AU2007202943A1 - Polymorph of a pharmaceutical - Google Patents

Description

S&FRef: 536731D2

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AUSTRALIA

PATENTS ACT 1990 COMPLETE SPECIFICATION FOR A STANDARD PATENT Name and Address Abbott Laboratories, of CHAD-0377/AP6D-2 100 Abbott of Applicant Park Road, Abbott Park, Illinois, 60064-6050, United States of America Actual Inventor(s): Kimberly A. Allen, John F. Bauer, Philip E. Bauer, Sanjay R. Chemburkar, Bikshandarkoil A. Narayanan, Ketan Patel, Azita Saleki-Gerhardt, Harry O. Spiwek Address for Service: Spruson Ferguson St Martins Tower Level 31 Market Street Sydney NSW 2000 (CCN 3710000177) Invention Title: Polymorph of a pharmaceutical The following statement is a full description of this invention, including the best method of performing it known to me/us:- 5845c(844828_1) Polymorph of a Pharmaceutical Technical Field This invention relates to a novel crystalline polymorph of (2S,3S,5S)-5-(N- (N -methyl-N 2 -isop ropy 1-4 th iazo lyl)methyl)a mi no)ca rbonyl)-L valinyl)amino)-2-(N((5-thiazolyl)methoxycarbonyl)amino)-1,6-diphenyl-3hydroxyhexane, methods for its preparation, methods for its use as a pharmaceutical agent and pharmaceutical compositions comprising the novel crystalline polymorph. This invention also relates to an amorphous form of (2S, 3

S,

5

S)-

5 -(N-(N-((N-methyl-N-((2-isopropyl-4thiazolyl)methy)amino)carbonyl)-L-valinyl)amino)2(N-((5-thiazolyl)methoxycarbonyl)amino)-1,6diphenyl-3-hydroxyhexane and methods for its preparation Background of the Invention Inhibitors of human immunodeficiency virus (HIV) protease have been approved for use in the treatment of HIV infection for several years. A particularly effective HIV protease inhibitor is 2 S,3S,5S)-5-(N-(N-((N-methy-N-((2.isopropy..

4 methoxycarbonyl)amino)-1,6-diphenyl-3-hydroxyhexane (ritonavir), which is marketed as NORVIRO.. Ritonavir is known to have utility for the inhibition of HIV protease, the inhibition of HIV infection, the inhibition of cytochrome P450 monooxygenase and the enhancement of the pharmacokinetics of compounds which are metabolized by cytochrome P450 monooxygenase. Ritonavir is particularly effective for the inhibition of HIV infection when used alone or in D combination with one or more reverse transcriptase inhibitors and/or one or more other HIV protease inhibitors.

SRitonavir and processes for its preparation are disclosed in U.S. Patent No. 5,541,206, issued July 30, 1996. This patent discloses processes for O preparing ritonavir which produce a crystalline polymorph of ritonavir which is termed crystalline Form I. Substantially pure Form I has the powder X-ray N\ diffraction pattern, 13 solid state nuclear magnetic resonance spectrum, the FT 10 near infrared spectrum and the FT mid infrared spectrum which appear in FIGS.

1, 4, 6 and 8, respectively. The angular positions (two theta) of the characteristic peaks in the powder X-ray diffraction pattern of substantially pure Form I shown in FIG. 1 are 3.33° 0.10, 6.760 8.330 0.10, 14.610 0.10, 16.330 0.10, 16.760 0.10, 17.03° 0.10, 18.020 0.10, 18.620 0.10, 19.470 0.1°, 19.860 0.10, 20.250 0.10, 21.460 23.460 0.1° and 24.360 0.1°.

Another process for the preparation of ritonavir is disclosed in U.S. Patent No. 5,567,823, issued October 22, 1996. The process disclosed in this patent also produces ritonavir as crystalline Form I.

Pharmaceutical compositions comprising ritonavir or a pharmaceutically 2o acceptable salt thereof are disclosed in U.S. Patent Nos. 5,541,206, issued July 1996; 5,484,801, issued January 16, 1996; 5,725,878, issued March 1998; and 5,559,158, issued September 24, 1996 and in International Application No. WO98/22106, published May 28, 1998 (corresponding to U.S. Serial No.

08/966,495, filed November 7, 1997).

The use of ritonavir to inhibit an HIV infection is disclosed in U.S. Patent No. 5,541,206, issued July 30, 1996. The use of ritonavir in combination with one or more reverse transcriptase inhibitors to inhibit an HIV infection is disclosed in U.S. Patent No. 5,635,523, issued June 3, 1997. The use of ritonavir in combination with one or more HIV protease inhibitors to inhibit an HIV infection is disclosed in U.S.

Patent No. 5,674,882, issued October 7, 1997. The use of ritonavir to inhibit cytochrome P450 monooxygenase and to enhance the pharmacokinetics of compounds metabolized by cytochrome P450 monooxygenase is disclosed in W097/01349, published January 16, 1997 (corresponding to U.S. Serial No. 08/687,774, filed June 26, 1996).

It has now been unexpectedly discovered that ritonavir can be prepared as a new crystalline polymorph which is termed crystalline Form II.

All publications, issued patents and patent applications cited herein are hereby incorporated by reference.

