TREA

ENROFLOXACIN HEXAHYDRATE

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Information

  • Patent Application
  • 20110003829
  • Publication Number
    20110003829
  • Date Filed
    January 18, 2008
    17 years ago
  • Date Published
    January 06, 2011
    14 years ago
Information
Abstract
The present invention relates to a novel hexahydrate of enrofloxacin, to processes for its preparation, to pharmaceuticals containing it, and to its use in combating diseases.
Description

The present invention relates to a novel hexahydrate of enrofloxacin, to processes for its preparation, to pharmaceuticals containing it, and to its use in combating diseases.


The compound enrofloxacin is disclosed for example in EP-A 49 355 and EP-A 78 362 and is as defined in the Formula (I):







The compound of the Formula (I) is a fluoroquinolone antibiotic which is suitable for the treatment of bacterial diseases. Enrofloxacin-containing products are applied in veterinary medicine and have been commercially available for many years under the name Baytril®.


The compound of the Formula (I) can be prepared as described in EP-A 49 355 and EP-A 78 362. To date, only one crystal modification was known of the compound of the Formula (I), which is hereinbelow referred to as modification A. Modification A has a melting point of 224° C. and a characteristic x-ray diffractogram, IR spectrum, Raman spectrum, FIR spectrum and NIR spectrum (Tab. 1-5, FIG. 1-5).


Surprisingly, there has now been found a novel enrofloxacin hexahydrate of the Formula (II).







The hexahydrate of the Formula (II) contains 23.1% of hydrate water.


The present invention relates to the enrofloxacin hexahydrate of the Formula (II).


Surprisingly, the hexahydrate according to the invention shows better filtration properties and is easier to dry than modification A. Moreover, the hexahydrate according to the invention can be prepared in a better space-time yield and with a better secondary component profile than modification A.


The improved product properties are retained when the known modification A is prepared from the hexahydrate by drying.


In comparison with modification A, the hexahydrate of the Formula (II) has a clearly distinguishable X-ray diffractogram, IR spectrum, Raman spectrum, FIR spectrum and NIR spectrum (FIG. 1-5).


The invention relates in particular to enrofloxacin hexahydrate which, in the X-ray diffractogram, has a reflection at a 2 theta angle of 24.2.


The invention furthermore relates in particular to an enrofloxacin hexahydrate which, in the NIR spectrum, has a band at 5097 cm−1.


The invention furthermore relates to the use of the hexahydrate of the Formula (II) for the treatment and/or prophylaxis of bacterial diseases. The enrofloxacin hexahydrate can be employed essentially for the same indications as enrofloxacin and its pharmaceutically acceptable salts.


The present invention furthermore relates to the use of the compound according to the invention for the treatment and/or prophylaxis of diseases, in particular of bacterial diseases.


The present invention furthermore relates to the use of the compound according to the invention for the preparation of a pharmaceutical for the treatment and/or prophylaxis of diseases, in particular of bacterial diseases.


The present invention furthermore relates to a method of treating bacterial diseases, where a suitable amount of enrofloxacin hexahydrate is administered.


The present invention furthermore relates to pharmaceuticals which comprise the compound according to the invention, conventionally together with one or more inert non-toxic pharmaceutically acceptable adjuvants, and to their use for the abovementioned purposes.


The present invention furthermore relates to pharmaceuticals comprising the compound according to the invention and, if appropriate, one or more further active substances, in particular for the treatment and/or prophylaxis of the abovementioned diseases.


Like enrofloxacin and its salts, enrofloxacin hexahydrate, too, shows low toxicity and is active against a broad spectrum of microorganisms, including those which are resistant to a variety of antibiotics such as, for example, penicillins, cephalosporins, aminoglycosides, sulphonamides, tetracyclins. Enrofloxacin hexahydrate can be used for controlling Gram-negative and Gram-positive bacteria and bacteria-like microorganisms, and the diseases caused by these pathogens can be prevented, alleviated and/or cured. Accordingly, the hexahydrate is suitable in human and veterinary medicine for the prophylaxis and chemotherapy of local and systemic infections which are caused by these pathogens.


It is furthermore also suitable as an agent for the preservation of inorganic and organic materials, in particular organic materials of various types, for example polymers, lubricants, colours, fibres, leather, paper and wood, of foodstuffs and of water.


