U.S. patent application number 10/490213 was filed with the patent office on 2004-11-25 for pharmaceutical preparation useful for treating tumors and lesions of the skin and the mucous membranes and methods and kits using same.
Invention is credited to Burstein, Pinchas.
Application Number | 20040234625 10/490213 |
Document ID | / |
Family ID | 25514753 |
Filed Date | 2004-11-25 |
United States Patent
Application |
20040234625 |
Kind Code |
A1 |
Burstein, Pinchas |
November 25, 2004 |
Pharmaceutical preparation useful for treating tumors and lesions
of the skin and the mucous membranes and methods and kits using
same
Abstract
A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion is provided. The pharmaceutical preparation
including, as active ingredients, a therapeutically effective
amount of trichloroacetic acid and hydrochloric acid, or
trichloroacetic acid and formic acid or all three of these acids
and optionally a crosslinking/fixating/preserving agent. Additional
preparations are also described.
Inventors: |
Burstein, Pinchas; (Ramat
Hasharon, IL) |
Correspondence
Address: |
Anthony Casrorina
G E Ehrlich
Suite 207
2001 Jefferson Davis Hwy
Arlington
VA
22202
US
|
Family ID: |
25514753 |
Appl. No.: |
10/490213 |
Filed: |
March 31, 2004 |
PCT Filed: |
October 2, 2002 |
PCT NO: |
PCT/IL02/00804 |
Related U.S. Patent Documents
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Application
Number |
Filing Date |
Patent Number |
|
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10490213 |
Mar 31, 2004 |
|
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09968771 |
Oct 3, 2001 |
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Current U.S.
Class: |
424/666 ;
514/557 |
Current CPC
Class: |
A61K 33/00 20130101;
A61K 31/19 20130101; A61P 17/00 20180101; A61P 43/00 20180101; A61K
33/00 20130101; A61K 2300/00 20130101; A61K 2300/00 20130101; A61K
31/19 20130101 |
Class at
Publication: |
424/666 ;
514/557 |
International
Class: |
A61K 033/18; A61K
031/19 |
Claims
What is claimed is:
1. A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion comprising, as active ingredients,
therapeutically effective amounts of at least two active
ingredients selected from the group consisting of trichloroacetic
acid, hydrochloric acid and formic acid.
2. The pharmaceutical preparation of claim 1, wherein a
concentration of said trichloroacetic acid said hydrochloric acid
and said formic acid is selected such that application of the
preparation to the skin or mucous membrane lesion leads to drying
and separation of the skin or mucous membrane lesion from a base
tissue thereof.
3. The pharmaceutical preparation of claim 1, wherein a
concentration of trichloroacetic acid, said hydrochloric acid and
said formic acid is selected such that application of the
pharmaceutical preparation to the skin or mucous membrane lesion
preserves a morphology of tissue thereof thereby enabling
histopathological analysis of said tissue.
4. The pharmaceutical preparation of claim 1, wherein a
concentration of said trichloroacetic acid is selected from a range
of 5% to 97% (w/w), said concentration of said hydrochloric acid is
selected from a range of 3% to 38% (w/w) and said concentration of
said formic acid is selected from a range 0.1% to 85% (w/w).
5. The pharmaceutical preparation of claim 1, further comprising at
least one crosslinking/fixating/preserving agent.
6. The pharmaceutical preparation of claim 5, wherein said at least
one crosslinking/fixating/preserving agent is selected from the
group consisting of formaldehyde, paraformaldehyde, glutaraldehyde,
glyoxal, carbodi-imide, a formaldehyde donor, sodium hydroxymethyl
glycinate, diazolidinyl urea, imidazolidinyl urea,
dimethilol-5,5-dimethilhydantoin, dimethilol urea,
2-bromo-2-nitropropane 1,3-diol, quarternium-15, parabens,
5-chloro-2 methylisothiazolin-3-one, 1,2-dibromo-2,4-dicyanobut-
ane, ethanol and other alcohols and polyol.
7. A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion comprising, as active ingredients, about 48%
(w/w) trichloroacetic acid, about 8% (w/w) hydrochloric acid and
about 3% (w/w) formic acid.
8. The pharmaceutical preparation of claim 7, further comprising
about 4% formaldehyde.
9. The pharmaceutical preparation of claim 1, further comprising at
least one agent selected from the group consisting of cytotoxic
drugs, anti acne drugs, corticosteroids, anti-inflammatory agents,
antibiotics, anti-viral agents, anti-psoriatic agents,
keratinolytic agents, skin penetration enhancers, local anaesthetic
agents, antiseptic agents metal ions, tars and urea.
10. An ampoule containing the pharmaceutical preparation of
claiml.
11. An ampoule containing the pharmaceutical preparation of claim
7.
12. A kit containing the pharmaceutical preparation of claim 8, the
kit including at least two ampoules.
13. An article-of-manufacturing comprising packaging material and a
pharmaceutical preparation being identified for treatment of skin
or mucous membrane lesions, said pharmaceutical preparation
including, as active ingredients, therapeutically effective amounts
of at least two agents selected from the group consisting of
trichloroacetic acid, hydrochloric acid and formic acid.
14. An article-of-manufacturing comprising packaging material and a
pharmaceutical preparation being identified for treatment of skin
or mucous membrane lesions, said pharmaceutical preparation
including, as active ingredients, about 48% (w/w) trichloroacetic
acid, about 8% (w/w) hydrochloric acid and about 3% (w/w) formic
acid.
15. The article-of-manufacturing of claim 13, wherein said
pharmaceutical preparation further comprises at least one
crosslinking/fixating/preservi- ng agent.
16. The pharmaceutical preparation of claim 15, wherein the at
least one crosslinking/fixating/preserving agent is selected from
the group consisting of formaldehyde, paraformaldehyde,
glutaraldehyde, glyoxal, carbodi-imide, a formaldehyde donor,
sodium hydroxymethyl glycinate, diazolidinyl urea, imidazolidinyl
urea, dimethilol-5,5-dimethilhydantoin, dimethilol urea,
2-bromo-2-nitropropane 1,3-diol, quarternium-15, parabens,
5-chloro-2 methylisothiazolin-3-one, 1,2-dibromo-2,4-dicyanobut-
ane, ethanol and other alcohols and polyol.
17. The pharmaceutical preparation of claim 14, further comprising
4% (w/w) formaldehyde.
18. A method of treating a skin or mucous membrane lesion, the
method comprising applying to the skin or mucous membrane lesion a
pharmaceutical preparation including, as active ingredients, a
therapeutically effective amount of at least two agents selected
from the group consisting of trichloroacetic acid, hydrochloric
acid and formic acid.
19. The method of claim 18, wherein a concentration of said
trichloroacetic acid is selected from a range of 5% to 97% (w/w),
said concentration of said hydrochloric acid is selected from a
range of 3% to 38% (w/w) and said concentration of said formic acid
is selected from a range of 0.1% to 85% (w/w).
20. The method of claim 18, wherein said pharmaceutical preparation
includes, as active ingredients, about 48% (w/w) trichloroacetic
acid, about 8% (w/w) hydrochloric acid and about 3% (w/w) formic
acid.
21. The method of claim 18, wherein said pharmaceutical preparation
further includes at least one crosslinking/fixating/preserving
agent selected from group consisting of formaldehyde,
paraformaldehyde, glutaraldehyde, glyoxal, carbodi-imide, a
formaldehyde donor, sodium hydroxymethyl glycinate, diazolidinyl
urea, imidazolidinyl urea, dimethilol-5,5-dimethilhydantoin,
dimethilol urea, 2-bromo-2-nitropropane 1,3-diol, quarternium-15,
parabens, 5-chloro-2 methylisothiazolin-3-one,
1,2-dibromo-2,4-dicyanobutane, ethanol and other alcohols and
polyol.
22. The method of claim 20, wherein the pharmaceutical preparation
further comprises 4% (w/w) formaldehyde.
23. The method of claim 18, further comprising repeating said
applying to the skin or mucous membrane lesion said pharmaceutical
preparation at predetermined time intervals.
24. A method of treating and biopsying a skin or mucous membrane
lesion, the method comprising: (a) applying to the skin or mucous
membrane lesion at least one mummifying preparation, so as to
obtain, following a mummification period, a mummified skin or
mucous membrane lesion; and (b) collecting said mummified skin or
mucous membrane lesion.
25. The method of claim 24, wherein said mummifying preparation
includes, as active ingredients, therapeutically effective amounts
of at least two agents selected from the group consisting of
trichloroacetic acid, hydrochloric acid and formic acid.
26. The method of claim 25, wherein a concentration of said
trichloroacetic acid is selected from a range of 5% to 97% (w/w),
said concentration of said hydrochloric acid is selected from a
range of 3% to 38% (w/w) and said concentration of said formic acid
is selected from a range of 0.1% to 85% (w/w).
27. The method of claim 24, wherein said mummifying preparation
includes about 48% (w/w) trichloroacetic acid, about 8% (w/w)
hydrochloric acid and about 3% (w/w) formic acid.
28. The method of claim 24, wherein said mummifying preparation
further includes at least one crosslinking/fixating/preserving
agent selected from group consisting of formaldehyde,
paraformaldehyde, glutaraldehyde, glyoxal, carbodi-imide, a
formaldehyde donor, sodium hydroxymethyl glycinate, diazolidinyl
urea, imidazolidinyl urea, dimethilol-5,5-dimethilhydantoin,
dimethilol urea, 2-bromo-2-nitropropane 1,3-diol, quartemium-15,
parabens, 5-chloro-2 methylisothiazolin-3-one,
1,2-dibromo-2,4-dicyanobutane, ethanol and other alcohols and
polyol.
