CA2075970A1 - Heparin derivatives - Google Patents
Heparin derivativesInfo
- Publication number
- CA2075970A1 CA2075970A1 CA002075970A CA2075970A CA2075970A1 CA 2075970 A1 CA2075970 A1 CA 2075970A1 CA 002075970 A CA002075970 A CA 002075970A CA 2075970 A CA2075970 A CA 2075970A CA 2075970 A1 CA2075970 A1 CA 2075970A1
- Authority
- CA
- Canada
- Prior art keywords
- heparin
- process according
- salts
- molecular weight
- heparin derivatives
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Abandoned
Links
Classifications
-
- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08B—POLYSACCHARIDES; DERIVATIVES THEREOF
- C08B37/00—Preparation of polysaccharides not provided for in groups C08B1/00 - C08B35/00; Derivatives thereof
-
- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08B—POLYSACCHARIDES; DERIVATIVES THEREOF
- C08B37/00—Preparation of polysaccharides not provided for in groups C08B1/00 - C08B35/00; Derivatives thereof
- C08B37/006—Heteroglycans, i.e. polysaccharides having more than one sugar residue in the main chain in either alternating or less regular sequence; Gellans; Succinoglycans; Arabinogalactans; Tragacanth or gum tragacanth or traganth from Astragalus; Gum Karaya from Sterculia urens; Gum Ghatti from Anogeissus latifolia; Derivatives thereof
- C08B37/0063—Glycosaminoglycans or mucopolysaccharides, e.g. keratan sulfate; Derivatives thereof, e.g. fucoidan
- C08B37/0075—Heparin; Heparan sulfate; Derivatives thereof, e.g. heparosan; Purification or extraction methods thereof
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P7/00—Drugs for disorders of the blood or the extracellular fluid
- A61P7/02—Antithrombotic agents; Anticoagulants; Platelet aggregation inhibitors
Abstract
Low molecular weight heparin derivatives and salts thereof are prepared by treating a quaternary ammonium salt of a heparin, dissolved in a heterocyclic organic solvent or in an aprotic solvent, with an alkylating agent having from 6 to 30 carbon atoms at a temperature of about 20· to 60 ·C for a prolonged period of time, treating the resultant reaction product at a temperature of about 5· to 120 ·C with an inorganic or organic base, such as an alkaline hydroxide, in aqueous solution, and isolating the obtained heparin derivatives in their free form or as alkaline salts thereof.
The heparin derivatives obtained according to the procedure of the invention constitute a mixture of mostly depolymerized products with a narrow range of molecular weight. These products are useful as anti-thrombotic agents.
The heparin derivatives obtained according to the procedure of the invention constitute a mixture of mostly depolymerized products with a narrow range of molecular weight. These products are useful as anti-thrombotic agents.
Description
~ 2~970 wo 92/11294 Pcr/~Ps2~o~7 Hepar 1 n derl vat 1 ve s Background and Summary of th,e Invention The pre~ent invention concerns new heparin derivatives with pharmacological properties which ar~ , modified with respect to those of the heparin preparations currently available on the market and used in anticoagulant therapies. The relationship between the anti-thrombin activity and the activity on the Xa factox a~d the platelet factor 4 (PF4) of the new derivatives diffexs from that of heparin. In other words, their considerable affinity for PF4 is accompanied by reduced activity on the reaction between anti-thrombin III and thrombin, catalyzed by heparin.
In parallel, the reaction between antith_ombin III
and the.Ya factor, catalyzed by heparin itself, is even more sensitive to the new derivatives. Because of their different ratio of activity from that of heparin, on PF4 and on the reactions activated by thrombin and Xa factGr, the derivatives of the invention are able to pravent -' thrombosis without the risk of hemorrhage which accompanies the anti-thrombotic action of heparin. It ,~ must be noted that hemorrhagic activity can be caused by ''' an excessive action of thrombin inhibition. The ability ' of the new derivatives of the invention to bind PF4, to catalyze at low concentrations the reaction activated by the Xa factor, and only at higher concentrations reactions catalyzed by thrombin, make these compounds suitable zs drugs for ~he treab~t of arterial and venous thro~kosis.
; The new heparin derivatives and their salts are obtained by (1) prolonged treatment of an alkylating - (etherifying) agent derived from a hydrocarbon with more than 6 carbon atoms, at room temperature or slightly '~
over, with a quaternary ammonium salt of heparin, dissolved in a heterocyclic organic solvent chosen from ; N-hydrocarbyl-pyrrolidine-2-one or . . ~.
: .
. ~ , . . .
- ~ :
'' . ' ~ ~ ~ . . ' : ' , .
: :. .. .
In parallel, the reaction between antith_ombin III
and the.Ya factor, catalyzed by heparin itself, is even more sensitive to the new derivatives. Because of their different ratio of activity from that of heparin, on PF4 and on the reactions activated by thrombin and Xa factGr, the derivatives of the invention are able to pravent -' thrombosis without the risk of hemorrhage which accompanies the anti-thrombotic action of heparin. It ,~ must be noted that hemorrhagic activity can be caused by ''' an excessive action of thrombin inhibition. The ability ' of the new derivatives of the invention to bind PF4, to catalyze at low concentrations the reaction activated by the Xa factor, and only at higher concentrations reactions catalyzed by thrombin, make these compounds suitable zs drugs for ~he treab~t of arterial and venous thro~kosis.
; The new heparin derivatives and their salts are obtained by (1) prolonged treatment of an alkylating - (etherifying) agent derived from a hydrocarbon with more than 6 carbon atoms, at room temperature or slightly '~
over, with a quaternary ammonium salt of heparin, dissolved in a heterocyclic organic solvent chosen from ; N-hydrocarbyl-pyrrolidine-2-one or . . ~.
: .
. ~ , . . .
- ~ :
'' . ' ~ ~ ~ . . ' : ' , .
: :. .. .
2~7r~97~
W092/11294 v Pc~/P9~lo~7 N-hydrocarbyl~piperidine-2-one, not substituted or substituted by lower alkyl groups, and their derivatives interrupted in the heterocyclic ring ~y a heteroatom or hetero group chosen from 0-, -S- or -NH- or in a concentrated solution of one such compound in an aprokic solvent, (2) treating the reaction product at a high temperature with an organic or inorganic base in a~eous solution, (3) isolating the heparin derivatives obtained ln free form or their alkaline salts, and, if desired, (4) converting the resulting compounds into the free form or into the alkaline salts or as salts of other metals or organic bases.
The new heparin derivatives, whose aforesaid pharmacological properties are different from those of heparin, also have a modified chemical structure and different molecular weight; their chemical structure has - not yet been completely defined. It has however been ascertained that they:
a) constitute a mixture of mostly depolymerized products and therefore have a medium-to-low molecular weight compared the starting products, which are rich in fragments similar to one another and with molecular weights coming within the same narrow range, and with a minimum of fragments which deviate from this mean.
b) Compared to their starting products, they have a notably diminished ratio between the iduronic-type saccharide unit and the glucuronic-type unit.
Other modifications of the chemical structure, with respect to heparin, which can be found in the new derivatives, are in part also those which have already ' - ~ ; ;, ' ~ ' " :., ' -;
- - - , .
: - .. .
2 ~ 7 ~
' W092/11294 Pc~r/~s~
been described for some heparin fragments obtained by alkaline treatment of heparin esters, for example desulfation and the presence of unsaturated monosic units.
The identification of the new derivatives can be carried out, a~t from said chemical tests, by spectroscopy, especially nuclear magnetic resonance (NMR), which allows in particular to differentiate the new derivatives from heparin fragments already described in the literature.
The treatment of a quaternary ammonium salt of heparin with an alkylating agent chosen from those commonly used, that is, derived from a lower hydrocarbon, such as a lower alkyl halide, for example ethyl bromide~
in a normally used solvent, such as dimethylsulfoxide or dimethylformamide, leads to heparin esters, such as those described in British patent No. 1501095. If these esters undergo alkaline treatment, such as that included in the second phase of the procedure of the present invention, different heparin fragments are obtained, as can be demonstrated by NMR analysis.
The new low-molecular-weight heparin derivative descr:~d in the examples, constitutes a novel product, which can be characterized mainly on the basis of NMR spectroscopic 25 data at high frequency (400-500 MHz for the proton analysis;
100-125 MHz for C-13 analysis), utilizing traditional one-dimensional spectres in FT (Fourier Transformation), corroborated with the latest two-dimensional techniques (H-H and C-H correlation), optionally resorting to more recent methods (e~g. TOCSY - total correlation spectroscopy), wher2 necessary for the study of such complex products.
.
, ,'.
' ' '.
,, ' , ..
.. . .
., : :
. . , 20 15'370 WO92/1129~ PCr/EP~3/02479 ~;
From an overall examination of the results obtainable by the cited methods, it can be determined that:
1) The new "low-molecular-weight heparin" of the invention is a complex mixture of oligosaccharides, sulfated both at N and at O, reflecting the heterogeneity of the starting heparin. Its fundamental constituents IdoA and GlcnAc, differently sulfated, and secondary constituents (essentially GlcA) link together, giving rise to different sequential combinations.
2) With respect to the starting heparin, the product which is the object of the present invention shows a considerable decrease in the IdoA/GlcN ratio, this decrease being detectable by NMR. Accordingly, the signals of the anomeric sites of the typical IdoA
seguence (2SO3)-GlcNSO3) (6SO3) (102 and 99.5 ppm for carbon; 5.18 and 5.32 ppm for the proton) prove to be drastically diminished. Such transformations cannot be detected in the known, low-molecular-weight ; heparins, or if they can, it is to a far lesser degree. Concomitantly, markedly intense siynals appear of a new unsaturated monosaccharide unit (see point 4).
3) Another characteristic fact is the appearance of new signals (at 54.2 and S3.3 ppm for carbon, correlatable to protons at 3.73 and 3.68 ppm respectively) which is compatible, in the present context, only with the 2-position of a GlcN residue, with no SO3H groups at the nitroqen). This characteristic, dete~ctable by 2-D NMR, is - practically absent in samples of Xnown, low-molecular-weight heparins.
.
:. .
~ , . .
- . . -, - :
: : .: . - , - . . . . . : . :
2 ~
WO92/1129~ PC'r/~ 79 4) Typically, most of the aforesaid oligosaccharides terminate with an unsaturated monosaccharide unit, three-substituted in positions 1-2, as can be shown by NMR (signals at 147 and 172 ppm in C-13: doublet at 6 ppm for the proton). These signals are absent or very reduced in the other known, low-molecular-weight heparins.
It must therefore be concluded that as early as the first step of the procedure of the present inventionj what happens is not just a simple esterification, but a more complex chemical reaction.
It can therefore be assumed from these findings that the heparin-like products of the present invention are new and different from the heparin fragments already described in the literature. For example, they are different from the fragments described in European patent No. 0 302 034, obtained by alkaline treatment of heparin esters, these fragments being suitable for the formation of complexes with copper ions having an angiogenic action. In the same way, the heparin fragments described in U.S. patent No. 4,440,926, obtained starting from well-defined heparin esters by treatment with NaOH
(0.1-0.5 N) between 20 and 60C, are not identical to the products of the present invention.
The aforesaid qualities of the new heparin derivatives of the present invention can be demonstrated by the following experiments, performed on the produck described in the illustrative Examples and abridged to the code name PE. In the experiments, unfractionated heparin (UFH) and a low-molecular-weight heparin derivative (CY
2l6 = Fraxiparine~) are used as comparison products. Both these products are commercially available for the treatment of thrombosis.
~: - : . . . . . . . .......................... ..
: - . `. :
. ~ , . , ., -2 ~ 7 ~ 7 i, ~
WO92/11294 PCT/EP9~/0~7 : -6-Brief Description of the Drawinqs Figure l shows the anticoagulant activity in vitro of PE compared to UFH and CY 216 in terms of thrombin time (sec.). The data obtained are mean values of 7-l0 replications for each test product.
Figure 2 shows the ex vlvo anticoagulant activity of PE, compared to UFH and CY 216, according to the e~fect on thrombin time after i.v. administration. The data are mean values from experiments on 5 rabbits for each test, product.
Figure 3 illustrates the ex vivo anticongulant activity of PE, compared to UFH and CY 216, based on anti-FXa activity (disappearance kinetics after s.c.
administration). The data are mean values from experiments on 5 rabbits per test product.
Figure 4 shows the ex vivo activity for PF4 after i.v. administration of PE, in comparison to UFH and CY
216.
.
1. ANTICOAGULANT ACTIVITY IN VITRO ON RECONSTRUCTED
HUMAN PLASMA
Materials and Methods Test products (solubilization and concentrations) The following products were tested:
- heparin derivative PE
- unfractionated heparin (UFH) - low-molecular-weight heparin derivative (CY 216 -Fraxiparine~) The test products were dissolved in sterile saline and tested at concentrations ranging from 0.5 to t2.5 ~g/ml.
' ' , ., :
~ .
.; .
.:-. :. -. . . , ~ ,, . . . : .
, - ~, .. .
- . .. ...
.. . . .. . . . . .
7$~7~
'-jW092/11294 PCr/EP~ 2~79 _7_ Parameters 1. Thrombin time (as an indicator of anticoagulant activity) 2. Anti-FXa activity (as an ~cator of anticoagulant activity) Results l. Thrombin time From Fig. l it is clear that:
- PE has anticoagulant activity starting at concentrations of l.25 ~g/ml - The anticoagulant activity of PE is considerably ~.
inferior to that of unfractionated heparin UFH
(thrombin time increases at concentrations about 4-5 times greater than UFH).
No significant differences from CY 216 can be observed.
2. Anti-FXa activity In Table l, the preliminary data indicate that: .
- PE has anti-FXa activity starting from concentrations of 3 ~g/ml - the anti-FXa activity is distinctly inferior to that of heparin.
It must also be noted that this activity is also inferior to that of CY Zl6; in this case, however, the difference is less e~ident than that observed in comparison to UFH.
' f ' I . .
'. '~ ' ' , ' ' ' . ' ' ' .: ' ' ' , ' ' . ' ' ~ , . , , .: . .
. ' ~ ' ' . ~ . ' , ' ' ' ' ' . ~ ' ' ' ' ' . ' ' , ~ ' ,' ' ' . ", ' ' ' . ' ' ' ' ' ' ' ~ ' ' , , ' ' , . .
'.: ' .' " .~. . '.""' " '. ' ' ' ~ ' . ' ' ' , ' '. ' ' ' ' '' .. ' . ' ' ~ ' .' '.' ''' ' " ' ' " ' ' ''' ' ' . ' ' .' ' ' ' ' ' .
, ' ' ' .
