AU4752099A - Treatment of neurological conditions by an interleukin-1 inhibiting compound - Google Patents
Treatment of neurological conditions by an interleukin-1 inhibiting compound Download PDFInfo
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- AU4752099A AU4752099A AU47520/99A AU4752099A AU4752099A AU 4752099 A AU4752099 A AU 4752099A AU 47520/99 A AU47520/99 A AU 47520/99A AU 4752099 A AU4752099 A AU 4752099A AU 4752099 A AU4752099 A AU 4752099A
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AUSTRALIA
Patents Act 1990 COMPLETE
SPECIFICATION
STANDARD
PATENT
Applicant(s): THE VICTORIA UNIVERSITY OF MANCHESTER Invention Title: TREATMENT OF NEUROLOGICAL CONDITIONS BY AN INTERLEUKIN-1 INHIBITING
COMPOUND
The following statement is a full description of this invention, including the best method of performing it known to me/us: 1A TREATMENT OF NEUROLOGICAL CONDITIONS BY AN INTERLEUKIN-1 INHIBITING COMPOUND This invention relates to a method for treatment of neurological conditions and to compositions and products useful for such treatment.
Neurological conditions pose serious clinical problems, as their effects are severe and long-lasting but little is known of any really effective means for curing or even controlling them.
There is, therefore, a considerable need for some treatment for such conditions.
In one aspect of the present invention there is provided the use of a compound which prevents, inhibits or modifies the action of interleukin-l as an active agent for the treatment of conditions of neurological 15 degeneration. In particular, there is provided the use of an agent in the treatment of a human being for a condition of cerebral neurological degeneration selected from: diseases arising from or related to cerebral 20 ischaemia; (ii) cerebral neurological damage resulting ":"from excitotoxicity; and (iii) chronic neurological disease associated with, or related to, cerebral amyloidosis; 25 wherein the agent prevents or inhibits the action of •interleukin-l and the use comprises administering to the human being in need of such treatment an effective amount of the agent.
The use of the agent in the treatment of a non-human mammal for a condition of cerebral neurological degeneration is also provided.
In another aspect of the present invention there is provided a formulation adapted for the use as defined in the previous paragraph, comprising an active agent as defined therein dispersed or dissolved in a pharmaceutically acceptable carrier (solvent or diluent), S:20535F 1B especially in water or an aqueous medium, especially in normal saline (an isotonic solution of sodium chloride in water).
Interleukin-i is commonly referred to as "IL-1".
The active agent thus defined has the effect of protecting neurons from adverse effects, neurodegeneration.
The active agent used may be in a variety of forms, for example a naturally occurring product or one produced by artificial or synthetic methods, for example a genetically engineered form. Particularly suitable is interleukin-l receptor antagonist protein (conveniently referred to as "IL-1 particularly recombinant
IL-
1 ra. It is also possible to use analogues of 15 IL-1 ra, as well as derivatives and fragments thereof (and analogues of these compounds).
Our treatment is useful for a variety of conditions of neurological degeneration, however caused, though the S. means by which the active agent we specify here works is 20 not yet clearly understood. It is believed that it is probably by blocking the action of a S:20535F 2 interleukin-1. The invention is especially applicable to treatment of the neurons in the brain, periphery and spinal chord.
Cerebral lesions in several chronic neurodegenerative conditions Alzheimer's disease (AD) and Down's Syndrome) are known to be associated with the formatior of beta-amyloid (beta-AP), apparently due to abnormal metabolism of beta-amyloid precursor protein (beta- APP) with consequent deposition of beta-AP.
IL-1 has been demonstrated to be present in the brains of patients with Down's Syndrome and Alzheimer's Disease (Griffin et al, 1989, Proc Nat Acad Sci 86, 7611) and in separate studies has been shown to induce synthesis of the precursor of beta-APP (Goldberg et al, 1989, Proc Nat Acad Sci 86, 7606).
