AU751118B2 - Pharmaceutical composition - Google Patents
Pharmaceutical composition Download PDFInfo
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- AU751118B2 AU751118B2 AU53496/00A AU5349600A AU751118B2 AU 751118 B2 AU751118 B2 AU 751118B2 AU 53496/00 A AU53496/00 A AU 53496/00A AU 5349600 A AU5349600 A AU 5349600A AU 751118 B2 AU751118 B2 AU 751118B2
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- Australia
- Prior art keywords
- analogue
- mannose
- phosphate
- formula
- healing
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Description
AUSTRALIA
Patents Act 1990 COMPLETE SPECIFICATION STANDARD PATENT Applicant(s): Ra04 TH
T
ITP..' NVESTYO DCES- Invention Title: Pharmaceutical Composition The following statement is a full description of this invention, including the best method of performing it known to me/us: 1A Pharmaceutical Composition The present invention concerns pharmaceutical compositions for promoting the healing of wounds or fibrotic disorders, in particular for promoting the healing of wounds or fibrotic disorders with reduced scarring.
By "wounds or fibrotic disorders" is meant any condition which may result in the formation of scar tissue. In particular, this includes the healing of skin wounds, the repair of tendon damage, the healing of crush injuries, the healing of eye wounds, including wounds to the cornea, the healing of central nervous system (CNS) injuries, 0: conditions which result in the formation of scar tissue in the CNS, scar tissue formation resulting from strokes, and tissue adhesion, for example, as a result of injury or surgery (this may apply to e.g. tendon healing and abdominal strictures and adhesions). Examples of fibrotic disorders include pulmonary fibrosis, glomerulonephritis, cirrhosis of the liver, and proliferative vitreoretinopathy.
9 By "reduced scarring" is meant reduced level of scarring relative to an untreated wound or fibrotic disorder.
In particular, there is a lack of compositions for promoting the healing of wounds or fibrotic disorders with reduced scarring. Scar tissue formation, although providing mechanical strength to a healed wound, can be unsightly and may impair the function of the tissue.
-2- This is particularly the case in wounds which result in scar tissue formation in the CNS, the scar tissue inhibiting the reconnection of severed or re-growing nerve ends, so significantly affecting their function.
Compositions for promoting the healing of wounds or fibrotic disorders may also be used together with compositions for use in the treatment of chronic wounds, for example venous ulcers, diabetic ulcers and bed sores (decubitus ulcers), especially in the elderly and wheel chair bound patients. Such compositions may be extremely useful in patients where wound healing is either slow or in whom the wound healing process has not yet started. Such compositions may be used to "kick-start" wound healing and may then be used in combination with the compositions of the present invention. Hence not only may a chronic wound be healed, but it may be healed with reduced scarring.
The activation of LTGF-p (Latent Transforming Growth Factor-p) to active TGF-p is a critical step in the healing process. LTGF-p (which comprises TGF-p bound to the LAP (Latency Associated Peptide) which in turn may be bound to the LTBP (LTGF-p Binding Protein)) binds to cell-surface M6P (mannose-6-phosphate) receptors via M 6 P-containing carbohydrates in the LAP (Purchio, M.F. et al.,1988, J. Biol.
Chem., 263: 14211-14215; Dennis, P.A. and Rifkin, 1991, Proc. Natl. Acad. Sci.
USA, 88: 580-584; Shah, M. et al., 1992, Lancet, 339: 213-214; Shah, M. et al., 1994, J. Cell Sci., 107: 1137-1157). This binding allows the activation of the LTGF-p a process also involving transglutaminase and plasminogen/plasmin.
-3- Due to the binding of LTGF-p to the M6P receptor, M6P itself may play a significant role in the healing process by competing with the M6P-containing carbohydrates in the LAP for the M6P receptor binding site. By increasing the quantity of M6P at a site (by "site" in this context is meant a site of wounding or a fibrotic disorder), the binding of LTGF-p to the M6P receptor may be inhibited (or at least reduced), and the levels of fibrotic and non-fibrotic TGF-P affected.