~o 92".294 ~ 0 7 ~ 9 7 0 p~r/Ep91/o247~
Table 1 ANTI-FXa ACTIVITY IN VITRQ OF PE IN COMPARISON TO
5 CONCENTRATIONS UF~ CY 216PE
(~g/ml) 0~5 0.336 - -1 - 0.3310.342 1.5 0.281 2.5 0.212 3 - 0.2610.296 3.5 0.179 - 0.2000.245 7 - 0.1580.201 The data are means of 3 experiments per concentratio~, 20 one for each test product.
`; ' 2. ANTICOAGULANT ACTIVITY EX VIVO ON R~BBIT PLAS~
AFTER I.V. AND S.C. ADMINISTRATION
.
The anticoagulant activity o~f the new heparin derivative PE was assessed by ex vivo methods on rabbit plasma. By "ex vivo" is meant in vitro measurement of ~: :
blood withdrawn from an animal to which the chemical substance has been administered. Examined in particular were the fol'lowing:
a) thrombin time, on arterial blood after acute bolus intravenous administration (i.v.) of the test products;
b) anti-FXa activity, on arterial blood after acute . ~
`
:.
- ., . . . . . . . . . . .
20 1~97~
~ WO92/11294 PCT/EP~1/02~'79 _g_ subcutaneous administration (s.c.).
This method, being highly sensitive, i5 indicative of the "bioavailability" of the test products, since it allows the kinetics of the disappearance of the test products to be monitored after subcutaneous administration.
The test products were dissolved in sterile saline solution and administered acutely at 0.86 mg/kg by the i.v. route and at 1-2 mg/kg by the s.c. route.
Test description a? Thrombin time - This test assesses thrombin time on samples of arterial blood from rabbits at various time intervals (2-5-10-20-30-40 minutes) after i.v.
administration of a bolus of test product.
b) Anti-FXa activitv By measuring the anti-FXa activity (by a chromogenic test which is sensitive at very low concentrations of compound) it is possible to monitor the presence of the test products in the circulation for a very long timeO
Samples of arterial blood (from the central artery of the ear) were taken at various intervals (1-2-3-4-5-6-7-8 hrs) after s.c. administration.
: 25 Results - a) Thrombin time : From Fig. 2 it is clear that:
- PE has a low anticoagulant activity at 0.86 mg/kg i.v., confirming the in vitro data - the anticoagulant activity of PE is distinctly inferior to that of UFH, but does not differ significantly from that ~F Cy 2 1 6 .
' ~ .
: . .
, :, ~
~ ' ' '"' .' , .
.
` ' ' : , ', .
~ . ' ' '. ~ -. .
~0~9'~
WO92/112~4 pc~r/Ep~ /0~7~ ~
b) anti-FXa activity Fig. 3 shows that:
- PE (after s.c. administratiun at 1 mg/kg) remains present in the circulation for longer than UFH, administered at twice the dose, that is, at 2 mg/kg s.c. -The disappearance kinetics of the heparin derivative PE is therefore slower than that of UFH, but similar to that of CY 216.
` 10 3. EX VIVO AFFINITY FOR PLATELET FACTOR 4 (PF4) By the experiments described hereafter, the affinity o~ the new heparin derivative PE of the present invention lS was assessed for human PF4, i.e. the ~binding properties"
of such products for PFb.
The ex vivo technique used monitored the kinetics of the disappearance of PF4 from the circulation in the absence and in the presence of heparin.
It is well known that heparin or glycosaminoglycans (GAGs), administered before PF4, markedly enhance its kinetics (G. Cella et al., "Human platelet factor 4 and protamine sulphate interaction with glycosaminoglycans in the rabbit", Eur. J. Clin. Invest., Vol. 17, pp. 548-554 (1987~.
Compounds able to bind PF4 should therefore greatly prolong its presence in the circulation. This effect is ; proportional to the quantity of GAG injected and to its ` affinity for PF4.
The test products were dissolved in sterile saline solution and administered at 0.86 mg/kg i.v.
. ~ , : , ,:, . ,: . . . . . . .
- , ' , ' ~ W092/11294 2 ~ 7 0 p~r/Ep9l/o2479 DescriPtion of the test Administrati.on of the test products was acute (intravenous bolus), at a dose of 0.86 mg/kg. Samples of arterial blood were taken 2-3 mins later from the central artery of the ear (baseline sample). 5 minutes after administration of the first bolus, a second bolus of purified human PF4 was given (30 ~g/kg).
Samples were taken 1.5-2.5-5-10-20-30 minutes after administration of PF4. These were centrifuged, stored and assessed by the RIA test (commercially available kit) for human PF4.
Results As reported in Fig. 4, the data obtained indicate that:
- PE has affinity for platelet factor PF4 and gradually disappears from the circulation reaching low values about 30 minutes after administration.
- The affinity of PE for PF4 i~ much lower (about 60%) than that of UFH and the kinetics of the disappearance of the complex with PF4 is far more rapid than that of UFH, while it is similar to that of CY 2160 4. ANTITHROMBOTIC ACTIVITY IN VIVO IN A MODEL OF
ARTERIAL THROMBOSIS IN RABBIT
The experiment described hereafter assessed the antithrombotic activity in vivo of the new heparin : 30 derivative PE. The objective was to test the efficacy of the products in preventing the formation of àn arterial thrombus in an acute model of arterial thrombosis in the rabbit carotid artery, following endothelial damage and reduction of the vascular '' ' , .~ - . . . .
.
-:
:-. : ~., .. :.:. .
.
WO92/11294 2 ~ 7 ~ ~ 7 ~ pcrlEp9l/o2~7~J~
diameter.
The test products were dissolved in sterile saline and administered by the i.v~ route at concentrations ranging from 1.2 to 6 mg/kg.
Descri~tion of the model The experiments were performed on rabbits anesthetized with Nembutal (30 mg/kg i.v., bolus) arld tracheotomized for forced breathing. A tube was inserted into the femoral vein and artery for the continuous administration of anesthetic and drug. Systemic blood pressure was monitored and the carotid was fixed with a flowmeter and snare. When the system stabilized, stenosis was p~ormed. After suitable intervals tnot less than 20 minutes), mechanical damage was induced with surgical forceps and sténosis was performed above the damaged vessel. The decrease in flow was moni~ored until it re~ched the value zero (0), corresponding to occlusion of the vessel. The controlateral carotidwas prepared in the same way. The test products were ~ infused i.v. for ~ight minutes in all, with mechanical damage being performed after two minutes of infusion. The flow was monitored constantly until at least one hour after the end of treatment. The animal was sacrificed by an overdose of anesthetic at the end of the experiment.
:
Results As reported in Table 2, the data obtained indicate that:
- PE is effective in completely preventing the ` formation of an occlusive thrombus. The effect is ' evident at a dose of 6 mg/kg i.v.;
; - The antithrombotic efficac~ of PE is inf erior `, .
. .
.. . .
' ~' . '' ' .,~.' ':., ', ':' ' , ' ' ' ' -'' ~, . ...... .. .
- . . , , , . , , :
'~ - ' ', ';' ' '' , :' ' ',. .. . .
2 ~ ~ ~ 9 7 ~
W092/11294 . P~r/EP9a/0'~7 (about 5x) to that of unfractionated heparin UFH
(which can ~e seen to inhibik the formation of occlusive thrombi at a dose as low as l.2 mg/kg), the pharmacological efficacy of PE is similar to that of CY 216.
Table 2 Antithrombotic activity of PE in comparison to unfractionated heparin (UFH) and CY 216 in a model of arterial stenosis in rabbit Products l.v. dose No. occluded animals No. treated animals UFH l.2 mg/kg 2/12 PE 6 mg/kg 2/12 3 mg/kg 6/8 CY 216 6 mg/kg 2/12 3 mg/kg 5/9 .
5. ANTITHROMBOTIC ACTIVITY IN A MODEL OF VENOUS
THROMBOSIS IN VIVO
: The experiment described hereafter was performed to assess the antithrombotic efficacy in vivo of PE in a model of venous thrombosis in the rat.
The venous stasis technique was used, by occluding : 30 the vena cava inferior, as this method causes the - formation of a mainly fibrinic thrombus due to the `. variation in blood flow at the level of the bifurcation o the vena cava with the left renal vein.
.
.
: : :
. ~ . ~ , ,:
. .
:. . .
-'~ - , .
W092/12294 æ o ~ ~ ~ 7 PCI/EP~/024Y9 The model under examination therefore proves to be sensitive to the activity of anticoagulant drugs and in particular to the antithrombotic potential of heparin (after administration and stasis).
The test products were dissolved in sterile saline and administered intravenously at doses ranging from 0~5 to 3 mg/kg i.v. (15 minutes before stasis induction).
Description of the test The experiments were performed on male CD-COBS rats, weighing 175-200 grams. The animals were anesthetised with sodium pentobarbital (40 mg/kg i.p.) and their undersides were disinfected with alcohol. A 4-cm incision was made along the middle of the abdomen starting from the ribs. The vena cava was isolated from the aorta to the common iliac artery and tied with a cotton thread immediately underneath the fork with the left renal vein~
The double occlusion was such as to exert constant ~Id continuous pressure for 5 seconds. The abdominal wall was then closed. Two hours later the abdomen was reopened to verify thrombus formation. After closing off the vena cava, in correspondence to the common iliac arteries, and the collateral circulation with a hemostat, the vascular ; section below the occlusion was cut longitudinally with a needle. The thrombus was removed and immersed in distilled water, blotted dry on paper and then placed in a dry box for 24 hours to determine the dry residue expressed in mg.
- .
~, . . .
: . . .. . . .
- .. ... , .. . - . ., . .: ... , ,.,,,.. ,. .: .,..... .. ,., . : .
~ W092/112~4 2 ~ 7 ~ ~ 7 0 PCItEP9ll/02,~
Results The data relative to the weight (mg) of the thrombi (Table 3) and incidence (~) of the thrombi (Table 4) two hours after venous stasis, show that:
- PE has antithrombotic efficacy; its protective effect (pre-treatment) is significant at a dose of 1.5 mg/kg i.v.
- the efficacy of PE is inferior to that of unfractionated heparin UFH (which already has a lo significant effect at 0.5 mg/kg i.v.) , ~ .. :,. .: ,. . ~, ' . ' : , .
- . : ,, :~
2a7~i~7~
W092/11294 P~/EP91/02~79 Table 3 Antithrombotic effect in vivo of PE compared to UFH
in a venous stasis model: weight ~mg) of the thrombi obtained 2 hrs after venous stasis (effec.ted 15 minu~es after i.v. administration of the test products) .
Doses (mg/kg i.v.) Products 0 0.5 1. 0 1.8 2 .0 3 . O
n = 1~ n = 14 n= 24 n = 20 n = 14 n = 14 `.
PE 2.2 1.4 1.5 0.8*0.0**0.0**
UFH 2.2 0.7* 0.5** 0.02** - -' * p < 0.05; ** p < O.Ol Dunnett's test n = number of animals . .
..... ~ . .. . .-.
~ 2 ~ D
W092~1~294 PCr/EPgl/0247g Table 4 Antithrombotic effect in vivo of PE compared to UFH in a venous stasis model: incidence (%) of thrombi obtained 2 hours after venous stasis (effected 15 minutes after 5 i.v. administration of the test products) _ Doses (mg/kg i.v.) ___ Products 0 0.5 1.0 1.5 2.0 3.0 n = 15n = 14n = 24 n = 20n = 14 n = 14 _ PE 93.3 85.7 62.5 60.0 0.0 0.0 UFH 93.3 57.1 50.0 14.3 - --n = number of animals - - -: : : . . : . . : . .
, ,. : . .. ~ .: . .: . , : -. : . - : ~ - ,:
~7~97~
WO 92/1 1 294 PC~ 7 6. EFFECT ON BLEEDING TIME IN RAT
The experiment described hereafter assessed the effect of PE on bleeding time 15 minutes after intravenous administration of the test products.The test products were dissolved in sterlle saline and administered i.v. at concentrations ranging from 1 to 3 mg/kg.
Description of the test The experiments were performed on male, CD-COBS rats (17S-200 grams) in which the test substances were administered acutely by the intravenous route.The bleeding time (in seconds) was assessed 15 minutes later by the standard template method of cutting the tail (Dejana et al., "sleeding time in rats: A comparison of different experimental conditions", Thromb. HaemostatO, Vol. 48, pp. 108-111 (1982)).
Results The data obtained (Table 5) show that:
- The effect of PE on "bleeding time" is significantly increased at a dose of 2.0 mg/kg i .v .
- the effect of PE is notably inferior to that obtained with unfractionated heparin UF~ (in which the bleeding value already increases significantly at a dose of 1 mg/kg i.v.), but it is comparable to that of CY 216 (data not reported)`.
` 30 It is interesting to note that in order to obtain the same valuès for the bleeding time it is necessary to administer a dose of PE which is at least 3 times greater than that of UFh.
:' ~`
.
: : -. . : , , , - . .
~ 092/11294 2 0 7 ~ 9 7 0 PCT/~ ,47~ , ~19-- ' Table_5 The effects of PE and UFH on bleeding time (sec) 15 minutes after i.v. administration of the test products Doses (mg/kg e.v.) Products 0 1.0 1.5 2.0 3O0 n = 14n = 14 n = 14n = 14 n = 14 -PE 130 146 147 250* 3~9**
UFH 130 413** 487** - --* p < 0.05; ** p < 0.01 Dunnett's test n = number of animals .. . . . . .
. . ,: . . . . . .
- ,,; , , , :
: . . .
, .. :.. . . . .
.. . .
WO92/11294 2 ~ 7 ~ 9 ~ 9 P~r/~pt~ 7~
W092/11294 v Pc~/P9~lo~7 N-hydrocarbyl~piperidine-2-one, not substituted or substituted by lower alkyl groups, and their derivatives interrupted in the heterocyclic ring ~y a heteroatom or hetero group chosen from 0-, -S- or -NH- or in a concentrated solution of one such compound in an aprokic solvent, (2) treating the reaction product at a high temperature with an organic or inorganic base in a~eous solution, (3) isolating the heparin derivatives obtained ln free form or their alkaline salts, and, if desired, (4) converting the resulting compounds into the free form or into the alkaline salts or as salts of other metals or organic bases.
The new heparin derivatives, whose aforesaid pharmacological properties are different from those of heparin, also have a modified chemical structure and different molecular weight; their chemical structure has - not yet been completely defined. It has however been ascertained that they:
a) constitute a mixture of mostly depolymerized products and therefore have a medium-to-low molecular weight compared the starting products, which are rich in fragments similar to one another and with molecular weights coming within the same narrow range, and with a minimum of fragments which deviate from this mean.
b) Compared to their starting products, they have a notably diminished ratio between the iduronic-type saccharide unit and the glucuronic-type unit.