29. The method of claim 27, wherein said mummifying preparation
further includes 4% (w/w) formaldehyde.
30. The method of claim 24, further comprising repeating step (a)
at predetermined time intervals.
31. A method of treating, biopsying and histopathologically
examining a skin or mucous membrane lesion, the method comprising:
(a) applying to the skin or mucous membrane lesion at least one
mummifying preparation, so as to obtain, following a mummification
period, a mummified skin or mucous membrane lesion; (b) collecting
said mummified skin or mucous membrane lesion; (c) rehydrating said
mummified skin or mucous membrane lesion; and (d)
histopathologically examining said mummified skin or mucous
membrane lesion.
32. The method of claim 31, wherein said mummifying preparation
includes, as active ingredients, a therapeutically effective amount
of at least two active ingredients selected from the group
consisting of trichloroacetic acid, hydrochloric acid and formic
acid.
33. The method of claim 31, wherein a concentration of said
trichloroacetic acid is selected from a range of 5% to 97% (w/w),
said concentration of said hydrochloric acid is selected from a
range of 3% to 38% (w/w) and said concentration of said formic acid
is selected from a range of 0.1% to 85% (w/w).
34. The method of claim 31, wherein said mummifying preparation
further comprises at least one crosslinking/fixating/preserving
agent.
35. The method of claim 34, wherein said at least one
crosslinking/fixating/preserving agent is selected from group
consisting of formaldehyde, paraformaldehyde, glutaraldehyde,
glyoxal, carbodi-imide, a formaldehyde donor, sodium hydroxymethyl
glycinate, diazolidinyl urea, imidazolidinyl urea,
dimethilol-5,5-dimethilhydantoin, dimethilol urea,
2-bromo-2-nitropropane 1 ,3-diol, quarternium-15, parabens,
5-chloro-2 methylisothiazolin-3-one, 1,2-dibromo-2,4-dicyanobut-
ane, ethanol and other alcohols and polyol.
36. The method of claim 31, wherein said mummifying preparation
includes about 48% (w/w) trichloroacetic acid, about 8% (w/w)
hydrochloric acid and about 3% (w/w) formic acid.
37. The method of claim 36, wherein said mummifying preparation
further includes 4% (w/w) formaldehyde.
38. The method of claim 31, further comprising staining said
mummified skin or mucous membrane lesion prior to (d).
39. A kit useful for treating a skin or mucous membrane lesion
comprising: (a) an applicator including a reservoir configured for
storing a pharmaceutical preparation, said reservoir being capped
at one end by a removable applicator tip; (b) a mechanism for
forcing a pharmaceutical preparation stored by said reservoir
through said applicator tip; and (c) a plurality of applicator
tips, each being sized and configured for applying said
pharmaceutical preparation stored by said reservoir to a specific
type, shape or size of a skin or mucous membrane lesion.
40. The kit of claim 39, further comprising at least one ampoule
containing a pharmaceutical preparation including, as active
ingredients, a therapeutically effective amount of at least two
agents selected from the group consisting of trichloroacetic acid,
hydrochloric acid, and formic acid.
41. The kit of claim 39, wherein a concentration of said
trichloroacetic acid is selected from a range of 5% to 97% (w/w),
said concentration of said hydrochloric acid is selected from a
range of 3% to 38% (w/w) and said concentration of said formic acid
is selected of 0.1% to 85% (w/w).
42. The kit of claim 39, further comprising at least one ampoule
containing a pharmaceutical preparation including about 48% (w/w)
trichloroacetic acid, about 8% (w/w) hydrochloric acid and about 3%
(w/w) formic acid.
43. The kit of claim 39, wherein the pharmaceutical preparation
further comprises at least one crosslinking/fixating/preserving
agent selected from group consisting of formaldehyde,
paraformaldehyde, glutaraldehyde, glyoxal, carbodi-imide, a
formaldehyde donor, sodium hydroxymethyl glycinate, diazolidinyl
urea, imidazolidinyl urea, dimethilol-5,5-dimethilhydantoin,
dimethilol urea, 2-bromo-2-nitropropane 1,3-diol, quarternium-15,
parabens, 5-chloro-2 methylisothiazolin-3-one,
1,2-dibromo-2,4-dicyanobutane, ethanol and other alcohols and
polyol.
44. The kit of claim 42, wherein the pharmaceutical preparation
further includes 4% (wa/w) formaldehyde.
45. An adhesive bandage useful for treating skin lesions
comprising: (a) an applicator pad containing a pharmaceutical
preparation including at least two active ingredients selected from
the group consisting of trichloroacetic acid, hydrochloric acid and
formic acid; and (b) an adhesive tape attached to said applicator
pad, said adhesive tape being configured for attaching to a skin
region so as to position said applicator pad against a portion of
said skin region including a skin lesion thereby applying said
pharmaceutical preparation to said skin lesion.
46. The adhesive bandage of claim 45, wherein a concentration of
said trichloroacetic acid is selected from a range of 5% to 97%
(w/w), said concentration of said hydrochloric acid is selected
from a range of 3% to 38% (w/w) and said concentration of said
formic acid is selected from a range of 0.1% to 85% (w/w).
47. The adhesive bandage of claim 45, wherein the pharmaceutical
preparation further includes at least one
crosslinking/fixating/preservin- g agent selected from the group
consisting of formaldehyde, paraformaldehyde, glutaraldehyde,
glyoxal, carbodi-imide, a formaldehyde donor, sodium hydroxymethyl
glycinate, diazolidinyl urea, imidazolidinyl urea,
dimethilol-5,5-dimethilhydantoin, dimethilol urea,
2-bromo-2-nitropropane 1,3-diol, quarternium-15, parabens,
5-chloro-2 methylisothiazolin-3-one, 1,2-dibromo-2,4-dicyanobutane,
ethanol and other alcohols and polyol.
48. The adhesive bandage of claim 45, wherein the pharmaceutical
preparation includes about 48% (w/w) trichloroacetic acid, about 8%
(w/w) hydrochloric acid and about 3% (w/w) formic acid.
49. The adhesive bandage of claim 48, wherein the pharmaceutical
preparation further includes about 4% (w/w) formaldehyde.
50. A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion comprising, as active ingredients,
therapeutically effective amounts of at least two agents selected
from the group consisting of trichloroacetic acid, hydrochloric
acid, formic acid, monochloroacetic acid, dichloroacetic acid,
glycolic acid, citric acid, kojic acid, acetic acid, azelaic acid,
phosphoric acid, thioglycolic acid, salicylic acid and their salts
and phenol.
51. A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion comprising, as active ingredients,
therapeutically effective amounts of at least one agent selected
from the group consisting of trichloroacetic acid, hydrochloric
acid, formic acid, monochloroacetic acid, dichloroacetic acid,
glycolic acid, citric acid, kojic acid, acetic acid, azelaic acid,
phosphoric acid, thioglycolic acid, salicylic acid and their salts
and phenol and at least one crosslinking/fixating/preserving
agent.
52. The pharmaceutical preparation of claim 51, wherein said at
least one crosslinking/fixating/preserving agent is selected from
the group consisting of formaldehyde, paraformaldehyde,
glutaraldehyde, glyoxal, carbodi-imide, a formaldehyde donor,
sodium hydroxymethyl glycinate, diazolidinyl urea, imidazolidinyl
urea, dimethilol-5,5-dimethilhydantoin, dimethilol urea,
2-bromo-2-nitropropane 1,3-diol, quarternium-15, parabens,
5-chloro-2 methylisothiazolin-3-one, 1,2-dibromo-2,4-dicyanobut-
ane, ethanol and other alcohols and polyol.
53. The pharmaceutical preparation of claim 52, wherein a
concentration of said formaldehyde is selected from a range of
0.01% to 0.1%.
54. The pharmaceutical preparation of claim 52, wherein a
concentration of said formaldehyde is selected from a range of 0.1%
to 1%.
55. The pharmaceutical preparation of claim 52, wherein a
concentration of said formaldehyde is selected from a range of 1%
to 10%.
56. A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion, comprising, as active ingredients,
therapeutically effective amounts of at least one agent selected
from the group consisting of trichloroacetic acid, hydrochloric
acid, formic acid, monochloroacetic acid, dichloroacetic acid,
glycolic acid, citric acid, kojic acid, acetic acid, azelaic acid,
phosphoric acid, thioglycolic acid, salicylic acid and their salts
and phenol, and at least one nonoxidizing organic or inorganic
acid.
57. A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion, comprising at least one nonoxidizing
organic or inorganic acid and at least one
crosslinking/fixating/preserving agent, selected from the group
consisting of formaldehyde, paraformaldehyde, glutaraldehyde,
glyoxal, carbodi-imide, a formaldehyde donor, sodium hydroxymethyl
glycinate, diazolidinyl urea, imidazolidinyl urea,
dimethilol-5,5-dimethilhydantoin, dimethilol urea,
2-bromo-2-nitropropane 1,3-diol, quarternium-15, parabens,
5-chloro-2 methylisothiazolin-3-one, 1,2-dibromo-2,4-dicyanobutane,
ethanol and other alcohols and polyol.
58. The pharmaceutical preparation of claim 57, wherein a
concentration of said formaldehyde is selected from a range of
0.01% to 0.1%.
59. The pharmaceutical preparation of claim 57, wherein a
concentration of said formaldehyde is selected from a range of 0.1%
to 1%.
60. The pharmaceutical preparation of claim 57, wherein a
concentration of said formaldehyde is selected from a range of 1%
to 10%.
