GB2383038A - Anhydrous crystalline valaciclovir hydrochloride - Google Patents

Anhydrous crystalline valaciclovir hydrochloride Download PDF

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Publication number
GB2383038A
GB2383038A GB0225771A GB0225771A GB2383038A GB 2383038 A GB2383038 A GB 2383038A GB 0225771 A GB0225771 A GB 0225771A GB 0225771 A GB0225771 A GB 0225771A GB 2383038 A GB2383038 A GB 2383038A
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Prior art keywords
valaciclovir hydrochloride
anhydrous crystalline
hydrochloride
crystalline valaciclovir
anhydrous
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GB2383038B (en
GB0225771D0 (en
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Helene S Fain
David Alan Jones
Philip George Lake
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Glaxo Group Ltd
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Glaxo Group Ltd
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    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07DHETEROCYCLIC COMPOUNDS
    • C07D473/00Heterocyclic compounds containing purine ring systems
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/12Antivirals
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/12Antivirals
    • A61P31/20Antivirals for DNA viruses
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/12Antivirals
    • A61P31/20Antivirals for DNA viruses
    • A61P31/22Antivirals for DNA viruses for herpes viruses

Abstract

The invention relates to an anhydrous crystalline, form of valaciclovir hydrochloride, pharmaceutical compositions containing the same, its use against herpes viral infections and processes for preparing the same.

Description

--at 1 2383038 AN HYDROUS CRYSTAL FORM OF VALACICLOVIR HYDROCI I LORIDE
BACKGROUND OF THE INVENTION
s The present invention relates to a crystalline form of the antiviral compound valaciclovir hydrochloride, pharmaceutical formulations comprising this crystalline form, their use in therapy and processes for preparing the same.
10 The L-valine ester of acyclovir, namely (2-[(2-amino-1,6-dihydro-6-oxo9H purin-9-yl)methoxy]ethyl L-valinate, (otherwise known as valaciclovir) has been shown to possess much improved bioavailability while retaining the antiviral properties of acyclovir. A preferred form of this compound is its hydrochloride salt which is otherwise known as valaciclovir hydrochloride. The L-valinate 15 ester of acyclovir and its salts including the hydrochloride salt are disclosed in US patent no. 4,957,924, European patent no. 0308,065 and Beauchamp eta/., An vira/Chemist y and Chemotherapy 3(3):157-164 (1992), the subject matter of which is incorporated herein by reference in their entirety.
20 An anhydrous crystal form of valaciclovir hydrochloride was found and chara*erized and is described in U.S. Patent No. 6,107,302, the subject matter of which is incorporated herein by reference in its entirety. This crystal form is characterized by the X-ray powder diffraction pattern described in the '302 patent. BRIEF SUMMARY OF THE INVENTION
As a first aspect, the present invention provides anhydrous crystalline 30 valaciclovir hydrochloride characterized by substantially the same infrared (JR) absorption spectrum as Figure I, wherein the IR absorption spectrum is
obtained using a mull in mineral oil on an Ff-IR spectrometer at 2 cm i resolution. As a second aspect, the present invention provides anhydrous crystalline s valaciclovir hydrochloride characterized by an IR absorption spectrum obtained using a mull in mineral oil on an FT-IR spectrometer at 2 cm t resolution, comprising peaks at five or more positions selected from the group consisting of 3286+1, 3197+1, 1750+1, 1686+1, 1632+1, 1607+1, 1152+1, 701+1, and 688+1 cm.
As a third aspect, the present invention provides anhydrous crystalline vaiaciclovir hydrochloride characterized by substantially the same X-ray powder diffraction (XRD) pattern as Figure 2, wherein the XRD pattern is expressed in terms of 2 theta angles and obtained with a diffractometer 15 equipped with a diffracted beam graphite monochromator using copper Ka X radiation. As a fourth aspect, the present invention provides anhydrous crystalline valaciclovir hydrochloride characterized by an XRD pattern expressed in terms 20 of 2 theta angles and obtained with a diffractometer equipped with a diffracted beam graphite monochromator using copper Ka X-radiation, wherein the XRD pattern comprises 2 theta angles at four or more positions selected from the group consisting of 6. 7 +0.1, 8.1 +0.1, 9.3 +0.1, 11.4 +0.1, 13.9+0.1, 15.7+0.1, 16.3+0.1, and 17.1+0.1 degrees.
As a fifth aspect, the present invention provides anhydrous crystalline valaciclovir hydrochloride characterized by an XRD pattern expressed in terms of 2 theta angles and obtained with a diffractometer equipped with a diffracted beam graphite monochromator using copper Ka X-radiation, 30 wherein the XRD pattern comprises 2 theta angles 6.7 +0.1, 8.1 +0.1, 9.3 + 0.1, and 11.4 +0.1 degrees
As a sixth aspect, the present invention provides anhydrous crystalline valaciclovir hydrochloride characterized by substantially the same Raman spectrum as Figure 3, wherein the Raman spectrum is obtained using a Ff-
Raman spectrometer at 4 cm t resolution.
As a seventh aspect, the present invention provides anhydrous crystalline valaciclovir hydrochloride characterized by a Raman spectrum obtained using a FT-Raman spectrometer at 4 cm i resolution, wherein the Raman spectrum 10 comprises at least four peaks selected from the group consisting of 1684+1, 1364il,1348il,1191+l, and 810+1 cm-1.
As an eighth aspect, the present invention provides anNydrous crystalline valaciclovir hydrochloride characterized by substantially the same solid state 15 nuclear magnetic resonance (NMR) spectrum as Figure 4, wherein the solid state NMR is obtained on a spectrometer operating at a frequency of 90.55MHz for t3C observation at a temperature of 300K, a spinning speed 10kHz and a recycle delay of 15 seconds.
20 As a ninth aspect, the present invention provides anhydrous crystalline valaciclovir hydrochloride characterized by a solid state NMR spectrum obtained using a spectrometer operating at a frequency of 90. 55MHz for t3C observation at a temperature of 300K, a spinning speed of 10kHz and a recycle delay of 15 seconds, wherein the solid state NMR comprises chemical 2s shifts at 15.1+0.1, 17.2iO.1, 20.2+0.1, 20.9+O.1, 29.2+0.1, 29.9iO.1, 58.4+O.1, 64.6+O.1, 66.8+O.1, 69.3iO.1, 70.7+0.1, 73. 9iO.1, 74.4+O.1, 116.6iO.1, 117.3iO.1, 140.4+0.1, 150.4iO.1, 151.3+O.1, 153.6+0.1, 158.3iO.1, 169.1+0.1 and 169.6+0.1 ppm 30 As another aspect, the present invention provides a pharmaceutical composition comprising anhydrous crystalline valaciclovir hydrochloride
according to the present invention. The pharmaceutical composition may further comprise one or more pharmaceutically acceptable carriers or diluents.
As another aspect, the present invention provides a composition comprising 5 anhydrous crystalline valaciclovir hydrochloride according to the present invention and hydrated valaciclovir hydrochloride.
As another aspect, the present invention provides a composition comprising anhydrous crystalline valaciclovir hydrochloride according to the present 10 invention and Form valaciclovir hydrochloride.
As another aspe*, the present invention provides a method for the treatment or prophylaxis of a herpes viral infection in a mammal comprising administering to the mammal, an effective amount of anhydrous crystalline 15 valaciclovir hydrochloride according to the present invention.
As another aspect, the present invention provides a method for the treatment or prophylaxis of a condition or disease associated with a herpes viral Infection in a mammal, comprising administering to the mammal an effe*ive 20 amount of anhydrous crystalline valaciclovir hydrochloride according to the present invention.
As another aspect, the present invention provides anhydrous crystalline valaciclovir hydrochloride according to the present invention for use in 25 therapy. For example, the anhydrous crystalline valaciclovir hydrochloride can be for use in the treatment or prophylaxis of a herpes viral infection, for example in a mammal such as a human.
As another aspect, the present invention provides the use of anhydrous 30 crystalline valaciclovir hydrochloride according to the present invention in the
s preparation of a rr edicament-fOr the treatment or prophylaxis of a herpes viral infection, for exampiein a mammal such as a human.
The herpes viral infection may be selected from the group consisting of s herpes simplex virus i, herpes simplex virus 2, cytomegalovirus, Epstein Barr virus, varicella zoster virus, human herpes virus 6, human herpes virus 7, and human herpes virus 8.
As another aspect, the present invention provides the use of anhydrous 10 crystalline valaciclovir hydrochloride according to the present invention in the preparation of a medicament for the treatment or prophylaxis of a condition or disease associated with a herpes viral infection, for example in a mammal such as a human.
15 As another aspect, the present invention provides a process for preparing anhydrous crystalline valaciclovir hydrochloride according to the present invention comprising slurrying damp valaciclovir hydrochloride or hydrated valaciclovir hydrochloride in a solvent capable of removing water by azeotropic distillation, under azeotropic distillation conditions.
As another aspect, the present invention provides another process for preparing anhydrous crystalline valaciclovir hydrochloride according to the present invention comprising the steps of: a) optionally removing unbound process solvent from damp 25 valaciclovir hydrochloride to provide hydrated valaciclovir hydrochloride; b) slurrying damp valaciclovir hydrochloride or hydrated valaciclovir hydrochloride in a solvent capable of removing water by azeotropic distillation, under azeotropic distillation conditions to prepare the anhydrous crystalline valaciclovir hydrochloride; and 30 c) isolating the anhydrous crystalline valaciclovir hydrochloride.