Other modifications of the chemical structure, with respect to heparin, which can be found in the new derivatives, are in part also those which have already ' - ~ ; ;, ' ~ ' " :., ' -;
- - - , .
: - .. .
2 ~ 7 ~
' W092/11294 Pc~r/~s~
been described for some heparin fragments obtained by alkaline treatment of heparin esters, for example desulfation and the presence of unsaturated monosic units.
The identification of the new derivatives can be carried out, a~t from said chemical tests, by spectroscopy, especially nuclear magnetic resonance (NMR), which allows in particular to differentiate the new derivatives from heparin fragments already described in the literature.
The treatment of a quaternary ammonium salt of heparin with an alkylating agent chosen from those commonly used, that is, derived from a lower hydrocarbon, such as a lower alkyl halide, for example ethyl bromide~
in a normally used solvent, such as dimethylsulfoxide or dimethylformamide, leads to heparin esters, such as those described in British patent No. 1501095. If these esters undergo alkaline treatment, such as that included in the second phase of the procedure of the present invention, different heparin fragments are obtained, as can be demonstrated by NMR analysis.
The new low-molecular-weight heparin derivative descr:~d in the examples, constitutes a novel product, which can be characterized mainly on the basis of NMR spectroscopic 25 data at high frequency (400-500 MHz for the proton analysis;
100-125 MHz for C-13 analysis), utilizing traditional one-dimensional spectres in FT (Fourier Transformation), corroborated with the latest two-dimensional techniques (H-H and C-H correlation), optionally resorting to more recent methods (e~g. TOCSY - total correlation spectroscopy), wher2 necessary for the study of such complex products.
.
, ,'.
' ' '.
,, ' , ..
.. . .
., : :
. . , 20 15'370 WO92/1129~ PCr/EP~3/02479 ~;
From an overall examination of the results obtainable by the cited methods, it can be determined that:
1) The new "low-molecular-weight heparin" of the invention is a complex mixture of oligosaccharides, sulfated both at N and at O, reflecting the heterogeneity of the starting heparin. Its fundamental constituents IdoA and GlcnAc, differently sulfated, and secondary constituents (essentially GlcA) link together, giving rise to different sequential combinations.
2) With respect to the starting heparin, the product which is the object of the present invention shows a considerable decrease in the IdoA/GlcN ratio, this decrease being detectable by NMR. Accordingly, the signals of the anomeric sites of the typical IdoA
seguence (2SO3)-GlcNSO3) (6SO3) (102 and 99.5 ppm for carbon; 5.18 and 5.32 ppm for the proton) prove to be drastically diminished. Such transformations cannot be detected in the known, low-molecular-weight ; heparins, or if they can, it is to a far lesser degree. Concomitantly, markedly intense siynals appear of a new unsaturated monosaccharide unit (see point 4).
3) Another characteristic fact is the appearance of new signals (at 54.2 and S3.3 ppm for carbon, correlatable to protons at 3.73 and 3.68 ppm respectively) which is compatible, in the present context, only with the 2-position of a GlcN residue, with no SO3H groups at the nitroqen). This characteristic, dete~ctable by 2-D NMR, is - practically absent in samples of Xnown, low-molecular-weight heparins.
.
:. .
~ , . .
- . . -, - :
: : .: . - , - . . . . . : . :
2 ~
WO92/1129~ PC'r/~ 79 4) Typically, most of the aforesaid oligosaccharides terminate with an unsaturated monosaccharide unit, three-substituted in positions 1-2, as can be shown by NMR (signals at 147 and 172 ppm in C-13: doublet at 6 ppm for the proton). These signals are absent or very reduced in the other known, low-molecular-weight heparins.
It must therefore be concluded that as early as the first step of the procedure of the present inventionj what happens is not just a simple esterification, but a more complex chemical reaction.
It can therefore be assumed from these findings that the heparin-like products of the present invention are new and different from the heparin fragments already described in the literature. For example, they are different from the fragments described in European patent No. 0 302 034, obtained by alkaline treatment of heparin esters, these fragments being suitable for the formation of complexes with copper ions having an angiogenic action. In the same way, the heparin fragments described in U.S. patent No. 4,440,926, obtained starting from well-defined heparin esters by treatment with NaOH
(0.1-0.5 N) between 20 and 60C, are not identical to the products of the present invention.
The aforesaid qualities of the new heparin derivatives of the present invention can be demonstrated by the following experiments, performed on the produck described in the illustrative Examples and abridged to the code name PE. In the experiments, unfractionated heparin (UFH) and a low-molecular-weight heparin derivative (CY
2l6 = Fraxiparine~) are used as comparison products. Both these products are commercially available for the treatment of thrombosis.
~: - : . . . . . . . .......................... ..
: - . `. :
. ~ , . , ., -2 ~ 7 ~ 7 i, ~
WO92/11294 PCT/EP9~/0~7 : -6-Brief Description of the Drawinqs Figure l shows the anticoagulant activity in vitro of PE compared to UFH and CY 216 in terms of thrombin time (sec.). The data obtained are mean values of 7-l0 replications for each test product.
Figure 2 shows the ex vlvo anticoagulant activity of PE, compared to UFH and CY 216, according to the e~fect on thrombin time after i.v. administration. The data are mean values from experiments on 5 rabbits for each test, product.
Figure 3 illustrates the ex vivo anticongulant activity of PE, compared to UFH and CY 216, based on anti-FXa activity (disappearance kinetics after s.c.
administration). The data are mean values from experiments on 5 rabbits per test product.
Figure 4 shows the ex vivo activity for PF4 after i.v. administration of PE, in comparison to UFH and CY
216.
.
1. ANTICOAGULANT ACTIVITY IN VITRO ON RECONSTRUCTED
HUMAN PLASMA
Materials and Methods Test products (solubilization and concentrations) The following products were tested:
- heparin derivative PE
- unfractionated heparin (UFH) - low-molecular-weight heparin derivative (CY 216 -Fraxiparine~) The test products were dissolved in sterile saline and tested at concentrations ranging from 0.5 to t2.5 ~g/ml.
' ' , ., :
~ .
.; .
.:-. :. -. . . , ~ ,, . . . : .
, - ~, .. .
- . .. ...
.. . . .. . . . . .
7$~7~
'-jW092/11294 PCr/EP~ 2~79 _7_ Parameters 1. Thrombin time (as an indicator of anticoagulant activity) 2. Anti-FXa activity (as an ~cator of anticoagulant activity) Results l. Thrombin time From Fig. l it is clear that:
- PE has anticoagulant activity starting at concentrations of l.25 ~g/ml - The anticoagulant activity of PE is considerably ~.
inferior to that of unfractionated heparin UFH
(thrombin time increases at concentrations about 4-5 times greater than UFH).
No significant differences from CY 216 can be observed.
2. Anti-FXa activity In Table l, the preliminary data indicate that: .
- PE has anti-FXa activity starting from concentrations of 3 ~g/ml - the anti-FXa activity is distinctly inferior to that of heparin.
It must also be noted that this activity is also inferior to that of CY Zl6; in this case, however, the difference is less e~ident than that observed in comparison to UFH.
' f ' I . .
'. '~ ' ' , ' ' ' . ' ' ' .: ' ' ' , ' ' . ' ' ~ , . , , .: . .
. ' ~ ' ' . ~ . ' , ' ' ' ' ' . ~ ' ' ' ' ' . ' ' , ~ ' ,' ' ' . ", ' ' ' . ' ' ' ' ' ' ' ~ ' ' , , ' ' , . .
'.: ' .' " .~. . '.""' " '. ' ' ' ~ ' . ' ' ' , ' '. ' ' ' ' '' .. ' . ' ' ~ ' .' '.' ''' ' " ' ' " ' ' ''' ' ' . ' ' .' ' ' ' ' ' .
, ' ' ' .
~o 92".294 ~ 0 7 ~ 9 7 0 p~r/Ep91/o247~
Table 1 ANTI-FXa ACTIVITY IN VITRQ OF PE IN COMPARISON TO
5 CONCENTRATIONS UF~ CY 216PE
(~g/ml) 0~5 0.336 - -1 - 0.3310.342 1.5 0.281 2.5 0.212 3 - 0.2610.296 3.5 0.179 - 0.2000.245 7 - 0.1580.201 The data are means of 3 experiments per concentratio~, 20 one for each test product.
`; ' 2. ANTICOAGULANT ACTIVITY EX VIVO ON R~BBIT PLAS~
AFTER I.V. AND S.C. ADMINISTRATION
.
The anticoagulant activity o~f the new heparin derivative PE was assessed by ex vivo methods on rabbit plasma. By "ex vivo" is meant in vitro measurement of ~: :
blood withdrawn from an animal to which the chemical substance has been administered. Examined in particular were the fol'lowing:
a) thrombin time, on arterial blood after acute bolus intravenous administration (i.v.) of the test products;
b) anti-FXa activity, on arterial blood after acute . ~
`
:.
- ., . . . . . . . . . . .
20 1~97~
~ WO92/11294 PCT/EP~1/02~'79 _g_ subcutaneous administration (s.c.).
This method, being highly sensitive, i5 indicative of the "bioavailability" of the test products, since it allows the kinetics of the disappearance of the test products to be monitored after subcutaneous administration.
The test products were dissolved in sterile saline solution and administered acutely at 0.86 mg/kg by the i.v. route and at 1-2 mg/kg by the s.c. route.
Test description a? Thrombin time - This test assesses thrombin time on samples of arterial blood from rabbits at various time intervals (2-5-10-20-30-40 minutes) after i.v.
administration of a bolus of test product.
b) Anti-FXa activitv By measuring the anti-FXa activity (by a chromogenic test which is sensitive at very low concentrations of compound) it is possible to monitor the presence of the test products in the circulation for a very long timeO
Samples of arterial blood (from the central artery of the ear) were taken at various intervals (1-2-3-4-5-6-7-8 hrs) after s.c. administration.
: 25 Results - a) Thrombin time : From Fig. 2 it is clear that:
- PE has a low anticoagulant activity at 0.86 mg/kg i.v., confirming the in vitro data - the anticoagulant activity of PE is distinctly inferior to that of UFH, but does not differ significantly from that ~F Cy 2 1 6 .
' ~ .
: . .
, :, ~
~ ' ' '"' .' , .
.
` ' ' : , ', .
~ . ' ' '. ~ -. .
~0~9'~
WO92/112~4 pc~r/Ep~ /0~7~ ~
b) anti-FXa activity Fig. 3 shows that:
- PE (after s.c. administratiun at 1 mg/kg) remains present in the circulation for longer than UFH, administered at twice the dose, that is, at 2 mg/kg s.c. -The disappearance kinetics of the heparin derivative PE is therefore slower than that of UFH, but similar to that of CY 216.
` 10 3. EX VIVO AFFINITY FOR PLATELET FACTOR 4 (PF4) By the experiments described hereafter, the affinity o~ the new heparin derivative PE of the present invention lS was assessed for human PF4, i.e. the ~binding properties"
of such products for PFb.
The ex vivo technique used monitored the kinetics of the disappearance of PF4 from the circulation in the absence and in the presence of heparin.
It is well known that heparin or glycosaminoglycans (GAGs), administered before PF4, markedly enhance its kinetics (G. Cella et al., "Human platelet factor 4 and protamine sulphate interaction with glycosaminoglycans in the rabbit", Eur. J. Clin. Invest., Vol. 17, pp. 548-554 (1987~.
Compounds able to bind PF4 should therefore greatly prolong its presence in the circulation. This effect is ; proportional to the quantity of GAG injected and to its ` affinity for PF4.
The test products were dissolved in sterile saline solution and administered at 0.86 mg/kg i.v.
. ~ , : , ,:, . ,: . . . . . . .
- , ' , ' ~ W092/11294 2 ~ 7 0 p~r/Ep9l/o2479 DescriPtion of the test Administrati.on of the test products was acute (intravenous bolus), at a dose of 0.86 mg/kg. Samples of arterial blood were taken 2-3 mins later from the central artery of the ear (baseline sample). 5 minutes after administration of the first bolus, a second bolus of purified human PF4 was given (30 ~g/kg).
Samples were taken 1.5-2.5-5-10-20-30 minutes after administration of PF4. These were centrifuged, stored and assessed by the RIA test (commercially available kit) for human PF4.
Results As reported in Fig. 4, the data obtained indicate that:
- PE has affinity for platelet factor PF4 and gradually disappears from the circulation reaching low values about 30 minutes after administration.
- The affinity of PE for PF4 i~ much lower (about 60%) than that of UFH and the kinetics of the disappearance of the complex with PF4 is far more rapid than that of UFH, while it is similar to that of CY 2160 4. ANTITHROMBOTIC ACTIVITY IN VIVO IN A MODEL OF
ARTERIAL THROMBOSIS IN RABBIT
The experiment described hereafter assessed the antithrombotic activity in vivo of the new heparin : 30 derivative PE. The objective was to test the efficacy of the products in preventing the formation of àn arterial thrombus in an acute model of arterial thrombosis in the rabbit carotid artery, following endothelial damage and reduction of the vascular '' ' , .~ - . . . .
.
-:
:-. : ~., .. :.:. .
.
WO92/11294 2 ~ 7 ~ ~ 7 ~ pcrlEp9l/o2~7~J~
diameter.
The test products were dissolved in sterile saline and administered by the i.v~ route at concentrations ranging from 1.2 to 6 mg/kg.
Descri~tion of the model The experiments were performed on rabbits anesthetized with Nembutal (30 mg/kg i.v., bolus) arld tracheotomized for forced breathing. A tube was inserted into the femoral vein and artery for the continuous administration of anesthetic and drug. Systemic blood pressure was monitored and the carotid was fixed with a flowmeter and snare. When the system stabilized, stenosis was p~ormed. After suitable intervals tnot less than 20 minutes), mechanical damage was induced with surgical forceps and sténosis was performed above the damaged vessel. The decrease in flow was moni~ored until it re~ched the value zero (0), corresponding to occlusion of the vessel. The controlateral carotidwas prepared in the same way. The test products were ~ infused i.v. for ~ight minutes in all, with mechanical damage being performed after two minutes of infusion. The flow was monitored constantly until at least one hour after the end of treatment. The animal was sacrificed by an overdose of anesthetic at the end of the experiment.
:
Results As reported in Table 2, the data obtained indicate that:
- PE is effective in completely preventing the ` formation of an occlusive thrombus. The effect is ' evident at a dose of 6 mg/kg i.v.;
; - The antithrombotic efficac~ of PE is inf erior `, .
. .
.. . .
' ~' . '' ' .,~.' ':., ', ':' ' , ' ' ' ' -'' ~, . ...... .. .
- . . , , , . , , :
'~ - ' ', ';' ' '' , :' ' ',. .. . .