The hexahydrate can be used in a variety of pharmaceutical preparations. Preferred pharmaceutical preparations which may be mentioned are tablets, including sugar-coated tablets, capsules, pills, granules, suppositories, solutions, suspensions and emulsions for injection, oral solutions, suspensions and emulsions, furthermore pastes, ointments, gels, creams, lotions, powders and sprays.


Usually, a pharmaceutical formulation will, for stability reasons, contain mainly the hexahydrate of the Formula (II) and no substantial amounts of another form such as, for example, of another modification or of a solvate of the compound of the Formula (II). The pharmaceutical preferably contains more than 90 percent by weight, especially preferably more than 95 percent by weight, of the hexahydrate of the Formula (II), based on the total amount of the compound which it contains.


Enrofloxacin hexahydrate has favourable toxicity to warm-blooded species and is preferably suitable for combating bacterial diseases which occur in animal keeping and animal breeding in productive livestock, breeding stock, zoo animals, laboratory animals, experimental animals and pets. In this context, they are active against all or individual developmental stages and against resistant and normally sensitive strains. By combating the bacterial diseases, it is intended to reduce illness, deaths and reduced performance (for example in the production of meat, milk, wool, hides, eggs, honey and the like), so that, by using the active substances, more economical and simpler animal keeping is possible. The productive livestock and breeding stock include mammals such as, for example, cattle, horses, sheep, pigs, goats, camels, water buffalos, donkeys, rabbits, fallow deer, reindeer, fur-bearing animals such as, for example, mink, chinchilla, raccoon, birds such as, for example, chickens, geese, turkeys, ducks, pigeons, bird species kept on domestic premises and in zoos. They furthermore include farmed fish and ornamental fish.


The laboratory and experimental animals include mice, rats, guinea pigs, golden hamsters, dogs and cats.


The pets include dogs and cats.


In general, it has proved advantageous to administer amounts of from approximately 0.5 to approximately 50 mg, preferably 1 to 20 mg, of active substance per kg body weight per day in order to achieve effective results. The active substances can also be administered together with the animals' feed or drinking water.


Feed and foodstuffs usually contain from 0.01 to 100 ppm, preferably from 0.5 to 50 ppm, of the active substance in combination with a suitable edible material.


Such a feeding stuff and foodstuff can be used both for curative purposes and for prophylactic purposes.


Such a feeding stuff or foodstuff is prepared by mixing, with customary feeding stuffs, a concentrate or a blend which contains from 0.5 to 30% by weight, preferably from 1 to 20% by weight of an active substance in a mixture with an edible organic or inorganic carrier. Examples of edible carriers are maize meal or maize and soybean meal or mineral salts which preferably contain a small amount of an edible dust-prevention oil, for example corn oil or soya oil. The blend thus obtained can then be added to the complete feeding stuff before it is fed to the animals.


The invention furthermore relates to a process for the preparation of the hexahydrate of the Formula (II) by dissolving the compound of the Formula (I) in modification A in an inert solvent or in solvent/water mixtures and by converting the active substance into the hexahydrate of the Formula (II) by the addition of water at a temperature of between 5° C. and 25° C., preferably of from 20 to 25° C. The precipitate is isolated and dried at room temperature. This gives the hexahydrate of the Formula (II). The identity of the hexahydrate of the Formula (II) can be verified for example by X-ray diffractometry and by thermogravimetric analysis (TGA).


The invention furthermore relates to a process for the preparation of the hexahydrate of the Formula (II) by suspending the compound of the Formula (I) in modification A in water and by converting it into the hexahydrate of the Formula (II) by stirring or shaking the suspension. The residue is isolated and dried at room temperature. The identity of the hexahydrate of the Formula (II) can be verified for example by X-ray diffractometry and by thermogravimetric analysis (TGA).


Suitable inert solvents are mainly water-miscible solvents with boiling points of up to approximately 120° C. such as, for example, lower alcohols, in particular aliphatic alcohols with one hydroxyl group and 1 to 4 carbon atoms such as, for example, methanol, ethanol, isopropanol, or other volatile solvents such as, for example acetonitrile, or mixtures of the abovementioned solvents, or mixtures of the abovementioned solvents with water. Preferred are acetonitrile, methanol and isopropanol or mixtures of the abovementioned solvents or mixtures of the abovementioned solvents with water, very especially preferably ethanol or mixtures of ethanol with water.


