WO2001041800A2 - Compositions and methods for stabilizing biological molecules upon lyophilization - Google Patents

Compositions and methods for stabilizing biological molecules upon lyophilization Download PDF

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WO2001041800A2
WO2001041800A2 PCT/US2000/042484 US0042484W WO0141800A2 WO 2001041800 A2 WO2001041800 A2 WO 2001041800A2 US 0042484 W US0042484 W US 0042484W WO 0141800 A2 WO0141800 A2 WO 0141800A2
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menc
buffer
amoφhous
mixture
lyophilization
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PCT/US2000/042484
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French (fr)
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WO2001041800A3 (en
WO2001041800A9 (en
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Irina Esikova
Sidney Wolfe
James Thomson
Hora Maninder
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Chiron Corporation
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Priority to CA2393298A priority Critical patent/CA2393298C/en
Priority to DE60039450T priority patent/DE60039450D1/en
Priority to DK00992589T priority patent/DK1233784T3/en
Priority to JP2001543144A priority patent/JP4948731B2/en
Priority to EP00992589A priority patent/EP1233784B1/en
Publication of WO2001041800A2 publication Critical patent/WO2001041800A2/en
Publication of WO2001041800A3 publication Critical patent/WO2001041800A3/en
Publication of WO2001041800A9 publication Critical patent/WO2001041800A9/en

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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K39/02Bacterial antigens
    • A61K39/095Neisseria
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/10Antimycotics
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/60Medicinal preparations containing antigens or antibodies characteristics by the carrier linked to the antigen
    • A61K2039/6031Proteins
    • A61K2039/6037Bacterial toxins, e.g. diphteria toxoid [DT], tetanus toxoid [TT]

Definitions

  • the present invention relates to compositions and methods for stabilizing biological molecules upon lyophilization, and methods for lyophilizing biological molecules.
  • Meningococcal meningitis is one such disease for which prevention and/or therapy can be provided through a vaccine.
  • the meningococcal meningitis vaccine utilizes the meningococcal polysaccharide (PS) which is of relatively low immunogenicity.
  • PS vaccines are conjugated to protein carriers to increase immunogenicity and provide long-term protection in young children.
  • MenC-CRM 197 against meningococcus C (MenC) has been prepared using CRM 197 as the protein carrier (Costantino et al, Vaccine, 1992, Vol. 10, No. 10: 691 -8).
  • MenC-CRM 197 conjugate meningococcal polysaccharide vaccine MenC-CRM 197, and, indeed, with protein-containing vaccines in general.
  • formulations are frequently lyophilized. Lyophilization of MenC-CRM 197, however, can lead to protein aggregation during freezing and storage. In the case of MenC-CRM 197, the aggregates represent non- covalently bound, multimers of MenC-CRM 197 which apparently associate through hydrophobic interactions.
  • compositions and methods which overcome the problem of aggregation by stabilizing biological molecules against aggregation during lyophilization can yield aggregation as high as 9.5 to 10%.
  • concentration of available immunogen decreases. Therefore, a need exists for compositions and methods which overcome the problem of aggregation by stabilizing biological molecules against aggregation during lyophilization.
  • 197 vaccine is composed of two fragments, A and B, covalently bound to one another. Fragment A has been found to be stable and highly resistant to denaturation. Fragment B, however, is highly sensitive to denaturation and is subject to proteolytic breakdown during lyophilization. As proteolytic breakdown increases, the concentration of available functional immunogen decreases. Therefore, a further need exists for compositions and methods of preparation of biological molecules that will minimize breakdown during lyophilization and storage.
  • Arakawa et al. assessed the stabilization of proteins in aqueous solutions using various sugars (Arakawa et al, Biochemistry, 1982, 21 : 6536-6544). Arakawa et al. link the protection of component proteins in aqueous solution to the cohesive force of sugars which are responsible for the increase in the surface tension of the water. This factor, however, is not relevant in lyophilized solutions. Arakawa et al. do not address the stabilization of lyophilized solutions. Further, Arakawa et al. report that sucrose present in aqueous solutions actually decreases the activity of some enzymes. Pikal et al.
  • Izutsu et al. report that maintaining mannitol in an amo ⁇ hous state stabilizes ⁇ -galactosidase (Izutsu et /., Pharm. Res., 1993, Vol. 10, No. 8, 1232-1237). Izutsu et al. report that in 200 mM sodium phosphate buffer, mannitol, at 200-5 OOmM is amo ⁇ hous and acted to stabilize ⁇ -galactosidase. In 10 and 50 mM sodium phosphate buffer, mannitol at 50- lOOnM is amo ⁇ hous and exhibited a stabilizing effect. Izutsu et al. also report that glucose in sodium phosphate buffer protects enzyme activity, but does not provide any data on concentrations of glucose suitable to attain such an effect.
  • DeLuca et al. (1965) report that the eutectic temperature of a product is an important factor in the design of lyophilization cycles and that the eutectic temperatures for various organic and inorganic salts are similar (Table I). The authors state that other factors important in the design of lyophilization cycles include the supercooling effect and the thermal conductive property of the frozen mass. DeLuca et al. (1965) report that neither mannitol nor sucrose exert a significant effect on the solubility of organic salts or the eutectic temperature of the system. DeLuca et al.
  • the present invention arises from the su ⁇ rising discovery that it is possible to stabilize biological molecules against aggregation and breakdown during and following, i. e. "upon", lyophilization, using a dissolution buffer comprising an amo ⁇ hous excipient and an amo ⁇ hous buffer.
  • the present invention provides a dissolution buffer comprising at least one amo ⁇ hous excipient, at least one amo ⁇ hous buffer, and at least one MenC immunogen.
  • the present invention provides a method for stabilizing one or more MenC immuogens upon lyophilization. The method comprises dissolving the MenC immuogen in a dissolution buffer comprising at least one amo ⁇ hous excipient and an amo ⁇ hous buffer to form a mixture, and then lyophilizing the mixture.
  • the present invention provides a method for storing one or more MenC immunogens.
  • the method comprises dissolving the MenC immunogen in a dissolution buffer comprising at least one amo ⁇ hous excipient and an amo ⁇ hous buffer to form a mixture, and then lyophilizing the mixture.
  • the present invention provides a method for lyophilization of a MenC immunogen.
  • the method comprises dissolving a MenC immunogen in a dissolution buffer comprising at least one amo ⁇ hous excipient and an amo ⁇ hous buffer to form a mixture, loading the mixture from about 10°C to about 20°C under from about 1000 Pa to about 2000 Pa of pressure, freezing the mixture from about 1 hour to about 4 hours to a temperature from about -70°C to about -50°C under from about 1000 Pa to about 2000 Pa of pressure, drying the mixture for from about 18 hours to about 30 hours at a temperature from about -50°C to about -35°C under a pressure from about 5 Pa to about 10 Pa, and drying the mixture for from 2 hours to about 12 hours at a temperature from about 10°C to about 20°C under a pressure from about 5 Pa to about 10 Pa.
  • the present invention provides a method for lyophilization o f a M e n C i m m u n o g e n . T h e m e t h o d c o m p r i s e s dissolving a MenC immunogen in a dissolution buffer comprising at least one amo ⁇ hous excipient and an amo ⁇ hous buffer to form a mixture, loading the mixture at about 10°C under 1000 Pa of pressure, freezing the mixture for about 2 hours to a temperature of about -50°C under about 1000 Pa of pressure, drying the mixture for about 24 hours at a temperature of about -35°C under a pressure of about 5 Pa, and drying the mixture for about 8 hours at a temperature of about 20°C under a pressure of about 5 Pa.