2 ~ ~ ~ 9 7 ~
W092/11294 . P~r/EP9a/0'~7 (about 5x) to that of unfractionated heparin UFH
(which can ~e seen to inhibik the formation of occlusive thrombi at a dose as low as l.2 mg/kg), the pharmacological efficacy of PE is similar to that of CY 216.
Table 2 Antithrombotic activity of PE in comparison to unfractionated heparin (UFH) and CY 216 in a model of arterial stenosis in rabbit Products l.v. dose No. occluded animals No. treated animals UFH l.2 mg/kg 2/12 PE 6 mg/kg 2/12 3 mg/kg 6/8 CY 216 6 mg/kg 2/12 3 mg/kg 5/9 .
5. ANTITHROMBOTIC ACTIVITY IN A MODEL OF VENOUS
THROMBOSIS IN VIVO
: The experiment described hereafter was performed to assess the antithrombotic efficacy in vivo of PE in a model of venous thrombosis in the rat.
The venous stasis technique was used, by occluding : 30 the vena cava inferior, as this method causes the - formation of a mainly fibrinic thrombus due to the `. variation in blood flow at the level of the bifurcation o the vena cava with the left renal vein.
.
.
: : :
. ~ . ~ , ,:
. .
:. . .
-'~ - , .
W092/12294 æ o ~ ~ ~ 7 PCI/EP~/024Y9 The model under examination therefore proves to be sensitive to the activity of anticoagulant drugs and in particular to the antithrombotic potential of heparin (after administration and stasis).
The test products were dissolved in sterile saline and administered intravenously at doses ranging from 0~5 to 3 mg/kg i.v. (15 minutes before stasis induction).
Description of the test The experiments were performed on male CD-COBS rats, weighing 175-200 grams. The animals were anesthetised with sodium pentobarbital (40 mg/kg i.p.) and their undersides were disinfected with alcohol. A 4-cm incision was made along the middle of the abdomen starting from the ribs. The vena cava was isolated from the aorta to the common iliac artery and tied with a cotton thread immediately underneath the fork with the left renal vein~
The double occlusion was such as to exert constant ~Id continuous pressure for 5 seconds. The abdominal wall was then closed. Two hours later the abdomen was reopened to verify thrombus formation. After closing off the vena cava, in correspondence to the common iliac arteries, and the collateral circulation with a hemostat, the vascular ; section below the occlusion was cut longitudinally with a needle. The thrombus was removed and immersed in distilled water, blotted dry on paper and then placed in a dry box for 24 hours to determine the dry residue expressed in mg.
- .
~, . . .
: . . .. . . .
- .. ... , .. . - . ., . .: ... , ,.,,,.. ,. .: .,..... .. ,., . : .
~ W092/112~4 2 ~ 7 ~ ~ 7 0 PCItEP9ll/02,~
Results The data relative to the weight (mg) of the thrombi (Table 3) and incidence (~) of the thrombi (Table 4) two hours after venous stasis, show that:
- PE has antithrombotic efficacy; its protective effect (pre-treatment) is significant at a dose of 1.5 mg/kg i.v.
- the efficacy of PE is inferior to that of unfractionated heparin UFH (which already has a lo significant effect at 0.5 mg/kg i.v.) , ~ .. :,. .: ,. . ~, ' . ' : , .
- . : ,, :~
2a7~i~7~
W092/11294 P~/EP91/02~79 Table 3 Antithrombotic effect in vivo of PE compared to UFH
in a venous stasis model: weight ~mg) of the thrombi obtained 2 hrs after venous stasis (effec.ted 15 minu~es after i.v. administration of the test products) .
Doses (mg/kg i.v.) Products 0 0.5 1. 0 1.8 2 .0 3 . O
n = 1~ n = 14 n= 24 n = 20 n = 14 n = 14 `.
PE 2.2 1.4 1.5 0.8*0.0**0.0**
UFH 2.2 0.7* 0.5** 0.02** - -' * p < 0.05; ** p < O.Ol Dunnett's test n = number of animals . .
..... ~ . .. . .-.
~ 2 ~ D
W092~1~294 PCr/EPgl/0247g Table 4 Antithrombotic effect in vivo of PE compared to UFH in a venous stasis model: incidence (%) of thrombi obtained 2 hours after venous stasis (effected 15 minutes after 5 i.v. administration of the test products) _ Doses (mg/kg i.v.) ___ Products 0 0.5 1.0 1.5 2.0 3.0 n = 15n = 14n = 24 n = 20n = 14 n = 14 _ PE 93.3 85.7 62.5 60.0 0.0 0.0 UFH 93.3 57.1 50.0 14.3 - --n = number of animals - - -: : : . . : . . : . .
, ,. : . .. ~ .: . .: . , : -. : . - : ~ - ,:
~7~97~
WO 92/1 1 294 PC~ 7 6. EFFECT ON BLEEDING TIME IN RAT
The experiment described hereafter assessed the effect of PE on bleeding time 15 minutes after intravenous administration of the test products.The test products were dissolved in sterlle saline and administered i.v. at concentrations ranging from 1 to 3 mg/kg.
Description of the test The experiments were performed on male, CD-COBS rats (17S-200 grams) in which the test substances were administered acutely by the intravenous route.The bleeding time (in seconds) was assessed 15 minutes later by the standard template method of cutting the tail (Dejana et al., "sleeding time in rats: A comparison of different experimental conditions", Thromb. HaemostatO, Vol. 48, pp. 108-111 (1982)).
Results The data obtained (Table 5) show that:
- The effect of PE on "bleeding time" is significantly increased at a dose of 2.0 mg/kg i .v .
- the effect of PE is notably inferior to that obtained with unfractionated heparin UF~ (in which the bleeding value already increases significantly at a dose of 1 mg/kg i.v.), but it is comparable to that of CY 216 (data not reported)`.
` 30 It is interesting to note that in order to obtain the same valuès for the bleeding time it is necessary to administer a dose of PE which is at least 3 times greater than that of UFh.
:' ~`
.
: : -. . : , , , - . .
~ 092/11294 2 0 7 ~ 9 7 0 PCT/~ ,47~ , ~19-- ' Table_5 The effects of PE and UFH on bleeding time (sec) 15 minutes after i.v. administration of the test products Doses (mg/kg e.v.) Products 0 1.0 1.5 2.0 3O0 n = 14n = 14 n = 14n = 14 n = 14 -PE 130 146 147 250* 3~9**
UFH 130 413** 487** - --* p < 0.05; ** p < 0.01 Dunnett's test n = number of animals .. . . . . .
. . ,: . . . . . .
- ,,; , , , :
: . . .
, .. :.. . . . .
.. . .
WO92/11294 2 ~ 7 ~ 9 ~ 9 P~r/~pt~ 7~
7. IN VIVO TOL~RANCE AFTER I.V. AND S.C.
ADMINIST~TION IN MOUSE
The present experiment assessed the maximum tolerated dose of the compound PE after administration by the intravenous and subcutaneous route in the mouse.
The test products were dissolved-in sterile saline and tested at concentrations ranging between 125 and 2000 mg/kg i.v. and s.c.
Descri~tion of the test The experiment was performed on male and female CD-l mice (C. River) (25-35 grams) and comprised two steps.
l) Screening. Groups of one male mouse and one female mouse were treated with one of the following doses: 125, 250, 500, 1000 and 2000 mg/kg. Mortality within 7 days of treatment was monitored.
2~ Groups of five male and five female mice were treated (for each compound and each administration route) with the highest : tolerated dose found on screening. The animals were observed for 14 days, during which mortality and the presence of altered behaviour and general toxicity symptoms were observed. In the case of mortality a lower dose was used, until the maximum tolerated dose was found.
Where possible, autopsy was performed on the deceased animals.
~`
:
:-.
. . . :
9 7 ~
W0 92/ll294 ' ' ' / PCt'/;~R~)a/02'179 Results 1. Intravenous tolerance dose As reported in Tables 6 and 7, the maximum tolerated dose of the test compounds proved to be the following:
- PE: 1000 mg/kg i.v.
- unfractionated heparin UFH: 125 mg/kg i.v.
- CY 216: 1000 mg/kg i.v.
It must be noted therefore that PE has greater tolerance lo dose than unfractionated heparin UFH.
Autopsy of the animals which died after treatment with unfractionated heparin UFH at 500 and 250 mg/kg, reve~led no macroscopic findings except, in some animals, the presence of probable residues of internal hemorrhage in the intestine.
2. Subcutaneous tolerance dose The results obtained, as reported in Tables 8 and 9, show that the maximum tolerated doses of the test products are as follows:
- PE: 2000 mg/kg s.c.
- unfractionated heparin UFH: 125 mg/kg s.c.
- CY 216: 2000 mg/kg s.c.
25 As with the intravenous route, therefore, the .tolerance dose of PE is far greater than that of unfractionated heparin (UFH), while it is similar to that of CY 216. It is however important to highlight that:
- In all the animals (10/10~ treated with CY 216 (2000 mg/kg s.c.) a circular area of skin affected by necrosis was observed on the back, corresponding to the injection site, the size of which differed from animal to animal (maximum diameter about 1 cm).
.
. . . .
,: , . -.. . .
WO 92/11294 2 0 7 S 9 7 ~ I'CI/EP91/0~47') ~
-22- !
.
Autopsy revealed necrosis to be limited to the skin, it did not therefore affect the underlying muscle~
- No anomalies were observed in animals treated with PE (2000 mg/kg s.c.).
- The animals which died after treatment with UFH (250 mg/kg) presented extensive bruising in the subcutaneous dorsal region, where treatment had been performed.
The subcutaneous tolerance data therefore show a lo difference between the compoun~s PE and CY 216.
Indeed, although the maximum tolerance doses are the same, in the case of CY 216 a marked area of necrosis of the skin is present at the injection site, which indicates that CY 216 is tolerated to a lesser degree locally than PE (which presented no anomalie,).
'' ' , .
. .
. : , . :
.. . .
:. .
- - . . : :
07~97~
O92/11294 P~!EP~]/02479 Tabl e 6 Lethality of compounds PE, CY 216 and unfractionated heparin UFH after a single intravenous administration (screening) , . . _ . .
Treatment Deceased animals/Treated animals (mg/kg i.v.) males females 10 PE 2000 0/1 0/1 : :
Heparin UFH 2000 1/1 1/1 Heparin UFH 1000 1/1 1/1 Heparin UFH 500 0/1 0/1 Heparin UFH 250 0/1 0/1 Heparin UFH 125 0/1 0/1 ; ~ .,. : ' , ''''' ' ~, ' '', ~ ' ' ., , , ' :, . ' . . .
'. : '. . ' :' : , . . .
-207597~ 1 WO92/11294 PCT/EP'31/0247')~
-2~-Table 7 Lethality of compounds PE, CY 216 and unfractionated heparin (UFH) after a single intravenous administration . . _ ~
Treatment Deceased animals/Treated animals Tlme of death (mg/kg i.v~)males females days after ~ treatment immëdiate* 1 2 3 4 PE 1000 0/5 o/5 - - - -Heparin 5000/5 2/5 - 2 125 o/5 0/5 *Within minutes of tre~tment ~ ' .
., .
. :
' ~'~' ~ ''"' '' ' '' ''` ' '' " ' '. ,' ' ' ' ' ' ' ' " ' . ', ' ' ' ' ' ' ' ~ ' ', . '. ' '' ' ' . ,'' ' ~ ~O92~11294 ~ 7 ~ 9 ~ ~ pcr/~ 79 Table 8 Lethality of the compounds PE, CY 216 and unfractiona~ed heparin UFH after a single subcutaneous administration (screening) _ Treatmen~ Deceased animals/Treated animals tmg/kg s.c.) males females CY216 500 0/1 - o/
Heparin UFH 2000 1/1 1/1 ~eparin UFH 1000 1/1 0/1 .
Heparin UFH 500 1/1 0/1 Heparin UFH 250 0/1 0/1 Heparin UFH 125 0/1 0/1 - ., - - . . ..
. -- - -, .. . : ,. . .
, - ,- - ... . ..
. - - : - : ., ... :. -:. : : , . .
: - . : . : , . . .
- - - .. ... : .. " .. , .: : : ... : . . . .:.
. . .. :.: . .. ~ - . - , ..
2~7~70 WO92/11294 PCr'/~P91/~2~'7~) -2s- .
'rabl e 9 Lethality of compounds PE, CY 216 and unfractionated heparin (UFH) after a single subcutaneous administration Treatment Deceased animals/Treated animals Time of deat~
(mg/kg i.v.) males females treatment immediate 1 2 3 PE 2000 0/5 o/5 _ _ _ _ _ Heparin 250 1/5 2/5 - 2 15 UFH 125 0/5 0/5 ~
~ .
.
' '' ~ . ' '': ' ' . :
. . . . . .
." ' ' ; ,", . .
. . ~ , .. . .
-W092/11294 PC~ 10~75 CONCLUSIONS
The in vitro and in vivo results previously described outline an interesting pharmacological profile of the heparin derivative PE, setting it apart from unfractionated heparin (UXF) and rendering its pharmacological activities more valuable.
The activity of PE differs slightly ~rom that of CY
216, which i5 one of the best low-molecular-weight heparins currently on sale in France, and shows in particular better local tolerability after s.c.
administration in the mouse. Indeed, although the maximum tolerated doses are the same, all animals treated with CY 216 (2000 mg/kg s.c.) had evident necrosis of the skin at the injectidn site, while the skin of the animals treated with PE was unaffected.
In the case of pharmacological activity in vitro and in vivo, it is interesting to note that PE has:
- anticoagulant activity, far inferior to that of UFH;
- bioavailability, a~ter s.c. administration, much greater than that of UFH, thereby allowing fewer daily administrations for the same pharmacological effect;
- lesser side effects, with regard to UFH, as shown by the reduced bleeding time and by the absence of skin necrosis at the injection site, with regard to CY 216 (the best low-molecular-weight heparin ; on sale in France) which caused a local intolerance phenomena (necrosis) in all the animals treated;
- antithrombotic activity in vivo, as shown in both the model of venous stasis in the rat and in the m~del of arterial thrombosis in the rabbit. The product is therefore efficacious in preventing these .
.
'; :,, , . , . ,, ,, .' ,' , .- . - : : ,, - : . :. :. . .. . : ...
~,arl~7 ~
WO92/11294 pcr/E~9l/o2~7s pathologies at dosages of 1.5 and 6 mg/kg i.v., respectively, which do not induce any signif icant variations in the side effects.
In particular, with regard to the ven~us antithrombotic activity, the derivative PE, at a dose of 1.5 mg/kg i.v., does not induce:any alterations in bleeding time, unlike UFH;
- The new, low-molecular-weight heparin derivatives according to the present invention can therefore be used in the place of unfractionated heparin in all its indications, as an anticoagulant and thrombocyte aggregation inhibitor. The dose is adapted to each particular case, and is normally around 1-7 mg/kg per day, by the intravenous route.