Summary of the Invention According to one embodiment of this invention there is provided substantially pure amorphous ritonavir.

According to another embodiment of this invention there is provided a composition comprising amorphous ritonavir.

According to a further embodiment of this invention there is provided a pharmaceutical composition encapsulated in a soft elastic gelatin capsule and having the following composition: Amorphous ritonavir, dehydrated ethanol, oleic acid, butylated hydroxy toluene, polyoxyl 35 castor oil (Cremophor EL) and water.

Brief Description of the Drawings FIG. 1 is the powder X-ray diffraction pattern of the substantially pure Form I crystalline polymorph of ritonavir.

FIG. 2 is the powder X-ray diffraction pattern of the substantially pure Form II crystalline polymorph of ritonavir.

FIG. 3 is the powder X-ray diffraction pattern of substantially pure amorphous ritonavir.

FIG. 4 is the 400 MHz solid state 13C nuclear magnetic resonance spectrum of the substantially pure Form I crystalline polymorph of ritonavir.

FIG. 5 is the 400 MHz solid state 13C nuclear magnetic resonance spectrum of the substantially pure Form II crystalline polymorph of ritonavir.

FIG. 6 is the FT near infrared spectrum of the substantially pure Form I crystalline polymorph of ritonavir.

FIG. 7 is the FT near infrared spectrum of the substantially pure Form II crystalline polymorph of ritonavir.

FIG. 8 is the FT mid infrared spectrum of the substantially pure Form I crystalline polymorph of ritonavir.

844525 IDOC FIG. 9 is the FT mid infrared spectrum of the substantially pure Form II crystalline polymorph of ritonavir.

D FIG. 10 is the differential scanning calorimetric thermogram for substantially pure amorphous ritonavir.

Disclosure of the Invention In accordance with the present invention, there is a novel substantially pure crystalline polymorph of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4j methoxycarbonyl)amino)-1, 6 -diphenyl-3-hydroxyhexane (ritonavir). For the sake 'o of identification, this crystalline polymorph is designated as the Form II crystalline polymorph of ritonavir.

Substantially pure Form II has the powder X-ray diffraction pattern, 13C solid state nuclear magnetic resonance spectrum, the FT near infrared spectrum and the FT mid infrared spectrum which appear in FIGS. 2, 5, 7 and 9, 1' respectively. The two-theta angle positions of characteristic peaks in the powder X-ray diffraction pattern of substantially pure Form II as shown in FIG. 2 are: 8.670 0.10, 9.880 16.110 0.10, 16.700 0.10, 17.360 ±0.10, 17.780 ±0.10, 18.400 0.10, 18.93" 0.10, 20.070 20.650 0.1°, 21.71° 0.1°and 25.38 0.10.

More preferably, substantially pure Form II is characterized by peaks in the powder X-ray diffraction pattern having two-theta angle positions as shown in FIG. 2 of: 8.670 0.10, 9.51° 0.10, 9.880 0.10, 10.970 13.740 0.10, 16.110 0.10, 16.700 0.10, 17.360 0.10, 17.780 0.10, 18.400 0.1°, "2 18.930 0.10, 19.520 19.800 20.07° 0.10, 20.650 0.10, 21.490 0.10, 21.71° 0.10, 22.230 25.380 0.10, 26.150 0.1° and 28.620 0.10.

The substantially pure Form II crystalline polymorph of ritonavir can be Snprepared from amorphous ritonavir by contacting amorphous ritonavir with a IN C1-C3 alcohol. The method of contacting may be either by saturating the amorphous compound in the solvent at ambient temperature and then allowing 5 the mixture to stand for an extended period of time (for example, overnight) or by dissolving the amorphous compound in the solvent at elevated temperature, C preferably, at reflux, followed by cooling the solution to room temperature and 0 isolating Form II.

cN In one embodiment of the process, the substantially pure Form II crystalline polymorph of ritonavir can be prepared from amorphous ritonavir by preparing a saturated solution of amorphous ritonavir in a C1-C3 alcohol at room temperature and isolating Form II which results. In practice this can be accomplished by dissolving a sufficient amount of amorphous ritonavir in the C1-C3 alcohol at elevated temperature (up to reflux) such that when the solution is allowed to cool to room temperature a saturated solution is obtained, from which Form II precipitates and can be isolated. A preferred solvent for the preparation of Form II is anhydrous ethanol. Isolation of the resulting solid provides Form II.

Substantially pure amorphous ritonavir is prepared from the Form I t o crystalline polymorph of ritonavir by melting Form I ritonavir and rapidly cooling the melt. Isolation of the resulting solid provides amorphous ritonavir.

Substantially pure amorphous ritonavir can also be prepared by slowly adding a solution of ritonavir Form I in a suitable solvent (methylene chloride and the like; preferably, methylene chloride) at a concentration of, preferably, about 1 2 s g of ritonavir per about 1.5-2.0 mL of solvent (preferably, about 1 g of ritonavir/ about 1.5 mL of methylene chloride) to an anti-solvent (for example, hexane or heptane and the like; preferably, hexane) at a concentration of about 60-110 mL of antisolvent/ g of ritonavir; preferably, about 85-90 mL of hexane/ g of ritonavir, followed by isolation (for example, by filtration) of the resulting solid.