  • the present invention provides a method for stabilizing a MenC vaccine upon lyophilization.
  • the method comprises dissolving the MenC vaccine in a dissolution buffer comprising at least one amo ⁇ hous excipient and an amo ⁇ hous buffer to form a mixture, and lyophilizing the mixture.
  • Figure 1 depicts a chromatogram of MenC-CRM 197 obtained by Size Exclusion Chromatography (SEC). The main peak is seen between 19 and 24 minutes. A peak representing aggregation products is seen at about 15-17 minutes, and a peak representing fragmentation products is seen at greater than 24 minutes.
  • Figures 2A-C depict Differential Scanning Calorimetry (DSC) diagrams of a mannitol buffer (A), a mannitol-sucrose buffer (B), and a sucrose buffer (C). Replacement of 25% of the mannitol with sucrose in the buffer resulted in a decrease of the re- crystallization peak and a shift of the glass transition temperatures.
  • DSC Differential Scanning Calorimetry
  • Figure 3 depicts the effects of freeze temperature and presence of sucrose on the stability of MenC-CRM 197 formulation upon lyophilization as determined by percent recovery of MenC. MenC-CRM 197 exhibits greater stability in the presence of 5.0% sucrose when compared to formulations without sucrose.
  • Figures 4A-B show the effect of the excipient-buffer composition on the aggregation of MenC-CRM 197 as determined by Size Exclusion Chromatography.
  • Figure 4A depicts the use of a lOmM sodium phosphate buffer containing varying amounts of mannitol and/or sucrose.
  • Figure 4B depicts the use of a 5mM sodium phosphate buffer containing varying amounts of mannitol and/or sucrose.
  • the amount of amo ⁇ hous excipient, in this case sucrose in the formulation increased, aggregation of MenC-CRM 197 decreased.
  • Figure 5 depicts the effect of stress (37°C) on the aggregation of MenC-CRM 197 as determined by Size Exclusion Chromatography.
  • Formulations with amo ⁇ hous buffers demonstrated less aggregation after prolonged incubation at 37°C than did formulations with non-amo ⁇ hous buffers (sodium phosphate buffer).
  • the present invention provides buffer compositions, biological molecule compositions, and methods for the preparation and stabilization of biological molecules by reducing aggregation and breakdown of biological molecules upon lyophilization.
  • the compositions and methods involve replacing the crystallizable (non- amo ⁇ hous) buffers and excipients with completely or partially amo ⁇ hous buffers and excipients.
  • the phrase “dissolution buffer” refers to the solution in which the protein or proteins are dissolved for lyophilization.
  • the “dissolution buffer” comprises at least one amo ⁇ hous excipient and at least one amo ⁇ hous buffer.
  • the dissolution buffer further comprises a MenC immunogen.
  • the dissolution buffer further comprises MenC-CRM 197.
  • biological molecule includes, but is not limited to, proteins, nucleic acids, and saccharides. Biological molecules may be used individually or in combination with other biological molecules.
  • the biological molecule is an immunogen.
  • the biological molecule is a MenC immunogen.
  • the biological molecule is MenC-CRM 197.
  • protein refers to polypeptides, peptides, and analogs thereof.
  • Protein also includes polypeptides and peptides which are conjugated to other biological molecules.
  • the protein is an immunogen.
  • immunogen refers to any compound capable of eliciting a cellular and/or humoral immune response when in contact with a cell, and includes, without limitation, vaccines and compositions comprising immunogens. Preferably, an antibody response and a T cell response are elicited. Such immunogens would be expected to be useful in prophylactic and therapeutic applications as well as for research applications including the generation of antibodies.
  • nucleic acid refers to oligonucleotides and polynucleotides, and includes DNA and RNA.
  • saccharides includes oligosaccharides and polysaccharides.
  • amo ⁇ hous excipient refers to an excipient which remains amo ⁇ hous upon lyophilization. Excipients which remain amo ⁇ hous under certain conditions but may crystallize under other conditions are included. Conditions which maintain the amo ⁇ hous nature of the excipient are included in the present invention.
  • Amo ⁇ hous excipients are well known to those skilled in the art and include, without limitation, sugars, including sucrose, lactose, and, under conditions described herein, mannitol. Amo ⁇ hous excipients also may include, under conditions well known to those of skill in the art, without limitation, celluloses, especially sorbitol.
  • amo ⁇ hous excipients can be used either individually or as a mixture containing two or more different amo ⁇ hous excipients.
  • the amo ⁇ hous excipient is sucrose.
  • the final sucrose concentration in the dissolution buffer is from about 1.5% to about 5%.
  • the phrase "MenC vaccine" refers to a vaccine comprises at least one MenC immunogen.
  • the MenC vaccine comprises MenC- CRM 197.
  • amo ⁇ hous buffers refers to buffers which remain amo ⁇ hous upon lyophilization, e.g., organic buffers. Buffers which remain amo ⁇ hous under certain conditions but may crystallize under other conditions are included. Conditions for maintaining the amo ⁇ hous nature of the buffer are also included.
  • Amo ⁇ hous buffers are well known to those skilled in the art and include, without limitation, imidazole buffer and histidine buffer, piperidine, and diisopropylethylamine.
  • the amo ⁇ hous buffer is imidazole buffer.
  • the amo ⁇ hous buffer is imidazole buffer and has a concentration of about 1 OmM.
  • stabilizing is used synonymously with inhibiting, reducing, suppressing, decreasing, diminishing, and lowering aggregation and/or breakdown.
  • the present invention includes methods that substantially inhibit aggregation and/or breakdown of biological molecules.
  • Substantial inhibition of aggregation or breakdown refers to a reduction of aggregation or breakdown from about 25% to about 100% compared to controls which use crystallizable buffers and/or excipients.
  • aggregation or breakdown is inhibited by about 50%, more preferably by about 75%, and even more preferably by about 100%.
  • the term “upon lyophilization” refers to the period during lyophilization of the biological molecules and during subsequent storage of the lyophilized biological molecules.
  • an immunogen includes a mixture of two or more such immunogens.
  • methods for lyophilization of biological molecules comprise dissolving the biological molecule in a dissolution buffer which comprises at least one amo ⁇ hous excipient and an amo ⁇ hous buffer to form a mixture, and then lyophilizing the mixture.
  • lyophilization includes loading the samples at 20°C, freezing the samples to about -50°C for about 2 hours, and drying at about -35°C for about 24 hours under about 25 microns of vacuum pressure and at a ramp rate of about 25°C per hour.
  • the biological molecule is a MenC immunogen.
  • the biological molecule is MenC-CRM 197.
  • This invention satisfies a long felt-need for compositions and methods for preparing biological molecules which reduce aggregation and minimize breakdown upon lyophilization.
  • the group C menningococcal polysaccharide is a 2-9 linked homopolymer of sialic acid (N-acetyl neuraminic acid) partially O-acetylated in position C7 and/or C8.
  • CRM 197 is a mutant of the wild-type diphtheria toxin (Constantino et al, Vaccine, 1992, Vol. 10, No. 10, 691-8). Replacement of the glycine present at amino acid position 52 with glutamic acid leads to complete loss of enzymatic activity.