The heparins to be used in the previously described procedure of the present invention can be of any type and of various origin, for example heparins extracted from the intestine of pigs, cattle, and sheep and from ox ; 20 heart, especially any one of the products which are commercially available or described in the literature.
Such products have widely ranging molecular weights, for example between 2,000 and 30,000 daltons, especially unfractionated heparin UFH, and also low-molecular-weight heparins obtained by fractionation of standard heparins (2,000-lO,000 daltons) and heparin fragments with a molecular weight of 500-lO,000 daltons obtained by ~ partial depolymerization of standard heparins by chemical : or enzymatic means. The quaternary ammonium salts to be used as starting material for said procedure can be ~` prepared in the known way, for instance by ion exchange of the heparin in aqueous solution as a sodium or ` potassium salt with resins based on quaternary ammonium salts, for example a salified sulfonic resin with a .
- , , . , . : . .
, ~ ~. . ' ~ 2~97~
WO 92/11294 PC-r/EP91/024'7g quaternary ammonium base. The quaternary ammonium salt can be obtained by freeze-drying the eluate. As quaternary ammonium salts, tetraalkylammonium salts derived from lower alkyls may be advantageously used, particularly tetraalkylammonium salts with alkyl groups having a maximum of 6 carbon atoms. Optionally, alkyl-aryl-ammonium salts may also be used, for example those having long-chained alkyl groups. of the tetraalkylammonium salts, tetrabutylammonium salts are preferably used. The quaternary ammonium salts to be used as starting substance for the procedure of the present invention are those obtainable by ion exchange i~ the aforesaid manner using alkaline salts, for example sodium or potassium salts, of heparin of the type used commercially, that is, neutral salts. They are reacted with an excess of quaternary ammonium ions so as to obtain also the corresponding neutral salts.
Quaternary ammonium salts are soluble both in the aforesaid heterocyclic solvents, and in aprotic organic solvents, such as dimethylsulfoxide and dimethylfor~amide. The reaction with khe alkylating ; agent, according to the first step of the procedure, can be performed both in the aforesaid heterocyclic solvents, or in a solution of the same in one of the aforesaid aprotic organic solvents, prefexably in a concentrated solution. Of the aforesaid heterocyclic solvents, the preferred ones are above all those which are not substituted in the cyclic structure, that is, N-alkyl-o~aryl-2-pyrrolidone, or their derivatives containing a heterocyclic atom in the cyclic structure, such as the corresponding derivatives of imidazoline, piperazine or morpholine. The N-alkyl groups of ; heterocyclic solvents are derived preferably from a lower ~ alkyl with a maximum of 6 carbon atoms, and the aryl '~:
.. . .. . .
~,. . . ,., ' '" ' ~ ,. ' ' ,. - ~ , . . , , ~ .:
- . : . , . , ~ :
.
'': .,~.. , -, ' , ' : :. , 20~970 ~ I
WO 92/11294 PCr/EP(~/02~'79 group is primarily a pheny1 group, optionally substituted by 1 to 3 lower alkyl groups, especially methyl groupsO
Preferably, N-methyl-2-pvrrolidone is used.
An alkylating agent derived from a hydrocarbon having from 6 to 30 carbon atoms, preferably from 8 tQ 18 carbon atoms, is a compound easily capable of yielding the corresponding hydrocarbyl groups, such as a reagent ester group of an acid with an alcohol with a corxesponding number of carbon atoms, which can be an aliphatic or araliphatic alcohol having preferably a maximum of 18 carbon atoms, for example a hexyl, heptyl, octyl or nonyl alcohol. The reagent esters can be derived from inorganic or organic acids, such as hydracids, sulfuric or sulfurous acid, or alkyl- or aryl-sulfonic l~ acids, for example methane-sulfonic or p-toluenesulfonic acid. The esters of the hydracids are in particular chlorides, bromides and iodides. The reaction between the quaternary ammonium salt of the aforesaid alkylating agent is performed at room temperature (20C.)or slightly higher, for example at a temperature of from 30 ~ 35Co but not exceeding 60C, and is maintained for a prolonged period of time of about 5 to 20 hours, typically about 16 hours.
The reaction product can be isolated and subsequently submitted to the second step of the procedure, that is, to alkaline treatment, or it can be converted directly into the final product, performing the alkaline treatment directly on the solution, optionally concentrated, of the reaction product of the first step.
3 0 It is also possible to evaporate the solvent under bland (mildj conditions after the first step of the procedure and to perform alkaline treatment on the residue. It is therefore possible to perform the procedure of the ~ invention as a "one-pot" process. The basic treatment of :' -,., . ~. ~ :
-'WO92/1129~ ~ O~ PCT/~ Z47 -31~
the reaction product between the quaternary ammonium salt of heparin with the alkylating agent is performed at a temperature of from 5O to 120 C ., suitably at a temperature between 50C and 120C, preferably about 70OC, for about two hours. Alkaline hydrates are used~
such as NaOH or KOH, or other inorganic and/or organic bases, preferably at a concentration of between 0.l and lM. The bases are used in aqueous or alcoholic solutio~s/
but other solvents can be present which are miscible with water or with an aqueous-alcoholic mixture, such as, for example, the residue solvents used in the first step of the procedure in the case of the aforesaid "one-pot"
process.
If it is desired to isolate the reaction product of the first step of the proc-dure, it can be precipitated by the addition of an organic polar solvent, preferably an aliphatic alcohol such as methyl or ethyl alcohol, to which a basic buffer has preferably been added, such as especially a basic salt of a carboxylic acid, e.g., an acetate or propionate of sodium or potassium. Other basic buffers can be used, such as alkaline bicarbonates or alkaline phosphates. The precipitated product is preferably washed with the polar solvent used in the precipitation, for example methanol. It is advisable to purify the precipitated product further by reprecipitating it once more or several times, that is, by dissolving the product in water and precipitating it with an alcohol.
- The reaction product, comprising the low-molecular-weight heparin derivative and having the previously described properties, can be released in free form either from a metal salt or from an organic base in the conventional way. The alkaline salt corresponding to the alkaline hydrate used in the second step of the .
~` . ' " ' ' ~ ~ ' ~ ' ' ~ , , ' . , .
. ~ .~ , ~, ' , ' ' ' .
207~7~ f~7;, WO92/1l294 PCI/EP~1/02~7l) procedure may be obtained by neutralizing the solution with an acid, e.g., 2M hydrochloric acid, purifying the solution, extracting it with an organic solvent which cannot be mixed with water, for example methylene chloride, and repeating this operation several timesO
The salt is then dialyzed with distilled water and sodlum chloride and freeze-dried.
The products of the invention are used mainly in the form of their metal salts or organic base salts. If it ls desired to obtain metal salts other than alkaline sal~s corresponding to the ions of the alkaline hydrates used in the aforesaid alkaline treatment, it is possible ko use ion exchange methods by known t~chniques.
Alternatively, it is possible to isolate the heparin product in its acid form, adding the alkaline salt obtained with the calculated quantity of a diluted strong acid, such as hydrochloric acid or sulfuric acid, extracting the product with a suitable organic solvent, isolating the heparin compound in ~ree form and then converting it into the desired salt.
Of the metal or organic base salts which can be used according to the present invention, of particular importance are those which are therapeutically acceptable, such as alkali and alkaline-earth metals, for example sodium, potassium, ammonium, calcium, and magnesium salts, or heavy metal salts, such as copper and iron salts. The salts of organic bases can be derived ~rom primary, secondary or tertiary aliphatic, aromatic or heterocyclic amines, such as methylamine, ethylamine, propylamine, piperidine, morpholine, ephedrine, furfurylaminecholine, ethylenediamine and aminoethanolO
Salts which cannot be directly used in therapy, which are also part of the invention, are for example those which can be used for the purification of the new ' :
: , ~ .
, ~- ~ ' ' ''' ' .
.,, ~ " , - .
3 9 7 ~ 1 ' W092/11294 PCr/EP~1/02~79 heparin derivatives of the invention, such as some of the heavy metal salts.
The invention also includes pharmaceutical preparations containing as active substance a new low-molecular-weight heparin derivative obtainable by the procedure described herein, especially in the form o~
their therapeutically acceptable salts. Such preparations can be for parenteral use, for example for subcutaneous or intravenous administration, or for topical use, for example in the form of creams or ointments, or suppositories, or nose sprays. They can therefore be formulated as solutions of the active compounds or as freeze-dried powders of the active compounds to be mixed with one or more pharmaceutically lS acceptable excipients or diluents which are convenient for the aforesaid uses and with an osmolarity which is compatible with physiological fluids.The invention includes, besides the new low-molecular-weight heparin derivatives, the aforesaid procedure for their p:eparation. Included in the invention is also the performance of the single steps of the preparation procedure, that is, the reaction of a quaternary ammonium salt of heparin with an alkylating agent as defined above in on of said solvents and the alkaline treatment of the 1 25 reaction product.
The invention is illustrated in the following Examples which, however, are not to be considered as limiting.
' ..
.
. .
- ~ . - .. - . - . . .
.. . . .. .. . ..
, . , ~ .:
:, . -. . , ~ . : ~ .
.... . . ... : , , : , .
- : , - : , , . ; . . : . ., : :. ,, . : . :: .
: . : , . . . .
.. . . . . . .. ... .. . .
: - , . . .. . , :. ~ :
- .. . ... : . ,, : ,. .: . .
. . .. . . . .
207597~ ~ ' W092/11294 PC~'/EP91/0247~ i 1) F RMULATIONS FOR INJECTION
1 . 1 PE mg 10 20 30 40 water for injection in ml 0.1 0.2 0.3 004 Package with ready-to-use syringe containing sterile solution for subcutaneous admlnistration~
: 1.2 PE mg 150 300 other components:
water for injection in ml 4 Package with vial containing sterile solution for intravenous administration.
.
15 1.3 PE mg 10 20 30 40 other components:
sodium chloride mg 0.3 0.6 0.9 1.2 - water for injection in ml 0.1 0.2 0.3 0.4 Package with ready-to-use syringe containing sterile solution for suboutaneous administration.
. . - ' ' ' ' . . .
~ , . . .
.. - I .
-.: - ., . . . . :
:', ': . . ' -- W092/11~94 PCT/~P~1/02~7 1.4 PE mg 150 300 other components:
sodium chloride mg 35 70 water for injection in ml 5 10 ; Package with vial containing sterile solution ~or intravenous administration.
1.5 PE mg 150 300 other components:
sodium chloride mg 35 70 sodium metabisulfite mg 5 10 ~ .
chlorbutanol (*) . mg 25 50 ; 15 water for injection in ml 5 10 Package with vial containing sterile solution for multidose intravenous administration.
(*) in Example 1.5 the preservative chlorbutanol can 20 be substituted by:
benzyl alcohol mg 50 100 or by:
chlorocresol mg 5 10 ~ ,, .
,, , . , ,, ., ~. " . ", -,- . . .. : ,.. . .. , : , . ... . .. . .. .. .. . . . . .
.,: .. .. . , , . , , : . . ,., : ,, ., ",... . , .: . :. . : . ., . , : ,-. - .. ,: : : .
.. : -:: . : .: : .,::: . .. : .. . . .
: , :- -. : .... , . : . .. .
.: - . , ~ : . -- , .. .. - , , , - "
,: , .,, : . , , :
WO92/11294 2 0 ~ ~ 9 7 0 -36- PCr/EY~1/1)2~7~) 2) FORMULATIONS FOR ORAL ADMINISTRATION
2.l (pill or capsule) PE mg 3060 120 other components:
phosphatidylcholine ~
~ phosphatidylserine (*) mg 80160 320 : lactose mg 50l00 200 microcrystalline cellulose mg l020 40 talc mg 3 5 12 colloidal silica mg 3 6 12 (*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary 2.2 (pill or capsule) PE mg 3060 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg 80160 320 cholesterol mg 2 4 8 lactose mg 50l00 200 - microcrystalline cellulose mg l020 40 talc mg 3 6 12 colloidal silica mg 3 6 12 ; ~*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may 30 vary.
-' , ~: . -,. , . , . . :
, ~ . , , .
. ':, ,,: ': ' , . ,~ .
. . .. .... . . . .
.~ : , . . : . " ,, . : . . :
~ 092/11294 2 ~ ~ ;3 9 ~ Opcr/E~)l/o2479 2.3 (packet of powder) PE mg 60120 180 other components:
phosphatidylcholine ~
phosphatidylserine (*) mg250 500 750 cholesterol mg S lo 15 lactose mg 100 200 300 fla~oring and sweetener as required sucrose (**) to mg20004000 6000 (*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary (**) sucrose may be substituted by fructose 2.4 (retard effect tablet) PE mg 30 60 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg80 160 320 lactose mg 30 60 120 microcrystalline ;; 25 cellulose mg 5 10 20 hydroxypropyl-methylcellulose mg 10 20 40 talc mg 3 6 12 colloidal silica mg 3 6 12 (*~ the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary - ' :
'' , .
, . .
.~: . .. ,, . . ,, . . , : . . .
: ~ . ,, . - ,........ .: . . : .
- , .: . . . : .. . .. ~ :
~: . , : , .
.~ , . . . .
WO92/1]294 2 0 l 5 !~ 7 ~ pc~/Epl)l/n247t) ~;
-38- ~
. . , 2.5 (gastroresistant tablet) PE mg3060 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg 80 160 320 lactosa mg 50 100 200 microcrystalline cellulose mg 10 20 40 talc mg 30 60 120 colloidal silica mg 3 6 12 methacrylic acid copolymer mg 15 30 60 (*~ the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary .
2.6 (gastroresistant, retard effect tablet) PE mg 30 60 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg80 lS0 320 : lactose mg 50 100 200 mi~rocrystalline cellulose mg 10 20 40 hydroxypropyl_ methylcellulose mg 5 10 20 talc mg 30 60 120 colloidal silica mg ~ 6 12 . 30 methacrylic acid copolymer mg 15 30 60 ~` (*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may Yary `
wo92/1129~ 207~ i3 7 o pcr/Ep~ ItU~79 - 3 g -2.7 (solution to be administered orally as drops) PE mg 30 60120 other components:
citric acid mg 7.5 15 30 purified water to ml 0.250.5 2.8 tgranules *) PE mg 30 60120 other components:
citric acid mg 7.5 15 30 sucrose mg 30 60 60 corn starch mg 12.5 25 25 talc mg 5 10 10 polyvinylpyrrolidone mg 4 8 8 (*? 3 granules administered in a hard gelatin capsule 2.9 (gastroresistant granules *) PE mg 30 60 120 other components:
citric acid mg 7.5 15 30 sucrose mg 30 60 60 corn starch mg 12.5 25 25 - talc mg 5 10 lO
polyvinylpyrrolidone mg 4 8 8 .
methacrylic acid .