Similarly, substantially pure amorphous ritonavir can also be prepared by slowly adding a solution of ritonavir Form I in a suitable solvent such as methanol or the like at a concentration of, preferably, about 1 g of ritonavir per about mL of solvent (preferably, about 1 g of ritonavir/ about 1.5 mL of methanol) to an anti-solvent such as methyl t-butyl ether (MTBE) or the like at a concentration of about 60-150 mL of antisolvent/ g of ritonavir, preferably, about 90-110 mL of MTBE/ g of ritonavir and, most preferably, about 100 mL of MTBE/ g of ritonavir, (o followed by isolation (for example, by filtration) of the resulting solid.

Substantially pure amorphous ritonavir can also be prepared by slowly adding a solution of ritonavir Form I in a suitable solvent (for example, methanol and the like; preferably, methanol) at a concentration of about 1 g of ritonavir per about 1.5-2.0 mL of solvent (preferably, about 1 g of ritonavir/ about 1.6 mL of methanol) to water at about 0°C at a concentration of about 400-500 mL of water/ g of ritonavir (preferably, about 400 mL of water/ g of ritonavir), followed by isolation (for example, by filtration) and drying of the resulting solid.

Substantially pure amorphous ritonavir can also be prepared by lyophilization of a solution of ritonavir Form I. Preferred solvents are C1-C6 alcohols. A more preferred solvent is isobutanol.

Alternatively, in a preferred process, substantially pure Form II can be prepared by seeding a solution of ritonavir Form I in a suitable solvent (preferably, a C1-C3 alcohol; most preferably, ethanol) with undissolved (2S)-N-((1S)-1-Benzyl-2-((4S,5S)-4-benzyl-2-oxo-1,3-oxazolidin-5-yl)ethyl)-2- ((((2-isopropyl-1, 3 -thiazol- 4 -yl)methyl)amino)-carbonyl)amino)-3methylbutanamide. In a preferred method, ritonavir Form I is dissolved in ethanol (preferably, 200 proof ethanol) at a concentration of from about 150 g/ L to about 200 g/ L, preferably, about 160 g/ L. To the solution is added seed crystals of S)-1-Benzyl-2-((4S,5S)-4-benzyl-2-oxo-1,3-oxazolidin-5-yl)ethyl)-2- 2 -isopropyl-1, 3 -thiazol-4-yl)methyl)amino)carbonyl)-amino)-3methylbutanamide in the amount of from about 0.02 g to about 0.10 g of seed crystals/ g of ritonavir. The amount of seed crystals added is such that it exceeds the saturation amount in the solvent being used so that there are undissolved seed crystals present in the ritonavir solution. The mixture is allowed to stand at a temperature of from about 00 C to about 150 C (preferably, about 50 C) for from about 12 hours to about 48 hours (preferably, about 24 hours). The resulting crystalline ritonavir Form II is isolated by filtration.

(o In yet another preferred alternative method, substantially pure Form II can be prepared by recrystallization of Form I or mixtures of Form I and Form II from a solution in a suitable solvent (for example, ethyl acetate or isopropyl acetate or chloroform and the like other solvents with like dielectric constant; preferably, ethyl acetate), with seeding with Form II crystals, followed by addition of an anti- CI solvent (for example, heptane, hexane, toluene, petroleum ether and the like other anti-solvents with like dielectric constant; preferably, heptane). The amount of seed crystals added is such that it exceeds the saturation amount in the solvent being used so that there are undissolved seed crystals present in the ritonavir solution. In a preferred method, ritonavir (Form I or a mixture of Form I .0 and Form II) is dissolved in ethyl acetate (from about 4.0 L to about 6.0 L/kg of ritonavir) with heating (at from about 65°C to about 700C). The solution is slowly cooled to from about 550C to about 500C, preferably about 52°C. Seed crystals of ritonavir Form II (from about 0.5 g of Form II seed crystals/kg of ritonavir to about 10.0 g of Form II seed crystals/kg of ritonavir, preferably about 1.25 g of Form II seed crystals/kg of ritonavir) are added and the mixture is stirred for about 1 hour at a temperature of from about 55 0 C to about 50 0 C, preferably about 52°C. The amount of seed crystals added is such that it exceeds the saturation amount in the solvent being used so that there are undissolved seed crystals present in the ritonavir solution. Heptane (from about 1.0 L/kg of ritonavir to Z about 4.0 L/kg of ritonavir; preferably, about 2.8 L/kg of ritonavir) is added with Smixing and the mixture is allowed to slowly cool to about 250C and is then stirred for at least 12 hours at about 25°C. The product is isolated by M 5 filtration/centrifugation and is dried under vacuum with heating. On a manufacturing scale (300-400 kg batches), it has been observed that isolation by filtration/centrifugation is considerably faster for Form II than for the Scorresponding amount of Form I (16 hours versus 24-30 hours).