Furthermore chronic degenerative processes associated with over-expression of beta-APP for an extended period can lead to loss of synapses, deposition of beta-AP and degeneration of neurones. We have shown that this process is related to emergence of the clinical symptoms of cognitive and neurological deficits and demention (Gentleman S.L .et al. (1991). Neuropath.Applied Neurobioi.17,531). Our experimental data show that these mechanisms are probably active ii, many of the diseases described in Chapters 5 and 6 of the International Classification of Disease (10th edition) Dementia in Alzheimer's disease, Parkinson's Disease, Cortical Lewy Body Disease, etc.) Interleukin-l a 17KDa cytokine is synthesised Farrar et al., Immunol.Rev. 100, 361, 1981) and acts within the central nervous system to mediate several aspects of the acute phase response, and directly modifies neuronal and glial function. An endogenous IL-1 receptor antagonist (IL-ira) has been identified Eisenberg et al.; Nature, 343, 341, 1990) which binds to IL- \receptors in peripheral tissues and hippocampal neurones, and has been shown to inhibit many peripheral actions of IL-1.
Further evidence that IL-ira may be of benefit derives from observations that the concentrations of IL-1 and related cytokines are increased in brain in response to traumatic injury, cerebral ischaemia, and HIV infection and administration of IL-1 worsens ischaemic brain damage. (Gentleman et al (1993) Progr. Exp. Brain Res.(in press)) Thus, blocking its actions by administration of IL-ira or related inhibitors of IL-1 action may limit many forms of neurological damage.
The molecular weight of the active agent defined herein may vary over a considerable range. It may thus usually be of molecular weight up to about 40 KDa (kilodaltons) though products of higher or lower molecular weight may be used if desired and preferably in the range 5 to 25 KDa, especially in the range 15 to 20 KDa. Commonly, products of molecular weight about 17 KDa are convenient and accessible.
The active agents may be administered by various modes, conventional in the art, and the choice depends upon what may be considered most appropriate for the patient's condition. Thus they may be introduced directly into the site of an identified or suspected neuro-degeneration, taking appropriate care that the administration does not itself cause undue damage to the tissue or affect the Scondition adversely. This may be done by injection, e.g. central injection, (for example stereotaxic injection) via hypodermic needles, cannulae, or the like. For intra-cranial administration piarrr-assisted apparatus may be used.
Altern-atively, they iay be 'administered by indirect metnods, so •that they then migrate within the body from the site of introduction to the site at which they are required and are to have effect. Thus, adminstration by infusion can be used, and this can be preferred when direct access to the site of action is either difficult or considered to be less desirable, or even may not be easily determinable. The mode by which this migration occurs may vary, and may be for example by transfer through the blood stream or the cerebro-spinal fluid. Thus, the active agent may be administered by introduction at a peripheral site, for example by intravenous infusion.
So, for the treatment of brain conditions, the invention gives the user a considerable choice, as administration may be by direct injection into the intra-cranial cavity, by infusion into the intracranial cavity, conveniently by way of the cerebro-spinal fluid, or by introduction at a peripheral site, for example by intravenous infusion.
Combinations of more than one administration technique may be used if desired.
Administration may be achieved by conventional apparatus.
Furthermore the active agent may be administered in conjunction with 4 other known treatment agents and/or procedures.
The formulations used may be any in which the defined compound (active agent) is contained in a medium which is safe and compatible with the tissues into which it is to be introduced. Thus the compound may be dispersed or dissolved in a pharmaceutically acceptable carrier (solvent or diluent). This is most conveniently water or an aqueous medium especially normal saline (an isotonic solution of sodium chloride in water) though other media may be used if desired provided they are pharmaceutically acceptable and compatible with the area to be treated. Thus, conventional adjuvants and additives may be used, for example in normal saline.