:- 6
As another aspe*, the present invention provides a process for preparing anhydrous crystalline valaciclovir hydrochloride according to the present invention comprising the steps of: a) removing unbound process solvent from damp valaciclovir 5 hydrochloride to provide hydrated valaciclovir hydrochloride; - b) slurrying hydrated valaciclovir hydrochloride in an anKydrous solvent at a temperature of from about ambient temperature to about the boiling point of the anhydrous solvent for a period of time sufficient to convert the hydrated valaciclovir hydrochloride to the anhydrous crystalline 10 valaciclovir hydrochloride; and c) isolating the anhydrous crystalline valaciclovir hydrochloride.
BRIEF DESCRIPTION OF THE SEVERAL VIEWS OF THE DRAWINGS
Figure 1. The IR absorption spectrum of the anhydrous crystal form of valaciclovir hydrochloride according to the present invention ( 'Form 2 valaciclovir hydrochloride"). The x-axis is wavenumber in cm i and the yaxis is percent transmittance. The IR absorption spectrum is obtained using a 20 mull in mineral oil on an FT-IR spectrometer at 2cm t resolution according to the procedures described herein.
Figure 2. The XRD pattern of Form 2 valaciclovir hydrochloride according to the present invention. The XRD pattern is expressed in terms of 2 theta 25 angles and obtained with a diffractometer equipped with a diffracted beam graphite monochromator using copper Ka X-radiation, according to the procedures described herein.
Figure 3. The Raman spectrum of Form 2 valaciclovir hydrochloride 30 according to the present invention. The Raman spectrum is obtained using a Fr-Raman spectrometer at 4 cm-1 resolution and 400mW power, with a
minimum of 600 scans accumulation, a InGaAs detector, and a CaF2 beamsplitter, according to the procedures described herein.
Figure 4. The solid state NMR spectrum of Form 2 valaciclovir hydrochloride 5 according to the present invention. The solid state NMR spectrum is obtained on a spectrometer operating at a frequency of 90. 55MHz for t3C observation at a temperature of 300K, a spinffing speed of 10kHz and a recycle delay of 15 seconds, according to the'procedures described herein.
- D Figure S. The differential scanning calorimetry (DSC) thermogram for Form 2 valaciclovir hydroc>hlorid according to the present invention. The DSC was carried out on a Perldn-61 tiler Pyris-'1 DCS system at a scan rate of 10 C per minute, using a sample size of 2.789mg, according to the procedures described herein.
Figure 6. The thermogravimetric analysis (TGA) of Form 2 valaciclovir hydrochloride according to the present invention. The TGA was carried out on a Perkin-Elmer Pyris-1 TGA system at a scan rate of 10 C per minute, using a sample size of 3.757mg, according to the procedures described 20 herein.
Figure 7. The IR spectrum of valaciclovir hydrochloride according to U.S. Patent No. 6,107,302 ( 'Form 1 valaciclovir hydrochloride']. The IR absorption spectrum is obtained using a mull in mineral oil on an FT-IR 2s spectrometer at 2cm t resolution according to the procedures described in the Comparative Example.
Figure 8. The solid stateNMR spectrum of Form 1 valaciclovir hydrochloride.
The solid state NMR spectrum is obtained on a spectrometer operating at a frequency of 90.55MHz for t3C observation at a temperature of 300K, a 30 spinning speed of 10kHz and a recycle delay of 15 seconds, according to the procedures described in the Comparative Example.
Figure 9. The IR spectrum of hydrated valaciclovir hydrochloride. The IR absorption spectrum is obtained using a mull in mineral oil on an FT-IR spectrometer at Acme resolution according to the procedures described in the s Comparative Example.
Figure 10. The solid state NMR spectrum of hydrated vaiaciclovir hydrochloride. The solid state NMR spectrum is obtained on a spectrometer operating at a frequency of 90.55MHz for t3C observation at a temperature of 10 300K, a spinning speed of 10kHz and a recycle delay of 15 seconds, according to the procedures described in the Comparative Example.
DETAILED DESCRIPTION OF THE INVENTION
The present invention provides a novel anhydrous crystalline form of valaciclovir hydrochloride exhibiting one or more advantageous pharmaceutical properties or other advantages over hydrated and other anhydrous crystal forms of valaciclovir hydrochloride. The anhydrous crystal form of the present 20 invention possesses as one distinct advantage, that it can be prepared by processes which are simpler and more economical, particularly on a commercial scale, than other forms of valaciclovir hydrochloride. Unit operations such as filtration and drying add greatly to the cost of a pharmaceutical product on large scale production. The particles of the anhydrous crystal form of the 25 present invention are more easily dried and filtered allowing downstream processing advantages and/or cost of goods advantages. The processes for the preparation of the anhydrous crystal form of the present invention also show a high degree of robustness, an advantage for a highly regulated compound.
Batches of this crystalline form can, by the processes of this invention, be made 30 consistently to a high crystal form purity i.e., where the proportion of hydrated and other anhydrous crystalline forms of valaciclovir hydrochloride is limited
f 9 (particularly less than 10%, more particularly less than 5% and still more particularly less than 3%). As another advantage, the anhydrous crystal form of the present invention is stable and essentially nonhygroscopic. It also has good storage properties and can be readily formulated into pharmaceutical 5 compositions such as tablets and capsules.
As another one of its advantages, the anhydrous crystal form of the present invention is in the form a more powdery material than Form valaciclovir hydrochloride. This advantage reduces or eliminates the need for a pre 10 grinding stage to reduce larger, harder pellets into finer, more powdery material for formulating.
The various forms of valaciclovir hydrochloride may be characterized and differentiated using a number of conventional analytical techniques, including 15 but not limited to X-ray powder diffraction (XRD) patterns, infrared (JR) spectra, Raman spectra, differential scanning calorimetry (DSC), thermogravimetric analysis (TGA) and solid state NMR.
"Form 2 valaciclovir hydrochloride" as used herein refers to any of: I) an 20 anhydrous crystalline form of valaciclovir hydrochloride having substantially the same IR spectrum as shown in Figure 1, obtained using a mull in mineral oil on an Fr-IR spectrometer at 2 cm resolution; 2) an anhydrous crystalline form of valaciclovir hydrochloride having substantially the same XRD pattern as shown in Figure 2 when measured with a properly aligned diffractometer 25 equipped with a diffracted beam graphite monochromator using copper Kcc X-
radiation; 3) an anhydrous crystalline form of valaciclovir hydrochloride having substantially the same Raman spectrum as shown in Figure 3, obtained using a FF-Raman spectrometer at 4 cm i resolution; or 4) an anhydrous crystalline form of valaciclovir hydrochloride having substantially 30 the same solid state NOR spectra a shown in Figure 4, obtained on a spectrometer operating at a frequency of 90.55MHz for t3C observation at a
/ temperature of 300K, a spinning speed 10kHz and a recycle delay of 15 seconds. "Form 1 valaciclovir hydrochloride" as used herein shall refer to the anhydrous s crystalline valaciclovir hydrochloride described in U. S. Patent No. 6,107,302, having the identifying characteristics described therein.
"Hydrated valaciclovir hydrochloride" as used herein shall refer to any hydrated form of valaciclovir hydrochloride, including valaciclovir 10 hydrochloride monohydrate, valaciclovir hydrochloride dihydrate and mixtures thereof. "Damp valaciclovir hydrochloride" as used herein shall refer to the hydrated valaciclovir hydrochloride in the presence of process solvent.
"Process solvent" as used herein shall refer to any solvent employed for the preparation of valaciclovir hydrochloride, such as by recrystallization, by slurry, by the processes described in either U.S. Patent No. 4,957,924 or 6,107,302, or by any other suitable synthesis method.
The IR spectrum of the anhydrous crystalline form of valaciclovir hydrochloride according to the present invention (i.e., Form 2 valaciclovir hydrochloride) can be determined using conventional equipment and techniques known to those skilled in the art of analytical chemistry and 25 physical characterization. The IR spectra of Figures 1, 7, and 9 were obtained with a Perkin-Elmer System 2000 FT-IR spectrometer at 2 cm-1 resolution. The wavenumber in cm t (x-axis) is plotted against percent transmittance (y-axis). All samples were prepared as a mull in mineral oil.
Representative peaks observed in the IR spectrum of Form 2 valaciclovir 30 hydrochloride as a mull in mineral oil are as follows: 3286+1, 3197+1, 1750+1, 1686+1, 1632+1, 1607+1, 1572+1, 1533+1, 1463+1, 1394+1,
1377+1, 1365+1, 1341+1, 1298+1, 1258+1, 1247+1, 1224+1, 1191+1,
1152+1, 1132+1, 1096+1, 1042+1, 1017+1, 868+1, 830+1, 778+1, 759+1,
729+1, 701+1, 688+1 and 631+1 cm.
5 As will be apparent to those skilled in the art, not all of these peaks are necessary to conclusively identify an analyzed sample as Form 2 valaciclovir hydrochloride. Form 2 valaciclovir hydrochloride can be identified by the presence of peaks at 5 or more positions selected form the group consisting of 3286+1, 3197+1, 1750+1, 1686+1, 1632+1, 1607+1, 1152+1, 701+1, and 10 688+1 Amy. More particularly, at least 7 of these peaks are present and in one embodiment, all of the foregoing peaks are present.
Slight variations in observed peaks are expected based on the specific spectrometer employed and the analyst's sample preparation technique.
15 Some margin of error is present in each of the peak assignments reported above. The margin of error in the foregoing peak assignments is approximately +1 cm t Since some margin of error is possible in the peak assignments, a useful 20 method of comparing IR spectra in order to identify the particular form of a sample of valaciclovir hydrochloride is to overlay the IR spectrum of the sample over the IR spectrum of each of the known forms. For example, one skilled in the art can overlay an IR spectrum of an unknown form of valaciclovir hydrochloride, obtained using the methods described herein, over 25 Figure 1 and, using expertise and knowledge in the art, readily determine whether the IR spectrum of the unknown sample is substantially the same as the IR spectrum of Form 2 valaciclovir hydrochloride. If the IR spectrum is substantially the same as Figure 1, the previously unknown form can be readily and accurately identified as Form 2 valaciclovir hydrochloride.