CN- It has also been found that Form II or mixtures of Form II and Form I can to be converted to substantially pure Form I by dissolving the Form II or mixture of Form II and Form I in a suitable solvent (for example, ethyl acetate or isopropyl acetate and the like; preferably, ethyl acetate) at a concentration of about 1 kg of ritonavir/4 L of solvent (preferably, ethyl acetate) with heating. The hot solution of ritonavir is slowly added (preferably, through a filter) to a slurry of seed crystals of ritonavir Form I (from about 0.5% to about 10% by weight relative to amount of ritonavir Form II or mixture of Form II and Form I; preferably, from about 0.5% to about 5% by weight and, most preferably, from about 0.5% to about 1% by weight) in an anti-solvent (for example, heptane or hexane and the like; preferably, heptane) at a concentration of about 1 kg of ritonavir (Form II or 1.o mixture of Form II and Form I) per about 4-8 L of antisolvent (preferably, about 1 kg of ritonavir (Form II or mixture of Form II and Form about 4 L of heptane).

The mixture is cooled to about 20°C and stirred for at least 3 hours. Isolation (for example, by filtration) and drying of the resulting solid provides ritonavir Form I.

The following examples will serve to further illustrate the preparation of the novel forms of ritonavir of the invention and the conversion of Form II to Form I.

Example 1 Preparation of Amorphous Ritonavir Form I crystalline polymorph of ritonavir (100 g) was melted at 125°C by heating Form I. The melt was maintained at a temperature of 125°C for 3 hours.

The melt was rapidly cooled by placing the container holding the melt into a Dewar flask containing liquid nitrogen. The resulting glass was ground with a mortar and pestle to provide amorphous ritonavir (100 Powder X-ray diffraction analysis confirmed that the product was amorphous. Differential scanning calorimetric analysis determined that the glass transition point was from to about 45°C to about 490C. (Measured onset at 45.4°C and which ends at 49.08°C, with a midpoint of 48.99°C).

Example 2 Preparation of Crystalline Ritonavir (Form II) Amorphous ritonavir (40.0 g) was dissolved in boiling anhydrous ethanol (100 mL). Upon allowing this solution to cool to room temperature, a saturated solution was obtained. After standing overnight at room temperature, the resulting solid was isolated from the mixture by filtration and was air dried to provide Form II (approximately 24.0 g).

Example 3 2 o Preparation of (2S)-N-((1S)-1-Benzvl-2-((4S,5S)-4-benzyl-2-oxo- 13-oxazolidin-5yl)ethyl)-2-((((2-isopropyl-1, 3 -thiazol-4-yl)methyl)amino)carbonyl)amino)-3methylbutanamide Example 3a Preparation of 4 2 S)-2-t-butvloxvcarbonvlamino-3-phenylprpvI)-4benzvl-1,3-oxazolidin-2-one 2

S,

3 S,5S)-2-Amino-3-hydroxy-5-t-butyloxycarbonylamino-1,6diphenylhexane succinate salt (30 g, 63 mmol; U.S. Patent No. 5,654,466), ((5-thiazolyl)methyl)-(4-nitrophenyl)carbonate hydrochloride (22.2 g; U.S. Patent No. 5,597,926) and sodium bicarbonate (16.2 g) were mixed with 300mL of water and 300 mL of ethyl acetate and the mixture was stirred at room temperature for about 30 minutes. The organic layer was then separated and heated at about 'o 60 0 C for 12 hours, and then stirred at 20-25oC for 6 hours. 3 mL of ammonium hydroxide (29% ammonia in water) was added and the mixture stirred for hours. The resulting mixture was washed with 4 x 200 mL of 10% aqueous potassium carbonate and the organic layer was separated and evaporated under vacuum to provide an oil. The oil was suspended in about 250 mL of heptane.

s The heptane was evaporated under vacuum to provide a yellow solid. The yellow solid was dissolved in 300 mL of THF and 25 mL of 10% aqueous sodium hydroxide was added. After stirring for about 3 hours, the mixture was adjusted to pH 7 by addition of 4N HCI (about 16 mL). The THF was evaporated under vacuum to leave an aqueous residue, to which was added 300 mL of distilled So water. After stirring this mixture, a fine suspension of solids resulted. The solid was collected by filtration and the filtered solid was washed with water (1400 mL) in several portions, resulting in the desired product.

Example 3b Preparation of 4 S,5S)-5-((2S)-2-amino-3-phenylpropyl)- 4-benzvl-1,3-oxazolidin-2-one The crude, wet product of Example 3a was slurried in 1N HCI (192 mL) and the slurry was heated to 70°C with stirring. After 1 hour, THF (100 mL) was added and stirring at 65°C was continued for 4 hours. The mixture was then Sallowed to cool to 20-25°C and was stirred overnight at 20-25 0 C. The THF was D removed by evaporation under vacuum and the resulting aqueous solution was cooled to about 5°C, causing some precipitation to occur. The aqueous mixture 5 was adjusted to pH 7 by addition of 50% aqueous sodium hydroxide (about 18.3 1- The resulting mixture was extracted with ethyl acetate (2 x 100 mL) at about 15 0 C. The combined organic extracts were washed with 100 mL of brine and the organic layer was separated and stirred with sodium sulfate (5 g) and Darco q (3 This mixture was warmed on a hot plate for 1 hour at 45°C. The hot FO mixture was then filtered through a bed of diatomaceous earth and the filter pad was washed with ethyl acetate (100 mL). The filtrate was evaporated under vacuum to provide an oil. The oil was redissolved in methylene chloride (300 mL) and the solvent was evaporated under vacuum. The resulting oil was dried at room temperature under vacuum to provide the desired product (18.4 g) as a glassy syrup.