  • the capsular polysaccharide of ' Neisseria meningitidis group C was hydrolyzed and the resulting oligosaccharide (OS) was coupled to CRM 197.
  • the coupling of CRM 197 to the capsular polysaccharide was based on selective end-reducing group activation of the oligosaccharide and subsequent coupling to the protein through a special spacer (Constantino et al, Vaccine, 1992, 10: 691-698).
  • the ratio of sialic acid to CRM 197 in the conjugate is about 0.6.
  • the average length of oligosaccharides was estimated by ion exchange chromatography (Mono-Q analysis, elution on Q Sepharose FFTM) as 14.2.
  • the K d of the oligosaccharide was between 0.33 and 0.41, and the free saccharide concentration was about 2.5%.
  • MenC conjugate vaccine lyophilized antigen obtained from Siena had the following composition: 12 ⁇ g (as measured by sialic acid content) of meningococcal C oligosaccharide antigen (Siena, Italy) conjugated to 19.7 ⁇ g of CRM 197, 9 mg of mannitol, and lOmM phosphate buffer, pH 7.2.
  • the lyophilized antigen Prior to administration, the lyophilized antigen is solubilized with 0.6 mL of aluminum hydroxide adjuvant. Of this solution, 0.5 mL is injected.
  • DSC Densilic Acid Deformation : The SII Seiko instrument with a Hewlett-Packard operating system was used to calculate DSC by analyzing additive crystallinity. Sample solutions of the excipient solutions were frozen at a ramp rate of 10°C/minute to a temperature of about -50°C. Using dry nitrogen as the atmosphere, thermal changes were monitored while warming samples at various ramp rates (0.625°C/minute to 10°C/minute). The effect of excipient composition on thermal change was assessed.
  • MenC Bulk Dialysis of MenC Bulk was performed using Spectra/Por Membrane ® (Spectrum Laboratories, Madison Hills, CA) with a 10,000 MW cutoff to replace the sodium phosphate buffer with the various buffers tested herein. Following dialysis, the MenC Bulk solution was diluted with various volumes of buffer and appropriate amounts of excipient to yield a desired protein concentration of 1.045 mg/mL. Sodium phosphate, histidine hydrochloride, and imidazole hydrochloride buffers, all pH 7.2, were used in the formulations. Buffer concentrations varied from 5 to 10 mM. Excipients used were mannitol, mannitol- sucrose mixtures, or sucrose.
  • Excipient concentrations were 1.5%, 3%, or 5%. In some formulations, Tween-80 ® was also added. After preparation, all formulated MenC Bulk solutions were filtered through 0.22 ⁇ m sterile Millipore filters and stored at 4°C.
  • Lyophilization The final product was prepared by lyophilization of the MenC Bulk.
  • the Freeze-Drying Cycle included several different stages and was different for mannitol (A*), mannitol-sucrose (B), and sucrose (C) formulations (see Table 1).
  • HPSEC High Performance Size Exclusion Chromatography analysis: TSK GEL R G4000SW XL columns (30cm x 7.8 mm inner diameter) (TosoHaas, Montgomeryville, PA), columns of small-particle hydrophilic gels for SEC (Size Exclusion Chromatography) separation in aqueous mobile phase were used for analysis of MenC-CRM 197 vaccine following lyophilization and solubilization. According to the instructions supplied by the manufacturer, the number of theoretical plates was greater than 16,000 and the asymmetry factor was from 0.7 to 1.6.
  • HPSEC analysis showed the retention times of 18.3 minutes and 22.8 minutes for MenC-CRM 197 (Siena) and MenC Bulk, respectively.
  • the recovery of MenC as measured with the fluorescence detector was about 95% (value calculated from 5 measurements for 10 ⁇ L injection volumes).
  • Increasing injection volume led to a proportional increase in the area of major peaks.
  • the reproducibility of injections was high with a standard error (standard deviation x 100/ Average peak area) less than 1%.
  • FIG. 1 A typical chromatogram of MenC-CRM 197 (lyophilized) is presented in Figure 1 , and shows a broad, non-symmetrical peak between 19-24 minutes (main peak). After sample stress, two additional peaks appeared; one related to the product with a higher molecular weight (an aggregation product) with a retention time between 15-17 minutes, and another with a lower molecular weight (fragmentation product) with a retention time over 24 minutes.
  • the flow rate was 0.5 mL/min.
  • pressure was between 350-400 psi.
  • Example 1 Freeze Experiment with pH indicator Eighteen different formulations were prepared to study the influence of the solution composition on the pH change during freezing. Table 2 shows the variations of phosphate buffer concentrations, excipient concentrations, and mannitol-sucrose ratio in these formulations. The initial pH value for all formulations was pH 7.2. The freeze experiment was performed in a lyophilizer chamber and included several steps. Samples were loaded into the lyophilizer chamber and held for 0.2 hours at 20°C. Samples were then cooled to -50°C with a ramp rate of 60°C/minute and then held at -50°C for 0.5 hours. Next, samples were warmed to -20°C with a ramp rate of 60°C/minute and held at -20°C for 0.5 hours.
  • phosphate buffers change pH during freezing from a temperature of 20°C (2) to -20°C (4).
  • the formulations containing either a mannitol or mannitol-sucrose mixture displayed fewer changes in pH (see Table 2).
  • pH was between about 5 and 5.5
  • pH was between about 6 to 6.5.
  • No significant changes in pH of the various formulations were observed during the initial 5 hours.
  • certain color changes took place after 34.5 hours, namely the appearance of orange and red spots at the interface of the yellow and orange solid.
  • the area of the red spots increased with time.
  • two salts, monosodium phosphate and disodium phosphate had different crystallization points, -9.7°C and -0.5°C, respectively.
  • phosphate buffers change pH during freezing from a temperature of 20°C (2) to -20°C (4).
  • the formulations containing either a mannitol or mannitol-sucrose mixture displayed fewer changes in pH (see Table 2).
  • pH was between about 5 and 5.5
  • pH was between about 6 to 6.5.
  • No significant changes in pH of the various formulations were observed during the initial 5 hours.
  • certain color changes took place after 34.5 hours, namely the appearance of orange and red spots at the interface of the yellow and orange solid.
  • the area of the red spots increased with time.
  • two salts, monosodium phosphate and disodium phosphate had different crystallization points, -9.7°C and -0.5°C, respectively.
  • Example 4 Replacement of the sodium phosphate buffer with amorphous buffer increases the stability of the MenC Bulk formulations.
  • the freeze drying cycle included a single freeze without annealing and primary drying at -35°C, a temperature lower than the glass transition temperature of sucrose. Because of the amo ⁇ hous state of the excipient during lyophilization, the total freeze cycle time was increased as was the vacuum pressure.
  • Table 3 demonstrate that aggregation during lyophilization was completely prevented. In control experiments, i.e., non- amo ⁇ hous buffers and/or excipients, aggregation was higher than that observed for test solutions. For example, aggregation was 3.3% in lOmM sodium phosphate buffer with sucrose and 9.5% in 1 OmM sodium phosphate buffer with mannitol. Aggregation was 0% in lOmM imidazole buffer with 1.5% sucrose and 0.78% in lOmM histidine buffer with 1.5% sucrose.