The amount and concentration of the active agent appropriate for administration may be varied according to the particular need of the patient and the type and/or severity of the condition to be treated. The amount of the active agent is most suitably (for injection into the site of damage) in the range 100 to 10,000 micrograms (and preferably in the range 1000 to 5000 micrograms), on the basis of a patieii-t. !i 80 k-g body weght, and an amount of about 2400 micrograms is usually typical and convenient, though larger or smaller amounts may be used if desired.
If it is considered more convenient, these amounts can be •coo converted into "micrograms per kilogram of body weight" figures by *W simple calculation, and expressed in this way so that the dosages can be calculated more readily for various patients.
These amounts are those which it is intended should be at the site at which the agent is to act. Thus, if the agent is not introduced directly into the desired site, the amounts required for indirect introduction by infusion from a peripheral site) should be adjusted so as to give the amount stated above at the site of action.
In such cases, the amount used at the peripheral site will usually need to be greater than in the ranges stated above, but the optimum amount in any individual case may be determined by clinical factors, having regard to factors as the patient's condition and the response to the treatment. For example, a relatively high dosage may be most appropriate for a condition of acute trauma or at the commencement of treatment, while a lower or reduced dosage may be most appropriate for a chronic or continuing condition calling for an extended period of treatment.
The mode of treatment may be varied to suit the condition being treated. Thus, for example, a single adminstration may suffice in some cases to provide the desired protection rapidly in acute conditions, but this may be enhanced by continuing administration, while chronic conditions may need continuous administration. The optimum mode and dosage for any particular patient or condition can thus be determined by simple trial, and can be modified as treatment continues, in the light of the results shown by the patient's response and needs.
.0#0 The treatment of the present invention may be applied to a variety of acute and chronic conditions.
Our invention may be applicable to the treatment of relatively long-term neuro-degeneration of non-ischaemic origin epilepsy, Alzheimers disease, Huntingdon's chorea, Downs syndrome, Multiple Sclerosis and Parkinson's disease) and neurological damage resulting from chronic infection for example HIV producing the syndrome of
AIDS.
It may also be used for the treatment of ischaemic conditions.
a for example cerebral ischaemia (stroke, haemorrhage or brain injury as a result of trauma) which involve various forms of brain damage and may lead to acute or delayed damage to the brain neurons, and to degeneration for example after head trauma.
The time of treatment is also significant and can be important.
Administration may be before or after an ischaemic condition has occurred or is suspected. Administration before an ischaemic condition can be of value for prophylactic treatment, for example when the patient or subject is considered to be at risk of an ischaemic condition. Such conditions could be for example be in cardiac bypass surgery, in which a significant proportion of patients can suffer minor cerebral damage, or in childbirth, in which the foetus may be liable to problems in the foetal circulation potentially leading to anoxia and cerebral palsy and the like. The more common time of administration is after ischaemic damage has occurred or is suspected, for example in the conditions of treating a stroke or a head injury, and in such cases it is desirable to make the administration as soon as possible after the event to get best results preferably within an 6 hour or less, though administration later than that time may still be beneficial.
The efficacy of.our invention is illustrated by the ability of treatment by administration of active agents we now specify herein to reduce lesions caused by cerebral ischaemia or excitotoxins by up to or even more, and to reduce the amounts of beta-amyloid precursor protein (beta-APP) by 20% or more which are/produced by cerebral ischaemia.
The invention is illustrated but not limited by the following Examples and drawings.
In the appended drawings:- Figure 1 illustrates the effect of IL-1 receptor antagonist protein (IL-1 ra) on neuronal damage after cerebral ischaemia. The lower panel shows the volume of damage (mm 3 computed from the volume under the curve for upper panel). Mean SEM, one way ANOVA, *p<0.05.
'Figure 2 illustrates the effect of IL-1 receptor antagonist protein (IL-1 ra) on NMDA receptor mediated neuronal damage. Upper panel shows the area of damage (mm 2 and the lower panel shows the lesion volume (mm computed from the volume under the curve for upper panel). Mean SEM, unpaired Students t-test. *P<0.001.
In the claims which follow and in the preceding summary 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", i.e. the features specified may be associated with further features in various embodiments of the invention.
