suitable formulations for
preparing pharmaceutical or cosmetic compositions of telomerase activating and/or
wound healing extracts are described further in Sections V and II, respectively.
EXAMPLES
The following examples are intended to illustrate but not to limit the invention.
Example 1. Exemplary Extraction Protocol
Raw herbal material (Astragalus membranaceus root) was soaked in 95% aqueous
EtOH, at a level of 100 mL solvent/20 g plant material, for 30 min, then refluxed for 2
hours. The solid material was filtered, and the reflux step was repeated with fresh
solvent. The solvent fractions were combined. This solution could be used directly for
screening or dried to obtain the solid extract. Total yields from extraction of 20g samples
of plant material from two sources were, respectively, 1.8 g (Mongolia) and 3.2 g
(ShanXi).
Example 2. Short Term and Long Term Photoaging Assays
Keratinocytes were plated three days prior to (1) addition of vehicle control, (2)
addition of 25 ug/ml extract GRN925, or (3) transduction with 10 MOI (multiplicity of
infection) AdhTERT. At this point cells were about 40% confluent.
Short term experiment: After 3 additional days (at about 75% confluence), medium
was removed, and the cells were rinsed twice with PBS. Cells in each of groups (1), (2)
and (3) were then exposed to (a) 7.5 mJ/cm2 UVB radiation, (b) 10 mJ/cm2UVB
radiation, or (c) ambient radiation. One day later, the cells were harvested, and the extent
of apoptosis was determined by an annexin V-FACS assay, using the Immunotech
Annexin V-FITC kit. (For descriptions of this assay see e. g. Vermes et al., J. Immunol.
Methods 184 (1) : 39-51,1995 ; Koopman etal., Blood 84 (5): 1415-20,1994 ; Wilkins et al.
Cytometry 48 (1) 14-9,2002.)
Long term experiment: After 3 additional days (at about 75% confluence), the cells
were passaged onto new culture dishes, trypsinized, counted, and replated at a density of
3.5 x 105 ceIls/lOOcm in fresh media. The cells were allowed to grow for an additional 5-
6 days, to regain about 75% confluence, then treated as above (removal of medium, UVB
exposure, and apoptosis assay).
Example 3. Exemplary Cosmetic Formulations
The following are examples of cosmetic formulations incorporating the subject
extracts. In each case,"Extract"refers to an extract of an Astragalus or Cimicifuga
species, preferably an Astragalus extract, and most preferably an Astragalus
nzembranaceus root extract, prepared as described in Example A.
An exemplary oil-in-water emulsion can be prepared using the following ingredients:
Ingredient Weight %
Phase A Water U. S. P. (to 100)
Disodium EDTA 0. 15
Glycerin 5
Phase B Cetyl hydroxy ethyl cellulose 0. 15
Methyl Paraben 0. 25
Phase C Cetyl alcohol 0. 5
Stearyl alcohol 0. 5
Behenyl alcohol 0. 5
Cetyl ricinoleate 3
Steareth-2 (Brij 72) 1
Distearyldimonium chloride 0. 25
Propyl Paraben 0. 1
Myristyl myristate 1. 5
Caprylic/Capritryglycerides 1. 5
Mineral oil 2
Sugar fatty acid ester* 1
Polypropylene glycol-15 stearyl ether1
Phase D Dimethicone 10 CST (Dow Coming) 2
Phase E Extract (to give 2. 5% w/v)
Isopropanol 10
Benzyl alcohol 10
Phase F 50% NaOH to pH 7
*For example, a sucrose polyester having a degree of esterification of 7-8, where the fatty acids
are C18 mono-and/or di-unsaturated and C22 saturated, e. g. SEFA Cottonate.
The phase A components are blended at a temperature of about 70-80°C, and the
phase B components are then added at the same temperature and blended to form a
uniform mixture. The phase C components are milled to obtain an acceptably smooth
mixture, then added to the above mixture. The mixture is blended and allowed to cool to
about about 45°C, at which point dimethicone (phase D) is added, followed by the extract
in a lower alcohol such as ethanol (phase E), and NaOH (phase F) to pH 7.
Further exemplary oil-in-water emulsions can be prepared from ingredients as shown
in the tables below, again using conventional formulating techniques, such as follows.
Distilled water (Phase A) is purged with nitrogen, followed by addition of Phase B
ingredients. Phase C ingredients are then dispersed into Phase A/B until uniform, heating
to about 75°C. Phase D ingredients are blended separately and heated to about 75°C,
then blended into phases A/B/C under nitrogen for approx. 30 minutes, followed by
addition of the combined phase E ingredients. The mixture is blended until homogeneous
and then cooled. The phase F, G, and H ingredients are added, respectively, to the
mixture when it has cooled to 50°C (phase F), 40°C (phase G) and 30°C (phase H).