The hexahydrate of the Formula (II) is preferably prepared by dissolving the compound of the Formula (I) in modification A in ethanol/water (1:1) or methanol and precipitating the hexahydrate by addition of water at a temperature of between 5 and 25° C., preferably at a temperature of from 20 to 25° C. The precipitate is isolated and dried. This gives the hexahydrate of the Formula (II).


The invention furthermore relates to a process for the preparation of a purified form of enrofloxacin in modification A. Here, the hexahydrate is prepared by seeding an aqueous suspension of modification A with the hexahydrate of the Formula (II), subsequently removing the solvent and converting back the hexahydrate into modification A. This last step can be effected by drying at a higher temperature, in vacuo, at low atmospheric humidity or by stirring in anhydrous solvents such as, for example, absolute ethanol.







USE EXAMPLES

The DSC and TGA thermograms were obtained using a Differential Scanning Calorimeter DSC 7 or Pyris-1 (heating rate 2 K/min, flushing with dry nitrogen) and a Thermogravimetric Analyser TGA 7 (heating rate 10 K/min, flushing with dry nitrogen) from Perkin-Elmer. The X-ray diffractograms were registered in a Stoe transmission diffractometer using CuKα radiation. The IR, FIR, NIR and Raman spectra were recorded with Fourier IR spectrometers IFS 66/IFS 66 v (IR) with 32 scans and a resolution of 2 cm−1, IFS 66v (FIR) with 100 scans and a resolution of 2 cm−1, IFS 28/N (NIR) with 15 scans and a resolution of 8 cm−1 and RFS 100 (Raman) with 64 scans and a resolution of 2 cm−1 from Bruker.


Preparation of the Hexahydrate of Enrofloxacin
Example 1

Approximately 100 mg of enrofloxacin in modification A are suspended in approximately 2 ml of water and shaken at 25° C. After 8 days, the residue is filtered off and dried at room temperature. It is analysed by X-ray diffractometry and corresponds to the title compound as hexahydrate.


Example 2

Approximately 100 mg of enrofloxacin in modification A are dissolved with heating in approximately 10 ml of acetonitrile. The solution is filtered, treated with approximately 100 ml of water and left to stand in the refrigerator. On the next day, the active substance which has precipitated is filtered off and dried at room temperature. It is analysed by thermogravimetric analysis and corresponds to the title compound as hexahydrate.


Example 3

Approximately 100 mg of enrofloxacin in modification A are dissolved with heating in approximately 10 ml of methanol. The solution is filtered and treated with approximately 10 ml of water. The solution is left to stand at room temperature until the solvent has evaporated. The residue is analysed by thermogravimetric analysis and corresponds to the title compound as hexahydrate.


Example 4

Approximately 100 mg of enrofloxacin in modification A are suspended in approximately 2 ml of isopropanol:water (1:1) and shaken at 5° C. After one week, the residue is filtered off and dried at room temperature. It is analysed by thermogravimetric analysis and corresponds to the title compound as hexahydrate.


Example 5

Approximately 4 g of enrofloxacin in modification A are suspended in approximately 80 ml of ethanol:water (1:1) and stirred at room temperature. After one week, the residue is filtered off and dried at room temperature. It is analysed by thermogravimetric analysis and corresponds to the title compound as hexahydrate.


Example 6

Approximately 500 mg of enrofloxacin in modification A are suspended in approximately 20 ml of ethanol:water (1:1) and stirred at room temperature. After 1.5 h, the suspension is seeded with the hexahydrate. After 24 h, the residue is filtered off and dried at room temperature. It is analysed by thermogravimetric analysis and corresponds to the title compound as hexahydrate.


Preparation of Modification a from Enrofloxacin Hexahydrate
Example 7

100 mg of enrofloxacin hexahydrate are dried for one hour in the drying oven at 60° C. The residue is analysed by thermogravimetric analysis and corresponds to the title compound in modification A.


Example 8

100 mg of enrofloxacin hexahydrate are suspended in approximately 2 ml of absolute ethanol and shaken at 25° C. After 24 h, the residue is filtered off and dried at room temperature. It is analysed by thermogravimetric analysis and corresponds to the title compound in modification A.


Example 9

100 mg of enrofloxacin hexahydrate are dried for 24 h at room temperature in vacuo. The residue is analysed by thermogravimetric analysis and corresponds to the title compound in modification A.