30 Figures 7 and 9 can be used in the same manner to determine whether the
sample is Form 1 valaciclovir hydrochloride or hydrated valaciclovir hydrochloride, respectively.
The X-ray powder diffraction pattern of Form 2 valaciclovir hydrochloride can s be determined using conventional techniques and equipment known to those skilled in the art of analytical chemistry and physical characterization. The diffraction pattern of Figure 2 was obtained with a Philips X-Pert Pro diffractometer system equipped with a diffracted beam graphite monochromator using copper Ka X-radiation and an automated divergent slit.
10 A xenon proportional counter was used as the detector. The powder sample used to generate the X-ray powder diffraction data was prepared by conventional back filled sample preparation techniques using a 10 mm diameter holder about 1.5 mm thick.
15 A powder sample of Form 2 valaciclovir hydrochloride was used to produce the XRD pattern of Figure 2. 2 Theta angles in degrees (x-axis) is plotted again* peak intensity in terms of the count rate per seconds (y-axis). The XRD pattern for each anhydrous crystalline form and hydrated valaciclovir hydrochloride is unique to the particular form; exhibiting a unique set of 20 diffraction peaks which can be expressed in 2 theta angles (a), d-spacings (A) and/or relative peak intensities.
2 Theta diffraction angles and corresponding d-spacing values account for positions of various peaks in the XRD pattern. D-spacing values are 25 calculated with observed 2 theta angles and copper Koc1 wavelength using the Bragg equation. Slight variations in observed 2 theta angles and dspacings are expected based on the specific diffractometer employed and the analyst's sample preparation technique. More variation is expected for the relative peak intensities. Identification of the exe* crystal form of a compound 30 should be based primarily on observed 2 theta angles or d-spacings with lesser importance place on relative peak intensities. To identify Form 2
valaciclovir hydrochloride, the certain characteristic 2 theta angle peaks occur at 6.7+0.1, 8.1+0.1, 9.3+0.1, and 11.4+0.1 degrees, or 24.63, 13.17, 10.88 and 9.52' d-spacing.
5 Although one skilled in the art can identify Form 2 valaciclovir hydrochloride from these characteristic 2 theta angle peaks, in some circumstances it may be desirable to rely upon additional 2 theta angles or d-spacings for the identification of Form 2 valaciclovir hydrochloride. In one embodiment at least five, particularly seven and more particularly all, of the following 2 theta 10 angles are employed to identify Form 2 valaciclovir hydrochloride: 6.7 +0.1, 8.1 +0.1, 9.3 +0.1, 11.4 +0.1, 13.9+0.1, 15.7+0.1, 16.3+0.1, and 17.1+0.1 degrees Form 2 valaciclovir hydrochloride typically exhibits 2 theta angle peaks in 15 addition to the foregoing peaks. For example, Form 2 valaciclovir hydrochloride may exhibit 2 theta angle peaks at essentially the following positions: 6.7+0.1, 8.1+0.1, 9.3+0.1, 11.4+0.1, 13.3+0.1, 13.9+ 0.1, 15.4+0.1, 15.7+0.1, 16.3+0.1, 17.1+0.1, 18.6+0.1, 19.0+0.1, 19.3+0.1, 19.8+0.1,
20.6+0.1, 21.4+0.1, 22.6+0.1, 22.9+0.1, 24.2+0.1, 25.5+0.1, 26.4+0.1,
20 27.2+0.1, 27.5+0.1, 27.8+0.1, 28.0+0.1, 28.9+0.1, 30.2+0.1, 30.9+0.1,
31.9+0.1, 32.6+0.1, 34.9+0.1, 35.3+0.1 and 35.9+0.1 degrees, or about 24. 63, 13.17, 10.88, 9.52, 7.75, 7.27, 6.63, 6.36, 6.25, 6.07, 5.73, 5.62,
5.44, 5.18, 4.77, 4.67, 4.59, 4.49, 4.42, 4.30, 4.15, 3.94, 3.88, 3.67, 3. 49,
3.38, 3.28, 3.24, 3.20, 3.18, 3.09, 3.04, 2.96, 2.89, 2.81, 2.74, 2.57, 2. 54,
2s 2.50, 2.43, 2.30, 2.21, 2.15 and 2.10 A d-spacing.
Some margin of error is present in each of the 2 theta angle assignments and d-spacings reported above. The error in determining d-spacings decreases with increasing diffraction scan angle or decreasing d-spacing. The margin of error in the foregoing 2 theta angles is approximately +0.1 degrees for each 30 of the foregoing peak assignments.
Since some margin of error is possible in the assignment of 2 theta angles and d-spacings, the preferred method of comparing XRD patterns in order to identify a the particular form of a sample of valaciclovir hydrochloride is to overlay the XRD pattern of the unknown sample over the XRD pattern of a 5 known form. For example, one skilled in the art can overlay an XRD pattern of an unknown sample of valaciclovir hydrochloride, obtained using the methods described herein, over Figure 2 and, using expertise and knowledge in the art, readily determine whether the XRD pattern of the unknown sample is substantially the same as the XRD pattern of Form 2 valaciclovir 10 hydrochloride. If the XRD pattern is substantially the same as Figure 2, the previously unknown form can be readily and accurately identified as Form 2 valaciclovir hydrochloride. The same technique can be used to determine if the unknown sample is Form 1 valaciclovir hydrochloride by overlaying the XRD pattern over Figures 1, 2 or 3 of U.S. Patent No. 6,107,302.
Although 2 theta angles or d-spacings are the primary method of identifying a particular crystalline form, it may be desirable to also compare relative peak intensities. As noted above, relative peak intensities may vary depending upon the specific diffractometer employed and the analyst's sample 20 preparation technique. The peak intensities are reported as intensities relative to the peak intensity of the strongest peak. The intensity units on the XRD are counts/sec. The absolute counts = counts/time x count time = counts/sec x 10 sec.
25 Considering 2 theta angles, d-spacing (a) and relative peak intensity (I), Form 2 valaciclovir hydrochloride exhibits the following XRD pattern characteristics:
Form 2 Valaciclovir Hydrochloride 2 theta angle I (o)1 3.6 24.63 0.2
6.7 13.17 75.6
8.! 10.88 5.2
9.3 9.52 100.0
11.4 7.75 28.3
12.2 7.27 2.5
13.3 6.63 11.2
13.9 6.36 16.9
14.2 6.25 8.7
14.6 6.07 7.0
15.5 5.73 22.1
15.8 5.62 40.8
16.3 5.44 18.5
17.1 5.18 48.4
18.6 4.77 13.6
19.0 4.67 26.5
19.3 4.59 17.1
19.8 4.49 16.1
20.1 4.42 9.8
20.6 4.30 11.3
21.4 4.15 50.0
22.6 3.94 18.9
22.9 3.88 34.1
24.2 3.67 23.7
25.5 3.49 18.8
26.4 3.38 49.7
27.2 3.28 32.0
Form 2 Valaciclovir Hydrochloride A 2 theta angle I (o) 27.5 3.24 50.9
27.8 3.20 46.9
28.0 3.18 52.0
28.9 3.09 14.9
29.3 3.04 6.4
30.2 2.96 11.8
31.0 2.89 18.8
31.9 2.81 13.5
32.7 2.74 12.0
34.9 2.57 14.4
35.3 2.54 14.5
35.9 2.50 10.3
37.0 2.43 3.2
39.1 2.30 3.2
40.7 2.21 5.2
41.9 2.15 4.8
43.1 2.10 7.3
Margin of error = approx. +0.1 degrees.
Based upon the foregoing characteristic features of the XRD pattern of Form 2 valaciclovir hydrochloride, one skilled in the art can readily identify Form 2 5 valaciclovir hydrochloride. It will be appreciated by those skilled in the art that the XRD pattern of a sample of Form 2 valaciclovir hydrochloride, obtained using the methods described herein, may exhibit additional peaks.
The foregoing table provides the most intense peaks which are characteristic of that particular crystalline form or solvate. This table does not represent an 10 exhaustive list of peaks exhibited by Form 2 vaiaciclovir hydrochloride.
Raman spectroscopy is another useful analytical technique for identifying the physical characteristics of a sample of valaciclovir hydrochloride and distinguishing between Form 2 valaciclovir hydrochloride, Form valaciclovir hydrochloride and hydrated valaciclovir hydrochloride. The Raman spectrum 5 of the anhydrous crystalline form of valaciclovir hydrochloride according to the present invention (i.e., Form 2 valaciclovir hydrochloride) can be determined using conventional equipment and techniques known to those skilled in the art of analytical chemistry and physical characterization. The Raman spectrum of Figure 3 was obtained using a N col.960 E.S.P. -Reman 10 spectrometer. Data were acquired at 4 cram resolution. Laser excitation was at 1064 rim (as is inherent by the use of an FT-Raman spectrometer) with a power of 400 mW and a minimum of 600 scans accumulation. The number of sample scans was 1200 using an InGaAs detector and CaF2 beasmsplitter.
Samples were prepared by placing the solid sample as received irTto a glass 15 NOR tube. The sample was rotated during the measurement. In Figure 3, Raman shift in cm-t (x-axis) is plotted against Raman intensity (y-axis).