EXAMPLE 1 Rats were treated to induce in them a stroke condition (a middle cerebral artery occlusion) by electro-cautery of the middle cerebral artery in the manner customary for such experimental study.
Male Sprague-Dawley rats (Charles River, weighing 200-250g.
were used in all experiments. The animals were injected icy (via previously implanted indwelling guide cannulae in the third ventricle 6a of the brain), 10 minutes prior to surgery, with IL-I ra (1.0 micrograms in 4 microlitres, i.e. 0.6 nmol, n=12, Synergen, Colorado. USA) or 0.9%6 saline (4 microlitres, control, n=14), 30 minutes before and 10 minutes after surgery. Cerebral ischaemia was induced by permanent occlusion of the left middle cerebral artery Lye et al., Neurosci.Meth. 22, 133, 1987)* under Iflalothane anausth-esia (2%j in ox-Ygcn!nirou xd) All animals recovered consciousness within 10 minutes after completion of surgery and were allowed free access to food and water thereafter.
7 The degree of damage, or protection against damage, was assessed by histologica i examination of the lesion size to assess the amount of non-viable tissue present. The data were summed from multiple experiments and derived from study of the rat brains 24 hours after the stroke condition commenced and also compared with control animals in which the treatment was not applied. The area of damage (mm 2 was assessed by tetrazolium staining on 500 p coronal sections of brain (area computed by Seescan image analysis).
The data summarised in Figure 1 demonstrate that injection of (IL-1 ra) into the third ventricle of the brain 30 minutes before and 10 minutes after unilateral focal cerebral ischaemia (MCAo) in the rat inhibits neuronal damage (volume of infarct, measured 24 hours later) by approximately In vehicle-treated ischaemic rats, histological damage (absence of mitochondrial respiratory activity) occurred reproducibly in basal ganglia and neocortex (Figure Injection of IL-lra inhibited the extent of damage in these areas, reducing the total volume of the lesion from 84 12 mm 3 to 42 8 mm 3 Our results therefore sho-w that focal cer-cbra 1 ischaemia i markedly inhibited (ca 50%) by cerebral injection of recombinant IL-1 ra in the rat.
We have also shown effects of peripheral injection of IL-1 ra on brain damage.
This was carried out by intravenous injection.
The IL-1 ra was given as a dose of 0.5 mg/kg., as a solution in normal saline.
This was administered as a first injection 30 minutes BEFORE the stroke, followed by a second injection 10 minutes AFTER the stroke.
lesion size.
after the above treatment 104 14 mm 3 control (no IL-1 ra) 57 15 mm 3 This may be expressed as being a 45% reduction in the size of the lesion or as a 45% protection against the effects of the stroke a great clinical improvement.
8 EXAMPLE 2.
Study of neuronal death resulting from focal cerebral ischaemia or excitotoxic damage due to striatal infusion of an NMDA-receptor agonist.
Excitatory amino acids are potent endogenous neurotoxic agents which can induce neuronal damage and have been proposed as mediators of neuronal death following ischaemia, mechanical brain injury, seizures or neuro-degenerative conditions such as Parkinson's disease, Huntingdon's chorea and damage caused by-infections such as HIV. The NMDA receptor has been strongly implicated in these excitotoxic actions of amino acids. Synthetic antagonists of NMDA receptors MK801) are potent neuroprotective agents in ischaemia, while pharmacological NMDA receptor activation results in neuronal damage. Infusion of cis-2,4-methanoglutamate, a potent and selective NMDA agonist into the striatum of rats causes dose-dependent lesions which are markedly inhibited by pre-treatment with MK801. Data presented in Figure 2 show that infusion of 10 nmoles of cis-2,4e iethmio-glutamate caused reproducible sions -(12.3 1.3 mm 3 Infusion ofIL-1 ra with the NMDA agonist significantly reduced the volume of lesions induced by the cis- 2, 4 -methanoglutamate by 71.1 This indicates that protection against excitotoxic damage is offered by IL-1 ra.