; copol~ner mg 10 15 15 .', , . : , (*) 3 granules administered in a hard gelatin capsule :
. .
' -, . , ., , ' , . ' ' ' , ~':
, , , :.. ..
, . . , . :
' ':
WO 92/11294 2 0 7 ~ ~ 7 0 Pcr/E~l/~2~79 3. NASAL OR PUL~ONARY FORMULATIONS
3.1 PE fine white powder mg 20 40 The active principle, as a fine white powder, is contained in a gelatin capsule to be broken open when ready for use and loaded into suitable apparatus for inhalation.
3.2 (powder for inhalation) PE fine white powder mg 20 40 phosphatidylcholine +
phosphatidylserine * mg 30 60 ' The active principle, as a fine white powder, is contained in a gelatin capsule to be broken open when ready for use and loaded into suitable apparatus for inhalation.
(*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary 4. FORMULATIONS FOR RECTAL ADMINISTRATION
4.1 PE mg 30 120 semisynthetic glyceride mg1940 1880 4.2 PE mg 30 120 phosphatidylserine +
phosphatidylcholinemg 100 200 semisynthetic glyceride mg1840 1680 .
.. . . . .. . .. :
. ~. , . ., . .. . :
~. , :: ',' ' ' , , .
. : .
092/11294 PCT/EP~1/Oz479 -4l~
In summary, the low molecular weight heparin derivatives and salts ~hereof according to the present invention are obtainable by treatment of a quaternary ammonium salt of a heparin, dissolved in a heterocyclic organic solvent chosen from the group formed by N-alkyl pyrrolidine-2-one, N-alkyl-piperidine-2-one, unsubstituted or substituted by lower alkyl groups, and their derivatives interrupted in the heterocyclic ring by another heteroatom or heterogroup selected from -o-, -s-, and -NH-, or in a concentrated solution of said compound in an aprotic solvent, with an alkylating (etherifying) agent derived from a hydrocarbon having from 6 to 30 carbon atoms, preferably from 8 to 18 carbon atoms, at a temperature of from about 20 (room temperature) to 60~C.
for a prolonged period of time, e.g., about 5 to 20 hours. The resulting reaction product is then treated at a temperature of from 5 to 120C., preferably about 70C., with an inorganic or organic base in an aqueous solution. The product resulting from this alkaline treatment is then isolated in free form or as an alkali metal or alkaline earth metal salt thereof. Salts of other metals or organic base salts may be obtained therefrom by conversion from one to the other.
Preferably, in the second step of the procedure, the reaction product is treated with an alkaline hydroxide in aqueous solution. The resulting low molecular weight heparin derivatives and salts thereof are useful therapeutically, for example, as anti-thrombotic agents.
- ~ .
- : ,.':~. ., , . ~ . , . .:
.:
. ,,:, ~ . ~
ADMINIST~TION IN MOUSE
The present experiment assessed the maximum tolerated dose of the compound PE after administration by the intravenous and subcutaneous route in the mouse.
The test products were dissolved-in sterile saline and tested at concentrations ranging between 125 and 2000 mg/kg i.v. and s.c.
Descri~tion of the test The experiment was performed on male and female CD-l mice (C. River) (25-35 grams) and comprised two steps.
l) Screening. Groups of one male mouse and one female mouse were treated with one of the following doses: 125, 250, 500, 1000 and 2000 mg/kg. Mortality within 7 days of treatment was monitored.
2~ Groups of five male and five female mice were treated (for each compound and each administration route) with the highest : tolerated dose found on screening. The animals were observed for 14 days, during which mortality and the presence of altered behaviour and general toxicity symptoms were observed. In the case of mortality a lower dose was used, until the maximum tolerated dose was found.
Where possible, autopsy was performed on the deceased animals.
~`
:
:-.
. . . :
9 7 ~
W0 92/ll294 ' ' ' / PCt'/;~R~)a/02'179 Results 1. Intravenous tolerance dose As reported in Tables 6 and 7, the maximum tolerated dose of the test compounds proved to be the following:
- PE: 1000 mg/kg i.v.
- unfractionated heparin UFH: 125 mg/kg i.v.
- CY 216: 1000 mg/kg i.v.
It must be noted therefore that PE has greater tolerance lo dose than unfractionated heparin UFH.
Autopsy of the animals which died after treatment with unfractionated heparin UFH at 500 and 250 mg/kg, reve~led no macroscopic findings except, in some animals, the presence of probable residues of internal hemorrhage in the intestine.
2. Subcutaneous tolerance dose The results obtained, as reported in Tables 8 and 9, show that the maximum tolerated doses of the test products are as follows:
- PE: 2000 mg/kg s.c.
- unfractionated heparin UFH: 125 mg/kg s.c.
- CY 216: 2000 mg/kg s.c.
25 As with the intravenous route, therefore, the .tolerance dose of PE is far greater than that of unfractionated heparin (UFH), while it is similar to that of CY 216. It is however important to highlight that:
- In all the animals (10/10~ treated with CY 216 (2000 mg/kg s.c.) a circular area of skin affected by necrosis was observed on the back, corresponding to the injection site, the size of which differed from animal to animal (maximum diameter about 1 cm).
.
. . . .
,: , . -.. . .
WO 92/11294 2 0 7 S 9 7 ~ I'CI/EP91/0~47') ~
-22- !
.
Autopsy revealed necrosis to be limited to the skin, it did not therefore affect the underlying muscle~
- No anomalies were observed in animals treated with PE (2000 mg/kg s.c.).
- The animals which died after treatment with UFH (250 mg/kg) presented extensive bruising in the subcutaneous dorsal region, where treatment had been performed.
The subcutaneous tolerance data therefore show a lo difference between the compoun~s PE and CY 216.
Indeed, although the maximum tolerance doses are the same, in the case of CY 216 a marked area of necrosis of the skin is present at the injection site, which indicates that CY 216 is tolerated to a lesser degree locally than PE (which presented no anomalie,).
'' ' , .
. .
. : , . :
.. . .
:. .
- - . . : :
07~97~
O92/11294 P~!EP~]/02479 Tabl e 6 Lethality of compounds PE, CY 216 and unfractionated heparin UFH after a single intravenous administration (screening) , . . _ . .
Treatment Deceased animals/Treated animals (mg/kg i.v.) males females 10 PE 2000 0/1 0/1 : :
Heparin UFH 2000 1/1 1/1 Heparin UFH 1000 1/1 1/1 Heparin UFH 500 0/1 0/1 Heparin UFH 250 0/1 0/1 Heparin UFH 125 0/1 0/1 ; ~ .,. : ' , ''''' ' ~, ' '', ~ ' ' ., , , ' :, . ' . . .
'. : '. . ' :' : , . . .
-207597~ 1 WO92/11294 PCT/EP'31/0247')~
-2~-Table 7 Lethality of compounds PE, CY 216 and unfractionated heparin (UFH) after a single intravenous administration . . _ ~
Treatment Deceased animals/Treated animals Tlme of death (mg/kg i.v~)males females days after ~ treatment immëdiate* 1 2 3 4 PE 1000 0/5 o/5 - - - -Heparin 5000/5 2/5 - 2 125 o/5 0/5 *Within minutes of tre~tment ~ ' .
., .
. :
' ~'~' ~ ''"' '' ' '' ''` ' '' " ' '. ,' ' ' ' ' ' ' ' " ' . ', ' ' ' ' ' ' ' ~ ' ', . '. ' '' ' ' . ,'' ' ~ ~O92~11294 ~ 7 ~ 9 ~ ~ pcr/~ 79 Table 8 Lethality of the compounds PE, CY 216 and unfractiona~ed heparin UFH after a single subcutaneous administration (screening) _ Treatmen~ Deceased animals/Treated animals tmg/kg s.c.) males females CY216 500 0/1 - o/
Heparin UFH 2000 1/1 1/1 ~eparin UFH 1000 1/1 0/1 .
Heparin UFH 500 1/1 0/1 Heparin UFH 250 0/1 0/1 Heparin UFH 125 0/1 0/1 - ., - - . . ..
. -- - -, .. . : ,. . .
, - ,- - ... . ..
. - - : - : ., ... :. -:. : : , . .
: - . : . : , . . .
- - - .. ... : .. " .. , .: : : ... : . . . .:.
. . .. :.: . .. ~ - . - , ..
2~7~70 WO92/11294 PCr'/~P91/~2~'7~) -2s- .
'rabl e 9 Lethality of compounds PE, CY 216 and unfractionated heparin (UFH) after a single subcutaneous administration Treatment Deceased animals/Treated animals Time of deat~
(mg/kg i.v.) males females treatment immediate 1 2 3 PE 2000 0/5 o/5 _ _ _ _ _ Heparin 250 1/5 2/5 - 2 15 UFH 125 0/5 0/5 ~
~ .
.
' '' ~ . ' '': ' ' . :
. . . . . .
." ' ' ; ,", . .
. . ~ , .. . .
-W092/11294 PC~ 10~75 CONCLUSIONS
The in vitro and in vivo results previously described outline an interesting pharmacological profile of the heparin derivative PE, setting it apart from unfractionated heparin (UXF) and rendering its pharmacological activities more valuable.
The activity of PE differs slightly ~rom that of CY
216, which i5 one of the best low-molecular-weight heparins currently on sale in France, and shows in particular better local tolerability after s.c.
administration in the mouse. Indeed, although the maximum tolerated doses are the same, all animals treated with CY 216 (2000 mg/kg s.c.) had evident necrosis of the skin at the injectidn site, while the skin of the animals treated with PE was unaffected.
In the case of pharmacological activity in vitro and in vivo, it is interesting to note that PE has:
- anticoagulant activity, far inferior to that of UFH;
- bioavailability, a~ter s.c. administration, much greater than that of UFH, thereby allowing fewer daily administrations for the same pharmacological effect;
- lesser side effects, with regard to UFH, as shown by the reduced bleeding time and by the absence of skin necrosis at the injection site, with regard to CY 216 (the best low-molecular-weight heparin ; on sale in France) which caused a local intolerance phenomena (necrosis) in all the animals treated;
- antithrombotic activity in vivo, as shown in both the model of venous stasis in the rat and in the m~del of arterial thrombosis in the rabbit. The product is therefore efficacious in preventing these .
.
'; :,, , . , . ,, ,, .' ,' , .- . - : : ,, - : . :. :. . .. . : ...
~,arl~7 ~
WO92/11294 pcr/E~9l/o2~7s pathologies at dosages of 1.5 and 6 mg/kg i.v., respectively, which do not induce any signif icant variations in the side effects.
In particular, with regard to the ven~us antithrombotic activity, the derivative PE, at a dose of 1.5 mg/kg i.v., does not induce:any alterations in bleeding time, unlike UFH;
- The new, low-molecular-weight heparin derivatives according to the present invention can therefore be used in the place of unfractionated heparin in all its indications, as an anticoagulant and thrombocyte aggregation inhibitor. The dose is adapted to each particular case, and is normally around 1-7 mg/kg per day, by the intravenous route.
The heparins to be used in the previously described procedure of the present invention can be of any type and of various origin, for example heparins extracted from the intestine of pigs, cattle, and sheep and from ox ; 20 heart, especially any one of the products which are commercially available or described in the literature.
Such products have widely ranging molecular weights, for example between 2,000 and 30,000 daltons, especially unfractionated heparin UFH, and also low-molecular-weight heparins obtained by fractionation of standard heparins (2,000-lO,000 daltons) and heparin fragments with a molecular weight of 500-lO,000 daltons obtained by ~ partial depolymerization of standard heparins by chemical : or enzymatic means. The quaternary ammonium salts to be used as starting material for said procedure can be ~` prepared in the known way, for instance by ion exchange of the heparin in aqueous solution as a sodium or ` potassium salt with resins based on quaternary ammonium salts, for example a salified sulfonic resin with a .
- , , . , . : . .
, ~ ~. . ' ~ 2~97~
WO 92/11294 PC-r/EP91/024'7g quaternary ammonium base. The quaternary ammonium salt can be obtained by freeze-drying the eluate. As quaternary ammonium salts, tetraalkylammonium salts derived from lower alkyls may be advantageously used, particularly tetraalkylammonium salts with alkyl groups having a maximum of 6 carbon atoms. Optionally, alkyl-aryl-ammonium salts may also be used, for example those having long-chained alkyl groups. of the tetraalkylammonium salts, tetrabutylammonium salts are preferably used. The quaternary ammonium salts to be used as starting substance for the procedure of the present invention are those obtainable by ion exchange i~ the aforesaid manner using alkaline salts, for example sodium or potassium salts, of heparin of the type used commercially, that is, neutral salts. They are reacted with an excess of quaternary ammonium ions so as to obtain also the corresponding neutral salts.
Quaternary ammonium salts are soluble both in the aforesaid heterocyclic solvents, and in aprotic organic solvents, such as dimethylsulfoxide and dimethylfor~amide. The reaction with khe alkylating ; agent, according to the first step of the procedure, can be performed both in the aforesaid heterocyclic solvents, or in a solution of the same in one of the aforesaid aprotic organic solvents, prefexably in a concentrated solution. Of the aforesaid heterocyclic solvents, the preferred ones are above all those which are not substituted in the cyclic structure, that is, N-alkyl-o~aryl-2-pyrrolidone, or their derivatives containing a heterocyclic atom in the cyclic structure, such as the corresponding derivatives of imidazoline, piperazine or morpholine. The N-alkyl groups of ; heterocyclic solvents are derived preferably from a lower ~ alkyl with a maximum of 6 carbon atoms, and the aryl '~:
.. . .. . .
~,. . . ,., ' '" ' ~ ,. ' ' ,. - ~ , . . , , ~ .:
- . : . , . , ~ :
.
'': .,~.. , -, ' , ' : :. , 20~970 ~ I
WO 92/11294 PCr/EP(~/02~'79 group is primarily a pheny1 group, optionally substituted by 1 to 3 lower alkyl groups, especially methyl groupsO
Preferably, N-methyl-2-pvrrolidone is used.