61. A pharmaceutical preparation useful for treating a skin or
mucous membrane lesion, comprising, as active ingredients,
therapeutically effective amounts of at least one agent selected
from the group consisting of trichloroacetic acid, hydrochloric
acid, formic acid, monochloroacetic acid, dichloroacetic acid,
glycolic acid, citric acid, kojic acid, acetic acid, azelaic acid,
phosphoric acid, thioglycolic acid, salicylic acid and their salts
and phenol, and at least one agent selected from the group
consisting of cytotoxic drugs, anti acne drugs, corticosteroids,
anti-inflammatory agents, antibiotics, anti-viral agents,
anti-psoriatic agents, keratinolytic agents, skin penetration
enhancers, local anaesthetic agents, antiseptic agents metal ions,
tars and urea.
Description
FIELD AND BACKGROUND OF THE INVENTION
[0001] The present invention relates to pharmaceutical preparations
useful in the treatment of tumors and lesions of the skin and the
mucous membranes, and methods and kits using same.
[0002] Human skin and mucousal membranes support a wide range of
growth abnormalities which exhibit a wide range of sizes, shapes
and colors. Although not always dangerous to the individual, such
growth abnormalities are frequently cosmetically unappealing and as
such are oftentimes a cause of great discomfort. In addition, such
growth abnormalities are also prone to injury and infection and can
be a source of physical pain or discomfort.
[0003] Genital warts (condylomata acuminata) are a sexually
transmitted disease caused by the human papilloma virus (HPV).
Since the 1970's it has been increasingly clear that infections by
the same virus are closely implicated in the aetiology of
anogenital squamous cell carcinomas and in their precursors known
as dysplasia, intraepithelial neoplasia (CIN) or squamous
intraepithelial lesions (SIL).
[0004] Cutaneous melanoma, another skin lesion, which is also known
as "the great masquerader", is often recognized by its dark color,
although some tumors, defined as amelanotic melanomas, have little
or no pigmentation and as such are hard to detect and diagnose.
[0005] Due to limited diagnostic capabilities, physicians often
rely upon biopsy specimen analysis for accurate diagnosis of a
suspected malignant melanoma.
[0006] However, at present, most lesions which are not suspected as
being malignant are not biopsied but are rather treated via methods
such as cryosurgery, laser therapy or electrocauterization which
destroy the treated skin region making histopathological diagnosis
impossible.
[0007] In addition, such treatment methods oftentimes lead to
complications including pain, bleeding and discharge as well as
infections, blistering and hematomas. Such complications often
necessitate the application of localized antibiotics as well as
bandaging and as such are liable to cause further discomfort to the
individual treated.
[0008] Furthermore, with such treatments, the healing process is
liable to be slow and prolonged inevitably concluding with the
formation of an ugly scar which can be a source of discomfort,
particularly when appearing on exposed areas of the body such as
the neck and face.
[0009] Finally, such methods are also limited by the use of
expensive equipment not available in most clinics; furthermore,
cryosurgery requires a current and permanent supply of liquid
nitrogen, and is thus limited by the logistic hardships imposed by
such requirements.
[0010] An alternative method of treating lesions such as, warts and
condylomata acuminata, involves topical application of
Solcoderm.TM. (manufactured and distributed by Solco Basel AG,
Switzerland), a medication which includes nitric acid and nitrous
acid or metal nitrite.
[0011] Adequate results using Solcoderm.TM. are achieved only if
the recommended storage temperature and the use-by dates indicated
are observed as accurately as possible, since fluctuations in the
nitrite concentration due to storage temperature, storage time or
prolonged exposure to oxygen may severely decrease the
effectiveness of Solcoderm.TM..
[0012] In addition, it has been observed that preparations such as
Solcoderm.TM.. when inactive, present an increased danger of side
effects and may for example lead to ulcerations on healthy
skin.
[0013] Furthermore, due to the use of nitric acid, which is a
strong oxidizing acid, Solcoderm.TM. treatment tends to destroy
lesion tissue to an extent substantially negating the possibility
of accurate post treatment histopathological study and
diagnosis.
[0014] U.S. Pat. No. 5,573,786 describes an improved composition of
Solcoderm.TM. which overcomes the stability limitations described
above. This composition includes nitric acid and nitrite reduction
products formed by reacting aqueous nitric acid with a primary
C.sub.1-C.sub.5 alkanol. The primary alkanol is converted to
C.sub.1-C.sub.5 alkanoic acid and carbon dioxide. with the
simultaneous formation of nitrate reduction products.
[0015] As stated in U.S. Pat. No. 5,573,786 this improved
composition is useful for the treatment of common and plantar
warts, pedal mycosis and onychomycosis.
[0016] Topical treatment methods using Solcoderm.TM. or its
derivatives are oftentimes preferred over laser therapy or
cryotherapy, since such treatment methods cause less of a
discomfort to the treated individual and are easier and less
expensive to conduct. However, the currently available composition
is indicated for the treatment of warts and condylomata only.
[0017] Although a study performed by Cesarini from the Department
of Dermatology, Foundation Rothschild, Paris, France (Dermatologica
168; suppl. 1. pp. 15-25 (1984)) suggested that the fixative
properties of Solcoderm.TM. are adequate for histopathological
diagnosis of post-treatment scabs, the same study demonstrated that
when H & E staining is used (the single histochemical staining
method used), the cellular elements stain in pale pink while the
extra cellular compartment does not stain at all; furthermore,
anisocytosis, anisokariosis and polychromatophilia, the usual
landmarks of cytologists, cannot be observed and described.
[0018] There is thus a widely recognized need for, and it would be
highly advantageous to have, compositions and methods of using same
for effectively treating skin or mucous membrane lesions while
enabling post treatment histopathological analysis of treated
tissue.
SUMMARY OF THE INVENTION
[0019] According to one aspect of the present invention there is
provided a pharmaceutical preparation useful for treating a skin or
mucous membrane lesion comprising, as active ingredients,
therapeutically effective amounts of at least two active
ingredients selected from the group consisting of trichloroacetic
acid, hydrochloric acid and formic acid.
[0020] According to another aspect of the present invention there
is provided a pharmaceutical preparation useful for treating a skin
or mucous membrane lesion comprising, as active ingredients,
therapeutically effective amounts of at least two said active
ingredients selected from the group consisting of trichloroacetic
acid, hydrochloric acid and formic acid and a
crosslinking/fixating/preserving agent.
[0021] According to further features in preferred embodiments of
the invention described below, there is provided an ampoule
containing the pharmaceutical preparation described herein.
[0022] According to an additional aspect of the present invention
there is provided an article-of-manufacturing comprising packaging
material and a pharmaceutical preparation being identified for
treatment of skin or mucous membrane lesions, the pharmaceutical
preparation including, as active ingredients, therapeutically
effective amounts of trichloroacetic acid and hydrochloric acid, or
trichloroacetic acid and formic acid, or hydrochloric acid and
formic acid, or all three acids.
[0023] According to still an additional aspect of the present
invention there is provided a method of treating a skin or mucous
membrane lesion, the method comprising: (a) applying to the skin or
mucous membrane lesion a pharmaceutical preparation including, as
active ingredients, therapeutically effective amounts of at least
two active ingredients selected from the group consisting of
trichloroacetic acid, hydrochloric acid and formic acid.
[0024] According to still further features in the described
preferred embodiments the method further comprising repeating step
(a) at predetermined time intervals.
[0025] According to still further features in the described
preferred embodiments, a concentration of the trichloroacetic acid,
the hydrochloric acid and the formic acid is selected such that
application of the preparation to the skin or mucous membrane
lesion leads to drying and separation of the skin or mucous
membrane lesion from a base tissue thereof.
[0026] According to still further features in the described
preferred embodiments a concentration of the trichloroacetic acid,
the hydrochloric acid and the formic acid is selected such that
application of the pharmaceutical preparation to the skin or mucous
membrane lesion preserves a morphology of tissue thereof thereby
enabling histopathological analysis of the tissue.
[0027] According to still further features in the described
preferred embodiments a concentration of the trichloroacetic acid
is selected from a range of 5%-97% (w/w), the concentration of the
hydrochloric acid is selected from a range of 3%-38% (w/w) and the
concentration of the formic acid is selected from a range of
0.1%-85% (w/w), preferably about 3 %.
[0028] According to still further features in the described
preferred embodiments the pharmaceutical preparation further
comprising at least one crosslinking/fixating/preserving agent
selected from the group consisting of formaldehyde;
paraformaldehyde; glutaraldehyde; glyoxal; carbodi-imide; a
formaldehyde donor; sodium hydroxymethyl glycinate; diazolidinyl
urea; imidazolidinyl urea; dimethilol-5,5-dimethilhydantoin;
dimethilol urea; 2-bromo-2-nitropropane 1,3-diol; quarternium-15;
parabens; 5-chloro-2 methylisothiazolin-3-one;
1,2-dibromo-2,4-dicyanobut- ane; ethanol and other alcohols;
polyol.
[0029] According to still further features in the described
preferred embodiments the pharmaceutical preparation further
comprising at least one agent selected from the group consisting of
cytotoxic drugs, anti acne drugs, corticosteroids,
anti-inflammatory agents, antibiotics, anti- viral agents,
anti-psoriatic agents, keratinolytic agents, skin penetration
enhancers, local anaesthetic agents, antiseptic agents, metal ions,
tars and urea.
[0030] According to yet an additional aspect of the present
invention there is provided an article-of-manufacturing comprising
packaging material and a pharmaceutical preparation being
identified for treatment of skin or mucous membrane lesions, the
pharmaceutical preparation including, as active ingredients, about
48% (w/w) trichloroacetic acid, about 8% (w/w) hydrochloric acid
and about 3% (w/w) formic acid.