Example 3c Preparation of (2S)-N-((1S)-1-Benzyl-2-((4S,5S)-4-benzl-2-oxo-1,3-oxazolidin-5yl)ethyl)-2-((((2-isopropyl-1, 3 -thiazol-4-yl)methyl)amino)carbonyl)amino)-3methylbutanamide -o N-((N-Methyl-N((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valine (10.6 g, 33.9 mmol; U.S. Patent No. 5,539,122 and International Patent Application No. W098/00410), the product of Example 3b (10.0 g, 32.2 mmol) and 1-hydroxybenzotriazole (5.2 g, 34 mmol) were dissolved in THF (200 mL).

1, 3 -dicylcohexylcarbodiimide (DCC, 7.0 g, 34 mmol) was then added to the THF mixture and the mixture was stirred at 22°C for 4 hours. Citric acid (25 mL of aqueous solution) was added and stirring continued for 30 minutes. The THF was then evaporated under vacuum. The residue was dissolved in ethyl ;Z acetate (250 mL) and washed with 10% citric acid solution (175 mL). NaCI (5 g) Swas added to accelerate the separation of the layers. The organic layer was sequentially washed with 10% aq. sodium carbonate (2 x 200 mL) and water (200 ¢q 5 mL). The organic layer was then dried over sodium sulfate (20 filtered and evaporated under vacuum. The resulting product (20.7 g of a foam) was dissolved in hot ethyl acetate (150 mL) and then heptane (75 mL) was added.

SUpon cooling, another 75 mL of heptane was added and the mixture was heated cN to reflux. Upon cooling to room temperature, no precipitate formed. The solvents were evaporated under vacuum and the residue was redissolved in a mixture of 200 mL ethyl acetate/100 mL heptane. The small amount of undissolved solid was removed by filtration. The filtrate was evaporated under vacuum and the residue was dissolved in a mixture of 100 mL ethyl acetate/ 50 mL heptane, giving a clear solution. The solution was cooled to -10oC and a white precipitate formed. The mixture was allowed to sit at -15°C for 24 hours. The resulting solid was collected by filtration, washed with 1:1 ethyl acetate/heptane (2 x 24 mL) and dried in a vacuum oven at 55 0 C to provide the desired product as a beige solid (16.4 g).

H NMR (DMSO-d 6 5 7.84 (1H, doublet 7.71 (1H, singlet), 7.32-7.11 2 0 (11H, multiplet), 6.09 (1H, doublet 4.51 (1H AB J=16.2), 4.43 (1H AB J=16.2), 4.22 (1H, multiplet), 4.07 (1H, multiplet), 3.96 (1H, doublet of doublet 3.65 (1H, multiplet), 3.23 (1H, septuplet 2.89 (3H, singlet), 2.84-2.60 (4H, multiplet), 1.94 (1H, multiplet), 1.76-1.49 (2H, multiplet), 1.30 (6H, doublet 0.80 (3H, doublet 0.77 (3H, doublet J=5.8) C 1C NMR (DMSO-d 6 8 177.2, 171.5, 157.6, 157.5, 152.8, 138.3, 136.5, 129.5, S129.2, 128.2, 128.0, 126.4, 126.0, 114.0, 77.2, 59.9, 57.6, 48.2, 46.2, 40.4, 40.1, S39.1, 34.5, 32.4, 30.3, 22.8, 22.8, 19.4, 18.3.

Example 4 5 Preparation of Crystalline Ritonavir (Form II) STo a solution of 1.595 g of ritonavir Form I in 10 mL of 200 proof ethanol 0was added an amount of the product of Example 3c (approximately micrograms) such that all of the added amount of the product of Example 3c did not dissolve. This mixture was allowed to stand at about 5°C for 24 hours. The ,0 resulting crystals were isolated by filtration through 0.45 micron nylon filter and air dried to provide ritonavir Form II.

Example Alternative Preparation of Crystalline Ritonavir (Form II) Ethyl acetate (6.0 L/kg of ritonavir) was added to ritonavir (Form I or a mixture of Form I and Form II) in a reaction vessel. The mixture was stirred and heated to 70°C until all solids were dissolved. The solution was filtered (utilizing a centrifuge pump and 5X20 inch cartridge filters having a porosity of 1.2 microns) and the filtrate was allowed to cool to 52 0 C at a rate of 2-10°C/hour. To this solution was added an amount of ritonavir Form II seed crystals (about 1.25 g of Form II seed crystals/kg of ritonavir) such that all of the seed crystals did not dissolve and the mixture was stirred at 52°C for not less than 1 hour at an agitation rate of 15 RPM. The mixture was then allowed to cool to 40°C at a rate of 10°C/hour. Heptane (2.8 Lkg of ritonavir) was added at a rate of 7L/minute with mixing. The mixture was allowed to cool to 25°C at a rate of 10°C/hour with mixing. Then the mixture was stirred for not less than 12 hours at 250C. The product was isolated by filtration using a Heinkel type centrifuge (run time approximately 16 hours). The product was dried at 55°C under vacuum (50 mm Hg) for 16-25 hours to provide ritonavir crystal Form II.