  • MenC-CRM 197 solid samples were stressed after lyophilization at 4°C, 25°C, or 37°C in an incubator for a period of 3 months. At selected time points, samples were removed from the incubator, reconstituted with 0.6 mL distilled water, and analyzed by HPSEC. All formulations were stable at 4°C, i.e., did not show an increase in aggregation upon storage. Samples of MenC-CRM 197 (Sienna) showed higher aggregation during stress testing than did formulations containing either imidazole or histidine buffers (Fig. 5). Use of the histidine or imidazole buffers in the MenC-CRM 197 formulation increased the vaccine stability. Although the inventors do not wish to be bound to this mechanism, it is thought that stabilization may be due to the interaction of the tryptophan of CRM 197 with the structurally similar imidazole ring.

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Abstract

The present invention is directed to compositions and methods for the preparation of biological molecules, in particular MenC-CRM 197. Biological molecules dissolved in dissolution buffers comprising at least one amorphous excipient and an amorphous buffer exhibit reduced aggregation and proteolytic breakdown.

Description

COMPOSITIONS AND METHODS FOR STABILIZING BIOLOGICAL MOLECULES UPON LYOPHILIZATION
FIELD OF THE INVENTION
The present invention relates to compositions and methods for stabilizing biological molecules upon lyophilization, and methods for lyophilizing biological molecules.
BACKGROUND OF THE INVENTION
Vaccines are widely used for the prevention and/or therapy of many different diseases. Meningococcal meningitis is one such disease for which prevention and/or therapy can be provided through a vaccine. The meningococcal meningitis vaccine utilizes the meningococcal polysaccharide (PS) which is of relatively low immunogenicity. To overcome the relatively low immunogenicity of meningococcus polysaccharide, PS vaccines are conjugated to protein carriers to increase immunogenicity and provide long-term protection in young children. One such vaccine ~ MenC-CRM 197 — against meningococcus C (MenC) has been prepared using CRM 197 as the protein carrier (Costantino et al, Vaccine, 1992, Vol. 10, No. 10: 691 -8).
Some problems are associated, however, with the use of the conjugate meningococcal polysaccharide vaccine MenC-CRM 197, and, indeed, with protein-containing vaccines in general. To extend the shelf-life of vaccines, formulations are frequently lyophilized. Lyophilization of MenC-CRM 197, however, can lead to protein aggregation during freezing and storage. In the case of MenC-CRM 197, the aggregates represent non- covalently bound, multimers of MenC-CRM 197 which apparently associate through hydrophobic interactions. The use of present dissolution buffer formulations, i.e., containing lOmM sodium phosphate (pH 7.2) as a buffer and 1.5% mannitol as an excipient, can yield aggregation as high as 9.5 to 10%. As aggregation increases, the concentration of available immunogen decreases. Therefore, a need exists for compositions and methods which overcome the problem of aggregation by stabilizing biological molecules against aggregation during lyophilization. 197 vaccine, is composed of two fragments, A and B, covalently bound to one another. Fragment A has been found to be stable and highly resistant to denaturation. Fragment B, however, is highly sensitive to denaturation and is subject to proteolytic breakdown during lyophilization. As proteolytic breakdown increases, the concentration of available functional immunogen decreases. Therefore, a further need exists for compositions and methods of preparation of biological molecules that will minimize breakdown during lyophilization and storage.
Although various theories exist that seek to explain and minimize aggregation and/or breakdown of biological molecules upon lyophilization, to date, no satisfactory techniques exist. Orii et al. report that glycerol and sugars protect biological materials from damage caused by freezing and thawing, presumably by minimizing pH changes (Orii et al, J. Biochem., 1977, 81 :163-168).
Arakawa et al. assessed the stabilization of proteins in aqueous solutions using various sugars (Arakawa et al, Biochemistry, 1982, 21 : 6536-6544). Arakawa et al. link the protection of component proteins in aqueous solution to the cohesive force of sugars which are responsible for the increase in the surface tension of the water. This factor, however, is not relevant in lyophilized solutions. Arakawa et al. do not address the stabilization of lyophilized solutions. Further, Arakawa et al. report that sucrose present in aqueous solutions actually decreases the activity of some enzymes. Pikal et al. report that excipients must remain at least partially amorphous to be effective in stabilizing a protein, but cautioned that an amorphous excipient is not a sufficient condition for stability enhancement and, indeed, observed that the addition of amoφhous excipients to protein solutions can actually destabilize the protein through molecular interactions between the excipient and protein (Pikal eta , Biopharm., 1990, 3, 26- 29.) Pikal et al. state that high levels of buffers are to be avoided as this is likely to lead to crystallization of one of the buffer components and a subsequent large pH shift during freezing and that even buffers that remain amoφhous are not suitable at high levels, as this normally lowers the collapse temperature and glass transition temperature of the dried material. The authors report that, in their experience, a low level of buffer tends to remain amoφhous yet does not dramatically affect the collapse temperature or glass transition temperature. Pikal et al, however, does not define high or low levels of buffer. In a later report al, however, Pikal et al. report that, based on reverse-phase HPLC, aggregation was at a maximum in 1.69 mM phosphate buffer while decomposition was at a minimum (Pikal et al, Pharm. Res., 1991, 8:427-436). The authors concluded, thus, that the level of phosphate buffer does not appear to be a relevant factor.
Izutsu et al. report that maintaining mannitol in an amoφhous state stabilizes β-galactosidase (Izutsu et /., Pharm. Res., 1993, Vol. 10, No. 8, 1232-1237). Izutsu et al. report that in 200 mM sodium phosphate buffer, mannitol, at 200-5 OOmM is amoφhous and acted to stabilize β-galactosidase. In 10 and 50 mM sodium phosphate buffer, mannitol at 50- lOOnM is amoφhous and exhibited a stabilizing effect. Izutsu et al. also report that glucose in sodium phosphate buffer protects enzyme activity, but does not provide any data on concentrations of glucose suitable to attain such an effect.
The protective effect of select amino acids on lyophilized enzyme solutions has also been tested (Seguro et al, Cryobiology, 1990, 27: 70-79). The protective effects of monosodium glutamate (MSG) and lysine hydrochloride (Lys-HCl) during lyophilization using lactate dehydrogenase in solution were assessed. Seguro et al note that the addition of either MSG or Lys-HCl to the enzyme solution reduces the loss of enzyme activity from about 40% (control using deionized water) to 20-25% (using MSG or Lys-HCl). The authors suggest that neither the salt concentration nor the ionic strength is important in the stabilization of the dissolved enzyme. Seguro et al. report that the most relevant factor in freeze denaturation is either the termination of supercooling phenomena produced by the additives, or the phase change from water to ice.
Procedures for lyophilization of various compositions have been described in several references (DeLuca, J. Vac. Sci. Technol., 1977, Vol. 14, No. 1, 620-629; DeLuca et al., J. Pharm. Sci., 1965, Vol. 54, No. 4, 617-624; Pikal et al, Biopharm., 1990, 3, 26- 29). The methods for lyophilizing described in these references include a series of cycles.
DeLuca et al. (1965) report that the eutectic temperature of a product is an important factor in the design of lyophilization cycles and that the eutectic temperatures for various organic and inorganic salts are similar (Table I). The authors state that other factors important in the design of lyophilization cycles include the supercooling effect and the thermal conductive property of the frozen mass. DeLuca et al. (1965) report that neither mannitol nor sucrose exert a significant effect on the solubility of organic salts or the eutectic temperature of the system. DeLuca et al. (1977) report that the eutectic point of the additive should not be lower than the drug as this will affect cycle times and suggests adding mono- and di-basic phosphate and sodium chloride to improve the characteristics of the finished cake. The authors conclude that it may be possible to optimize cycle time by determining the eutectic temperatures and the supercooling properties of the product. A need exists for compositions and methods for stabilizing biological molecules upon lyophilization.