We have also shown that brain damage caused by striatal infusion of quinolinic acid in rats is inhibited by IL-lra. Quinolinic acid caused lesions (assessed from mitochondrial viability) of 27.8 2.4 m 3 coinfusion of IL-lra (10pg) reduced the size of the lesion to 15.1 2.7 mm 3 by Quinolinic acid is a naturally occurring molecule which, when released in high quantities is toxic to neurons.
Excess release of quinolinic acid has been reported in the brain in various neurological conditions Huntingdon's chorea and AIDS) and may be a cause of neurological damage in these conditions. Therefore, inhibition of its actions by IL-lra could be of benefit.
We have thus shown also that IL-I ra inhibits brain damage induced by administration of excitotoxic agents (NMDA receptor agonists or quinolinic acid) to rat brain. Since this mechanism of damage underlies many other neurological conditions (such as epileptic degeneration, Huntingdon's chorea, Parkinson's disease and brain damage resulting from infections such as HIV or traumatic brain injury) as well as ischaemic damage, IL-ra may be of benefit in each of these .conditions.
EXAMPLE 3 Methods Rats (Sprague-Dawley 200-250 gms) were anaesthetized with halothane in oxygen/nitrous oxide) and treated so as to induce a neurological lesion (an infarct). This was achieved by permanent occlusion of the left middle cerebral artery following an established procedure (Lye RH et al 1987 Neurosci. Meth. 22,133). The animals had previously been fitted with an indwelling guide cannula in the third ventricle in the brain and were injected with a solution of IL- micrograms in 4 microlitres i.e. 0.6 nmol) or 0.9% saline (4 microlitres) at intervals of 10- minutes and 30 minutes following the lesion procedure.
A total of 32 animals were used in the various experimental and control procedures.
Animals in treated and non-treated groups were examined after 24 hours 20 total) and 7 day 12 total) survival times.
The brain from each animal was fixed embedded in paraffin and processed for immunocytochemistry to assess the degree of immunoreactivity to p amyloid precursor protein in the brain (using both polyclonal and monoclonal antibodies to P amyloid precursor protein).
Results Lesion size varied from animal to animal. However, increased immunoreactivity to the p amyloid precursor protein was consistently found in a region extending some 2 mm from the edge of the infarct.
Animals treated with IL-1 ra had a reduction in lesion size and also manifested a marked reduction of the levels of p amyloid protein precursor protein-immunoreactivity in the neurons surrounding the lesion.
Similar results were seen in animals with both 24 hour and day survival times.
Claims (30)
1. A method of treating a patient for a condition which is characterised by cerebral ischaemia, the method comprising administering a therapeutically effective amount of an active agent which inhibits IL-1 binding to the IL-1 R to the patient.
2. A method according to claim 1 wherein the ischaemia is 10 caused by a stroke, haemorrhage or a brain injury resulting from trauma.
3. A method of treating a patient for a condition which is characterised by excitoxicity, the method comprising administering a therapeutically effective amount of an active agent which inhibits IL-1 binding to the IL-1 R to the patient.
4. A method according to claim 3 wherein the condition is not characterised by cerebral ischaemia.
5. A method according to claim 3 wherein the excitoxicity is caused by an NMDA receptor agonist.
6. A method according to claim 3 wherein the excitoxicity is caused by excitatory amino acids.
7. A method according to claim 6 wherein the excitatory amino acid is quinolinic acid or cis- 2,4- methanoglutamate.
8. A method according to claim 3 wherein the condition is selected from the group consisting of epilepsy, Huntingdon's chorea, Down's syndrome and Parkinson's disease. 11
9. A method according to any one of claims 1 to 4 wherein the condition is a chronic neurodegenerative disorder. A method according to any one of the preceding claims wherein the active agent is an antagonist of the IL-1R.