[0031] As used herein throughout, the term "about" refers to
.+-.10%.
[0032] According to still further features in the described
preferred embodiments the pharmaceutical preparation includes about
48% (w/w) trichloroacetic acid, about 8% (w/w) hydrochloric acid,
about 3% (w/w) formic acid and about 4% (w/w) formaldehyde.
[0033] According to a further aspect of the present invention there
is provided a method of treating and biopsying a skin or mucous
membrane lesion, the method comprising: (a) applying to the skin or
mucous membrane lesion at least one mummifying preparation, so as
to obtain, following a mummification period, a mummified skin or
mucous membrane lesion; and (b) collecting the mummified skin or
mucous membrane lesion.
[0034] According to still further features in the described
preferred embodiments the mummifying preparation includes, as
active ingredients, therapeutically effective amounts of at least
two agents selected from the group consisting of trichloroacetic
acid, hydrochloric acid and formic acid.
[0035] According to still further features in the described
preferred embodiments a concentration of the trichloroacetic acid
is selected from a range of 5%-97% (w/w), the concentration of the
hydrochloric acid is selected from a range of 3%-38% (w/w) and the
concentration of the formic acid is selected from a range of
0.1%-85% (w/w).
[0036] According to still further features in the described
preferred embodiments the mummifying preparation further comprises
a crosslinking/fixating/preserving agent.
[0037] According to still further features in the described
preferred embodiments the mummifying preparation includes, as
active ingredients, about 48% (w/w) trichloroacetic acid, about 8%
(w/w) hydrochloric acid and about 3% (w/w) formic acid.
[0038] According to still further features in the described
preferred embodiments the pharmaceutical preparation further
comprises about 4 % (w/w) formaldehyde.
[0039] According to still further features in the described
preferred embodiments the method further comprising staining the
mummified skin or mucous membrane lesion prior to histopathological
examination.
[0040] According to still a further aspect of the present invention
there is provided a kit useful for treating a skin or mucous
membrane lesion comprising: (a) an applicator including a reservoir
configured for storing a pharmaceutical preparation, the reservoir
being capped at one end by a removable applicator tip; (b) a
mechanism for forcing a pharmaceutical preparation stored by the
reservoir through the applicator tip; and (c) a plurality of
applicator tips, each being sized and configured for applying the
pharmaceutical preparation stored by the reservoir to a specific
type, shape or size of a skin or mucous membrane lesion.
[0041] According to still further features in the described
preferred embodiments the kit further comprising at least one
ampoule containing a pharmaceutical preparation including, as
active ingredients, therapeutically effective amounts of at least
two active ingredients selected from the group consisting of
trichloroacetic acid. hydrochloric acid and formic acid.
[0042] According to still a further aspect of the present invention
there is provided an adhesive bandage useful for treating skin
lesions comprising: (a) an applicator pad containing a
pharmaceutical preparation including at least two active
ingredients selected from the group consisting of trichloroacetic
acid, hydrochloric acid and formic acid; and (b) an adhesive tape
attached to the applicator pad, the adhesive tape being configured
for attaching to a skin region so as to position the applicator pad
against a portion of the skin region including a skin lesion
thereby applying the pharmaceutical preparation to the skin
lesion.
[0043] According to still further features in the described
preferred embodiments the pharmaceutical preparation including, as
active ingredients, therapeutically effective amounts of at least
two active ingredients selected from the group consisting of
trichloroacetic acid, hydrochloric acid and formic acid.
[0044] According to still further features in the described
preferred embodiments a concentration of the trichloroacetic acid
is selected from a range of 5%-97% (w/w), the concentration of the
hydrochloric acid is selected from a range of 3%-38% (w/w) and the
concentration of the formic acid is selected from a range of
0.1%-85% (w/w).
[0045] According to still further features in the described
preferred embodiments the pharmaceutical preparation includes, as
active ingredients, about 48% (w/w) trichloroacetic acid, about 8 %
(w/w) hydrochloric acid and about 3% (w/w) formic acid.
[0046] According to still further features in the described
preferred embodiments the pharmaceutical preparation further
comprises about 4% (w/w) formaldehyde.
[0047] According to still a further aspect of the present invention
there is provided a pharmaceutical preparation useful for treating
a skin or mucous membrane lesion comprising, as active ingredients,
therapeutically effective amounts of at least two agents selected
from the group consisting of trichloroacetic acid, hydrochloric
acid, formic acid, monochloroacetic acid, dichloroacetic acid,
glycolic acid, citric acid, kojic acid, acetic acid, azelaic acid,
phosphoric acid, thioglycolic acid, salicylic acid and their salts
and phenol.
[0048] According to yet a further aspect of the present invention
there is provided a pharmaceutical preparation useful for treating
a skin or mucous membrane lesion comprising, as active ingredients,
therapeutically effective amounts of at least one agent selected
from the group consisting of trichloroacetic acid, hydrochloric
acid, formic acid, monochloroacetic acid, dichloroacetic acid,
glycolic acid, citric acid, kojic acid, acetic acid, azelaic acid,
phosphoric acid, thioglycolic acid, salicylic acid and their salts
and phenol and at least one crosslinking/fixating/preserving
agent.
[0049] According to still further features in the described
preferred embodiments the at least one
crosslinking/fixating/preserving agent is selected from the group
consisting of formaldehyde; paraformaldehyde; glutaraldehyde;
glyoxal; carbodi-imide; a formaldehyde donor; sodium hydroxymethyl
glycinate; diazolidinyl urea; imidazolidinyl urea;
dimethilol-5,5-dimethilhydantoin; dimethilol urea;
2-bromo-2-nitropropane 1,3-diol; quarternium-15; parabens;
5-chloro-2 methylisothiazolin-3-one; 1,2-dibromo-2,4-dicyanobutane;
ethanol and other alcohols; polyol.
[0050] According to still a further aspect of the present
invention, there is provided a pharmaceutical preparation useful
for treating a skin or mucous membrane lesion, comprising as active
ingredients, a therapeutically effective amounts of at least one
agent selected from the group consisting of trichloroacetic acid,
hydrochloric acid, formic acid, monochloroacetic acid,
dichloroacetic acid, glycolic acid, citric acid, kojic acid, acetic
acid, azelaic acid, phosphoric acid, thioglycolic acid, salicylic
acid and their salts and phenol, and at least one nonoxidizing
organic or inorganic acid.
[0051] According to yet a further aspect of the present invention,
there is provided a pharmaceutical preparation useful for treating
a skin or mucous membrane lesion, comprising, as active
ingredients, at least one nonoxidizing organic or inorganic acid
and at least one crosslinking/fixating/preserving agent selected
from the group consisting of formaldehyde; paraformaldehyde;
glutaraldehyde; glyoxal; carbodi-imide; a formaldehyde donor;
sodium hydroxymethyl glycinate; diazolidinyl urea; imidazolidinyl
urea; dimethilol-5,5-dimethilhydantoin; dimethilol urea;
2-bromo-2-nitropropane 1,3-diol; quarternium-15; parabens;
5-cbloro-2 methylisothiazolin-3-one; 1,2-dibromo-2,4-dicyanobut-
ane; ethanol and other alcohols; polyol.
[0052] The present invention successfully addresses the
shortcomings of the presently known configurations by providing a
pharmaceutical preparation useful for removing skin or mucous
membrane lesions and for fixating tissues of skin or mucous
membrane lesions thereby enabling both treatment and
histopathological analysis of skin or mucous membrane lesions.
BRIEF DESCRIPTION OF THE DRAWINGS
[0053] The invention is herein described, by way of example only,
with reference to the accompanying drawings. With specific
reference now to the drawings in detail, it is stressed that the
particulars shown are by way of example and for purposes of
illustrative discussion of the preferred embodiments of the present
invention only, and are presented in the cause of providing what is
believed to be the most useful and readily understood description
of the principles and conceptual aspects of the invention. In this
regard, no attempt is made to show structural details of the
invention in more detail than is necessary for a fundamental
understanding of the invention, the description taken with the
drawings making apparent to those skilled in the art how the
several forms of the invention may be embodied in practice.
[0054] In the drawings:
[0055] FIG. 1 is an image of a mouse skin section fixed with
preparation A-Ia according.to the present invention, and stained
with H&E; magnification .times.100.
[0056] FIG. 2 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with H&E; magnification .times.200.
[0057] FIG. 3 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with H&E; magnification .times.400.
[0058] FIG. 4 is an image of a mouse skin section fixed with
preparation A-lb according to the present invention, and stained
with H&E; magnification .times.100.
[0059] FIG. 5 is an image of a mouse skin section fixed with
preparation A-lb according to the present invention, and stained
with H&E; magnification .times.200.
[0060] FIG. 6 is an image of a mouse skin section fixed with
Solcoderm.TM. and stained with H&E;
magnification.times.100.
[0061] FIG. 7 is an image of a mouse skin section fixed with
Solcoderm.TM. and stained with H&E;
magnification.times.400.
[0062] FIG. 8 is an image of a mouse skin section fixed with
buffered formaldehyde 4% and stained with H&E;
magnification.times.100.
[0063] FIG. 9 is an image of a mouse skin section fixed with
buffered formaldehyde 4% and stained with H&E;
magnification.times.200.
[0064] FIG. 10 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with Van-Gieson; magnification.times.100.
[0065] FIG. 11 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with Van-Gieson; magnification.times.200.
[0066] FIG. 12 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with Van-Gieson; magnification.times.400.
[0067] FIG. 13 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with Van-Gieson; magnification.times.400.