SUMMARY OF THE INVENTION
The present invention arises from the suφrising discovery that it is possible to stabilize biological molecules against aggregation and breakdown during and following, i. e. "upon", lyophilization, using a dissolution buffer comprising an amoφhous excipient and an amoφhous buffer.
According to one aspect, the present invention provides a dissolution buffer comprising at least one amoφhous excipient, at least one amoφhous buffer, and at least one MenC immunogen. According to another aspect, the present invention provides a method for stabilizing one or more MenC immuogens upon lyophilization. The method comprises dissolving the MenC immuogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, and then lyophilizing the mixture.
In yet another aspect, the present invention provides a method for storing one or more MenC immunogens. The method comprises dissolving the MenC immunogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, and then lyophilizing the mixture.
In still another aspect, the present invention provides a method for lyophilization of a MenC immunogen. The method comprises dissolving a MenC immunogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, loading the mixture from about 10°C to about 20°C under from about 1000 Pa to about 2000 Pa of pressure, freezing the mixture from about 1 hour to about 4 hours to a temperature from about -70°C to about -50°C under from about 1000 Pa to about 2000 Pa of pressure, drying the mixture for from about 18 hours to about 30 hours at a temperature from about -50°C to about -35°C under a pressure from about 5 Pa to about 10 Pa, and drying the mixture for from 2 hours to about 12 hours at a temperature from about 10°C to about 20°C under a pressure from about 5 Pa to about 10 Pa.
In another aspect, the present invention provides a method for lyophilization o f a M e n C i m m u n o g e n . T h e m e t h o d c o m p r i s e s dissolving a MenC immunogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, loading the mixture at about 10°C under 1000 Pa of pressure, freezing the mixture for about 2 hours to a temperature of about -50°C under about 1000 Pa of pressure, drying the mixture for about 24 hours at a temperature of about -35°C under a pressure of about 5 Pa, and drying the mixture for about 8 hours at a temperature of about 20°C under a pressure of about 5 Pa.
In another aspect, the present invention provides a method for stabilizing a MenC vaccine upon lyophilization. The method comprises dissolving the MenC vaccine in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, and lyophilizing the mixture.
BRIEF DESCRIPTION OF THE DRAWINGS
Figure 1 depicts a chromatogram of MenC-CRM 197 obtained by Size Exclusion Chromatography (SEC). The main peak is seen between 19 and 24 minutes. A peak representing aggregation products is seen at about 15-17 minutes, and a peak representing fragmentation products is seen at greater than 24 minutes. Figures 2A-C depict Differential Scanning Calorimetry (DSC) diagrams of a mannitol buffer (A), a mannitol-sucrose buffer (B), and a sucrose buffer (C). Replacement of 25% of the mannitol with sucrose in the buffer resulted in a decrease of the re- crystallization peak and a shift of the glass transition temperatures.
Figure 3 depicts the effects of freeze temperature and presence of sucrose on the stability of MenC-CRM 197 formulation upon lyophilization as determined by percent recovery of MenC. MenC-CRM 197 exhibits greater stability in the presence of 5.0% sucrose when compared to formulations without sucrose.
Figures 4A-B show the effect of the excipient-buffer composition on the aggregation of MenC-CRM 197 as determined by Size Exclusion Chromatography. Figure 4A depicts the use of a lOmM sodium phosphate buffer containing varying amounts of mannitol and/or sucrose. Figure 4B depicts the use of a 5mM sodium phosphate buffer containing varying amounts of mannitol and/or sucrose. As the amount of amoφhous excipient, in this case sucrose, in the formulation increased, aggregation of MenC-CRM 197 decreased.
Figure 5 depicts the effect of stress (37°C) on the aggregation of MenC-CRM 197 as determined by Size Exclusion Chromatography. Formulations with amoφhous buffers (either histidine or imidazole) demonstrated less aggregation after prolonged incubation at 37°C than did formulations with non-amoφhous buffers (sodium phosphate buffer).
DETAILED DESCRIPTION OF THE INVENTION
The present invention provides buffer compositions, biological molecule compositions, and methods for the preparation and stabilization of biological molecules by reducing aggregation and breakdown of biological molecules upon lyophilization. The compositions and methods involve replacing the crystallizable (non- amoφhous) buffers and excipients with completely or partially amoφhous buffers and excipients.
As used herein, the phrase "dissolution buffer" refers to the solution in which the protein or proteins are dissolved for lyophilization. The "dissolution buffer" comprises at least one amoφhous excipient and at least one amoφhous buffer. In a preferred embodiment, the dissolution buffer further comprises a MenC immunogen. In a more preferred embodiment, the dissolution buffer further comprises MenC-CRM 197.
As used herein, the term "biological molecule" includes, but is not limited to, proteins, nucleic acids, and saccharides. Biological molecules may be used individually or in combination with other biological molecules. In a preferred embodiment of the present invention, the biological molecule is an immunogen. In a more preferred embodiment, the biological molecule is a MenC immunogen. In an even more preferred embodiment, the biological molecule is MenC-CRM 197. As used herein, the term "protein" refers to polypeptides, peptides, and analogs thereof. "Protein" also includes polypeptides and peptides which are conjugated to other biological molecules. In a preferred embodiment of the present invention, the protein is an immunogen.
As used herein, the term "immunogen" refers to any compound capable of eliciting a cellular and/or humoral immune response when in contact with a cell, and includes, without limitation, vaccines and compositions comprising immunogens. Preferably, an antibody response and a T cell response are elicited. Such immunogens would be expected to be useful in prophylactic and therapeutic applications as well as for research applications including the generation of antibodies.
As used herein, the term "nucleic acid" refers to oligonucleotides and polynucleotides, and includes DNA and RNA.
As used herein, the term "saccharides" includes oligosaccharides and polysaccharides.
As used herein, the phrase "amoφhous excipient" refers to an excipient which remains amoφhous upon lyophilization. Excipients which remain amoφhous under certain conditions but may crystallize under other conditions are included. Conditions which maintain the amoφhous nature of the excipient are included in the present invention. Amoφhous excipients are well known to those skilled in the art and include, without limitation, sugars, including sucrose, lactose, and, under conditions described herein, mannitol. Amoφhous excipients also may include, under conditions well known to those of skill in the art, without limitation, celluloses, especially sorbitol. The amoφhous excipients can be used either individually or as a mixture containing two or more different amoφhous excipients. In a preferred embodiment, the amoφhous excipient is sucrose. In a more preferred embodiment, the final sucrose concentration in the dissolution buffer is from about 1.5% to about 5%. As used herein, the phrase "MenC vaccine" refers to a vaccine comprises at least one MenC immunogen. In a preferred embodiment, the MenC vaccine comprises MenC- CRM 197.
As used herein, the phrase "amoφhous buffers" refers to buffers which remain amoφhous upon lyophilization, e.g., organic buffers. Buffers which remain amoφhous under certain conditions but may crystallize under other conditions are included. Conditions for maintaining the amoφhous nature of the buffer are also included. Amoφhous buffers are well known to those skilled in the art and include, without limitation, imidazole buffer and histidine buffer, piperidine, and diisopropylethylamine. In a preferred embodiment, the amoφhous buffer is imidazole buffer. In a further preferred embodiment, the amoφhous buffer is imidazole buffer and has a concentration of about 1 OmM.