Although M6P is extremely useful, it is quickly metabolised and so previous attempts to increase the levels of M6P at a wound site have focused upon providing a constant supply of M6P to the wound site by the use of slow/sustained/biocompatible non-inflammatory delivery systems. Such slow/sustained delivery systems are both costly and inconvenient and are extremely difficult to produce since it is difficult to achieve slow release from a non-inflammatory/biocompatible vehicle.
o. O The present inventors have found that, surprisingly, analogues of M6P may be used to promote the healing of wounds or fibrotic disorders with reduced scarring, the analogues having similar yet distinct structures and functioning as M6P and/or inhibiting the degradation of M6P.
4- In a first aspect, the present invention provides a method for promoting the healing of wounds or fibrotic disorders with reduced scarring comprising administering to a subject in need of treatment an analogue of mannose- 6-phosphate having an anion selected from the group consisting of: 0 (i) O CF2 0
CH
2 OH 0
HO
HO
OH
(ii) 0 O H
HOO--
OH
.OH O 25 0HO (iii) X and OH O
HO
r (iv) OH 0
HO
HO
OH
wherein X is fluorine or hydrogen.
The subject may be a human or animal body.
In a second aspect, the present invention provides an analogue of mannose-6-phosphate comprising an anion of formula:
HOO
P CF2
HO-
OH
In a third aspect, the present invention provides an analogue of mannose-6-phosphate comprising an anion of formula: 30 o 0--P
OH
H
H. O -6 In a fourth aspect, the present invention provides an analogue of mannose-6-phosphate comprising an anion of formula: 0 P 0
P
x ,0 OH 0O
HO
HO
OH
wherein X is fluorine or hydrogen.
In a fifth aspect, the present invention provides an analogue of mannose-6-phosphate comprising an anion of formula: 0 io OH 0
HO
HO
OH
wherein X is fluorine or hydrogen.
S.
S
7 Surprisingly, it has been found that the phosphonate analogues of M6P having an anion of the formula (ii), (iii) or (iv) are capable of binding to the M6P isomerase binding .site. This allows them to competitively inhibit the binding of M6P to the binding site and competitively inhibit M6P breakdown M6P metabolism), therefore increasing the half-life of M6P. Even more surprisingly, these phosphonate analogues of M6P, despite their molecular similarity to M6P and despite their ability to bind to the M6P isomerase binding site, have significantly greater half-lives than M6P are broken down at a significantly slower rate than M6P).
The analogue having an anion of the formula (iii) or (iv) may have a significantly greater halflife than M6P. The analogue may have a half-life at least approximately 10 times that of M6P. It may, for example, have a half-life at least approximately 100 or 1000 times greater than M6P. It may be metabolised by M6P isomerase at a significantly slower rate than M6P. The analogue may bind the M6P isomerase receptor binding site. It may bind to the cell-surface M6P receptor binding site.
The analogue having an anion of the formula (iii) or (iv) may bind to the M6P isomerase receptor binding site. It may bind to the cell-surface M6P receptor 25 binding site.
The analogue having an anion of the formula (iii) or (iv) may have a greater binding affinity than M6P for a M6P receptor. The analogue may have a greater affinity than M6P for the M6P isomerase receptor binding site. The analogue may have a binding affinity for the M6P receptor approximately 2 or 3 times that of M6P.
8 The analogue having an anion of the formula (iii) or (iv) may increase the half-life of M6P in an environment containing M6P isomerase. The analogue may be for use in increasing the half-life of. M6P in an environment containing M6P isomerase.
The analogue may be an inhibitor of M6P breakdown. It may be an inhibitor of M6P metabolism. It may be an inhibitor of M6P isomerase.
The analogue having an anion of the formula (iii) or (iv) may be used in conjunction with other agents or compositions for promoting the healing of wounds or fibrotic disorders with reduced scarring. Such agents or compositions may comprise M6P. For example, a method according to the present invention may comprise administering a phosphonate analogue of M6P having an anion of the formula (ii) (iii) or (iv) in conjunction with M6P itself.
The analogue having an anion of the formula (iii) or (iv) may be administered in the form of a 20 pharmaceutical composition comprising the analogue and a pharmaceutically acceptable carrier, diluent or excipient.
A single dose of a phosphonate analogue having an anion of the formula (iii) or (iv) may have a long-lasting effect upon a wound site, providing significant clinical and therapeutic advantages. This in turn means that instead of the present continual supply of M6P to a wound site, a site may be given a single dose, or several doses, of a phosphonate analogue of M6P having an Sanion of the formula (iii) or (iv).