[0068] FIG. 14 is an image of a mouse skin section fixed with
Solcoderm.TM. and stained with Van-Gieson;
magnification.times.100.
[0069] FIG. 15 is an image of a mouse skin section fixed with
buffered formaldehyde 4% and stained with Van-Gieson;
magnification.times.400.
[0070] FIG. 16 is an image of a mouse skin section fixed with
preparation A-lb according to the present invention, and stained
with Cytokeratin; magnification .times.200.
[0071] FIG. 17 is an image of a mouse skin section fixed with
Solcoderm.TM. and stained with Cytokeratin;
magnification.times.200.
[0072] FIG. 18 is an image of a mouse skin section fixed with
buffered formaldehyde 4% and stained with Cytokeratin;
magnification.times.400.
[0073] FIG. 19 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with AgNOR; magnification .times.200.
[0074] FIG. 20 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with AgNOR; magnification .times.400.
[0075] FIG. 21 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with AgNOR; magnification .times.400.
[0076] FIG. 22 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with AgNOR; magnification .times.400.
[0077] FIG. 23 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with AgNOR; magnification .times.1000 (oil).
[0078] FIG. 24 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with AgNOR; magnification .times.1000 (oil).
[0079] FIG. 25 is an image of a mouse skin section fixed with
preparation A-Ia according to the present invention, and stained
with AgNOR; magnification .times.1000 (oil).
[0080] FIG. 26 is an image of a mouse skin section fixed with
Solcoderm.TM. and stained with AgNOR; magnification.times.100.
[0081] FIG. 27 is an image of a mouse skin section fixed with
Solcoderm.TM. and stained with AgNOR; magnification.times.400.
[0082] FIG. 28 is an image of a mouse skin section fixed with
buffered formaldehyde 4% and stained with AgNOR;
magnification.times.400.
[0083] FIG. 29 is an image of a mouse skin section fixed with
buffered formaldehyde 4% and stained with AgNOR;
magnification.times.400.
[0084] FIGS. 30a1-38c2 are images of patients treated with one
embodiment of the pharmaceutical preparation of the present
invention, (a1, a2)-prior to treatment, (b1, b2, c1 and
c2)--following treatment. FIGS. 30a1-b2 --Intradermal nevus; 1
topical treatment; scab dropped 20 days after treatment; pictures
taken 27 days after treatment. FIGS. 31a1-b2--Veruca vulgaris; 3
topical treatments; complete healing after 50 days. FIGS. 32a1-b2
--Intradermal nevus; 1 topical treatment; scab dropped 25 days
after treatment; pictures taken 31 days after treatment. FIGS.
33a1-c2--Intradermal nevus; 1 topical treatment, scab dropped 22
days after treatment, pictures taken 36 (FIG. 33b1 and b2) and 65
(FIG. 33c1 and b2) days after treatment. FIGS. 34a-b--Veruca
vulgaris; 3 topical treatments; complete healing after 43 days.
FIGS. 35a-b--Intradermal nevus; 1 topical treatment; scab dropped
18 days after treatment; pictures taken 39 days after treatment.
FIGS. 36a1-b--Two intradermal nevi; 1 topical treatment; scabs
dropped 16 & 18 days after treatment; pictures taken 22 days
after treatment. FIGS. 37a1-b--Pigmented skin tags; 1 topical
treatment; scabs dropped 9-14 days after treatment; pictures taken
30 days after treatment. FIGS. 38a-c--Seborrheic keratosis; 2
topical treatments, the second performed 32 days after the first
one (FIG. 38b1 and 2); complete healing is observed 57 days
following initial treatment (FIG. 38c1 and 2).
[0085] FIGS. 39-50 illustrate sections of a scab formed and
detached following treatment of an intradermal nevus on the
forehead of a 31 year old woman by a single topical application of
one embodiment of the pharmaceutical preparation of the present
invention. FIGS. 39-42 illustrates Hematoxylin & eosin
staining. The specimens illustrate a skin fragment showing squamous
epithelium with dermis (magnifications: .times.40, .times.100,
.times.200, .times.400, respectively). The preservation of the
tissue (if normal is given a score 4 out of 4) is not as optimal as
routine formalin fixated tissue, shows some artifactual shrinkage,
and would be given a grading score of 3 to 3.5 of 4. The
architecture of epithelium and dermal tissues are sufficiently
preserved. The specimens present the following: (a) normal lining
keratinizing epithelium, (b) normal dermal adnexal structures, (c)
clusters and nests of intradermal melanocytic cells showing no
cellular atypia or pleomorphism. The diagnosis in these specimens
is that of an intradermal nevus. Had a suspected malignancy been
present in these specimens, the tissue preservation is sufficiently
good to enable its identification. FIG. 43 illustrates Van-Gieson
staining of the specimen of FIGS. 39-42. This stain highlights
connective tissue (preferential to elastic and collagen fibers)
with a red-pink uniform color. FIG. 44 illustrates Cytokeratin
staining of the specimen of FIGS. 39-42. Cytokeratin stain, which
is an immunohistochemical stain, stains the cell membranes of
epithelial cells of both the epidermis and adnexal structures (hair
follicles). The stain shows a "rim" of brown staining that is
limited to the cell membrane with no staining of the cytoplasm or
nucleus. In the skin, the stain is most prominent in the most
basally situated epithelial cells, and thereby delineates the
basement membrane of the skin. FIGS. 45-46 illustrates HMB 45
staining of the specimen of FIGS. 39-42. This stain is a selective
immunohistochemical (membrane) stain for malignant melanocytes and
does not stain the benign nevus cells in the specimen. FIGS. 47-50
illustrate AgNOR staining of the specimen of FIGS. 39-42. This
stain is not limited to cell types, and as such stains both
epithelial and stromal cells (e.g. squamous cells and smooth muscle
cells). The staining does not delineate cell membranes but rather
stains (in dark brown) the nuclei and para-nuclear cytoplasm in a
non-uniform punctate pattern.
[0086] FIGS. 51a-b illustrate an applicator configured for applying
the preparations of the present invention to skin or mucous
membrane lesions.
[0087] FIGS. 52a-b illustrate an adhesive bandage configured for
treating skin lesions according to the teachings of the present
invention.
DESCRIPTION OF THE PREFERRED EMBODIMENTS
[0088] The present invention is of a pharmaceutical preparation
which can be used to treat skin or mucous membrane lesions.
Specifically, the present invention can be used to remove skin or
mucous membrane lesions in a manner which enables histopathological
examination of removed lesion tissue.
[0089] The principles and operation of the present invention may be
better understood with reference to the drawings and accompanying
descriptions.
[0090] Before explaining at least one embodiment of the invention
in detail, it is to be understood that the invention is not limited
in its application to the details of construction and the
arrangement of the components set forth in the following
description or illustrated in the drawings. The invention is
capable of other embodiments or of being practiced or carried out
in various ways. Also, it is to be understood that the phraseology
and terminology employed herein is for the purpose of description
and should not be regarded as limiting.
[0091] As used herein, the phrase "skin or mucous membrane lesions"
generally refers to benign or malignant pathologies of skin or
mucousal membrane tissues. Examples of skin or mucous membrane
lesions treatable by the preparations and methods of the present
invention include, but are not limited to, dermatoses, seborrheic
keratosis, intradermal nevus, verucae, condylomata accminata,
seborrheic dermatitis, atopic dermatitis, eczema, hyperkeratosis,
acne (acne vulgaris), psoriasis; bacterial, fungal and/or viral
infections of the skin and/or the mucous membranes/tissues,
diabetic and/or ischemic wounds/ulcers, decubitus ulcers and oral
lesions (lesions of the oral mucosa) such as aphthous
stomatisis.
[0092] According to one aspect of the present invention there is
provided a pharmaceutical preparation useful for treating a skin or
mucous membrane lesion. The pharmaceutical preparation comprises,
as active ingredients, therapeutically effective amounts of at
least one, preferably at least two, active ingredients selected
from the following: trichloroacetic acid, hydrochloric acid, formic
acid, monochloroacetic acid, dichloroacetic acid, glycolic acid,
citric acid, kojic acid, acetic acid, azelaic acid, phosphoric
acid, thioglycolic acid, salicylic acid and their salts and phenol.
Preferably, the pharmaceutical preparation includes trichloroacetic
acid, hydrochloric acid and optionally formic acid.
[0093] The pharmaceutical preparation may also advantageously
include a crosslinking/fixating/preserving agent, examples of which
are given hereinbelow.
[0094] Table 1 below lists possible combinations and concentrations
of presently preferred active ingredients suitable for use as the
pharmaceutical preparation of the present invention.
1TABLE 1 Presently preferred active ingredient combinations
Hydrochloric trichloroacetic Formic acid acid acid Formaldehyde
Preparation 1 8% 48% 3% -- (A - Ib)* Preparation 2 10% 33% 4% -- (A
- Ia)* Preparation 3 13% 20% 5% -- Preparation 4 8% 48% -- --
Preparation 5 10% 33% -- -- Preparation 6 13% 20% -- -- Preparation
7 8% 48% 3% 4% (A - Ib+)* Preparation 8 10% 33% 4% 4% (A - Ia+)*
Preparation 9 13% 20% 5% 4% Preparation 10 -- 46% 5% -- Preparation
11 -- 46% 5% 4% final concentrations of active ingredients given in
weight per weight (w/w) *designation used hereinbelow for these
specific preparations.
[0095] According to a preferred embodiment of the present
invention, the concentration of each of the active ingredients is
selected such that application of the preparation to the skin or
mucous membrane lesion leads to drying (mummification) and
separation of the skin or mucous membrane lesion from its base
tissue.