As used herein, the term "stabilizing" is used synonymously with inhibiting, reducing, suppressing, decreasing, diminishing, and lowering aggregation and/or breakdown. The present invention includes methods that substantially inhibit aggregation and/or breakdown of biological molecules. Substantial inhibition of aggregation or breakdown refers to a reduction of aggregation or breakdown from about 25% to about 100% compared to controls which use crystallizable buffers and/or excipients. Preferably, aggregation or breakdown is inhibited by about 50%, more preferably by about 75%, and even more preferably by about 100%.
As used herein, the term "upon lyophilization" refers to the period during lyophilization of the biological molecules and during subsequent storage of the lyophilized biological molecules. As used in this specification and the appended claims, the singular forms "a",
"an", and "the" include plural references unless the content clearly dictates otherwise. Thus, for example, reference to "an immunogen" includes a mixture of two or more such immunogens.
In accordance with the present invention, methods for lyophilization of biological molecules are also provided. The methods comprise dissolving the biological molecule in a dissolution buffer which comprises at least one amoφhous excipient and an amoφhous buffer to form a mixture, and then lyophilizing the mixture. In one embodiment of the invention, lyophilization includes loading the samples at 20°C, freezing the samples to about -50°C for about 2 hours, and drying at about -35°C for about 24 hours under about 25 microns of vacuum pressure and at a ramp rate of about 25°C per hour. In a preferred embodiment, the biological molecule is a MenC immunogen. In a more preferred embodiment, the biological molecule is MenC-CRM 197. Through the practice of the present invention, the biological molecule is stabilized against aggregation and breakdown.
This invention satisfies a long felt-need for compositions and methods for preparing biological molecules which reduce aggregation and minimize breakdown upon lyophilization. By replacing non-amoφhous excipients and non-amoφhous buffers in the dissolution buffer with amoφhous excipients and amoφhous buffers, a reduction of aggregation and breakdown during lyophilization and subsequent storage is achieved. Materials and Methods
The following materials and methods were used unless otherwise noted.
The group C menningococcal polysaccharide (MenC) is a 2-9 linked homopolymer of sialic acid (N-acetyl neuraminic acid) partially O-acetylated in position C7 and/or C8. CRM 197 is a mutant of the wild-type diphtheria toxin (Constantino et al, Vaccine, 1992, Vol. 10, No. 10, 691-8). Replacement of the glycine present at amino acid position 52 with glutamic acid leads to complete loss of enzymatic activity. To prepare the conjugate, the capsular polysaccharide of 'Neisseria meningitidis group C was hydrolyzed and the resulting oligosaccharide (OS) was coupled to CRM 197. The coupling of CRM 197 to the capsular polysaccharide was based on selective end-reducing group activation of the oligosaccharide and subsequent coupling to the protein through a special spacer (Constantino et al, Vaccine, 1992, 10: 691-698). The ratio of sialic acid to CRM 197 in the conjugate is about 0.6. The average length of oligosaccharides was estimated by ion exchange chromatography (Mono-Q analysis, elution on Q Sepharose FF™) as 14.2. The Kd of the oligosaccharide was between 0.33 and 0.41, and the free saccharide concentration was about 2.5%.
MenC-CRM 197 Bulk Lot 1 ("MenC Bulk") consists of about 1.045 mg/mL CRM 197, and about 0.636 mg/mL MenC antigen (as measured by sialic acid content), in lOmM sodium phosphate buffer (pH=7.2) and is stored at 4°C. All MenC-CRM 197 solutions disclosed herein were filtered through 0.22 μm sterile Millipore™ filters before testing. The bulk solution is diluted before lyophilization.
MenC conjugate vaccine lyophilized antigen (MenC-CRM 197) obtained from Siena had the following composition: 12 μg (as measured by sialic acid content) of meningococcal C oligosaccharide antigen (Siena, Italy) conjugated to 19.7 μg of CRM 197, 9 mg of mannitol, and lOmM phosphate buffer, pH 7.2. Prior to administration, the lyophilized antigen is solubilized with 0.6 mL of aluminum hydroxide adjuvant. Of this solution, 0.5 mL is injected.
DSC (Differential Scanning Calorimetry): The SII Seiko instrument with a Hewlett-Packard operating system was used to calculate DSC by analyzing additive crystallinity. Sample solutions of the excipient solutions were frozen at a ramp rate of 10°C/minute to a temperature of about -50°C. Using dry nitrogen as the atmosphere, thermal changes were monitored while warming samples at various ramp rates (0.625°C/minute to 10°C/minute). The effect of excipient composition on thermal change was assessed.
Dialysis of MenC Bulk was performed using Spectra/Por Membrane® (Spectrum Laboratories, Laguna Hills, CA) with a 10,000 MW cutoff to replace the sodium phosphate buffer with the various buffers tested herein. Following dialysis, the MenC Bulk solution was diluted with various volumes of buffer and appropriate amounts of excipient to yield a desired protein concentration of 1.045 mg/mL. Sodium phosphate, histidine hydrochloride, and imidazole hydrochloride buffers, all pH 7.2, were used in the formulations. Buffer concentrations varied from 5 to 10 mM. Excipients used were mannitol, mannitol- sucrose mixtures, or sucrose. Excipient concentrations were 1.5%, 3%, or 5%. In some formulations, Tween-80® was also added. After preparation, all formulated MenC Bulk solutions were filtered through 0.22 μm sterile Millipore filters and stored at 4°C.
Lyophilization: The final product was prepared by lyophilization of the MenC Bulk. The Freeze-Drying Cycle included several different stages and was different for mannitol (A*), mannitol-sucrose (B), and sucrose (C) formulations (see Table 1).
HPSEC (High Performance Size Exclusion Chromatography) analysis: TSK GELR G4000SWXL columns (30cm x 7.8 mm inner diameter) (TosoHaas, Montgomeryville, PA), columns of small-particle hydrophilic gels for SEC (Size Exclusion Chromatography) separation in aqueous mobile phase were used for analysis of MenC-CRM 197 vaccine following lyophilization and solubilization. According to the instructions supplied by the manufacturer, the number of theoretical plates was greater than 16,000 and the asymmetry factor was from 0.7 to 1.6.
HPSEC analysis showed the retention times of 18.3 minutes and 22.8 minutes for MenC-CRM 197 (Siena) and MenC Bulk, respectively. The recovery of MenC as measured with the fluorescence detector was about 95% (value calculated from 5 measurements for 10 μL injection volumes). Increasing injection volume led to a proportional increase in the area of major peaks. The reproducibility of injections was high with a standard error (standard deviation x 100/ Average peak area) less than 1%. The accuracy of 10 injections (each 20 μL) from different vials was also high (average value = 19.83 μL, standard deviation = 0.085 μL). The minimum injection volume (standard deviation = 0.1 μL from 20 μL) was found to be 35 μL. A typical chromatogram of MenC-CRM 197 (lyophilized) is presented in Figure 1 , and shows a broad, non-symmetrical peak between 19-24 minutes (main peak). After sample stress, two additional peaks appeared; one related to the product with a higher molecular weight (an aggregation product) with a retention time between 15-17 minutes, and another with a lower molecular weight (fragmentation product) with a retention time over 24 minutes. For the column chromatography the flow rate was 0.5 mL/min. , pressure was between 350-400 psi., the mobile phase was 100 mM phosphate buffer (pH= 7.2) with 200 mM (NH4)2SO4 (HPLC grade, Bio-Rad), at room temperature. Sample emissions were detected with the UN detector at 214 nm and fluorescence detector at 280 run Ex. and 340 nm Em. A gel filtration standard containing Gamma-globulin, ovalbumin, myoglobin, and vitamin B- 12 (Bio-Rad) was used as a standard. Analysis was performed using a two-pump Waters 510 HPLC system consisting of a Waters Automated Gradient Controller and Model 510 pumps, a Waters 486 Tuneable Absorbance Detector, a Waters 712 WISP injection system, and a Hitachi Fl Detector L-7480 with a Xe lamp. The following examples are meant to illustrate the invention and are not to be construed to limit the invention in any way. Those skilled in the art will recognize modifications that are within the spirit and scope of the invention.