Mixing is continued until the mixture is uniform.
Ingredient Weight %
Phase B Glycerin 5
Phase C Glycerin 1
EDTA 0. 1
Carbopol 954 0. 5-0.68
Carbopol 1382 0. 1
Phase D Cetyl alcohol 0. 72
Stearyl alcohol 0. 48
Stearic acid 0. 1
PEG-100 stearate 0. 1
Arlatone 2121
Silicone Q21403 2
Sugar fatty acid ester 0. 67
Tocopherol acetate 0-0. 5
Niacinamide 2
Phase E Distilled water 2
NaOH (to pH 7
Phase F Urea 0-2
D-Panthenol 0-0. 5
Distilled water 5
Phase G Glydant Plus 0. 1
Glycerin _ _
Distilled water 1
Phase H Methyl/isopro l isostearate 1. 3-2. 6
BHT 0. 05
Tween 20 0. 04
Extract (to give 5% w/v)
Ingredient Weight %
Phase B Glycerin 6
Phase C Glycerin 3
Carbopol 954 0. 4
EDTA 0. 1
Phase D Cetyl palmitate 1. 5
Cetyl alcohol 2. 25
Stearyl alcohol 1. 5
Stearic acid 0. 31
PEG-100 stearate 0. 31
Silicone wax DC2501 2
DC 3225C 1. 88
Dimethicone 200/350CST 0.63
Tocopherol acetate 0-0. 5
Niacinamide 2
Phase E Distilled water 2
NaOH (to pH 7)
Phase F D-Panthenol 0-0. 5
Distilled water 0-5
Phase G Glydant Plus 0. 1
Distilled water 1
Glycerin 1
Phase H Isopropyl palmitate 1. 25
Tween 80 0-0. 04
BHT 0-0. 05
Extract (to give 2. 5% w/v)
A high internal phase water-in-oil emulsion can be prepared using the following
components:
Ingredient Weight %
Extract (to give 1.0% w/v)
1, 3-dimethyl-2-imidazolidinone 0. 2
Brij 92 (Polyoxyethylene (2) oleyl ether) 5
Bentone 38 (Quaternium 18-hectorite) 0.5
MgSO4#7H2O 0. 3
Butylated hydroxy toluene 0. 01
Perfumes
Water (to 100)
An oil-in-water cream can be prepared using the following components:
Ingredient Weight %
Extract to give 2.5% w/v
Glycolic Acid 8
Mineral oil 4
1, 3-dimethyl-2-imidazolidinone 1
Brij 56 (Cetyl alcohol POE (10)) 4
Cetyl alcohol 4
Triethanolamine 0. 75
Butane-1, 3-diol 3
Xanthan gum 0. 3
Perfumes
Butylated hydroxy toluene 0. 01
Water (to 100)
An alcoholic lotion can be prepared using the following components:
Ingredient Weight %
Extract (to give 6.5% w/v)
1, 3-dimethyl-2-imidazolidinone 0. 1
Ethanol 40
Perfume qs
Butylated hydroxy toluene 0. 01
Water (to 100)
A sunscreen cream can be prepared using the following components:
Ingredient Weight %
Extract (to give 4.0% w/v)
1, 3-dimethyl-2-imidazolidinone 0. 2
Silicone oil 200 cts 7.5
Glycerylmonostearate 3
Cetostery alcohol
Polyoxyethylene-(20)-cetyl alcohol 1. 4
Xanthan gum 0. 5
Parsol 1789 (Butylmethoxydibenzoylmethane) 1.5
Parsol MCX (Octyl methoxycinnamate) 7
Perfume qs
Color as
Water (to 100)
A non-aqueous skin care composition can be prepared using the following components:
Ingredient Weight %
Extract (to give 7.0% w/v)
1, 3-dimethyl-2-imidazolidinone
Silicone gum SE-30a 10
Silicone fluid 345b 20
Silicone fluid 344c (to 100)
Squalene 10
Linoleic acid 0. 01
Cholesterol 0. 03
2-hydroxy-n-octanoic acid 0. 7
Vitamin E linoleate 0. 5
Herbal oil 0. 5
Ethanol 2
(a) Dimethyl silicone polymer, MW # 50,000, available from GEC
(b) Dimethyl siloxane cyclic pentamer, available from Dow Coming Corp.
(c) Dimethyl siloxane tetramer, available from Dow Coming Corp.