Example 10

100 mg of enrofloxacin hexahydrate are dried for 24 h at room temperature over phosphorus pentoxide. The residue is analysed by thermogravimetric analysis and corresponds to the title compound in modification A.









TABLE 1







X-ray diffractometry


Reflections [2 theta]










Modification A
Hexahydrate














7.2
6.9



8.7
7.2



9.8
8.1



12.6
9.7



13.5
11.7



14.5
13.9



14.9
14.3



15.3
14.5



16.0
14.6



16.5
14.8



17.4
14.9



17.9
15.2



18.7
15.9



19.3
16.1



19.6
17.4



21.3
18.9



21.5
19.3



21.7
19.5



22.6
20.1



23.4
20.7



24.1
21.4



24.7
21.8



25.3
22.5



25.8
22.8



26.1
23.3



26.8
24.2



27.5
24.7



28.4
24.9



29.5
25.2




25.7




26.4




27.0




27.3




27.8




30.1




30.7

















TABLE 2







IR spectroscopy


Peak maxima [cm−1]










Modification A
Hexahydrate














625
533



639
547



708
625



749
707



785
744



803
788



831
803



855
824



890
830



935
844



954
890



1023
943



1044
951



1077
1012



1090
1025



1107
1042



1124
1090



1154
1107



1186
1130



1208
1165



1221
1182



1254
1256



1289
1294



1298
1311



1313
1339



1337
1360



1381
1378



1393
1387



1401
1394



1467
1471



1508
1496



1539
1547



1611
1582



1628
1628



1737
1738



2780
3394



2826



2875



2967



3090

















TABLE 3







Raman spectroscopy


Peak maxima [cm−1]










Modification A
Hexahydrate














112
85



196
114



207
200



260
254



292
299



300
323



362
372



383
395



442
496



495
548



538
637



638
667



666
701



691
744



711
775



748
794



771
830



786
853



890
891



1026
944



1044
959



1077
1028



1125
1048



1163
1107



1186
1129



1207
1177



1218
1195



1227
1224



1254
1256



1299
1282



1327
1313



1343
1341



1349
1359



1395
1377



1437
1390



1466
1421



1536
1449



1606
1466



1624
1478



1738
1495



2828
1530



2961
1551



3012
1585



3033
1618




2970




3011




3029




3097

















TABLE 4







FIR spectroscopy


Peak maxima [cm−1]










Modification A
Hexahydrate














85
93



102
97



127
101



154
109



195
118



236
145



257
151



303
188



313
190



322
236



336
247



364
254



386
280



394
303



410
322



423
338



444
368



463
387



473
395



493
410




423




459




472




475




495

















TABLE 5







NIR spectroscopy


Peak maxima [cm−1]










Modification A
Hexahydrate







4041
4049



4087
4129



4123
4212



4192
4277



4216
4341



4254
4383



4330
4433



4390
4501



4490
4553



4543
5097



4950
5857



5236
5943



5660
5980



5792
6053



5947
6133



6039
6162



6109
6679



7165
8515



7986
8788



8433



8733










FIGURES


FIG. 1: X-ray diffractograms of enrofloxacin modification A and hexahydrate



FIG. 2: Infrared spectra of enrofloxacin modification A and hexahydrate



FIG. 3: Raman spectra of enrofloxacin modification A and hexahydrate



FIG. 4: FIR spectra of enrofloxacin modification A and hexahydrate



FIG. 5: NIR spectra of enrofloxacin modification A and hexahydrate

Claims
  • 1. An enrofloxacin hexahydrate compound, of the Formula (II)
  • 2. The compound of claim 1 which, in the X-ray diffractogram, has a reflection at a 2 theta angle of 24.2.
  • 3. The compound of claim 1 which, in the NIR spectrum, has a band at 5097 cm 1.
  • 4. A pharmaceutical composition comprising enrofloxacin hexahydrate according to claim 1.
  • 5. (canceled)
  • 6. A method of treating bacterial diseases in an animal, which comprises administering an effective amount of enrofloxacin hexahydrate to an animal in need thereof
  • 7. (canceled)
Priority Claims (1)
Number Date Country Kind
10 2007 004 732.2 Jan 2007 DE national
PCT Information
Filing Document Filing Date Country Kind 371c Date
PCT/EP08/00357 1/18/2008 WO 00 7/28/2009