The power (mW) and minimum number of scans accumulation may be adjusted within conventional knowledge to provide a spectrum of similar 20 qualityto that provided in Figure 3. For example, if a higher power is employed, a lower number of minimum scans accumulation may be required to achieve a spectrum of similar quality to that reported in Figure 3.
Similarly, if a lower power is employed, a higher number of minimum scans accumulation may be required to obtain a spectrum of similar quality.
25 Preferably, when determining whether the Raman spe*rumof an unknown sample of valaciclovir hydrochloride is Form 2 valaciclovir hydrochloride, the spectrum will be obtained using a power of 400 mW and a minimum of 600 scans accumulation.
so The choice of detector is not believed to be critical to obtaining a spectrum suitable for comparison with that provided at Figure 3. As is known to those
skilled in the art, a different detector will likely affect the intensity of the peaks. However, peak positions should remain relatively the same. For a definitive comparison, when determining whether the Raman spectrumof an unknown form of valaciclovir hydrochloride is Form 2 valaciclovir 5 hydrochloride, preferably the spectrum will be obtained using an InGaAs detector. Certain main peaks observed in the Raman spectrum of Form 2 valaciclovir hydrochloride as using an FT-Raman spectrometer at a resolution of 4 cm-1 10 are as follows: 3285+1, 3201+1, 3114+1, 3003+1, 2960+1, 2931+1, 2894+1, 1749+1, 1684+1, 1630+1, 1568+1, 1477+1, 1449+1, 1416+1, 1397+1,
1364+1, 1348+1, 1310+1, 1226+1, 1191+1, 1133+1, 1070+1, 1039+1,
1014+1, 966+1, 902+1, 869+1, 850+1, 832+1, 810+1, 784 1, 760+1, 687+1,
646+1, 630+1, 527+1, 500+1, 364+1, 324+1, 278+1, 191+1, 120+1, 91+1 and 15 78+1 cm 1 As will be apparent to those skilled in the art, not all of these peaks are necessary to conclusively identify an analyzed sample as Form 2 valaciclovir hydrochloride. Form 2 valdciclovir hydrochloride can be identified by the 20 presence of peaks at 5 or more positions noted above. More particularly, at least 7 of these peaks are present and in one embodiment, all of the foregoing peaks are present. The most characteristic peaks of the Raman spectrum of Form 2 valaciclovir hydrochloride obtained using the foregoing methods, are at 1684+1, 1364+1, 1348+1, 1191+1, and 810+1cm-1.
Slight variations in observed peaks are expected based on the specific spectrometer employed, the resolution of the data and the analyst's sample preparation technique. Some margin of error is present in each of the peak assignments reported above. The margin of error in the foregoing peak 30 assignments is approximately +1 cm i
F Since some margin of error is possible in the peak assignments, the preferred method of determining whether an unknown form of valaciclovir hydrochloride is Form 2 valaciclovir hydrochloride is to overlay the Raman spectrum of the sample over the Raman spectrum provided in Figure 3. One 5 skilled in the art can overlay a Raman spectrum of an unknown form of valaciclovir hydrochloride, obtained using the methods described herein, over Figure 3 and, using expertise and knowledge in the art, readily determine whether the Raman spectrum of the unknown sample is substantially the same as the Raman spectrum of Form 2 valaciclovir hydrochloride.
Solid state nuclear magnetic resonance (NMR) is yet another conventional analytical technique for identifying the physical characteristics of a sample of valaciclovir hydrochloride and distinguishing between Form 2 valaciclovir hydrochloride, Form valaciclovir hydrochloride and hydrated valaciclovir 15 hydrochloride. The solid state NMR spectra of each form of valaciclovir hydrochloride is unique. The solid state NMR spectrum of the anhydrous crystalline form of valaciclovir hydrochloride according to the present invention (i.e., Form 2 valaciclovir hydrochloride) is determined using conventional Equipment and techniques known to those skilled in (hWart of 20 analytical chemistry and physical characterization. The solid state NMR spectrum of Figures 4, 8 and SO were obtained on a Bruker AMX360 spectrometer, operating at a frequency of 90.55MHz for t3C observation at 300 K (i.e., ambient temperature) a spinning speed of 10kHz and a recycle delay of 15 seconds. t3C ME spectra are acquired by cross-polarisation from 25 Hartmann-Hahn matched proton. 4k data points were acquired in 60ms, using a contact time of 3 ms and a recycle time of 15 s. Protons were decoupled during acquisition by using a two-pulse phase modulated (TPPM) composite sequence. The free induction decay (rid) was apodised by exponential multiplication using 5Hz of line broadening before Fourier 30 transformation into 32k data points. Chemical shifts were externally referenced to the carboxylate signal of glycine at 176.4 ppm relative to
tetramethyl silane (TMS). Samples were prepared by placing the solid sample into a glass NMR tube. Chemical shift in ppm (x-axis) is plotted against intensity (y-axis).
5 Certain characteristic chemical shifts observed in the solid state NMR spectrum of Form 2 valaciclovir hydrochloride using a spectrometer operating at a frequency of 90.55MHz for i3C observation at a temperature of 300K, a spinning speed 10kHz and a recycle delay of 15 seconds include the following: 15. +0.1, 17.2+0.1, 20.2+0.1, 20.9+0.1, 29.2+0.1, 29.9+0.1, 10 58.4+0.1, 64.6+0.l, 66.8+0.1, 69.3+0.l, 70.7+0.1, 73.9+0.l, 74.4+0.1, 116.6+0.1, 117.3+0.1, 140.4+0.1, 150.4+0.1, 151.3+0.1, 153.6+0.1,
158.3+0.1, 169.1+0.1 and 169.6+0.1 ppm Slight variations in observed chemical shifts are expected based on the 15 specific spectrometer employed and the analyst's sample preparation technique. Some margin of error is present in each of the chemical shifts reported above. The margin of error in the foregoing chemical shifts is approximately +0.1 ppm 20 Since some margin of error is possible in the assignment of chemical shifts, the preferred method of determining whether an unknown form of valaciclovir hydrochloride is Form 2 valaciclovir hydrochloride is to overlay the solid state NMR spectrum of the sample over the solid state NMR spectrum provided in Figure 4. One skilled in the art can overlay an NMR spectrum of an unknown 25 sample of valaciclovir hydrochloride, obtained using the methods described herein, over Figure 4 and, using expertise and knowledge in the art, readily determine whether the NMR spectrum of the unknown sample is substantially the same as the NMR spectrum of Form 2 valaciclovir hydrochloride. The same technique may be employed using Figures 8 and SO to determine 30 whether a particular sample is Form 1 valaciclovir hydrochloride or hydrated valaciclovir hydrochloride, respectively.
Any of the foregoing analytical techniques can be used alone or in combination to identify a particular form of valaciclovir hydrochloride. In addition, other methods of physical characterization can also be employed to 5 identify and characterize Form 2 valaciclovir hydrochloride. Examples of suitable techniques which are known to those skilled in the art to be useful for the physical characterization or identification of a crystalline form or solvate include but are not limited to melting point, differential scanning calorimetry, and thermogravimetric analysis. These techniques may be lo employed alone or in combination with other techniques to characterize a sample of an unknown form of valaciclovir hydrochloride, and to distinguish Form 2 valaciclovir hydrochloride from Form 1 and hydrated valaciclovir hydrochloride. 15 The present invention includes Form 2 valaciclovir hydrochloride both in substantially pure form and in admixture with other forms of valaciclovir hydrochloride; particularly one or both of hydrated valaciclovir hydrochloride and Form valaciclovir hydrochloride. By "substantially pure" is meant that the composition comprises at least 90 percent Form 2 valaciclovir 20 hydrochloride as compared to the other forms of valaciclovir hydrochloride in the composition, more particularly at least 95 percent Form 2 and in one embodiment, at least 97 percent Form 2 valaciclovir hydrochloride.
Form 2 valaciclovir hydrochloride may be in admixture with one or both of 25 Form valaciclovir hydrochloride or hydrated valaciclovir hydrochloride.
Additionally, Form 2 may be in admixture with damp valaciclovir hydrochloride. Since Form 2 valaciclovir hydrochloride is essentially free of water of 30 hydration, the proportion of hydrated valaciclovir hydrochloride in any batch may be measured by the overall water of hydration content of each batch. In
another aspect of the invention there is provided valaciclovir hydrochloride (either Form 2 valaciclovir hydrochloride or an admixture of Form 1 and Form 2 valaciclovir hydrochloride) having a water of hydration content of not more than 3% by weight (w/w) and including one or more of the characterizing s data described above. More particularly, the water of hydration content is not more than 2% w/w, and in one embodiment, it is not more than 1.5% w/w and in still another embodiment, it is not more than 1% w/w and in yet another embodiment, it is not more than 0.7% w/w.
10 The water of hydration content is measured by the Karl Fischer method which is well known in the art and is described in the 1990 US Pharmacopoeia at pages 1619-1621, and the European Pharmacopoeia, second edition (1992) part 2, sixteenth fascicule at v. 3.5-6.1.
15 The present invention expressly contemplates the foregoing mixtures of Form 2 valaciclovir hydrochloride with one or more of Form valaciclovir hydrochloride and hydrated valaciclovir hydrochloride. Admixtures of Form 2 valaciclovir hydrochloride with another form of the compound may result in the masking or absence of one or more of the foregoing X-ray powder 20 diffraction peaks and Raman spectrum described above for Form 2 valaciclovir hydrochloride. Methods are known in the art for analyzing such admixtures of forms in order to provide for the accurate identification of the presence or absence of particular form in the admixture. Suitable methods for the quantitation of the particular forms in a mixture are well known in the art, 25 e.g. IR, Raman, SSNMR, Near IR (NIR).