Example 6 G Preparation of Amorphous Ritonavir Ritonavir Form I (40 g) was dissolved in methylene chloride (60 mL). This solution was slowly added over 15 minutes to a round bottom flask equipped with an overhead stirrer and containing hexanes (3.5 The resulting slurry was allowed to stir for 10 minutes. The precipitate was filtered and dried at room o 1 temperature in a vacuum oven to provide amorphous ritonavir (40 g).

Example 7 Preparation of Amorphous Ritonavir Ritonavir Form I (5 g) was dissolved in methanol (8 mL). This solution was slowly added to a round bottom flask equipped with an overhead stirrer and containing distilled water (2 while maintaining the internal temperature near 0 0 C. The resulting solid was filtered to give a sticky solid which was dried in a vacuum oven at 20-25 0 C for 12-18 hours to give amorphous ritonavir (2.5 g).

Example 8 Preparation of Ritonavir Form I 112 Ritonavir Form II (1 kg) was added to a reactor followed by the addition of ethyl acetate (4 This mixture was refluxed until all of the solids were dissolved.

;Z

0-n

IND

To a separate reactor was added an amount of seed crystals of ritonavir Form I (5 followed by the addition of heptane (4 such that all of the seed crystals did not dissolve. This mixture (a slurry) was stirred at 230C The hot solution from reactor A was slowly filtered, using a 0.2 micron filter cartridge, into the mixture in reactor B over not less than 2 hours. The resulting slurry in reactor B was cooled to 20°C and stirred for not less than 3 hours. The resulting slurry was filtered, the filtered solid washed with heptane and then dried in a vacuum oven at 65°C to provide ritonavir Form I.

A preferred pharmaceutical composition comprising ritonavir, especially, ritonavir Form II, has the following composition, encapsulated in a soft elastic gelatin capsule.

Ritonavir Form II Ethanol, dehydrated Oleic acid Butylated hydroxytoluene Polyoxyl 35 castor oil (Cremophor

EL®)

Water 100.0 mg 1 2 0.0 mg 709.75 mg 0.25 mg 60.0 mg 10.0 mg The preferred composition can be prepared according to the following method.

The following protocol is employed in the preparation of 1000 soft gelatin capsules: D Scale Amount (mg/capsule) Name (g) Q.S. Nitrogen, N.F.

Q.S.

CN 118.0 Ethanol, 118.0 C dehydrated, USP, 200 Proof Ethanol, Cdehydrated, USP, 200 Proof 0.25 Butylated Hydroxytoluene, NF 0.25 704.75 Oleic Acid, NF 704.75 100.0 Ritonavir Form II 100.0 10.0 Water, purified, USP (distilled) 10.0 60.0 Polyoxyl 35 Castor Oil, NF 60.0 5.000 Oleic Acid, NF 5.000 A mixing tank and suitable container are purged with nitrogen. 118.0 g of ethanol is weighed, blanketed with nitrogen, and held for later use. The second aliquot of ethanol (2 g) is then weighed, and mixed with 0.25 g of butylated hydroxytoluene until clear. The mixture is blanketed with nitrogen and held. The main mixing tank is heated to 28 °C (not to exceed 30 704.75 g of oleic acid is then charged into the mixing tank. 100.0 g of ritonavir Form II is then added to the oleic acid with mixing. The ethanol/butylated hydroxytoluene is then added to the mixing tank, followed by the 118.0 g of ethanol measured previously, and mixed for at least 10 minutes. 10 g of water is then charged into the tank and mixed until the solution is clear (for not less than 30 minutes). 60.0 g of Polyoxyl castor oil is charged into the tank and mixed until uniform. The solution is stored at 2-8 °C until encapsulation. According to the procedures described in g International Patent Application W098/22106, 1.0 g of the solution is filled into each soft gelatin capsule and the soft gelatin capsules are then dried, and stored Sat 2-8 oC.

N As used herein, the term "substantially pure", when used in reference to a polymorph of ritonavir, refers to a polymorph of ritonavir, Form I or Form II, which Sis greater than about 90% pure. This means that the polymorph of ritonavir does C.i not contain more than about 10% of any other compound and, in particular, does not contain more than about 10% of any other form of ritonavir. More preferably, the term "substantially pure" refers to a polymorph of ritonavir, Form I or Form II, 0 which is greater than about 95% pure. This means that the polymorph of ritonavir does not contain more than about 5% of any other compound and, in particular, does not contain more than about 5% of any other form of ritonavir. Even more preferably, the term "substantially pure" refers to a polymorph of ritonavir, Form I or Form II, which is greater than about 97% pure. This means that the polymorph 15 of ritonavir does not contain more than about 3% of any other compound and, in particular, does not contain more than about 3% of any other form of ritonavir.

As used herein, the term "substantially pure", when used in reference to amorphous ritonavir, refers to amorphous ritonavir which is greater than about pure. This means that the amorphous ritonavir does not contain more than about 10% of any other compound and, in particular, does not contain more than about 10% of any other form of ritonavir. More preferably, the term "substantially pure", when used in reference to amorphous ritonavir, refers to amorphous ritonavir which is greater than about 95% pure. This means that the amorphous ritonavir does not contain more than about 5% of any other compound and, in 1Z particular, does not contain more than about 5% of any other form of ritonavir.