.o By reducing the dosage of M6P to a wound site, the osmotic effect upon the surrounding tissue at the site may 9 be significantly reduced when compared to the osmotic effect of a continual supply of M6P.
Hence the analogue having an anion of formula (iii)' or (iv) may be functionally equivalent to M6P, yet may have a significantly greater half-life and/or receptor binding affinity than M6P. The analogue may not only function as M6P, but also may act to increase the half-life and efficacy of any added or endogenous M6P by inhibiting the metabolism of M6P by, for example, M6P isomerase.
The method of the present invention may comprise the use of an analogue of M6P having an anion of formula (iii) or (iv) either immediately before or immediately after wounding/onset. It may comprise the use of an analogue of M6P having an anion of formula (iii) or (iv) within approximately 120 hours of wounding/onset, although it may be preferable to apply it within a shorter time, for example 120, 96, 72, 48, 24, or 12 hours post-wounding/onset. By "onset" is meant the 20 onset of a fibrotic disorder.
S.The efficacy of the treatment in promoting healing with reduced scarring may be significantly enhanced by increasing M6P levels at a site immediately following wounding when TGF-i complexed to LAP is released from degranulating platelets. The TGF-pi complexed to LAP is either free in the tissue fluid, bound to the fibrin clot/platelet complex, or is endocytosed into surrounding cells, e.g. fibroblasts, monocytes and macrophages, by the M6P receptor. This degranulation and release of fibrotic TGF-P upon initial wounding has a number of effects which affect subsequent healing. In particular, the TGF-P~ R attracts monocytes and macrophages to the site, which in 10 turn release more TGF-Pi. By inhibiting this initial activation of TGF-P, which is predominantly TGF-Pi, the ratio of fibrotic: non-fibrotic growth factors at a site may be altered in favour of non-fibrotic growth factors and enhanced healing with reduced scarring effected.
The method may be used in conjunction with a method for promoting the healing of wounds or fibrotic disorders with reduced scarring.
The method may be used in conjunction with a method for promoting the healing of chronic wounds.
Experimental work undertaken in treating wounds with non-phosphorylated mannose and glucose resulted in retarded healing when compared with controls. Galactose-6phosphate and glycerol-3-phosphate have no effect upon either wound healing or scarring.
The invention will be further apparent from the following example, which shows by way of example only, that the analogue of M6P having an anion of the following formula o
SCH
2 (I)
O
CH2OH 2
HO
HO
*OH
is metabolised at a significantly slower rate and has a greater M6P receptor binding affinity than M6P and may be used to inhibit M6P metabolism.
11 The analogue of M6P having an anion of the formula methods and uses thereof are the subject of Australian Patent No. 719992 of which the present application is.a divisional.
Of the figures, Figure 1 Figure 2 Figure 3 shows methods of synthesis of various phosphonate analogues of M6P; shows phosphonate analogues of M6P having the formula (iii) and and shows isosteric mannose phosphonate (formula non-isosteric mannose phosphonate (formula fructose-lphosphate (formula and maltose- 1-phosphate.
4.
4 4* 0 *0 4 *444 44
I*.
4444 *4 4* 444444
EXPERIMENTAL
The wound healing and anti-scarring properties of isosteric mannose phosphonate (formula and nonisosteric mannose phosphonate (formula fructose-lphosphate (formula (III)) and maltose-l-phosphate (Figure were tested as described below.
Additionally, the M6P phosphonate analogue of formula was prepared and a receptor binding assay performed with M6P isomerase to analyse its binding affinity for the 25 M6P receptor and also to analyse its half-life. Standard methods were used to obtain the data.
Method Adult male Sprague Dawley rats (200-250 g) were anaesthetised using equal parts halothane, nitrous oxide 12 and oxygen. Four linear full thickness incisions, 1 cm in length to the depth of the panniculus carnosus, were made on the dorsal skin, 1 cm from the midline and 5 and 8 cm from the base of the skull. The wounds were left unsutured to heal by secondary intention. Experimental treatments were administered by intradermal injection to the wound margins (50 pl down each wound margin). At selected time points animals were killed by chloroform overdose. Wounds were excised from the surrounding tissue and bisected.
Half the wounds were rapidly frozen in OCT for cryosection and immunocytochemistry and half fixed in formaldehyde for wax embedding and histology. Wax sections were routinely stained with haematoxylin and eosin, picrosirius red and Massons Lille trichrome, to display collagen fibre thickness, density and orientation to enable assessment of scar quality.