In another aspect, the present invention provides pharmaceutical compositions comprising Form 2 valaciclovir hydrochloride. Such pharmaceutical compositions may further comprise one or more other forms 30 of valaciclovir hydrochloride and/or one or more pharmaceutically acceptable carriers or diluents. Examples of suitable pharmaceutical compositions and
methods for their preparation are described in U.S. Patent Nos. 4,957,924, 5,879,706, European patent EP 0 806 943 Bat, and PCT Publication No. WO01/82905, the subject matter of which is incorporated herein by reference in their entirety. Conveniently, suitable pharmaceutical compositions can be prepared using conventional techniques, and when employed, carriers and diluents. Pharmaceutical compositions for oral administration, such as tablet (and caplet) and capsule formulations, are preferred.
Form 2 valaciclovir hydrochloride for use in the instant invention may be used 10 in combination with other therapeutic agents. Similarly, the pharmaceutical formulations of the present invention may include one or more additional therapeutic agents. Other therapeutic agents that may be combined with Form 2 valaciclovir hydrochloride include for example, nonnucleotide reverse transcriptase inhibitors, nucleoside reverse transcriptase inhibitors, protease 15 inhibitors and/or other antiviral agents. The invention thus provides in a further aspe* the use of a combination comprising Form 2 valaciclovir hydrochloride with a further therapeutic agent in the treatment of viral infections. Particular antiviral agents which may be combined with the compounds of the present invention include acyclovir, famcyclovir, 20 gancyclovir, docosanol, miribavir, amprenavir, lamivudine, zidovudine, and abacavir. When the compounds of formula (I) are used in combination with other therapeutic agents, the compounds may be administered either sequentially 25 or simultaneously by any convenient route.
The combinations referred to above may conveniently be presented for use in the form of a pharmaceutical formulation and thus pharmaceutical formulations comprising a combination as defined above optionally together 30 with a pharmaceutically acceptable carrier or diluent comprise a further aspec* of the invention. The individual components of such combinations
? 24 may be administered either sequentially or simultaneously in separate or combined pharmaceutical formulations.
When combined in the same formulation it will be appreciated that the two s compounds must be stable and compatible with each other and the other components of the formulation and may be formulated for administration.
When formulated separately they may be provided in any convenient formulation, in such a manner as is known for such compounds in the art.
10 When Form 2 valaciclovir hydrochloride is used in combination with a second therapeutic agent, the dose of each compound may differ from that when the compounds are used alone. Appropriate doses will be readily appreciated by those skilled in the art.
15 Form 2 valaciclovir hydrochloride and pharmaceutical compositions comprising the same are useful in therapy, particularly in the treatment or prophylaxis, including suppression of recurrence of symptoms, of a viral disease, in an animal, e.g. a mammal such as a human. The various therapeutic uses disclosed in U.S. Patent Nos. 4,957,924, and 5,879,706 and 20 PCf Publication no. WO 97/25989, the subject matter of which is incorporated herein by reference in their entirety, are similarly applicable to Form 2 valaciclovir hydrochloride. Form 2 valaciclovir hydrochloride is especially useful for the treatment or prophylaxis of viral diseases such as herpes viral infections. Herpes viral infections include, for example, herpes simplex virus 25 1 (HSV-1), herpes simplex virus 2 (HSV-2), cytomegalovirus (CMV) (including transplant CMV), Epstein Barr virus (EBV), varicella zoster virus (VZV) (also known as herpes zoster virus (HZV)), human herpes virus 6 (HHV-6), human herpes virus 7 (HHV-7), and human herpes virus 8 (HHV-8). Form 2 valaciclovir hydrochoride is also useful in the treatment or prophylaxis of the 30 symptoms or effects of herpes virus infections.
F 2s Form 2 valaciclovir hydrochloride is also useful in the treatment or prophylaxis of a condition or disease associated with a herpes virus infection, particularly a condition or disease associated with a latent herpes virus infection in an animal, e.g., a mammal such as a human. By"condition or disease s associated with a herpes viral/virus infection" is meant a condition or disease, excluding the viral infection per se, which results from the presence of the viral infection, such as chronic fatigue syndrome which is associated with EBV infection and multiple sclerosis which has been associated with herpes viral infections such as EBV and HHV-6.
In addition to those conditions and diseases, Form 2 valaciclovir hydrochloride may also be used for the treatment or prophylaxis of cardiovascular diseases and conditions associated with herpes virus infections, in particular atherosclerosis, coronary artery disease and restenosis and specifically 15 restenosis following angioplasty (RFA). Restenosis is the narrowing of the blood vessels which can occur after injury to the vessel wall, for example injury caused by balloon angioplasty or other surgical and/or diagnostic techniques, and is characterized by excessive proliferation of smooth muscle cells in the walls of the blood vessel treated. It is thought that in many 20 patients suffering from RFA, viral infection, particularly by CMV and/or HHV-6 of the patient plays a pivotal role in the proliferation of the smooth muscle cells in the coronary vessel treated. Restenosis can occur following a number of surgical and/or diagnostic techniques, for example, transplant surgery, vein grafting, coronary by-pass grafting and, most commonly following 25 angioplasty.
There is evidence from work done both in vitro and in vivo, indicating that restenosis is a multifactorial process. Several cytokines and growth factors, acting in concert, stimulate the migration and proliferation of vascular smooth 30 muscle cells (SMC) and production of extracellular matrix material, which accumulate to occlude the blood vessel. In addition growth suppressors act
to inhibit the proliferation of SMC's and production of extracellular matrix material. The present invention provides a method for the treatment or prophylaxis of a s viral infection in an animal such as a mammal (e.g., a human), particularly a herpes viral infection, which comprises administering to the animal an effective amount of Form 2 valaciclovir hydrochloride.
As used herein, the term "prophylaxis" refers to the prevention of infection, 10 the prevention of occurrence of symptoms in an infected subject, or a decrease in severity or frequency of symptoms of viral infection, condition or disease in the subject.
As used herein, the term "treatment" refers to the partial or total elimination 15 of symptoms or decrease in severity of symptoms of viral infection, condition or disease in the subject, or the elimination or decrease of viral presence in the subject.
As used herein, the term "effective amount" means an amount of a 20 compound of formula (I) which is sufficient, in the subject to which it is administered, to treat or prevent the stated disease, condition or infection.
For example, an effective amount of a compound of formula (I) for the treatment of a herpes virus infection is an amount sufficient to treat the herpes viral infection in the subject.
25 The present invention also provides a method for the treatment or prophylaxis of a condition or disease associated with a herpes viral infection in an animal such as a mammal (e.g., a human), which comprises administering to the animal an effective amount of Form 2 valaciclovir hydrochloride. In one embodiment, the present invention provides a method for the treatment 30 or prophylaxis of chronic fatigue syndrome or multiple sclerosis in an animal such as a mammal (e.g., a human), which comprises administering to the
animal an effective amount of Form 2 valaciclovir hydrochloride. The foregoing method is particularly useful for the treatment or prophylaxis of chronic fatigue syndrome or multiple sclerosis, associated with latent infection with a herpes virus.
In another embodiment, the present invention provides a method for the treatment or prophylaxis of a cardiovascular condition such as atherosclerosis, coronary artery disease or restenosis (particularly restenosis following surgery such as angioplasty), which comprises administering to the animal an lo effective antiviral amount of Form 2 valaciclovir hydrochloride.
The present invention also provides the use of Form 2 valaciclovir hydrochloride in the preparation of a medicament for the treatment or prophylaxis of a viral infection in an animal such as a mammal (e.g., a human), particularly a herpes viral infection and the use of Form 2 valaciclovir 15 hydrochloride in the preparation of a medicament for the treatment of a condition or disease associated with a herpes viral infection. In one embodiment, the present invention provides the use of a compound of formula (I) in the preparation of a medicament for the treatment or prophylaxis of cardiovascular disease, such as restenosis and atherosclerosis.
Simple dehydration of hydrated valaciclovir hydrochloride typically results in the formation of a partially amorphous and unstable form. The instantly claimed anhydrous crystal form can be conveniently prepared, however, by using the solvent mediated dehydrations described herein below. Accordingly, 25 as a further aspe*, the present invention provides a process for preparing Form 2 valaciclovir hydrochloride comprising slurrying damp valaciclovir hydrochloride or hydrated valaciclovir hydrochloride in a solvent capable of removing water by azeotropic distillation, under azeotropic distillation conditions. In one particular embodiment, the process comprises the steps 30 of:
a) optionally removing unbound process solvent from damp valaciclovir hydrochloride to provide (substantially dry) hydrated valaciclovir hydrochloride; b) slurrying the damp valaciclovir hydrochloride or the hydrated s valaciclovir hydrochloride in a solvent capable of removing water by azeotropic distillation, under azeotropic distillation conditions to prepare said anhydrous crystalline valaciclovir hydrochloride; and c) isolating the anNydrous crystalline (i.e., Form 2) valaciclovir hydrochloride. Valaciclovir hydrochloride can be prepared using the processes described in U.S. Patent Nos. 4,957,924 and 6,107,302, the subject matter of which is already incorporated herein by reference in their entirety. The synthesis of valaciclovir hydrochloride leads to the formation of hydrated valaciclovir 15 hydrochloride in solution in the reaction mixture (i.e., in process solvent) from which it may be separated and purified as a solid produ* (i.e., damp valaciclovir hydrochloride).
Damp valaciclovir hydrochloride can be dried to remove unbound process solvent, thereby providing hydrated valaciclovir hydrochloride in substantially 20 dry form. Drying can be accomplished by any suitable method. Examples of such methods are described in U.S. Patent No. 6,107, 302. In one preferred embodiment, unbound process solvent is removed from damp valaciclovir hydrochloride by slurrying damp valaciclovir hydrochloride in acetone, filtering and then drying, for example at about 30-70OC to provide hydrated 25 valaciclovir hydrochloride in substantially dry form.