Even more preferably, the term "substantially pure", when used in reference to amorphous ritonavir, refers to amorphous ritonavir which is greater than about 97% pure. This means that the amorphous ritonavir does not contain more than about 3% of any other compound and, in particular, does not contain more than about 3% of any other form of ritonavir.

Powder X-ray diffraction analysis of samples was conducted in the following manner. Samples for X-ray diffraction analysis were prepared by spreading the sample powder (with no prior grinding required) in a thin layer on the sample holder and gently flattening the sample with a microscope slide.

A Nicolet 12NV X-ray Diffraction System was used with the following parameters: t X-ray source: Cu-Kal; Range: 2.00-40.00' Two Theta; Scan Rate: 1.00 degree/minute; Step Size: 0.02 degrees; Wavelength: 1.540562 angstroms.

Characteristic powder X-ray diffraction pattern peak positions are reported for polymorphs in terms of the angular positions (two theta) with an allowable variability of 0.10. This allowable variability is specified by the U.S.

Pharmacopeia, pages 1843-1844 (1995). The variability of 0.10 is intended to be used when comparing two powder X-ray diffraction patterns. In practice, if a diffraction pattern peak from one pattern is assigned a range of angular positions (two theta) which is the measured peak position 0.10 and a diffraction pattern peak from the other pattern is assigned a range of angular positions (two theta) 26 which is the measured peak position 0. 1' and if those ranges of peak positions overlap, then the two peaks are considered to have the same angular position (two theta). For example, if a diffraction pattern peak from one pattern is determined to have a peak position of 5.200, for comparison purposes the allowable variability allows the peak to be assigned a position in the range of 5.10' 5.30 If a comparison peak from the other diffraction pattern is determined to have a peak position of 5.350, for comparison purposes the allowable variability allows the peak to be assigned a position in the range of 5.250 5.450. Because there is overlap between the iwo ranges of peak Spositions 5.100 5.300 and 5.250 5.450) the two peaks being compared are considered to have the same angular position (two theta).

r 5 Solid state nuclear magnetic resonance analysis of samples was conducted in the following manner. A Bruker AMX-400 MHz instrument was used with the following parameters: CP- MAS (cross-polarized magic angle spinning); Sspectrometer frequency for 13 C was 100.627952576 MHz; pulse sequence was cp2lev; contact time was 2.5 milliseconds; temperature was 27.0 spin rate o was 7000 Hz; relaxation delay was 6.000 sec; 1" pulse width was 3.8 microseconds; 2 nd pulse width was 8.6 microseconds; acquisition time was 0.034 seconds; sweep width was 30303.0 Hz; 2000 scans.

FT near infrared analysis of samples was conducted in the following manner. Samples were analyzed as neat, undiluted powders contained in a s 6 clear glass 1 dram vial. A Nicolet Magna System 750 FT-IR spectrometer with a Nicolet SablR near infrared fiber optic probe accessory was used with the following parameters: the source was white light; the detector was PbS; the beamsplitter was CaF2; sample spacing was 1.0000; digitizer bits was 20; mirror velocity was 0.3165; the aperture was 50.00; sample gain was 1.0; the high pass 2o filter was 200.0000; the low pass filter was 11000.0000; the number of sample scans was 64; the collection length was 75.9 seconds; the resolution was 8.000; the number of scan points was 8480; the number of FFT points was 8192; the laser frequency was 15798.0 cm the interferogram peak position was 4096; the apodization was Happ-Genzel; the number of background scans was 64 and 2 s 5 the background gain was FT mid infrared analysis of samples was conducted in the following manner. Samples were analyzed as neat, undiluted powders. A Nicolet Magna System 750 FT-IR spectrometer with a Spectra-Tech InspectlR video microanalysis accessory and a Germanium attenuated total reflectance (Ge ATR) crystal was used with the fol!owing parameters: the source was infrared; the 0 detector was MCT/A; the beamsplitter was KBr; sample spacing was 2.0000; digitizer bits was 20; mirror velocity was 1.8988; the aperture was 100.00; sample 5 gain was 1.0; the high pass filter was 200.0000; the low pass filter was 20000.0000; the number of sample scans was 128; the collection length was 79.9 seconds; the resolution was 4.000; the number of scan points was 8480; the number of FFT points was 8192; the laser frequency was 15798.0 cm the interferogram peak position was 4096; the apodization was triangular; the Io number of background scans was 128 and the background gain was Differential scanning calorimetric analysis of samples was conducted in the following manner. A T.A. Instruments Thermal Analyzer 3100 with Differential Scanning Calorimetry module 2910 was used, along with Modulated DSC software version 1.1A. The analysis parameters were: Sample weight: 2.28 mg, placed in a covered, uncrimped aluminum pan; Heating rate: room temperature to 150°C at 5°C/minute under a nitrogen purge.

The foregoing is merely illustrative of the invention and is not intended to limit the invention to the disclosed embodiments. Variations and changes which are obvious to one skilled in the art are intended to be within the scope and nature of the invention which are defined in the appended claims.