EXAMPLES
Example 1: Freeze Experiment with pH indicator Eighteen different formulations were prepared to study the influence of the solution composition on the pH change during freezing. Table 2 shows the variations of phosphate buffer concentrations, excipient concentrations, and mannitol-sucrose ratio in these formulations. The initial pH value for all formulations was pH 7.2. The freeze experiment was performed in a lyophilizer chamber and included several steps. Samples were loaded into the lyophilizer chamber and held for 0.2 hours at 20°C. Samples were then cooled to -50°C with a ramp rate of 60°C/minute and then held at -50°C for 0.5 hours. Next, samples were warmed to -20°C with a ramp rate of 60°C/minute and held at -20°C for 0.5 hours. Samples were cooled to -50°C with a ramp rate of 60°C/minute and then warmed to -20°C with a ramp rate of 60°C/minute. Following freeze-drying, pH measurements were taken at various time points and temperatures. The experiment was performed with a universal pH indicator that changed color with pH change. Each color was related to the relevant pH. pH measurements were taken at time zero at 20°C (point 1), after 3 hours at -20°C (point 2), after 4 hours at -50°C (point 3), and after 5 hours at -20°C (point 4). Samples were held at -20°C overnight and the next measurements were taken at -20°C after 34.5 hours (point 5). A statistical study of 144 vials containing various formulations (8 vials for each formulation; 18 formulations) was performed at -20°C after 34.5 hours.
It is known that phosphate buffers change pH during freezing from a temperature of 20°C (2) to -20°C (4). The formulations containing either a mannitol or mannitol-sucrose mixture displayed fewer changes in pH (see Table 2). At -50°C, pH was between about 5 and 5.5, and at -20°C, pH was between about 6 to 6.5. No significant changes in pH of the various formulations were observed during the initial 5 hours. However, certain color changes took place after 34.5 hours, namely the appearance of orange and red spots at the interface of the yellow and orange solid. The area of the red spots increased with time. This observation demonstrated that the crystallization of phosphate salts was a slow and random process. Further, two salts, monosodium phosphate and disodium phosphate, had different crystallization points, -9.7°C and -0.5°C, respectively.
Statistical study of the pH changes during freezing indicated that the observations could be divided into 3 groups:
Group 1 pH 6.0 Yellow pH 6.0 and spots with pH 5.5
Group 2 pH 5.5
Orange pH 5.5 and greater than 5 spots with pH 5.0
Group 3 pH 5.0
Red pH 5.0- 5.5 and greater than 5 spots with pH 5.0 The percentage of the samples belonging to each group was calculated using the formula: % = n x 100/N, where n was the number of samples in each group and N was the total number of samples analyzed (in this case N=8) (see Table 2).
The statistical analysis presented in Table 2 showed that, to a large extent, the formulations containing mannitol belonged to Groups 2 and 3 while the formulations with a high sucrose content belonged to Group 1. Thus, replacement of a portion of the mannitol color with pH change. Each color was related to the relevant pH. pH measurements were taken at time zero at 20°C (point 1), after 3 hours at -20°C (point 2), after 4 hours at -50°C (point 3), and after 5 hours at -20°C (point 4). Samples were held at -20°C overnight and the next measurements were taken at -20°C after 34.5 hours (point 5). A statistical study of 144 vials containing various formulations (8 vials for each formulation; 18 formulations) was performed at -20°C after 34.5 hours.
It is known that phosphate buffers change pH during freezing from a temperature of 20°C (2) to -20°C (4). The formulations containing either a mannitol or mannitol-sucrose mixture displayed fewer changes in pH (see Table 2). At -50°C, pH was between about 5 and 5.5, and at -20°C, pH was between about 6 to 6.5. No significant changes in pH of the various formulations were observed during the initial 5 hours. However, certain color changes took place after 34.5 hours, namely the appearance of orange and red spots at the interface of the yellow and orange solid. The area of the red spots increased with time. This observation demonstrated that the crystallization of phosphate salts was a slow and random process. Further, two salts, monosodium phosphate and disodium phosphate, had different crystallization points, -9.7°C and -0.5°C, respectively.
Statistical study of the pH changes during freezing indicated that the observations could be divided into 3 groups:
Group 1 pH 6.0 Yellow pH 6.0 and spots with pH 5.5
Group 2 pH 5.5
Orange pH 5.5 and greater than 5 spots with pH 5.0
Group 3 pH 5.0
Red pH 5.0- 5.5 and greater than 5 spots with pH 5.0 The percentage of the samples belonging to each group was calculated using the formula: % = n x 100/N, where n was the number of samples in each group and N was the total number of samples analyzed (in this case N=8) (see Table 2).
The statistical analysis presented in Table 2 showed that, to a large extent, the formulations containing mannitol belonged to Groups 2 and 3 while the formulations with a high sucrose content belonged to Group 1. Thus, replacement of a portion of the mannitol with sucrose resulted in fewer pH changes. The more sucrose present in the formulation resulted in a smaller pH change. The most notable results were obtained for either 1.5% excipients, (with either 80%, 90%, or 100% mannitol) in lOmM phosphate buffer, and 5% excipients (with 80% or 90% mannitol) containing sucrose in 5mM phosphate buffer, each of which lead to 100% of the samples falling into the yellow group .
Addition of inert organic compounds such as mannitol and sucrose decreased the pH changes of the phosphate buffer. Such an effect of these additives might be related to the increased viscosity of the formulation which might inhibit crystal growth and precipitation of the phosphate salts. Because visco-elastic properties of the solution could affect the temperature of crystallization (5) , the properties prevented crystallization of the salt upon cooling giving a supercooled liquid dispersed within an ice crystal meshwork.