An alkylating agent derived from a hydrocarbon having from 6 to 30 carbon atoms, preferably from 8 tQ 18 carbon atoms, is a compound easily capable of yielding the corresponding hydrocarbyl groups, such as a reagent ester group of an acid with an alcohol with a corxesponding number of carbon atoms, which can be an aliphatic or araliphatic alcohol having preferably a maximum of 18 carbon atoms, for example a hexyl, heptyl, octyl or nonyl alcohol. The reagent esters can be derived from inorganic or organic acids, such as hydracids, sulfuric or sulfurous acid, or alkyl- or aryl-sulfonic l~ acids, for example methane-sulfonic or p-toluenesulfonic acid. The esters of the hydracids are in particular chlorides, bromides and iodides. The reaction between the quaternary ammonium salt of the aforesaid alkylating agent is performed at room temperature (20C.)or slightly higher, for example at a temperature of from 30 ~ 35Co but not exceeding 60C, and is maintained for a prolonged period of time of about 5 to 20 hours, typically about 16 hours.
The reaction product can be isolated and subsequently submitted to the second step of the procedure, that is, to alkaline treatment, or it can be converted directly into the final product, performing the alkaline treatment directly on the solution, optionally concentrated, of the reaction product of the first step.
3 0 It is also possible to evaporate the solvent under bland (mildj conditions after the first step of the procedure and to perform alkaline treatment on the residue. It is therefore possible to perform the procedure of the ~ invention as a "one-pot" process. The basic treatment of :' -,., . ~. ~ :
-'WO92/1129~ ~ O~ PCT/~ Z47 -31~
the reaction product between the quaternary ammonium salt of heparin with the alkylating agent is performed at a temperature of from 5O to 120 C ., suitably at a temperature between 50C and 120C, preferably about 70OC, for about two hours. Alkaline hydrates are used~
such as NaOH or KOH, or other inorganic and/or organic bases, preferably at a concentration of between 0.l and lM. The bases are used in aqueous or alcoholic solutio~s/
but other solvents can be present which are miscible with water or with an aqueous-alcoholic mixture, such as, for example, the residue solvents used in the first step of the procedure in the case of the aforesaid "one-pot"
process.
If it is desired to isolate the reaction product of the first step of the proc-dure, it can be precipitated by the addition of an organic polar solvent, preferably an aliphatic alcohol such as methyl or ethyl alcohol, to which a basic buffer has preferably been added, such as especially a basic salt of a carboxylic acid, e.g., an acetate or propionate of sodium or potassium. Other basic buffers can be used, such as alkaline bicarbonates or alkaline phosphates. The precipitated product is preferably washed with the polar solvent used in the precipitation, for example methanol. It is advisable to purify the precipitated product further by reprecipitating it once more or several times, that is, by dissolving the product in water and precipitating it with an alcohol.
- The reaction product, comprising the low-molecular-weight heparin derivative and having the previously described properties, can be released in free form either from a metal salt or from an organic base in the conventional way. The alkaline salt corresponding to the alkaline hydrate used in the second step of the .
~` . ' " ' ' ~ ~ ' ~ ' ' ~ , , ' . , .
. ~ .~ , ~, ' , ' ' ' .
207~7~ f~7;, WO92/1l294 PCI/EP~1/02~7l) procedure may be obtained by neutralizing the solution with an acid, e.g., 2M hydrochloric acid, purifying the solution, extracting it with an organic solvent which cannot be mixed with water, for example methylene chloride, and repeating this operation several timesO
The salt is then dialyzed with distilled water and sodlum chloride and freeze-dried.
The products of the invention are used mainly in the form of their metal salts or organic base salts. If it ls desired to obtain metal salts other than alkaline sal~s corresponding to the ions of the alkaline hydrates used in the aforesaid alkaline treatment, it is possible ko use ion exchange methods by known t~chniques.
Alternatively, it is possible to isolate the heparin product in its acid form, adding the alkaline salt obtained with the calculated quantity of a diluted strong acid, such as hydrochloric acid or sulfuric acid, extracting the product with a suitable organic solvent, isolating the heparin compound in ~ree form and then converting it into the desired salt.
Of the metal or organic base salts which can be used according to the present invention, of particular importance are those which are therapeutically acceptable, such as alkali and alkaline-earth metals, for example sodium, potassium, ammonium, calcium, and magnesium salts, or heavy metal salts, such as copper and iron salts. The salts of organic bases can be derived ~rom primary, secondary or tertiary aliphatic, aromatic or heterocyclic amines, such as methylamine, ethylamine, propylamine, piperidine, morpholine, ephedrine, furfurylaminecholine, ethylenediamine and aminoethanolO
Salts which cannot be directly used in therapy, which are also part of the invention, are for example those which can be used for the purification of the new ' :
: , ~ .
, ~- ~ ' ' ''' ' .
.,, ~ " , - .
3 9 7 ~ 1 ' W092/11294 PCr/EP~1/02~79 heparin derivatives of the invention, such as some of the heavy metal salts.
The invention also includes pharmaceutical preparations containing as active substance a new low-molecular-weight heparin derivative obtainable by the procedure described herein, especially in the form o~
their therapeutically acceptable salts. Such preparations can be for parenteral use, for example for subcutaneous or intravenous administration, or for topical use, for example in the form of creams or ointments, or suppositories, or nose sprays. They can therefore be formulated as solutions of the active compounds or as freeze-dried powders of the active compounds to be mixed with one or more pharmaceutically lS acceptable excipients or diluents which are convenient for the aforesaid uses and with an osmolarity which is compatible with physiological fluids.The invention includes, besides the new low-molecular-weight heparin derivatives, the aforesaid procedure for their p:eparation. Included in the invention is also the performance of the single steps of the preparation procedure, that is, the reaction of a quaternary ammonium salt of heparin with an alkylating agent as defined above in on of said solvents and the alkaline treatment of the 1 25 reaction product.
The invention is illustrated in the following Examples which, however, are not to be considered as limiting.
' ..
.
. .
- ~ . - .. - . - . . .
.. . . .. .. . ..
, . , ~ .:
:, . -. . , ~ . : ~ .
.... . . ... : , , : , .
- : , - : , , . ; . . : . ., : :. ,, . : . :: .
: . : , . . . .
.. . . . . . .. ... .. . .
: - , . . .. . , :. ~ :
- .. . ... : . ,, : ,. .: . .
. . .. . . . .
207597~ ~ ' W092/11294 PC~'/EP91/0247~ i 1) F RMULATIONS FOR INJECTION
1 . 1 PE mg 10 20 30 40 water for injection in ml 0.1 0.2 0.3 004 Package with ready-to-use syringe containing sterile solution for subcutaneous admlnistration~
: 1.2 PE mg 150 300 other components:
water for injection in ml 4 Package with vial containing sterile solution for intravenous administration.
.
15 1.3 PE mg 10 20 30 40 other components:
sodium chloride mg 0.3 0.6 0.9 1.2 - water for injection in ml 0.1 0.2 0.3 0.4 Package with ready-to-use syringe containing sterile solution for suboutaneous administration.
. . - ' ' ' ' . . .
~ , . . .
.. - I .
-.: - ., . . . . :
:', ': . . ' -- W092/11~94 PCT/~P~1/02~7 1.4 PE mg 150 300 other components:
sodium chloride mg 35 70 water for injection in ml 5 10 ; Package with vial containing sterile solution ~or intravenous administration.
1.5 PE mg 150 300 other components:
sodium chloride mg 35 70 sodium metabisulfite mg 5 10 ~ .
chlorbutanol (*) . mg 25 50 ; 15 water for injection in ml 5 10 Package with vial containing sterile solution for multidose intravenous administration.
(*) in Example 1.5 the preservative chlorbutanol can 20 be substituted by:
benzyl alcohol mg 50 100 or by:
chlorocresol mg 5 10 ~ ,, .
,, , . , ,, ., ~. " . ", -,- . . .. : ,.. . .. , : , . ... . .. . .. .. .. . . . . .
.,: .. .. . , , . , , : . . ,., : ,, ., ",... . , .: . :. . : . ., . , : ,-. - .. ,: : : .
.. : -:: . : .: : .,::: . .. : .. . . .
: , :- -. : .... , . : . .. .
.: - . , ~ : . -- , .. .. - , , , - "
,: , .,, : . , , :
WO92/11294 2 0 ~ ~ 9 7 0 -36- PCr/EY~1/1)2~7~) 2) FORMULATIONS FOR ORAL ADMINISTRATION
2.l (pill or capsule) PE mg 3060 120 other components:
phosphatidylcholine ~
~ phosphatidylserine (*) mg 80160 320 : lactose mg 50l00 200 microcrystalline cellulose mg l020 40 talc mg 3 5 12 colloidal silica mg 3 6 12 (*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary 2.2 (pill or capsule) PE mg 3060 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg 80160 320 cholesterol mg 2 4 8 lactose mg 50l00 200 - microcrystalline cellulose mg l020 40 talc mg 3 6 12 colloidal silica mg 3 6 12 ; ~*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may 30 vary.
-' , ~: . -,. , . , . . :
, ~ . , , .
. ':, ,,: ': ' , . ,~ .
. . .. .... . . . .
.~ : , . . : . " ,, . : . . :
~ 092/11294 2 ~ ~ ;3 9 ~ Opcr/E~)l/o2479 2.3 (packet of powder) PE mg 60120 180 other components:
phosphatidylcholine ~
phosphatidylserine (*) mg250 500 750 cholesterol mg S lo 15 lactose mg 100 200 300 fla~oring and sweetener as required sucrose (**) to mg20004000 6000 (*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary (**) sucrose may be substituted by fructose 2.4 (retard effect tablet) PE mg 30 60 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg80 160 320 lactose mg 30 60 120 microcrystalline ;; 25 cellulose mg 5 10 20 hydroxypropyl-methylcellulose mg 10 20 40 talc mg 3 6 12 colloidal silica mg 3 6 12 (*~ the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary - ' :
'' , .
, . .
.~: . .. ,, . . ,, . . , : . . .
: ~ . ,, . - ,........ .: . . : .
- , .: . . . : .. . .. ~ :
~: . , : , .
.~ , . . . .
WO92/1]294 2 0 l 5 !~ 7 ~ pc~/Epl)l/n247t) ~;
-38- ~
. . , 2.5 (gastroresistant tablet) PE mg3060 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg 80 160 320 lactosa mg 50 100 200 microcrystalline cellulose mg 10 20 40 talc mg 30 60 120 colloidal silica mg 3 6 12 methacrylic acid copolymer mg 15 30 60 (*~ the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary .
2.6 (gastroresistant, retard effect tablet) PE mg 30 60 120 other components:
phosphatidylcholine +
phosphatidylserine (*) mg80 lS0 320 : lactose mg 50 100 200 mi~rocrystalline cellulose mg 10 20 40 hydroxypropyl_ methylcellulose mg 5 10 20 talc mg 30 60 120 colloidal silica mg ~ 6 12 . 30 methacrylic acid copolymer mg 15 30 60 ~` (*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may Yary `
wo92/1129~ 207~ i3 7 o pcr/Ep~ ItU~79 - 3 g -2.7 (solution to be administered orally as drops) PE mg 30 60120 other components:
citric acid mg 7.5 15 30 purified water to ml 0.250.5 2.8 tgranules *) PE mg 30 60120 other components:
citric acid mg 7.5 15 30 sucrose mg 30 60 60 corn starch mg 12.5 25 25 talc mg 5 10 10 polyvinylpyrrolidone mg 4 8 8 (*? 3 granules administered in a hard gelatin capsule 2.9 (gastroresistant granules *) PE mg 30 60 120 other components:
citric acid mg 7.5 15 30 sucrose mg 30 60 60 corn starch mg 12.5 25 25 - talc mg 5 10 lO
polyvinylpyrrolidone mg 4 8 8 .
methacrylic acid .
; copol~ner mg 10 15 15 .', , . : , (*) 3 granules administered in a hard gelatin capsule :
. .
' -, . , ., , ' , . ' ' ' , ~':
, , , :.. ..
, . . , . :
' ':
WO 92/11294 2 0 7 ~ ~ 7 0 Pcr/E~l/~2~79 3. NASAL OR PUL~ONARY FORMULATIONS
3.1 PE fine white powder mg 20 40 The active principle, as a fine white powder, is contained in a gelatin capsule to be broken open when ready for use and loaded into suitable apparatus for inhalation.
3.2 (powder for inhalation) PE fine white powder mg 20 40 phosphatidylcholine +
phosphatidylserine * mg 30 60 ' The active principle, as a fine white powder, is contained in a gelatin capsule to be broken open when ready for use and loaded into suitable apparatus for inhalation.
(*) the ratios between the phosphatidylcholine and phosphatidylserine present in the formulations may vary 4. FORMULATIONS FOR RECTAL ADMINISTRATION
4.1 PE mg 30 120 semisynthetic glyceride mg1940 1880 4.2 PE mg 30 120 phosphatidylserine +
phosphatidylcholinemg 100 200 semisynthetic glyceride mg1840 1680 .
.. . . . .. . .. :
. ~. , . ., . .. . :
~. , :: ',' ' ' , , .
. : .
092/11294 PCT/EP~1/Oz479 -4l~
In summary, the low molecular weight heparin derivatives and salts ~hereof according to the present invention are obtainable by treatment of a quaternary ammonium salt of a heparin, dissolved in a heterocyclic organic solvent chosen from the group formed by N-alkyl pyrrolidine-2-one, N-alkyl-piperidine-2-one, unsubstituted or substituted by lower alkyl groups, and their derivatives interrupted in the heterocyclic ring by another heteroatom or heterogroup selected from -o-, -s-, and -NH-, or in a concentrated solution of said compound in an aprotic solvent, with an alkylating (etherifying) agent derived from a hydrocarbon having from 6 to 30 carbon atoms, preferably from 8 to 18 carbon atoms, at a temperature of from about 20 (room temperature) to 60~C.
for a prolonged period of time, e.g., about 5 to 20 hours. The resulting reaction product is then treated at a temperature of from 5 to 120C., preferably about 70C., with an inorganic or organic base in an aqueous solution. The product resulting from this alkaline treatment is then isolated in free form or as an alkali metal or alkaline earth metal salt thereof. Salts of other metals or organic base salts may be obtained therefrom by conversion from one to the other.
Preferably, in the second step of the procedure, the reaction product is treated with an alkaline hydroxide in aqueous solution. The resulting low molecular weight heparin derivatives and salts thereof are useful therapeutically, for example, as anti-thrombotic agents.
- ~ .
- : ,.':~. ., , . ~ . , . .:
.:
. ,,:, ~ . ~
Claims (36)
1. A process for preparing low molecular weight heparin derivatives and/or salts thereof which is characterized by (1) treating a quaternary ammonium salt of a heparin dissolved in a heterocyclic organic solvent selected from N-alkyl-pyrrolidine-2-one, N-alkyl-piperidine-2-one, unsubstituted or substituted by lower alkyl groups, or derivatives thereof interrupted in the heterocyclic ring by another heteroatom or heterogroup selected from -O-, -S- or -NH-, or a concentrated solution of said compound in an aprotic solvent, with an alkylating agent derived from a hydrocarbon having from 6 to 30 carbon atoms, at room temperature or slightly higher, (2) treating the resulting reaction product, at a temperature of from 5° to 120°C., with an inorganic or organic base in an aqueous solution, and (3) isolating the heparin derivatives obtained in their free form or as alkali metal or alkaline earth metal salts thereof.