Claims (8)

1. 2. The substantially pure amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- 1,6- diphenyl-3-hydroxyhexane of Claim 1 characterized by a glass transition from about 45 0 C to about 490 C.
2. 3. A process for the preparation of the compound of Claim 1 comprising adding a i0 solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane to an antisolvent.
3. 4. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane in methylene chloride to hexane. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane Form I in methylene chloride at a concentration of about 1g of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2- isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5- th iazolyl) moth oxycarbonyl)am ino)-1, ,6-d iphe nyl -3-hyd roxyhexane per about 1.5-2.0 mL of methylene chloride to hexane at a concentration of about 60-110 mL of hexane per gram of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)- 2-(N-((5-thiazolyl)methoxycarbonyl)am ino)-1 ,6-diphenyl-3-hydroxyhexane.
4. 6. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane Form I in methylene chloride at a concentration of about 1 g of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2- isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5- thiazolyl)methoxycarbonyl)amino)-1,6-diphenyl-3-hydroxyhexane per about 1.5 mL of methylene chloride to hexane at a concentration of about 85-90 mL of hexane per gram of (2S,3S,5S)-5-(N-(N- ((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5- thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane. 844525 II)OC 22
5. 7. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane in methanol to methyl t-butyl ether.
6. 58. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane Form I in methanol at a concentration of about 1 g of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane per about 1.5-2.0 mL of methanol to hexane at a concentration of about
7. 60-150 mL of hexane per gram of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane. 9. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane Form I in methanol at a concentration of about 1 g of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane per about 1 .5 mL of methanol to hexane at a concentration of about 110 mL of hexane per gram of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane in methanol to water. 11. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane Form I in methanol at a concentration of about 1 g of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane per about 1.5-2.0 mL of methanol to water at a concentration of about
8. 400-500 mL of water per gram of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1,6- diphenyl-3-hydroxyhexane. 844525 1 DOC 12. A process for the preparation of the compound of Claim 1 comprising adding a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- ;Z valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane Form I in IND methanol at a concentration of about 1 g of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- dliphenyl-3-hydroxyhexane per about 1.6 mL of methanol to water at a concentration of about 400 mL of water per gram of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1,6- diphenyl-3-hydroxyhexane. 13. A process for the preparation of the compound of Claim 1 comprising lyophilization of (Ni a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane. 14. A process for the preparation of the compound of Claim 1 comprising lyophilization of a solution of (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane in isobutanol. A process for the preparation of amorphous (2S,3S,5S)-5-(N-(N..((N-methyl-N-((2- isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5- thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane which process is substantially as herein described with reference to any one of Examples 1, 6 or 7. 16. Amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane made by the process of Claim 17. Substantially pure amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane made by the process of any one of Claims 3-14. 18. A composition comprising amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl- 4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane. 19. The composition of Claim 18, wherein said amorphous (2S,3S,5S)-5-(N-(N-((N-methyl- N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)am thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane is substantially pure. The composition of Claim 18, wherein greater than about 90% of (2S,3S,5S)-5-(N-(N- ((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5- thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane in said composition is amorphous 844525 1DOC (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valilyl)amilo)- iazolyl)methoxycarbonyl)am ino)- 1,6-d iphenyl-3-hyd roxyhexane. 21. The composition of Claim 18, wherein greater than about 95% of (2S,3S,5S)-5-(N-(N- ((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5- thiazolyl)methoxycarbonyl)amino)-1,6-diphenyl-3-hydroxyhexane in said composition is amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)- 2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane. 22. The composition of Claim 18, wherein greater than about 97% of (2S,3S,5S)-5-(N-(N- ((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5- thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane in said composition is amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)- 2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane. 23. The composition of any one of Claims 18-22 comprising a pharmaceutically acceptable carrier. 24. A pharmaceutical composition encapsulated in a soft elastic gelatin capsule and having the following composition: Amorphous (2S,3S,5S)-5-(N-(N-((N-methyl.N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane, dehydrated ethanol, oleic acid, butylated hydroxy toluene, polyoxyl castor oil (Cremophor EL) and water. The pharmaceutical composition of Claim 24 wherein the composition is as follows: (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4-thiazolyl)methyl)amino)carbonyl)-L- valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6-diphenyl-3-hydroxyhexane Form 11 100.0 mg, ethanol, dehydrated 120.0 mg, oleic acid 709.75 mg, butylated hydroxy toluene 0.25 mg, polyoxyl 35 castor oil (Cremophor EL) 60.0 mg and water 10.0 mg. 26. Substantially pure amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazolyl)methoxycarbonyl)amino)-1 ,6- diphenyl-3-hydroxyhexane as defined in Claim 1, 2 or 17 which is greater than about 95% pure. 844525 1IDOC 27. Substantially pure amorphous (2S,3S,5S)-5-(N-(N-((N-methyl-N-((2-isopropyl-4- thiazolyl)methyl)amino)carbonyl)-L-valinyl)amino)-2-(N-((5-thiazoy)ethoxycarboflyl)amilo)-1,6- diphenyl-3-hydroxyhexane as defined in Claim 1, 2 or 17 which is greater than about 97% pure. Dated 26 June, 2007 Abbott Laboratories Patent Attorneys for the Applicant/Nominated Person SPRUSON FERGUSON 844525 1 X)C