Fructose-l-phosphate (F1P) (formula (III)) and maltose-l-phosphate (MaltlP) were purchased from Sigma Chemical Company. A range of doses (10 mM, 20 mM and S* 20 mM) was studied for each sugar, with PBS (phosphate buffered saline) as a control. Treatments were administered at the time of wounding and each day for the following seven days. Two animals per dose were studied at each of the three time points 40 and 80 days post 25 wounding) for each compound. Total n=12.
4** Isosteric mannose phosphonate (formula was synthesised and supplied by Dr Sally Freeman, Department of Pharmacy, University of Manchester. A range of doses mM, 10 mM, and 10 mM 10 mM M6P) were studied, with PBS as a negative control, and 10 mM M6P and 20 mM M6P as positive controls. Treatments were administered at the time of wounding and each day for the following two days.
13 One animal per dose was studied at each of the two time points (7 and 80 days post wounding). Total n=4.
Non-isosteric mannose phosphonate (formula was synthesised and supplied by Dr Sally Freeman, Department of Pharmacy, University of Manchester. A single concentration (20 mM) of this compound was studied, with PBS as a control. The time of administration varied to the previous experiments. Animals were split into three groups and treated on day 0 alone, days 0, 2 and 4, or days 0 to 7 inclusive. Two animals per treatment regime were studied at each of the three time points 7 and 80 days). Total n=18.
In addition to the animal studies an ELISA-type assay using purified M6P/IGF II (insulin-like growth factor II) receptor was developed to determine if these analogues of M6P bind to the M6P/IGF II receptor.
Results 9* Fructose-l-phosphate (formula (III)) and maltose-l-phosphate At 7 days post wounding histological analysis showed 20 that neither F1P or MaltlP had any effect on wound healing, when compared with PBS controls.
Immunocytochemical analysis also showed that treated 0 wounds resembled controls. Staining for fibronectin was consistent between treatments and controls as were S 25 monocyte/macrophage profiles. At 40 days post wounding histological analysis was inconsistent, with no clear see.
trend. At 80 days post wounding, MaltlP appeared to improve the dermal architecture very slightly whilst F1P appeared to reduce scarring more significantly, particularly at the highest dose studied (40 mM).
TRA
14 Isosteric mannose phosphonate (formula At 7 days post wounding histological analysis revealed that none of the treated wounds appeared different to PBS controls. At 80 days post wounding 'the isosteric analogue appeared to improve the dermal architecture when compared with controls, and showed a similar improvement in scarring as the M6P treatments.
Non-isosteric mannose phosphonate (formula (II)) Initial histological analysis of wounds treated with 20 mM non-isosteric analogue from days 0 to 7 post wounding indicate an anti-scarring effect, especially with the 20 mM treatment on days 0 to 7 post wounding.
The results so far obtained indicate that despite the similarity of the mannose-6-phosphate analogues tested (F1P, MaltlP, and the isosteric and non-isosteric mannose phosphonate analogues), the greater efficacy of the mannose phosphonate analogues may be due to their *se fulfilling an additional role or having special properties with regard to their interactions with other molecules.
0 0 20 Receptor binding assay Initial results from the receptor binding assay showed that F1P binds the M6P/IGF II receptor with similar affinity as M6P, whereas MaltlP does not bind to this S. receptor. The results also showed that the analogue having 25 an anion of formula had a binding affinity approximately 3 times that of M6P for the M6P receptor binding site. Surprisingly, the results also showed that despite this significantly increased binding affinity and despite its structural similarity to M6P, the analogue having an anion of formula had a half-life of \approximately 1000 times that of M6P.
15 A reference herein to a prior art document does not constitute an admission that the document forms part of the common general knowledge in the art in Australia.
In the claims' which follow and in the preceding description of the invention, except where the context requires otherwise due to express language or necessary implication, the word "comprising" is used in the sense of "including", ie. the features specified may be associated with further features in various embodiments of the invention.