Damp valaciclovir hydrochloride or hydrated valaciclovir hydrochloride may be used to prepare the anhydrous crystal form of the present invention. Certain favors influence which anhydrous crystal form results. These factors include, 30 but are not limited to nucleation, seeding (both active and inadvertent), solvent mediated effects and critically water content. The solvent
composition and solvent to product ratio is critical for the nucleation of the desired form. Typically seeding can influence the nucleation of the desired form from the solvent mixture. Variation in total water content of the processing solvent can also give rise to unexpected effects. In the following s methods, conditions of separation and further processing are selected to produce the anhydrous crystalline form of the present invention (i.e., Form 2 valaciclovir hydrochloride).
According to the present method, either damp valaciclovir hydrochloride or 10 hydrated valaciclovir hydrochloride is slurried in a solvent capable of removing water by azeotropic distillation. Suitable solvents capable of removing water by azeotropic distillation include but are not limited to toluene, Cat 6alcohols, ketones (such as C -6 ketones), esters (such as C -6 esters), ethers (such as C -6 ethers) and mixtures thereof. Specific examples of suitable solvents 15 include but are not limited to butanol (e.g., butan- -ol or butan-2-ol), propanol (e.g., propan-2-ol or propan-1-ol), toluene, ethyl acetate, butyl acetate, methyl isobutyl ketone (4-methyl-2-pentanone) and mixtures thereof. Additional solvents capable of removing water by azeotropic distillation which may be used in the processes of the present invention can 20 be readily determined by those skilled in the art. Preferably, the solvent capable of removing water by azeotropic distillation is selected from the group consisting of butanol (e.g., butan-1-ol), ethyl acetate, methyl isobutyl ketone and mixtures thereof. In one preferred embodiment, the solvent capable of removing water by azeotropic distillation is butan- -ol. In another preferred 25 embodiment, the solvent capable of removing water by azeotropic distillation is methyl isobutyl ketone.
The step of slurrying the damp valaciclovir hydrochloride or hydrated valaciclovir hydrochloride in the above-described solvent is preferably carried 30 out by creating a thin, suspension of valaciclovir hydrochloride in the solvent, preferably with agitation.
The slurrying step takes place under azeotropic distillation conditions.
Suitable azeotropic distillation conditions will be readily apparent to those skilled in the art and will depend upon the particular solvent selected.
s Typically, azeotropic distillation conditions involve heating the slurry, preferably with agitation, to the boiling point of the solvent capable of removing water by azeotropic distillation.
Preferably, the slurrying step comprises formation of the slurry, followed by lo subjecting the slurry to the azeotropic distillation conditions.
The reaction is preferably continued for a period of time sufficient to separate the water from the starting material, thus resulting in the anhydrous crystalline valaciclovir hydrochloride of the present invention. The amount of 15 time required to convert to Form 2 valaciclovir hydrochloride will vary depending upon the particular solvent or mixture of solvents chosen, but typically, the reaction is carried out for from about to about 6 hours.
The anhydrous crystalline valaciclovir hydrochloride produced by the slurrying 20 process (i.e., Form 2 valaciclovir hydrochloride) may be isolated from the slurry by filtration.
Optionally, the process further comprises the additional step of drying the Form 2 valaciclovir hydrochloride. Drying may be accomplished in an oven at 25 elevated temperature, with or without the presence of a desiccant, or at ambient temperature in the presence of a desiccant. In one embodiment, the product is dried under vacuum.
In another aspect, the present invention provides another process for 30 preparing Form 2 valaciclovir hydrochloride comprising the steps of:
a) removing unbound process solvent from damp valaciclovir hydrochloride to provide (substantially dry) hydrated valaciclovir hydrochloride; b) slurrying the hydrated valaciclovir hydrochloride in an anhydrous s solvent at a temperature of from about ambient temperature to about the boiling point of the anhydrous solvent for a period of time sufficient to convert the hydrated valaciclovir hydrochloride to anhydrous crystalline valaciclovir hydrochloride according to the present invention; and c) isolating the anhydrous crystalline valaciclovir hydrochloride.
The step of removing unbound process solvent from damp valaciclovir hydrochloride is preferably as described above.
Ambient temperature is usually about 15 to about 25 C, more preferably 15 about 18 to about 20 oc The step of slurrying hydrated valaciclovir hydrochloride in an anhydrous solvent is preferably carried out by creating a thin, suspension of hydrated valaciclovir hydrochloride in the solvent, preferably with agitation.
Suitable anhydrous solvents for use in the process of the present invention include but are not limited to water-free industrial methylated spirits (IMS, denatured ethanol), methanol, absolute ethanol, toluene, tetrahydrofuran, methyl isobutyl ketone (MIBK, methyl-2-pentanone) and mixtures thereof.
25 Other suitable anhydrous solvents can be determined by those skilled in the art. In one embodiment, the anhydrous solvent is water-free industrial methylated spirits or absolute ethanol. In one embodiment, the anhydrous solvent is absolute ethanol, particularly absolute ethanol containing 2% or less water.
The slurrying step may be carried out at temperatures ranging from about ambient temperature (e.g. about 15 to about 25 oC) up to the boiling point of the anhydrous solvent. According to this process, the temperature may be up to but not including the boiling point of the solvent; i.e., the temperature is s not sufficiently high to boil the anhydrous solvent. Thus the temperature is preferably lower than the boiling point of the anhydrous solvent. The optimum temperature for the slurrying step will depend upon the particular anhydrous solvent employed. Preferably the slurrying step is carried out at a temperature of from about 50 to about 60 C. The slurrying step is carried out for a period of time sufficient to
convert hydrated valaciclovir hydrochloride to Form 2 valaciclovir hydrochloride. The amount of time required to convert the hydrated valaciclovir hydrochloride to Form 2 valaciclovir hydrochloride will depend upon the choice of anhydrous 15 solvent and the temperature at which the slurrying step is carried out.
Typically, the slurrying step is carried out for from about 1 to about 24 hours, more particularly from about 1 to about 8 hours and in one embodiment from about to about 2 hours.
20 The anhydrous crystalline valaciclovir (Form 2 valaciclovir hydrochloride) may be isolated by filtration. Optionally, the Form 2 valaciclovir hydrochloride thus produced may be dried, preferably as described above.
The following examples are intended for illustration only and are not intended 25 to limit the scope of the invention in any way.
Example 1: Preparation of Hydrated Valaciclovir Hydrochloride Water (35 ml) was added to Form 1 valaciclovir hydrochloride (15 9). The mixture was heated at 60 C with stirring until all the solids dissolved. Ethanol 30 (70 ml) was added and the solution was allowed to cool to ambient temperature, the product started to precipitate after a few minutes. The
mixture was cooled to 0-5OC for 1 hour. The solid was collected by filtration, washed with ethanol (50 ml) and dried overnight under house vacuum to afford hydrated Valaciclovir hydrochloride.
s Example 2: Preparation of Form 2 Valaciclovir Hydrochloride A suspension of hydrated Valaciclovir hydrochloride (Example 1) in Butan-1 ol (100 ml) was heated at reflux and approximately 50 ml solvent removed by distillation. The suspension was stirred and heated at reflux for 1 hr then cooled to ambient temperature. Form 2 Valaciclovir hydrochloride anhydrate 10 was collected by filtration and dried in vacua. Infra red analysis of the damp paste showed Form 2 Valaciclovir hydrochloride.
Example 3: Preparation of Form 2 Valaciclovir Hydrochloride Butan-1-ol (50 ml) was added to hydrated Valaciclovir hydrochloride (3.5 9).
15 The suspension was heated and stirred at reflux. Approximately 20 ml solvent was removed by distillation and butan-1-ol (50 ml) added. A further 30 ml solvent was removed by distillation followed by the addition of butan-1 ol (30 ml). The suspension was stirred and heated at reflux for 2.5 furs. Form 2 Valaciclovir hydrochloride was collected by filtration and dried in vacuo 20 (2.649).
Example 4: Preparation of Form 2 Valaciclovir Hydrochloride 4-Methyl 2pentanone (methyl isobutyl ketone) (30 ml) was added to hydrated Valaciclovir hydrochloride (2 9), (Example 1). The suspension was 2s stirred and heated in an oil bath at 120-130 C for one hour. The temperature of the oil bath was increased to 150 C and 15 ml of solvent was removed by azeotropic distillation, and the suspension was stirred for one further hour at an oil bath temperature of 120-130 C. The solid was collected by filtration and the reaction flask rinsed with 4-methyl-2pentanone (10 ml). The solid 30 was dried under vacuum over phosphorus pentoxide overnight to afford Form 2 valacyclovir hydrochloride.
Example 5: Preparation of Form 2 Valaciclovir Hydrochloride Industrial methylated spirit (IMS) (20 ml) was added to hydrated Valaciclovir hydrochloride (2.0 9) (Example 1). The suspension was stirred at 50-60 C 5 for one hour. The solid was collec*ed by filtration and the reaction flask rinsed with IMS (30 ml). The solid was dried under vacuum over phosphorus pentoxide overnight to afford Form 2 Valaciclovir hydrochloride.
Example 6: Preparation of Form 2 Valaciclovir Hydrochloride 10 Absolute ethanol (35 ml) was added to hydrated Valaciclovir hydrochloride (2.0 9) (Example 1). The suspension was stirred at 50-60 C for two hours.
The solid was collected by filtration and the reaction flask rinsed with absolute ethanol (30 ml). The solid was dried under vacuum over phosphorus pentoxide for two days to afford Form 2 Valaciclovir hydrochloride.