11. A method according to claim 10 wherein the active agent is IL-lra.
12. A method according to claim 11 wherein the IL-1ra is 10 recombinant IL-lra. *r
13. A method according to active agent is a fragment inhibiting IL-1 binding to
14. A method according to IL-ira is synthetic. A method according to weight of the active agent
16. A method according to weight of the active agent
17. A method according to weight of the active agent claim 11 or 12 wherein the of IL-lra which is capable of the IL-1R. claim 13 wherein the fragment of claim 13 wherein the molecular is less than or equal to claim 13 wherein the molecular is from about 5 to 25 kDa. claim 13 wherein the molecular is from about 15 to 20 kDa.
18. A method according to any one of the preceding claims wherein the therapeutically effective amount of the active agent is between 100 and 10,000 mg per 80 kg body weight.
19. A method according to claim 18 wherein the therapeutically effective amount of the active agent is between 1,000 and 5,000 mg per 80kg body weight. 12 A method according to claim 18 wherein the therapeutically effective amount of the active agent is about 2,4000 micrograms per 80kg body weight.
21. A method according to any one of the preceding claims wherein the active agent is administered directly to a site of an identified or suspected neurological degeneration.
22. A method according to claim 21 wherein the active .1 0 agent is administered by injection.
23. A method according to any one of the preceding claims wherein the active agent is administered indirectly to a "site of an identified or suspected neurological degeneration.
24. A method according to claim 23 wherein the active agent is administered at a peripheral site from which it subsequently migrates to the site of the identified or 20 suspected neurological degeneration. o o
25. A method according to claim 24 wherein the active agent is administered through the blood stream.
26. A method according to claim 25 wherein the active agent is administered by intravenous infusion.
27. A method according to claim 24 wherein the active agent is administered to the cerebro-spinal fluid.
28. A method according to claims 21 or 23 wherein the active agent is administered to the intra-cranial cavity.
29. A method according to any one of the preceding claims wherein the active agent is dispersed or dissolved in a pharmaceutically acceptable carrier. 13 A method according to claim 29 wherein the carrier is an aqueous medium.
31. A method according to claim 30 wherein the aqueous medium is normal saline.
32. A method according to any one of the preceding claims wherein the active agent is administered continuously. 1
33. A method according to claim 2 wherein the active agent is administered prophylactically to a mammal at risk of ischaemia. 15 34. A method according to claim 2 wherein the active agent is administered after ischaemic damage has occurred or is suspected. a
35. A method of treating a patient for a condition characterised by cerebral neurological degeneration, the method being substantially as described herein with reference to the accompanying Examples 1 or 2. Dated this 10th day of September 1999 THE VICTORIA UNIVERSITY OF MANCHESTER By their Patent Attorneys GRIFFITH HACK
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| AU47520/99A AU755240B2 (en) | 1991-10-31 | 1999-09-10 | Treatment of neurological conditions by an interleukin-1 inhibiting compound |
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| GB9123161 | 1991-10-31 | ||
| GB9125670 | 1991-11-30 | ||
| AU76482/96A AU7648296A (en) | 1991-10-31 | 1996-12-24 | Treatment of neurological conditions by an interleukin-1 inhibiting compound |
| AU47520/99A AU755240B2 (en) | 1991-10-31 | 1999-09-10 | Treatment of neurological conditions by an interleukin-1 inhibiting compound |
Related Parent Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU76482/96A Division AU7648296A (en) | 1991-10-31 | 1996-12-24 | Treatment of neurological conditions by an interleukin-1 inhibiting compound |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| AU4752099A true AU4752099A (en) | 1999-10-28 |
| AU755240B2 AU755240B2 (en) | 2002-12-05 |
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| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU47520/99A Expired AU755240B2 (en) | 1991-10-31 | 1999-09-10 | Treatment of neurological conditions by an interleukin-1 inhibiting compound |
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| Country | Link |
|---|---|
| AU (1) | AU755240B2 (en) |
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1999
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| Publication number | Publication date |
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| AU755240B2 (en) | 2002-12-05 |
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