4 4 0 4* o
Claims (7)
1. A method for promoting the healing of wounds or fibrotic disorders with reduced scarring comprising administering to a subject in need of treatment an analogue of mannose-6-phosphate having an anion selected from the group consisting of: (ii) *r
9.. S S S 0- 0-P ;and (iii) 17 (iv) 0- O P OH 0 HO HO OH wherein X is fluorine or hydrogen. 2. A method for promoting the healing of wounds or fibrotic disorders according to claim 1 wherein the analogue of mannose-6-phosphate is administered either immediately before or immediately after wounding or onset of the fibrotic disorder. 3. A method for promoting the healing of wounds or fibrotic disorders according to claim 1 wherein the 20 analogue of mannose-6-phosphate is administered within 120 hours of wounding or onset of the fibrotic disorder. S. 4. An analogue of mannose-6-phosphate comprising an anion of formula: O 25 O PCF, COH 2 OH 0 30 HO HO OH 18 An analogue of mannose-6-phosphate comprising an anion of formula: 6. An analogue of mannose-6-phosphate comprising an anion of formula: C. C C 0@e C C. C C. C C. 4C 0 C C. CO I. wherein X is-fluorine or hydrogen. 7. An analogue of mannose-6-phosphate comprising an anion of formula: 30 HO wherein X is fluorine or hydrogen. 19 8. A medicament comprising an analogue according to any one of claims 4 7 in conjunction with a pharmaceutically acceptable carrier diluent or excipient. 9. Use of an analogue of mannose-6-phosphate having an anion selected from the group defined in claim 1 for promoting the healing of wounds or fibrotic disorders with reduced scarring.
10. Use according to claim 9 wherein the analogue of mannose-6-phosphate is administered either immediately before or immediately after wounding or onset of the fibrotic disorder.
11. Use according to claim 9 wherein the analogue of mannose-6-phosphate is administered within 120 hours of wounding or onset of the fibrotic disorder.
12. Use of an analogue of mannose-6-phosphate having an 20 anion selected from the group defined in claim i for the preparation of a medicament for promoting the healing of wounds or fibrotic disorders with reduced scarring.
13. Use according to claim 12 wherein the medicament is administered either immediately before or immediately after wounding or onset of the fibrotic disorder. *S.
14. Use according to claim 12 wherein the medicament is administered within 120 hours of wounding or onset of the 30 fibrotic disorder. Dated this 1 1 t h day of June 2002 RENOVO LIMITED By its Patent Attorneys GRIFFITH HACK
Priority Applications (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| AU53496/00A AU751118B2 (en) | 1995-08-04 | 2000-08-18 | Pharmaceutical composition |
| AU2002301776A AU2002301776B2 (en) | 1995-08-04 | 2002-10-29 | Pharmaceutical Composition |
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| GB9516012 | 1995-08-04 | ||
| AU53496/00A AU751118B2 (en) | 1995-08-04 | 2000-08-18 | Pharmaceutical composition |
Related Parent Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU66248/96A Division AU719992B2 (en) | 1995-08-04 | 1996-07-31 | Pharmaceutical composition |
Related Child Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU2002301776A Division AU2002301776B2 (en) | 1995-08-04 | 2002-10-29 | Pharmaceutical Composition |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| AU5349600A AU5349600A (en) | 2000-10-26 |
| AU751118B2 true AU751118B2 (en) | 2002-08-08 |
Family
ID=3739503
Family Applications (2)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU53496/00A Ceased AU751118B2 (en) | 1995-08-04 | 2000-08-18 | Pharmaceutical composition |
| AU2002301776A Ceased AU2002301776B2 (en) | 1995-08-04 | 2002-10-29 | Pharmaceutical Composition |
Family Applications After (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU2002301776A Ceased AU2002301776B2 (en) | 1995-08-04 | 2002-10-29 | Pharmaceutical Composition |
Country Status (1)
| Country | Link |
|---|---|
| AU (2) | AU751118B2 (en) |
-
2000
- 2000-08-18 AU AU53496/00A patent/AU751118B2/en not_active Ceased
-
2002
- 2002-10-29 AU AU2002301776A patent/AU2002301776B2/en not_active Ceased
Also Published As
| Publication number | Publication date |
|---|---|
| AU2002301776B2 (en) | 2005-03-24 |
| AU5349600A (en) | 2000-10-26 |
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Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| PC1 | Assignment before grant (sect. 113) |
Owner name: RENOVO LIMITED Free format text: THE FORMER OWNER WAS: THE VICTORIA UNIVERSITY OF MANCHESTER |
|
| FGA | Letters patent sealed or granted (standard patent) |