Example 7: Preparation of Form 2 Valaciclovir Hydrochloride Absolute Ethanol (20 ml) was added to Valaciclovir hydrochloride (2.0 9) (Example 1). The suspension was stirred at ambient temperature for four hours. The solid was collected by filtration and the reaction flask rinsed with 20 absolute ethanol (30 ml). The solid was dried under vacuum over phosphorus pentoxide overnight to afford Form 2 Valaciclovir hydrochloride.
Example 8: Preparation of Form 2 Valaciclovir Hydrochloride Absolute Ethanol (300 ml) was added to hydrated valacyclovir hydrochloride 25 (30. 0 9). The suspension was stirred at 50-60 C for 1 hour. Absolute Ethanol (40 ml) was added and stirring at 50-60 C was continued for 2.5 hours. The solid was collected by filtration and the reaction flask rinsed with absolute ethanol (2 x 30 ml). The solid was dried under house vacuum over phosphorus pentoxide for three days. Then in vacuum oven for three hours 30 to afford Form 2 valacyclovir hydrochloride (27.19).
Example 9: Preparation of Form 2 Valaciclovir Hydrochloride Tetrahydrofuran (20 ml) and methanol (20ml) were added to hydrated Valaciclovir hydrochloride (2.0 9) prepared in a similar fashion to that in Example 1. The suspension was stirred at ambient temperature for three 5 and half hours. The solvents were evaporated under reduced pressure. The solid was dried under house vacuum on phosphorus pentoxide overnight to afford Form 2 Valaciclovir hydrochloride.
Example 10: Preparation of Form 2 Valaciclovir Hydrochloride to Ethyl acetate (50 ml) was added to hydrated Valaciclovir hydrochloride (2.0 g). The suspension was heated and stirred at reflex. Approx. 30 ml solvent was added and removed by distillation. The suspension was stirred and heated at reflux for 3 hrs using a Dean and Stark apparatus. The suspension was cooled. Form 2 Valaciclovir hydrochloride (1.809) was collected by 15 filtration and dried in vacuo.
Example 11: Analysis of Form 2 Valaciclovir Hydrochloride Proton NMR.
The proton NMR spectrum was consistent with that of Valaciclovir 20 hydrochloride.
Water content (by Karl Fisher titration): 0.61% w/w Infra Red.
25 The IR absorption spectrum of a mineral oil dispersion of the product was obtained using a Perkin-Elmer System 2000 FT-IR spectrometer at 2 cm i resolution. Data were digitized at 0.5 cm t intervals (Figure 1). Bands were observed at (cm 1): 3286, 3197, 1750, 1686, 1632, 1607, 1572, 1533, 1463, 1394,1377, 1366, 1342, 1298, 1259, 1247, 1225, 1191, 1152, 1133, 1096,
30 1042, 1017, 868, 830, 778, 760, 729, 701, 689, 631, 570.
X-ray powder diffraction.
The XRD pattern was determined on a Philips X'Pert MPD diffractometer equipped with a monochromator using copper Ka X-radiation. The Pattern is provided in Figure 2. Characteristic XRD angles 20 (relative intensities %) 5 6.7 (75.63), 9.3 (100.00), 11.4 (28.34), 13.3 (11.23), 13.9 (16.91), 15.4
(22.07), 15.7 (40.81), 16.3 (18.54), 17.1 (48.40), 18.6 (13.55), 19.0 (26. 45),
19.3 (17.11), 19.8 (16.07), 20.6 (11.32), 21.4 (50.03), 22.6 (18.93), 22. 9
(34.14), 24.2(23.67), 25.5 (18.76), 26.4 (49.69), 27.2 (31.95), 27.5 (50. 86),
27.8 (46.94), 28.0 (51.96), 28.9 (14.85) 30.2 (11.80), 30.9 (18.75), 31.9
10 (13.47), 32.6 (11.99), 34.9 (14.40), 35.3 (14.54), 35.9 (10.28).
Raman. Raman Spectra were collected on a Nicolet FT-Raman 960 running at 4cm t resolution and 400mW power, with a minimum of 600 scans accumulation.
15 Number of sample scans was 1200 using an InGaAs detector and CaF2 beasmsplitter. Spectrum is provided at Figure 3. Shift bands were observed at (cm-): 3285, 3201, 3114, 3003, 2960, 2931, 2894, 1749, 1684, 1630, 1568, 1477, 1449, 1416, 1397, 1364, 1348, 1310, 1226, 1191, 1133, 1070,
1039, 1014, 966, 902, 869, 850, 832, 810, 784, 760, 687, 646, 630, 527,
20 500, 364, 324, 278, 191, 120, 91 and 78.
Thermal analysis.
Differential scanning calorimetry was carried out on a Perkin-Elmer Pyris1 DSC system. Scan rate of 10 C per minute. Sample size 2.789 mg. The 25 thermogram is provided at Figure 5.
Moderately sharp asymmetric melting endotherm T=216 C and exothermic decomposition is observed.
Thermogravimetric analysis was carried out on a Perkin-Elmer Pyris-1 TGA system. Scan rate of 10 C per minute. Sample size 3.757 mg. The TGA trace is provided at Figure 6.
s Weight loss from 182-310 C = 42.97% w/w associated with melting / decomposition Solid State Nuclear Magnetic Resonance.
Acquisition was performed at 300K on a Bruker AMX360 spectrometer, 10 operating at a frequency of 90.55MHz for i3C observation. i3C MAS spectra are acquired by cross-polarization from Hartmann-Hahn matched proton. 4k data points were acquired in 60ms, using a contact time of 3ms and a recycle time of 15s. Protons were decoupled during acquisition by using a two-pulse phase modulated (TPPM) composite sequence. The free induction decay (fid) 15 was apodised by exponential multiplication using 5Hz of line broadening before Fourier transformation into 32k data points. Chemical shifts were externally referenced to the carboxylate signal of glycine at 176.4 ppm relative to TMS.. Spectrum is provided at Figure 4.
20 Comparative Example The IR and solid state NMR spectra of Form 1 valaciclovir hydrochloride (Figures 7 and 8, respectively) and hydrated valaciclovir hydrochloride (Figures 9 and IO, respectively) were obtained using procedures analogous to those described above in Example 11 for the IR and solid state NMR 25 analysis of Form 2 valaciclovir hydrochloride.
- The foregoing Examples are illustrative of the present invention and are not to be construed as limiting thereof. The invention is defined by the following claims ncluding eq ival ts thereof.

Claims (47)

  1. l. Anhydrous crystalline valaciclovir hydrochloride characterized by substantially the same infrared (JR) absorption spectrum as Figure 1, 5 wherein said IR absorption spectrum is obtained using a mull in mineral oil on an Ff-IR spectrometer at 2 cm t resolution.
  2. 2. Anhydrous crystalline valaciclovir hydrochloride characterized by an IR absorption spectrum obtained using a mull in mineral oil on an FT-IR lo spectrometer at 2 cm i resolution, comprising peaks at five or more positions selected from the-group consisting of 3286+1, 3197+1, 1750+1, 1686+1, 1632+1, 1607+1, 1152+1, 701+1, and 688+1 cm 1.
  3. 3. Anhydrous crystalline valaciclovir hydrochloride characterized by 15 substantially the same X-ray powder diffraction (XRD) pattern as Figure 2, wherein said XRD pattern is expressed in terms of 2 theta angles and obtained with a diffractometer equipped with a diffracted beam graphite nonochromator using copper Ka X-radiation.
    20
  4. 4. Anhydrous crystalline valaciclovir hydrochloride characterized by an XRD pattern expressed in terms of 2 theta angles and obtained with a diffractometer equipped with a diffracted beam graphite monochromator using copper Ka X-radiation, wherein said XRD pattern comprises 2 theta angles at four or more positions selected from the group consisting of 6. 7 25 +0.l, 8.1 +0.1, 9.3 +0.1, 11.4 +0.1, 13.9+0.1, 15.7+0.1, 16.3+0.1, and 17.1+0.1 degrees.
  5. 5. Anhydrous crystalline valaciclovir hydrochloride characterized by an XRD pattern expressed in terms of 2 theta angles and obtained with a 30 diffractometer equipped with a diffracted beam graphite monochromator
    À À 39
    using copper Koc X-radiation, wherein said XRD pattern comprises 2 theta angles at 6.7 +0.1, 8.1 +0.1, 9.3 +0.1, and 11.4 +0.1 degrees.
  6. 6. Anhydrous crystalline valaciclovir hydrochloride characterized by substantially the same Raman spectrum as Figure 3, wherein said Raman spectrum is obtained using a FT-Raman spectrometer at 4 cm i resolution.
  7. A. Anhydrous crystalline valaciclovir hydrochloride characterized by a Parnan spectrum obtained using a FT-Raman spectrometer at 4 cm ' lo resolution, wherein said Raman spectrum comprises at lea* four peaks selected from the group consisting of 1684+1, 1364+1, 1348+1, 1191+1, and 810+1cm-1.
  8. 8 Anhydrous crystalline valaciclovir hydrochloride characterized by 15 substantially the same solid state nuclear magnetic resonance (NMR) spectrum as Figure 4, wherein said solid state NMR is obtained on a spectrometer operating at a frequency of 90.55MHz for t3C observation at a temperature of 300K, a spinning speed of 10kHz and a recycle delay of 15 seconds.