2. A process according to claim 1, which further comprises converting said heparin derivatives or salts obtained into salts of other metals or into organic base salts.
3. A process according to claim 1, which further comprises converting the heparin derivatives obtained in free form into pharmaceutically acceptable salts or converting said salts into heparin derivatives in free form.
4. A process according to claim 1, wherein in step (2) said reaction product is treated with an alkaline hydroxide in aqueous solution.
5. A process according to claim 1 or claim 4, wherein the product resulting from the reaction of the alkylating agent with the quaternary ammonium salt of heparin is isolated before being treated with the inorganic or organic base.
6. A process according to claim 1 or claim 4, wherein quaternary ammonium salts of heparin having molecular weights varying from 2,000 to 30,000 daltons are used as a starting material.
7. A process according to claim 1 or claim 4, wherein quaternary ammonium salts of unfractionated heparin are used as a starting material.
8. A process according to claim 1 or claim 4, wherein quaternary ammonium salts of low molecular weight heparin, obtained by fractionation of heparin having a molecular weight of 2,000 to 10,000 daltons and heparin fragments having a molecular weight of 500 to 10,000 daltons obtained by partial chemical or enzymatic depolymerization of heparin, are used as a starting material.
9. A process according to claim 1 or claim 4, wherein said quaternary ammonium salt is a tetraalkylammonium salt wherein the alkyl groups have from 1 to 6 carbon atoms.
10. A process according to claim 1 or claim 4, wherein said quaternary ammonium salt is the tetrabutyl ammonium salt.
11. A process according to claim 1 or claim 4, wherein the N-alkyl group in said heterocyclic organic solvent is a lower alkyl having from 1 to 6 carbon atoms.
12. A process according to claim 1 or claim 4, wherein said heterocyclic organic solvent is N-methyl-pyrrolidone.
13. A process according to claim 1 or claim 4, wherein an ester of an acid with an aliphatic or araliphatic alcohol having from 6 to 30 carbon atoms is used as the alkylating agent.
14. A process according to claim 13, wherein said alkylating agent has from 8 to 18 carbon atoms.
15. A process according to claim 14, wherein said alkylating agent is an iodide, bromide or alkyl chloride, or an ester of an alkyl- or arylsulfonic acid.
16. A process according to claim 1 or claim 4, wherein the alkylating agent is reacted with the quaternary ammonium salt of heparin dissolved in said heterocyclic organic solvent at a temperature of from about 20° to 60°C.
17. A process according to claim 1 or claim 4, wherein the reaction product resulting from the reaction of the alkylating agent with the quaternary ammonium salt of heparin is isolated by precipitation by the addition of a polar organic solvent.
18. A process according to claim 17, wherein said polar organic solvent is an aliphatic alcohol.
19. A process according to claim 18, wherein a basic buffer is added to said aliphatic alcohol.
20. A process according to claim 19, wherein said basic buffer is a basic salt of a carboxylic acid.
21. A process according to claim 17, wherein the precipitated product is reprecipitated several times with the same organic solvent.
22. A process according to claim 1, wherein in step (2) said reaction product is treated with an alkaline hydroxide or with another inorganic and/organic base at a concentration of between 0.1 and 1M in aqueous solution or alcoholic-aqueous solution at a temperature of from 5° to 120°C.
23. A process according to claim 22, wherein the alkaline treatment step is performed on the isolated reaction product resulting from step (1) with 0.1 - 1M
aqueous sodium hydroxide at a temperature of about 70°C.
for a sufficient time to obtain said low molecular weight heparin derivatives and/or salts thereof.
aqueous sodium hydroxide at a temperature of about 70°C.
for a sufficient time to obtain said low molecular weight heparin derivatives and/or salts thereof.
24. A process according to any of the preceding claims, wherein the reaction product obtained from step (2) is isolated by neutralization of the alkaline aqueous solution, extraction with a water-immiscible organic solvent, and dialysis with distilled water and sodium chloride.
25. A process for preparing lower molecular weight heparin derivatives and/or salts thereof which is characterized by (1) treating the tetrabutylammonium salt of heparin having a molecular weight of 15,000 daltons dissolved in N-methyl-pyrrolidone with 1-iodooctane at room temperature for about 16 hours, (2) precipitating the reaction product by pouring the resulting solution into methanol to which sodium acetate has been added, (3) purifying the resulting product several times by reprecipitation from methanol to which sodium acetate has been added, (4) treating the dried product with 0.5 N aqueous sodium hydroxide for about two hours at approximately 70°C., (5) neutralizing the resulting solution with 2M
hydrochloric acid, (6) extracting the solution several times with methylene chloride, (7) dialyzing the solution with distilled water and 0.1 M sodium chloride, and (8) freeze-drying the obtained solution.
hydrochloric acid, (6) extracting the solution several times with methylene chloride, (7) dialyzing the solution with distilled water and 0.1 M sodium chloride, and (8) freeze-drying the obtained solution.
26. Low molecular weight heparin derivatives and salts thereof, prepared by the process as recited in any of claims 1 - 25.
27. Alkali metal or alkaline earth metal salts of low molecular weight heparin derivatives prepared by the process as recited in any of claims 1 - 25.
28. A sodium, potassium or calcium salt of the heparin derivatives prepared according to any of claims 1 - 25.
29. Salts of therapeutically acceptable bases of the heparin derivatives prepared according to any of claims 1 - 25.
30. Sodium, potassium or calcium salt of the heparin derivatives prepared according to claim 29.
31. A pharmaceutical composition comprising low molecular weight heparin derivatives according to claim 26 as an active ingredient and a pharmaceutically acceptable carrier, diluent or excipient.
32. A pharmaceutical composition comprising an alkali metal or alkaline earth metal salt of low molecular weight heparin derivatives according to claim 26 as an active ingredient and a pharmaceutically acceptable carrier, diluent or excipient.
33. The use of low molecular weight heparin derivatives according to claim 26 as a therapeutic agent.
34. The use of alkali metal or alkaline earth metal salts of low molecular weight heparin derivatives according to claim 27 as a therapeutic agent.
35. The use of low molecular weight heparin derivatives or salts thereof according to claim 26 for the treatment of thrombosis.
36. A pharmaceutical composition according to claims 31 and 32 for use in the treatment of thrombosis.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| IT04175290A IT1243300B (en) | 1990-12-20 | 1990-12-20 | HEPARIN DERIVATIVES |
| IT41752A/90 | 1990-12-20 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2075970A1 true CA2075970A1 (en) | 1992-06-21 |
Family
ID=11253436
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002075970A Abandoned CA2075970A1 (en) | 1990-12-20 | 1991-12-20 | Heparin derivatives |
Country Status (13)
| Country | Link |
|---|---|
| EP (1) | EP0516792A1 (en) |
| JP (1) | JPH05504785A (en) |
| KR (1) | KR920703644A (en) |
| CN (1) | CN1062537A (en) |
| AU (1) | AU658594B2 (en) |
| BR (1) | BR9106234A (en) |
| CA (1) | CA2075970A1 (en) |
| FI (1) | FI923762A (en) |
| HU (1) | HUT62917A (en) |
| IT (1) | IT1243300B (en) |
| NO (1) | NO923240L (en) |
| PT (1) | PT99898A (en) |
| WO (1) | WO1992011294A1 (en) |
Families Citing this family (13)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| FR2663639B1 (en) * | 1990-06-26 | 1994-03-18 | Rhone Poulenc Sante | LOW MOLECULAR WEIGHT POLYSACCHARIDE BLENDS PROCESS FOR PREPARATION AND USE. |
| FR2704861B1 (en) * | 1993-05-07 | 1995-07-28 | Sanofi Elf | Purified heparin fractions, process for obtaining them and pharmaceutical compositions containing them. |
| ES2077533B1 (en) * | 1994-02-28 | 1996-07-01 | Bioiberica | PROCEDURE FOR OBTAINING OLIGOSACCHARIDE FRACTIONS BY CHEMICAL DEPOLYMERIZATION OF HEPARIN. |
| US5639469A (en) * | 1994-06-15 | 1997-06-17 | Minnesota Mining And Manufacturing Company | Transmucosal delivery system |
| US6001820A (en) * | 1995-03-31 | 1999-12-14 | Hamilton Civic Hospitals Research Development Inc. | Compositions and methods for inhibiting thrombogenesis |
| US5744457A (en) * | 1995-03-31 | 1998-04-28 | Hamilton Civic Hospitals Research Development Inc. | Compositions and methods for inhibiting thrombogenesis |
| US5763427A (en) * | 1995-03-31 | 1998-06-09 | Hamilton Civic Hospitals Research Development Inc. | Compositions and methods for inhibiting thrombogenesis |
| KR19990087665A (en) * | 1996-03-15 | 1999-12-27 | 오미야 히사시 | Heat-treatment products of uronic acid, foods, beverages or drugs containing them |
| US5767269A (en) * | 1996-10-01 | 1998-06-16 | Hamilton Civic Hospitals Research Development Inc. | Processes for the preparation of low-affinity, low molecular weight heparins useful as antithrombotics |
| FR2763848B1 (en) * | 1997-05-28 | 2000-01-28 | Rhone Poulenc Rorer Sa | USE OF LOW MOLECULAR WEIGHT HEPARINS FOR THE PREVENTION AND TREATMENT OF CENTRAL NERVOUS TRAUMA |
| WO2003088949A2 (en) * | 2002-04-19 | 2003-10-30 | Bioghurt Biogarde Gmbh & Co. Kg. | Matrix comprising a bioactive component containing phospholipid |
| DE10217557A1 (en) * | 2002-04-19 | 2003-11-06 | Degussa Bioactives Gmbh | Functional foods containing a phospholipid-containing stable matrix |
| CN100335506C (en) * | 2004-05-20 | 2007-09-05 | 汕头市金丰医疗器械科技有限公司 | Heparin compound, and its preparing method and use |
Family Cites Families (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| FR2482603A1 (en) * | 1980-05-14 | 1981-11-20 | Pharmindustrie | NOVEL HEPARIN ESTERS FOR USE IN THE PREPARATION OF MEDICAMENTS, AND METHODS FOR THEIR PREPARATION |
| ATE122059T1 (en) * | 1986-08-20 | 1995-05-15 | Univ Miami | LOW MOLECULAR WEIGHT ALKYLESTERS OF HEPARIN. |
| SE8702254D0 (en) * | 1987-05-29 | 1987-05-29 | Kabivitrum Ab | NOVEL HEPARIN DERIVATIVES |
-
1990
- 1990-12-20 IT IT04175290A patent/IT1243300B/en active IP Right Grant
-
1991
- 1991-12-20 CA CA002075970A patent/CA2075970A1/en not_active Abandoned
- 1991-12-20 KR KR1019920701996A patent/KR920703644A/en not_active Application Discontinuation
- 1991-12-20 PT PT99898A patent/PT99898A/en not_active Application Discontinuation
- 1991-12-20 EP EP92901426A patent/EP0516792A1/en not_active Withdrawn
- 1991-12-20 HU HU922685A patent/HUT62917A/en unknown
- 1991-12-20 AU AU90964/91A patent/AU658594B2/en not_active Ceased
- 1991-12-20 BR BR919106234A patent/BR9106234A/en unknown
- 1991-12-20 JP JP4501399A patent/JPH05504785A/en active Pending
- 1991-12-20 CN CN91111853A patent/CN1062537A/en active Pending
- 1991-12-20 WO PCT/EP1991/002479 patent/WO1992011294A1/en not_active Application Discontinuation
-
1992
- 1992-08-18 NO NO92923240A patent/NO923240L/en unknown
- 1992-08-20 FI FI923762A patent/FI923762A/en not_active Application Discontinuation
Also Published As
| Publication number | Publication date |
|---|---|
| EP0516792A1 (en) | 1992-12-09 |
| NO923240D0 (en) | 1992-08-18 |
| NO923240L (en) | 1992-10-19 |
| WO1992011294A1 (en) | 1992-07-09 |
| PT99898A (en) | 1992-12-31 |
| AU9096491A (en) | 1992-07-22 |
| AU658594B2 (en) | 1995-04-27 |
| FI923762A0 (en) | 1992-08-20 |
| CN1062537A (en) | 1992-07-08 |
| JPH05504785A (en) | 1993-07-22 |
| IT9041752A1 (en) | 1992-06-21 |
| IT9041752A0 (en) | 1990-12-20 |
| IT1243300B (en) | 1994-05-26 |
| FI923762A (en) | 1992-08-20 |
| KR920703644A (en) | 1992-12-18 |
| HUT62917A (en) | 1993-06-28 |
| BR9106234A (en) | 1993-03-30 |
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| DK173982B1 (en) | Depolymerized heparin derivatives, processes for their preparation and pharmaceutical composition and biological reagent containing them | |
| US5280016A (en) | Non-anticoagulant heparin derivatives | |
| AU618346B2 (en) | Sulfoamino derivatives of chondroitin sulfates, of dermatan sulfate and of hyaluronic acid and their pharmacological properties | |
| US5250519A (en) | Non-anticoagulant heparin derivatives | |
| US5696100A (en) | Method for controlling O-desulfation of heparin and compositions produced thereby | |
| CA2075970A1 (en) | Heparin derivatives | |
| EP0983304B1 (en) | Dermatan disulfate, an inhibitor of thrombin generation and complement activation | |
| US5084564A (en) | Production of oligosaccharide fractions having antithrombotic properties by controlled chemical depolymerization of heparin | |
| EP0862585A1 (en) | Method for controlling o-desulfation of heparin and compositions produced thereby | |
| EP2794666B1 (en) | Use of chemically modified heparin derivates in sickle cell disease | |
| WO1995030424A1 (en) | O-desulfated heparin derivatives, methods of making and uses thereof | |
| NZ214094A (en) | Xylan sulphates of low molecular weight, process for their preparation and medicaments containing them | |
| JPH0216733B2 (en) | ||
| US20240041918A1 (en) | Oligosaccharide Compound for Inhibiting Intrinsic Coagulation Factor X-Enzyme Complex, and Preparation Method Therefor and Uses Thereof | |
| JPS6357407B2 (en) | ||
| KR20110067130A (en) | Carboxyethylated cyclodextrin polysulfates useful as medicaments | |
| EP3924391A1 (en) | Safe bovine heparin, preparation method, and application | |
| JP2004507562A (en) | Antithrombotic composition | |
| AU2015203727A1 (en) | High Purity Heparin and Production Method Therefor |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| FZDE | Discontinued |