[0096] As used herein, the term "mummification" and its derivatives
include dehydration and/or fixation and/or preservation of tissue
in such manner that following rehydration a mummified tissue is (i)
rehydratable; and (ii) amenable to meaningful hystopathological
staining and analysis.
[0097] The phrase "meaningful hystopathological staining" refers to
a hystopathological staining that allows clear identification
between pathological and normal state. Examples of suitable stains
used for obtaining hystopathological staining are given in the
Brief Description of the Drawings section above.
[0098] As has already been stated in the background section above,
although a study performed by Cesarini from the Department of
Dermatology, Foundation Rothschild, Paris, France (Dermatologica
168; suppl. 1. pp. 15-25 (1984)) suggested that the fixative
properties of Solcoderm.TM. are adequate for histopathological
diagnosis of post-treatment scabs, the same study demonstrated that
when H & E staining is used (the single histochemical staining
method used) the cellular elements stain in pale pink while the
extra cellular compartment does not stain at all; furthermore,
anisocytosis, anisokariosis and polychromatophilia, the usual
landmarks of cytologists, cannot be observed and described. These
findings may be explained by the fact that prior art preparations
such as Solcoderm.TM., utilize nitric acid, a strong oxidizing
acid, which tends to destroy treated tissues.
[0099] Hence, the type and concentrations of the active
ingredient(s) of the preparation of the present invention are
preferably selected such that cellular and extracellular morphology
of treated lesions is preserved following detachment of the lesion
from its surrounding skin or membrane tissue.
[0100] Furthermore, the active ingredient(s) of the preparation of
the present invention are also preferably selected so as to
facilitate penetration of the pharmaceutical preparation into the
treated tissue. This feature is particularly advantageous
especially in cases where crosslinking agents are used, since such
agents oftentimes exhibit poor tissue penetration properties.
Hence, the active ingredients are preferably selected to synergize
with the crosslinking agents with respect to dehydration and
mummification.
[0101] As described in the Examples section below, lesions treated
according to the teachings of the present inventions completely
separated from their base tissue, and fell off, in some cases, a
few days following a single topical application of the preparation
of the present invention. It is important to note that since this
separation does not occur until re-epithelialization ends, the skin
exposed following separation of a lesion is dry, smooth, healthy,
and manifests no signs of local infection, i.e., suppuration,
bleeding or festering.
[0102] As is described in the Examples section which follows, the
preparations of the present invention are also capable of
preserving the morphology and composition of tissue and cells
treated thereby. It stands to reason that these preservation
capabilities of the present preparation underlie or contribute to
its effectiveness in treating skin lesions, since tissue
drying/mummification probably leads to separation of the skin
lesion from the skin. Thus, when formulating additional
pharmaceutical preparations useful for treating skin or mucous
membrane lesions, consideration can also be given to tissue
preservation qualities of preparation ingredients.
[0103] Due to these tissue preservation capabilities, treatment
with the pharmaceutical preparation of the present invention
enables meaningful post treatment analysis of the architectural and
histological morphology of treated tissues, a feature which is
extremely important especially in cases where lesion tissue cannot
be accurately diagnosed prior to treatment, which feature is absent
in prior art preparations. Example 1 below details morphology
preservation qualities of the pharmaceutical preparation of the
present invention and compares such qualities with those of a
tissue preservative (i.e., formaldehyde) and Solcoderm.TM., a prior
art pharmaceutical preparation.
[0104] To enhance such tissue preservation features, the
pharmaceutical preparation of the present invention preferably
includes at least one crosslinking/fixating/preserving agent, the
concentration of which is selected according to the lesion tissue
to be treated. Examples of suitable
crosslinking/fixating/preserving agents include, but not limited to
formaldehyde; paraformaldehyde; glutaraldehyde; glyoxal;
carbodi-imide; a formaldehyde donor (a formaldehyde releasing
substance); sodium hydroxymethyl glycinate; diazolidinyl urea;
imidazolidinyl urea; dimethilol-5,5-dimethilhydantoin; dimethilol
urea; 2-bromo-2-nitropropane 1,3-diol; quarternium-15; parabens;
5-chloro-2 methylisothiazolin-3-one; 1,2-dibromo-2,4-dicyanobutane;
ethanol and other alcohols; and polyols.
[0105] The pharmaceutical preparation of the present invention may
also include at least one agent which functions in improving
penetration of the preparation into lesion tissue, preventing
infections, preventing lesion cell proliferation and/or reducing
discomfort associated with treatment.
[0106] Examples of agents falling into this category include, but
are not limited to, cytotoxic drugs, anti acne drugs,
corticosteroids, anti-inflammatory agents, antibiotics, anti-viral
agents, anti-psoriatic agents, keratinolytic agents, skin
penetration enhancers, local anaesthetic agents, antiseptic agents,
metal ions, tars and urea.
[0107] According to another preferred embodiment of the present
invention the pharmaceutical preparation includes about 48% (w/w)
trichloroacetic acid, about 8% (w/w) hydrochloric acid and about 3%
(w/w) formic acid. As is described in the Examples section below,
such a formulation was extremely effective in treating various
forms of skin lesions.
[0108] The pharmaceutical preparation of the present invention is
preferably provided as an aqueous solution contained in, for
example, an ampoule or any other suitable container.
[0109] The pharmaceutical preparation of the present invention can
also be provided in a paste (ointment or cream), or gel form by
mixing the active ingredient(s) of the pharmaceutical preparation
of the present invention with suitable thickeners or gelating
materials the likes of which are well known in the art.
Alternatively, when possible, the pharmaceutical preparation can be
provided in a rehydratable powder form, as a tincture.
[0110] It will be appreciated that in cases of reactive or unstable
active ingredients, the preparation of the present invention can be
provided in two or more separate ampoules or other kinds of
containers which can be combined prior to use.
[0111] For example, when crosslinking/fixating/preserving agents
are used in the pharmaceutical preparation of the present
invention, such agents may be provided in a separate ampoule and
combined with other active ingredients immediately prior to
use.
[0112] Preferably, the preparation of the present invention is
provided as part of an article-of-manufacturing which also includes
packaging material identifying the pharmaceutical preparation of
the present invention as useful for treatment and/or preservation
of a skin or mucous membrane lesion.
[0113] As already mentioned hereinabove, the pharmaceutical
preparation of the present invention can be utilized to treat a
variety of skin and mucousal membrane lesions.
[0114] Such treatment is effected by applying the pharmaceutical
preparation to the lesion (see, Example 2 for further detail) using
a syringe, a swab or a specially adapted applicator. A presently
preferred applicator is further described in Example 5 of the
Examples section which follows.
[0115] In cases where collection of the lesion tissue (typically in
lesions of skin tissue) is desired for histopathological
examination, application of the pharmaceutical preparation is
followed by bandaging such that the mummified skin lesion tissue is
retained by the bandage following separation, thus allowing
post-collection treatment (e.g., rehydration) and histopathological
analysis of the lesion tissue.
[0116] Application of the pharmaceutical preparation of the present
invention can also be effected via a specialized adhesive bandage.
Such a bandage is also described in Example 5 of the Examples
section.
[0117] An adhesive bandage applicator is especially advantageous in
cases where histopathological examination is desired, since it can
also serve to collect the lesion tissue following separation.
[0118] Thus, the present invention provides a pharmaceutical
preparation and methods of using same for treating and/or
mummifying lesion tissue.
[0119] As is further detailed in the Examples section which
follows, the preparation of the present invention is effective at
both treating and mummifying lesion tissue.
[0120] In addition, the preparation of the present invention is
harmless for use, free of side effects, while treatment therewith
is only slightly discomforting to the patient.
[0121] Finally, since complete treatment can oftentimes be effected
using a single application, the preparation of the present
invention provides an easy, rapid and inexpensive method of
removing lesions while minimizing scar tissue, infections and any
other problems usually associated with prior art methods of skin
lesion removal.
[0122] Additional objects, advantages, and novel features of the
present invention will become apparent to one ordinarily skilled in
the art upon examination of the following examples, which are not
intended to be limiting. Additionally, each of the various
embodiments and aspects of the present invention as delineated
hereinabove and as claimed in the claims section below finds
experimental support in the following examples.
EXAMPLES
[0123] Reference is now made to the following examples, which
together with the above descriptions, illustrate the invention in a
non limiting fashion.
[0124] In histopathology, most tissues are fixed prior to
microscopic examination. Since fixation oftentimes precedes various
tissue preparation steps, such as, for example, tissue staining, it
is essential that a fixative is selected according to the tissue
type to be fixed, and purpose of fixation.
[0125] Tissue fixation is caused by a complex series of chemical
events which depend on the fixation protocol used and tissue type
fixed. It is important that tissue morphology and composition is
maintained as much as possible during fixation steps, such that
fixed tissue accurately represents the living state of the tissue
prior to fixation.
[0126] Although most fixation protocols aim to preserve tissue
morphology and composition, some substances, e.g. lipids, are
always lost unless special precautions are taken.
[0127] Most fixation protocols preserve the microanatomy of the
tissues well enough to allow fixed tissues to be used in, for
example, histopathological diagnosis.
[0128] To preserve microanatomy, most fixation protocols employ
reagents which form crosslinks between proteins, since such
crosslinks ensure preservation of protein structures which dictate
cellular morphology.
[0129] Protein crosslinking is typically mediated by aldehyde
groups; reactions between fixative agents, such as formaldehyde,
and amino acids, such as lysine, form crosslinks between protein
molecules.