  9. 9. Anhydrous crystalline valaciclovir hydrochloride characterized by a solid state NMR spectrum obtained using a spectrometer operating at a frequency of 90.55MHz for t3C observation at a temperature of 300K, a spinning speed 10kHz and a recycle elay of 15 seconds, wherein said solid state NMR 25 comprises chemical shifts at 15. 1+0.1, 17.2+0.1, 20.2+0.1, 20.9+0.1, 29.2+0.1, 29.9+0.1, 58.4+0.1, 64.6+0. 1, 66.8+0.1, 69.3+0.1, 70.7+0.1,
    73.9+0.1, 74.4+0.1, 116.6+0.1, 117.3+0.1, 140.4_0.1, 150.4+0.1, 151.3+0.1,
    153.6+0.1, 158.3+0.1, 169.1+0.1 and 169.6+0.1 ppm 30
  10. 10. A pharmaceutical composition comprising the anhydrous crystalline valac clovir hydrochloride according to any of claims 1 to 9.
    -
  11. 11. The pharmaceutical composition according to claim 10 further comprising one or more pharmaceutically acceptable carriers or diluents.
    5
  12. 12. A composition comprising the anhydrous crystalline valaciclovir hydrochloride according to any of claims 1 to 9 and hydrated valaciclovir hydrochloride.
  13. 13. A composition comprising the anhydrous crystalline valaciclovir 10 hydrochloride according to any of claims 1 to 9 and Form 1 valaciclovir hydrochloride.
  14. 14. Anhydrous crystalline valaciclovir hydrochloride according to any of claims 1 to 9 for use in therapy.
  15. 15. Anhydrous crystalline valaciclovir hydrochloride according to any of claims 1 to 9 for use in the treatment or prophylaxis of a herpes viral infection in a mammal.
    20
  16. 16. Use of anhydrous crystalline valaciclovir hydrochloride according to any of claims 1 to 9 in the preparation of a medicament for the treatment or prophylaxis of a herpes viral infection in a mammal.
  17. 17. Anhydrous crystalline valaciclovir hydrochloride according to claim 15, 25 or the use according to claim 16, wherein said herpes viral infection is selected from the group consisting of herpes simplex virus 1, herpes simplex virus 2, cytomegalovirus, Epstein Barr virus, varicella Poster virus, human herpes virus 6, human herpes virus 7, and human herpes virus 8.
    30
  18. 18. Use of anhydrous crystalline valaciclovir hydrochloride according to any of claims 1 to 9 in the preparation of a medicament for the treatment or
    prophylaxis of a condition or disease associated with a herpes viral infection in a mammal.
  19. 19. A process for preparing anhydrous crystalline valaciclovir hydrochloride S as defined in any of claims 1 to 9 comprising slurrving damp valaciclovir hydrochoride or hydrated valaciclovir hydrochloride in a solvent capable of removing water by azeotropic distillation, under azeotropic distillation conditions. 10 20. A process for preparing anhydrous crystalline valaciclovir hydrochloride as defined in any of claims 1 to 9 comprising the steps of: a) optionally removing unbound process solvent from damp valaciclovir hydrochloride to provide hydrated valaciclovir hydrochloride; b) slurrying said damp valaciclovir hydrochloride or said hydrated 15 valaciclovir hydrochloride in a solvent capable of removing water by azeotropic distillation, under azeotropic distillation conditions to prepare said anhydrous crystalline valaciclovir hydrochloride; and c) isolating said anhydrous crystalline valaciclovir hydrochloride.
  20. 20
  21. 21. The process according to claim 19 or 20, wherein the slurrying step comprises formation of the slurry, followed by subjecting the slurry to the azeotropic distillation conditions.
  22. 22. The process according to any of claims 19, 20 or 21, wherein the 2s azeotropic distillation conditions involve heating the slurry with agitation to the boiling point of the solvent capable of removing water by azeotropic Distillation.
  23. 23. The process according to any of claims 19 to 22, wherein said solvent 30 capable of removing water by azeotropic distillation is selected from the group
    l consisting of toluene, C1 6alcohols, C1 6ketones, C1 tethers, C1 resters, and mixtures thereof.
  24. 24. The process according to claim 23, wherein said solvent is selected s from the group consisting of butanol, propanol, toluene, ethyl acetate, butyl acetate, methyl isobutyl ketone and mixtures thereof.
  25. 25. The process according to claim 23, wherein the solvent capable of removing water by azeotropic distillation is selected from the group consisting lo of butan- -ol, ethyl acetate, methyl isobutyl ketone (4methyl-2-pentanone) and mixtures thereof.
  26. 26. The process according to any of claims 19 to 25, wherein in the azeotropic distillation step, the reaction is carried out for from about 1 hour to 15 about 6 hours.
    i
  27. 27. The process according to any of claims 19 to 26, further comprising drying said anhydrous crystalline valaciclovir hydrochloride.
    20
  28. 28. A process for preparing anhydrous crystalline valaciclovir hydrochloride as defined in any of claims 1 to 9 comprising the steps of: a) removing unbound process solvent from damp valaciclovir hydrochloride to provide hydrated valaciclovir hydrochloride; b) slurrying said hydrated valaciclovir hydrochloride in an 25 anhydrous solvent at a temperature of from about ambient temperature to about the boiling point of said anhydrous solvent for a period of time sufficient to convert said hydrated valaciclovir hydrochloride to said anhydrous crystalline valaciclovir hydrochloride; and c) isolating said anhydrous crystalline valaciclovir hydrochloride.
  29. 29. The process according to claim 28 wherein ambient temperature is about 15 to about 25 oc.
  30. 30. The process according to claim 28 or 29 wherein said anhydrous 5 solvent is selected from the group consisting of water-free industrial methylated spirits, methanol, absolute ethanol, toluene, tetrahydrofuran, methyl isobutyl ketone (4-methyl-2-pentanone) and mixtures thereof.
  31. 31. The process according to claim 28, 29 or 30, wherein said anhydrous 10 solvent is water-free industrial methylated spirits or absolute ethanol or a mixture thereof.
  32. 32. The process according to any of claims 28 to at, wherein said slurrying step b) is carried out at a temperature lower than the boiling point of the 15 - anhydrous solvent.
  33. 33. The process according to any of claims 28 to 32, wherein said Flurrying step b) is carried out at a temperature of from atom Onto about 60 C.
    i
  34. 3.4. The process according to any of claims 28 to 33, wherein said slurry 9 - step b) is carried out for from about 1 hour to about 8 hours.
  35. 35. The process according to any of claims 28 to 34, further comprising the step of drying said anhydrous crystalline valaciclovir hydrochloride.
  36. 36. Anhydrous crystalline valaciclovir hydrochloride substantially as described in one or mpre of the Examples and/or having spectroscopic properties substantially as shown in one or more of Figures 1 to when obtained under conditions substantially as described in the description.
  37. 37. Anhydrous crystalline valaciclovir hydrochloride substantially as described in one or more of the Examples and having spectroscopic properties substantially as shown in one or more of Figures to 6 when obtained under conditions substantially as described in the description.
  38. 38. A process for preparing anhydrous crystalline valaciclovir hydrochloride as defined in any of claims to 9 or claim 36 or 37, wherein the process is substantially as described in one or more of the Examples.
    10
  39. 39. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 or 37, or a process according to claim 38, wherein the anhydrous crystalline valaciclovir hydrochloride or the process for preparing the anhydrous crystalline valaciclovir hydrochloride is substantially as described in Example 2.
  40. 40. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 or 37, or a process according to claim 38, wherein the anhydrous crystalline valaciclovir hydrochloride or the process for preparing the anhydrous crystalline valaciclovir hydrochloride is substantially as described in Example 20 3.
  41. 41. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 or 37, or a process according to claim 38, wherein the anhydrous crystalline valaciclovir hydrochloride or the process for preparing the anhydrous 25 crystalline valaciclovir hydrochloride is substantially as described in Example 4.
  42. 42. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 or 37, or a process according to claim 38, wherein the anhydrous crystalline 30 valaciclovir hydrochloride or the process for preparing the anhydrous
    crystalline valaciclovir hydrochloride is substantially as described in Example 5.
  43. 43. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 S or 37, or a process according to claim 38, wherein the anhydrous crystalline valaciclovir hydrochloride or the process for preparing the anhydrous crystalline valaciclovir hydrochloride is substantially as described in Example 6. 10
  44. 44. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 or 37, or a process according to claim 38, wherein the anhydrous crystalline valaciclovir hydrochloride or the process for preparing the anhydrous crystalline valaciclovir hydrochloride is substantially as described in Example 7.
  45. 45. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 OF 37, or a process according to claim 38, wherein the anhydrous crystalline valaciclovir hydrochloride or the process for preparing the anhydrous crystalline valaciclovir hydrochloride is substantially as described in Example
  46. 46. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 or 37, or a process according to claim 38, wherein the anhydrous crystalline valaciclovir hydrochloride or the process for preparing the anhydrous 25 crystalline valaciclovir hydrochloride is substantially as described in Example 9.
  47. 47. Anhydrous crystalline valaciclovir hydrochloride according to claim 36 or 37, or a process according to claim 38, wherein the anhydrous crystalline 30 valaciclovir hydrochloride or the process for preparing the anhydrous
    crystalline valaciclovir hydrochloride is substantially as described in Example 10. s
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EP1465894A4 (en) * 2001-11-14 2008-10-08 Teva Pharma Synthesis and purification of valacyclovir
US20050043329A1 (en) * 2002-09-06 2005-02-24 Shlomit Wizel Crystalline forms of valacyclovir hydrochloride
US20060229322A1 (en) * 2002-12-09 2006-10-12 Pau Cid Anhydrous crystalline form of valacyclovir hydrochloride
WO2004106338A1 (en) * 2003-05-30 2004-12-09 Eos Eczacibasi Ozgun Kimyasal Urunler Sanayi Ve Ticaret A.S. Novel crystalline forms of valacyclovir hydrochloride
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