[0130] Formaldehyde, glyoxal and glutaraldehyde have long been used
as crosslinking agents. In the case of formaldehyde, the
crosslinking reaction can be reversed during the first 24 hours of
reaction by simply saturating the reaction with excess water. With
glutaraldehyde, on the other hand, the reaction is rapid and
irreversible.
[0131] One of the important effects of fixation on proteins is the
extent of denaturation. For most routine histopathology analysis
such denaturation is of no consequence. However, in the case of
immunofluorescence, immunohistochemistry and high resolution
electron microscopy it is clearly of considerable importance.
[0132] In such cases, mild fixating conditions are used such that
antigenic sites are not greatly altered or destroyed or that
morphology of large molecules remains unchanged.
[0133] Depending on the protein, glutaraldehyde fixation can cause
a loss of up to 30 percent of .alpha.-helix structures, while
fixation with osmium tetraoxide or post-osmication of
glutaraldehyde-fixed material can cause the complete denaturation
of the protein.
[0134] Due to tissue heterogeneity, no single fixation protocol is
ideal for all tissue components or types. As such, researchers
often use mixtures of fixatives which are formulated such that a
limitation of one fixative agent is compensated for by another
fixative agent in the mixture. In some mixtures, the components may
react together, such as the case with aldehydes and oxidizing
agents. If such mixtures are used, then the active components must
be mixed immediately before use, otherwise, the effective
concentration of each agent will be decreased, possibly to levels
that are no longer effective.
[0135] Histopathological staining, including the use of a basement
membrane/collagen stain to emphasize the basic architecture of a
tissue or a neoplasm, are currently used as preliminary tissue
analysis methods oftentimes prior to use of more accurate
immunohistochemical analysis methods. Several choices of stains,
including PAS, silver (reticulin) stains, or a trichrome stain,
which is a three dye stain used for selective demonstration of
muscle, collagen fibers, fibrin and erythrocytes.
[0136] The use of immunohistochemical methods has vastly improved
diagnosis of tumors of uncertain origin. By using monoclonal and
polyclonal antibodies for identifying protein structures,
immunohistochemical methods enable accurate differentiation between
various tumor types and as such represent the most valuable tool at
the disposal of a histopathology investigator.
[0137] Since keratins are present in all epithelial cells, they
represent highly sensitive markers for malignant cells of
epithelial origin (e.g., carcinomas). There are more than 20
different subtypes of human keratin proteins each distinguished by
a specific molecular weight and/or isoelectric point. Specific
monoclonal antibodies have been developed against many of these
subtypes and immunohistochemical studies have shown that some
carcinomas have characteristic keratin profiles.
[0138] Although keratin expression is characteristic of epithelial
cells, non- epithelial neoplasms may in rare instances show
aberrant expression of keratin. Such tumors include lymphomas
(especially anaplastic large cell lymphoma), various sacromas,
gliomas, epithelioid vascular tumors, and melanomas.
[0139] Melanoma, oftentimes presents as a poorly differentiated
malignant neoplasm. Traditionally, Fontanta-Masson or other
silver-based stains for melanin and for the ultrastructural
detection of melanosomes have assisted in the diagnosis of
melanomas.
[0140] Melanomas typically have very little or no cytoplasmic
keratin but do stain with antivimentin, antibodies directed against
the S-100 protein which is a fairly stable antigen that withstands
formaldehyde fixation and paraffin embedding, and antibodies
directed against melanosomes.
[0141] In melanoma analysis, anti-S-100 staining is typically
effected along with additional histopathological or
immunohistopathological staining since the S-100 also appears in
benign nevus cells, Langerhans histiocytes, many sacromas
(liposarcomas and chondrosacromas), neural tumors (schwanomas,
neurofibromas, and granular cell tumors), and certain carcinomas,
such as those derived from the salivary gland, breast, and
lung.
[0142] The identity of S-100 positive neoplasm as a melanoma is
typically confirmed by reaction with HMB45, an antibody which
recognizes a melanoma-specific antigen by reacting with melanoma
cells and junctional nevus cells, but not normal melanocytes or
intradermal nevus cells.
[0143] The distribution of nucleolar acidic proteins selectively
stained by silver has become an important parameter for the
cytohistologic diagnosis of malignancy. The silver-stained (Ag)
proteins are located in nucleolar components which contain
ribosomal genes and represent the interphase counterpart of
metaphase nucleolar organizer regions (NORs). These proteins are
therefore called Ag-NOR proteins. It has been repeatedly
demonstrated that malignant tumors can be easily distinguished from
corresponding benign lesions on the basis of a greater quantity of
nucleolar Ag-NOR proteins.
[0144] Although the argyrophil method for NORs, known as the AgNOR
technique, identifies NOR-associated proteins rather than NORs
themselves, it is still considered highly specific. Crocker and
Skilbek (J Clin Pathol 40; 885-889;1987) have shown that
melanocarcinomas can readily be distinguished from naevocellular
naevi by using the AgNOR method. Thus, the simplicity and
applicability of the AgNOR method makes it a potentially powerful
histopathological tool.
Example I
Fixative Properties of the Pharmaceutical Preparations of the
Present Invention
[0145] A series of tissue fixating/staining experiments were
conducted in order to examine the fixating capability of each of
the components of the pharmaceutical preparations of the present
invention. In order to uncover possible synergistic relationships,
all possible combinations of these components were tested.
[0146] The information obtained from these experiments was cross
referenced with data regarding the corrosive nature of these
components, the level of burning or pain they cause upon skin
contact, and their ability to penetrate deeply into the tissue and
soften it during treatment.
[0147] Three main components were tested: trichloroacetic acid
(TCA), hydrochloric acid (HCl) and Formic acid (FA). These three
main components of the preparation were tested alone and in various
combinations as detailed in Table 2 below. In addition,
Solcoderm.TM. and its new version (U.S. Pat. No. 5,573,786) were
also tested and used as controls.
[0148] Materials and methods
[0149] Sections of mouse skin 8 mm in diameter were submerged into
1 ml of a test preparation in glass tubes sealed with a rubber
stopper, and incubated for 24 hours. The treated sections of mouse
skin were then recovered, dried on absorbent paper and laid upon
Petrie dishes, lined with two layers of absorbent paper. The skin
sections were flattened and loosely taped to the absorbent paper
using strips of breathing micropore tape and dried at room
temperature (RT) for 30 days. Following complete skin drying, the
specimens were sent for routine processing prior to being stained
with histochemical and immunohistochemical stains, as detailed
below. Skin treated with buffered formaldehyde 4% served as a
control. The scoring of fixation quality seen in the different
staining methods was determined according to the following key:
[0150] Score 1: Only the keratin and hair structures remain.
[0151] Score 2: Keratin and hair structures preserved, and the
"architecture" of the tissue is present. Cellular detail is not
present.
[0152] Score 3: Keratin and hair structures preserved,
"architecture" preserved and the dermal tissue shows cellular
detail. If a foreign, malignant or abnormal infiltrate was present
in the specimen, identification thereof is likely.
[0153] Score 4: All elements of epithelium as well as the dermal
tissue are preserved.
[0154] Fixation and staining at levels 3-4 enable identification
and preliminary diagnosis of a space-occupying lesion or a
suspicion of malignancy.
[0155] Results and discussion
[0156] The results, as summarized in Table 2 below, indicate
synergism among TCA HCl and FA as expressed in preservation of both
the architecture and cellular detail of the tissue section.
[0157] As shown in FIGS. 1-29, tissue sections treated with
preparation A-Ia and stained with H&E (FIGS. 1-3), Van-Gieson
(FIGS. 10-13), or AgNOR (FIGS. 19-25), and tissue sections treated
with preparation A-lb and stained with H&E (FIGS. 4-5) or
cytokeratin (FIG. 16) exhibited morphology which more closely
resembles that of formaldehyde fixed controls (FIGS. 8, 9, 15, 18
and 28-29) as compared to tissue sections treated with
Solcoderm.TM. and stained with H&E (FIGS. 6-7), Van-Gieson
(FIG. 14), cytokeratin (FIG. 17) or AgNOR (FIGS. 26-27).
2TABLE 2 Results of a clinical study Compound in ml. Hcl FA TCA 35%
85% Score 90% (w/w) (w/w) Formaldehyde Average (w/w) Stock Stock
40% H.sub.2O H & E Ag NOR Cytokeratin Score 0.6 0.4 1-2 3 2
2.16 0.6 0.4 1 1 1 1.00 0.6 0.4 2 3-4 2 2.50 0.3 0.3 0.4 1-2 3 2
2.16 0.3 0.3 0.4 1-2 4 2 2.50 0.3 0.3 0.4 1 1 1 1.00 0.2 0.2 0.2
0.4 2-3 4 3 3.16 0.2 0.2 0.2 0.1 0.3 3 5** 3 3.66 Form A-I a (1.0
ml)* 2-3 4 3 3.16 Form A-I b (1.0 ml)* 3 5 2-3 3.5 Form A-I a+ (1.0
ml)* 3 5** 3 3.66 Form A-I b+ (1.0 ml)* 3-4 5** 2-3 3.66 Solcoderm
.TM. (1.0 ml) 1 1 1 1.00 Solcoderm .TM. new version 1996 (1.0 ml) 1
1 1 1.00 Control-buffered formaldehyde 4% (1.0 ml) 4 4 4 4.00 *For
compositions - see Table 1. **Better than control.
[0158] As shown in FIGS. 19-29, the AgNOR stained tissue sections
exhibited better than control morphology. Use of this stain enables
clear visualization of the basal membrane, the epidermis-dermis
border and nuclear matter, thus enabling quantification of NORs in
every cell and determination of abnormal mitotic activity. This
stain also enables evaluation of the proportion between nuclei and
stroma as a parameter of proliferation of epithelial cells and as
such is especially useful in the diagnosis of malignant
melanoma.
[0159] Various parameters were taken into account during the design
of the different versions of the preparation. If one considers the
tissue penetration ability on the one hand and fixation quality on
the other, versions a, b, a+ and b+ of Formulation A-I. (see Table
1) are particularly effective, where fixative treatment using
version b enables faster softening of the tissue and is therefore
more suitable for lesions and tumors with a harder consistency or
those well protected by an especially thick layer of keratin.
[0160] In light of the data presented herein, it is evident that
several versions of the pharmaceutical preparation of the present
invention can be effectively used as a treatment/fixative
preparation since it enables retrospective histopathological
diagnosis of tissue treated thereby.
[0161] Following determination of its fixative properties
preparation A-I was used in a series of clinical studies in order
to determine its effectiveness in treating skin lesions (Example 2)
as well as to determine the level of discomfort, if any, when used
in treatment (Example 3).
Example 2
Clinical Study
[0162] A clinical study involving 87 patients, with a total number
of 228 lesions was conducted. The patients were divided into 2 main
groups: group A --highly responsive STLs; group B--less responsive
STLs.
[0163] The diagnosed STLs of Group A included: Intradermal Nevus,
Fibroepithelial Polyp, Dermatofibroma, Seborrheic Keratosis,
Condyloma Acuminata and Veruca Plana. The diagnosed STLs of Group B
included Veruca vulgaris and Haemangioma.
[0164] The patients were treated with preparation A-lb described
hereinabove in Table 1. Treatment regimen was as follows: an
applicator was dipped into the preparation and used to wet the
lesion. The entire area of the lesion was moistened, while avoiding
contact between the preparation and surrounding healthy tissues. If
the healthy tissue adjacent to the lesion was moistened, it was
immediately wiped dry with a cotton swab.
[0165] Using moderate pressure on the applicator, both
perpendicularly to the skin and at a 45.degree. angle if the lesion
protrudes above the skin, the preparation was forced into the
treated tissue. As the liquid penetrated, the lesion softens, and
the application treatment was stopped. The patient was instructed
to moisten the treated area several times daily, using absorbent
cotton saturated with 70% alcohol, beginning 24 hours after the
treatment, and especially after showering.
[0166] Following this treatment regimen, the tissue undergoes
fixation and gradual drying, until the lesion completely separates
from its base tissue, and falls off. Since this separation does not
occur until re-epithelialization ends, the exposed skin is dry,
smooth, healthy, and manifests no signs of local infection, i.e.,
suppuration, bleeding, or festering. The slight hyperemia in the
treated area gradually subsides.
[0167] The patient usually feels a local, tolerable, burning
sensation, which does not require the use of local anesthesia, and
which subsides completely several minutes following the end of the
treatment. There is no need for local bandaging, as the scab in
itself serves as a biological bandage. If the fixed lesion is to be
sent for histopathological examination, the treated area is covered
with a breathing micropore bandage, to prevent loss of the
scab.
[0168] Results
[0169] Table 3 below summarizes the results of the clinical trial.
Among the 87 patients treated, 11 did not appear for the follow-up
examination carried out 6 months or more following treatment; these
cases have not been included in the data presented here.
[0170] FIGS. 30a1-38c2 are images of patients having skin lesions
prior to (a1 ans a2) and following (b1i, b2, c1 and c2) treatment
with the preparation of the present invention. STLs types treated
in this study were divided into highly responsive STLs and less
responsive STLs in order to obtain a more lo clear representation
of the collected results, thus permitting precise evaluation of the
data concerning the efficiency of the preparation of the present
invention.
3TABLE 3 Clinical trial results Number of Number of local Number
successful applications Group Diagnosis of STLs results Failures
(Average) Recurrences A Intradermal nevus 62 62 -- 1-2 -- (1.11)
Fibroepithelial 15 15 -- 1-2 -- Polyp (skin tag) (1.13)
Dermatofibroma 6 6 -- 1-2 -- (1.33) Seborrheic 20 20 -- 1-2 --
keratosis (1.30) Condyloma 19 19 -- 1-2 2 acuminata (1.36) (10.5%)
Veruca plana 12 12 -- 1-2 -- (1.25) B Veruca vulgaris 57 53 4 1-4 6
(common wart) (7.0%)* (2.81) (11.3%) Haemangioma 11 11 -- 1-3 --
(1.90) *The treatment was considered a failure when a lesion of
veruca vulgaris did not completely respond to 4 local
applications.
[0171] The crust which formed at the treated region was detached in
almost all cases 9-22 days following treatment (maximum 27 days).
Hyperpigmentation developed In 3.4% of treated STLs, while
hypopigmentation developed in 6.4% of the cases. Superficial
scarring was noted for 2.9% of the treated STLs. In most cases,
slight pigmentation changes, which usually appear after the crust
drops, gradually vanished in within a few days.
[0172] Thus, the preparation of the present invention provides a
suitable inexpensive and readily available alternative to
destructive treatment methods (e.g., laser and cryosurgery) while
providing the physician with the ability to use the treated tissue
for histopathological analysis if need be.
Example 3
Staining of Tissue Treated with the Pharmaceutical Preparation of
the Present Invention
[0173] Sections of a scab formed and detached following treatment
of an intradermal nevus on the forehead of a 31 year old woman by a
single topical application of preparation A-lb were stained with
Hematoxylin & eosin, Van-Gieson, Cytokeratin, HMB 45 and AgNOR.
The results are shown in FIGS. 39-50.
Example 4
Comparison of the Degree of Burning Sensation between the
Composition of the Present Invention and Solcoderm.TM.
[0174] Treatments were conducted concurrently on 14 men and women
with pairs of adjacent tumors that were more or less identical in
size and nature in order to compare the burning sensation of the
preparation of the present invention with that produced by
Solcoderm.TM., a commercially available preparation. The patients
were asked to answer two questions at the end of the treatment
regimens, which treated side burn/hurt more (with an option to
answer identical burning/pain) and if the one that burns more or is
more painful is defined as a level 3 burn/pain, how would you
define the other treated area, using the following scale:
[0175] Level 0: no sensation at all.
[0176] Level 1: slight sensitivity
[0177] Level 2: moderate sensitivity
[0178] Level 3: severe sensitivity
[0179] Results
[0180] As shown in Table 4 below, the preparation of the present
invention caused, on an average, slight to moderate sensitivity,
whereas Solcoderm.TM. caused severe sensitivity in most patients
treated.
4TABLE 4 Results of burning sensation assessment Patient No.
Average 1 2 3 4 5 6 7 8 9 10 11 12 13 14 Score Solcoderm .TM. 3 3 3
2 3 3 3 3 3 3 2 3 3 3 2.85 Form. A-Ib 2 1 2 3 1 3 3 1 1 1 3 1 1 2
1.78
[0181] Thus, treatment with the preparation of the present
invention causes far less discomfort to the patient as compared to
Solcoderm.TM..
Example 5
The Therapeutic Kit
[0182] The compositions of the present invention may be applied
using a therapeutic kit. Such a kit includes:
[0183] (i) an ampoule containing the medicine;
[0184] (ii) several specially adapted applicators of different
diameters (described in detail below);
[0185] (iii) breathing micropore adhesive tape;
[0186] (iv) small paper envelope for sending the specimen, that is
also a form for recording the patient's details, date, and name of
attending physician.
[0187] (v) stand and handle for ampoule; and
[0188] (vi) small cotton applicator.
[0189] The applicator, which is referred to herein as applicator
10, is illustrated in FIGS. 51a-b. Applicator 10 includes a syringe
like mechanism 12 (FIG. 51a) for dispensing the preparation of the
present invention through a specially adapted tip 14 (FIG. 51b).
The tip can be fabricated in a variety of diameters, dispensing
hole patterns, and shapes so as to enable efficient and accurate
provision of the preparation of the present invention onto skin or
mucous membrane lesions of various shapes and sizes.
[0190] Adhesive bandage
[0191] The preparation of the present invention can also be applied
via an adhesive bandage. As specifically shown in FIGS. 52a-b, such
a bandage 20 includes an applicator 21 (e.g., pad 22 or reservoir
22') which is soaked with or contains the pharmaceutical
preparation of the present invention and an adhesive tape 24 which
is attached to applicator 21. Adhesive tape 24 is configured for
attaching to a skin region thereby positioning applicator 21
against a portion of the skin region which includes the skin
lesion. Upon such positioning the pharmaceutical preparation of the
present invention is applied to the skin lesion via diffusion or
active release (e.g., physical pressure on applicator pad ruptures
microvesicles which release the preparation or slow release from
microcapsules). A removable (e.g., peelable) cover 26 protecting
applicator 21 may also be employed.
[0192] It is appreciated that certain features of the invention,
which are, for clarity, described in the context of separate
embodiments, may also be provided in combination in a single
embodiment. Conversely, various features of the invention, which
are, for brevity, described in the context of a single embodiment,
may also be provided separately or in any suitable
subcombination.
[0193] Although the invention has been described in conjunction
with specific embodiments thereof, it is evident that many
alternatives, modifications and variations will be apparent to
those skilled in the art. Accordingly, it is intended to embrace
all such alternatives, modifications and variations that fall.
within the spirit and broad scope of the appended claims. All
publications, patents, and patent applications mentioned in this
specification are herein incorporated in their entirety by
reference into the specification, to the same extent as if each
individual publication, patent, or patent application was
specifically and individually indicated to be incorporated herein
by reference. In addition, citation or identification of any
reference in this application shall not be construed as an
admission that such reference is available as prior art to the
present invention.
* * * * *