Example 2: Effect of Buffer Selection on Recrystallization
It has been reported that mannitol in water shows an exothermic peak at about -25°C due to the crystallization of mannitol (Gatlin et α/., J. Parent. Drug. Assoα, 1980, 344:398- 408). In the presence of sodium phosphate buffer, the exothermic peak temperature differed from that in aqueous solution (Williams et al, J. Parent Sci. Tech., 1991, 45:94-100; Seguro et al, Cryobiology, 1990, 27: 70-79). The thermal behavior differences observed might be related to the changes in crystallinity (Izutsu et al, Pharm. Res., 1993, 10, No. 8, 1232- 1237). The DSC diagram in Figures 2A-C show that a 3% mannitol solution in lOmM sodium phosphate buffer, pH 7.2, caused exothermic re-crystallization at -23.5°C (ΔH= - 7735.2 mJ/mg) and endothermic glass transition at -32°C (ΔCp=351mJ/deg.mg) and -30.1°C (ΔCp=442mJ/deg.mg) (Figures 2a and 2b). Replacement of 25% of the mannitol with sucrose resulted in a decrease of the re-crystallization peak (ΔH= -2572 mJ/mg) and a shift of the glass transition temperatures to -41.4°C (ΔCp=6.7mJ/deg.mg) and -31.0°C (ΔCp=93mJ/deg.mg). Thermal analysis of the sucrose solution (Figure 2C) in the sodium phosphate buffer showed only the glass transition at -29.2°C (ΔCp=289.8mJ/deg.mg). Thus, the addition of sucrose to the crystallizable mannitol solution resulted in the formation of amoφhous mannitol during cooling and prevented crystallization. Example 3: Stabilization of MenC Bulk with sucrose
Stabilization of MenC Bulk with sucrose was shown in a freeze experiment (Fig. 3). Fourteen formulations of MenC Bulk were prepared as described above with various amoφhous excipient compositions and phosphate buffer concentrations (Table 3). The formulations were lyophilized according to method B (see Table 1). The lyophilization included freezing with annealing as previously developed by Siena, Italy (Caφenter et al, 1988, 25: 244-255). The suppression of aggregation during lyophilization as determined by Size Exclusion Chromatography was used to gauge stabilization. As shown in Figure 4, suppression of aggregation was found to be directly related to the sucrose content.
Example 4: Replacement of the sodium phosphate buffer with amorphous buffer increases the stability of the MenC Bulk formulations.
Histidine-histidine hydrochloride and imidazole-imidazole hydrochloride solutions, both pH 7.2, were used as buffers. Pure sucrose without mannitol was used to stabilize the protein. Various formulations were tested in an attempt to stabilize MenC Bulk. These formulations were lyophilized according to method C (see Table 1).
The freeze drying cycle included a single freeze without annealing and primary drying at -35°C, a temperature lower than the glass transition temperature of sucrose. Because of the amoφhous state of the excipient during lyophilization, the total freeze cycle time was increased as was the vacuum pressure. The results presented in Table 3 demonstrate that aggregation during lyophilization was completely prevented. In control experiments, i.e., non- amoφhous buffers and/or excipients, aggregation was higher than that observed for test solutions. For example, aggregation was 3.3% in lOmM sodium phosphate buffer with sucrose and 9.5% in 1 OmM sodium phosphate buffer with mannitol. Aggregation was 0% in lOmM imidazole buffer with 1.5% sucrose and 0.78% in lOmM histidine buffer with 1.5% sucrose.
Example 5: Stability study
MenC-CRM 197 solid samples were stressed after lyophilization at 4°C, 25°C, or 37°C in an incubator for a period of 3 months. At selected time points, samples were removed from the incubator, reconstituted with 0.6 mL distilled water, and analyzed by HPSEC. All formulations were stable at 4°C, i.e., did not show an increase in aggregation upon storage. Samples of MenC-CRM 197 (Sienna) showed higher aggregation during stress testing than did formulations containing either imidazole or histidine buffers (Fig. 5). Use of the histidine or imidazole buffers in the MenC-CRM 197 formulation increased the vaccine stability. Although the inventors do not wish to be bound to this mechanism, it is thought that stabilization may be due to the interaction of the tryptophan of CRM 197 with the structurally similar imidazole ring.
All references cited herein are hereby incoφorated by reference in their entirety.
Table 1 Lyophilization process for MenC CRM 197 Formulations
Process step Total process time Shelf Temperature Pressure hr °C Pascals (Pa)
Loading A* 0.0 20 1000
B 0.0 20 1000
C 0.2 10 1000
Freezing 1 A* 2.0 -55 1000
B 1.0 -50 1000
C 2.0 -50 1000
Annealing A* 2.0 -24 1000
B 2.0 -25 1000
Freezing II A* 3 -37 1000
B 1.0 -50 1000
Primary drying A* 15 37 21
1.0 -37 1.5
B 24.0 -20 10
C 24.0 -35 5
Secondary drying A* 2.0 30 1.5
B 8.0 20 10
C 8.0 20 5
A* -previously developed by Biocine Freezing ramp -60βC/h, drying ramp - 25βC/h
Special steps are pre-aeration (Nj/air, pressure 0.85 bar), stoppering, aeration (N2/air), and storage at 4°C.
A= Freeze-Drying Cycle for mannitol ^
B= Freeze-Drying Cycle for mannitol-sucrose
C= Freeze-Drying Cycle for sucrose Table 2 The pH changes during the freeze experiment with pH indicator
Formulation pH Yellow group samples, %
% % Excipient mM 0 3 h 4h 5h 34.5h Mannitol P04
20°C -20 -50 -20 -20
100 1.5 10 7 6 5 6 6(5.5)* 100
100 1.5 5 7 6 5.5 6-5.5 6(5.5)* 78
90 1.5 10 7 6 5.5 6.5-6 6(5.5)* 100
90 1.5 5 7 6 5 6 6.5-5(6)* 100
80 1.5 10 7 6 5 6 6(5.5)* 100
80 1.5 5 7 6 5 6.5 6 100
100 3 10 7 6(5.5)* 5 6-5.5 6 50
100 3 5 7 6(5.5)* 5.5 6 6 63
90 3 10 7 6 6-5.5 6-5.5 7(5)* 25
90 3 6 7 6 5 <6 6(5.5-5)* 87
80 3 10 7 6 5 6 6 75
80 3 5 7 6 5.5-6 6 6.5-6(6)* 90
100 5 10 7 6(5.5)* 5.5 6-5.5 6 77
100 5 5 7 6 5.5 6.5 ? 25
90 5 10 7 6 5 6.5 6(5.5) 37
90 5 5 7 6 5 6.5-6 6.5(5.5)* 100
80 5 10 7 6(5.5)* 5.5 6.5 6.5-6 88
80 5 5 7 6 5.5 6 6 100
The pH value for spots on the surface of solid sample Table 3 Aggregation of Imidazole and Histidine formulation of MenC-CRM 197 vaccine under lyophilization
# Formulation % Aggregation product
1 10 mM Imidazole, 1.5% sucrose 0 la 10 mM Imidazole, 1.5% sucrose, 0.05% Tween 80 0
2 10 mM Imidazole, 3% sucrose 0.21 2a 10 mM Imidazole, 3% sucrose, 0.05% Tween 80 0
3 10 mM Imidazole, 5% sucrose 0 3a 10 mM Imidazole, 5% sucrose, 0.05% Tween 80 0
4a 10 mM Histidine, 1.5% sucrose, 0.05% Tween 80 0
4 10 mM Histidine, 1.5% sucrose 0
5 lOmM Histidine 3% sucrose 0.78 5a 1 OmM Histidine, 3% sucrose, 0.05% Tween 80 0
6 10 mM Histidine, 5% sucrose 0 6a 10 mM Histidine, 5% sucrose, 0.05% Tween 80 0
Control: 10 mM NaPO4, pH 7.2, 1.5% sucrose 3.3
Siena: 10 mM NaPO4, pH 7.2, 1.5% mannitol 9.5%

Claims

ClaimsWe claim:
1. A dissolution buffer comprising at least one amoφhous excipient, at least one amoφhous buffer, and at least one MenC immunogen.
2. The dissolution buffer of claim 1 wherein the amoφhous buffer is an organic buffer.
3. The dissolution buffer of claim 2 wherein the organic buffer is selected from the group consisting of imidazole buffer and histidine buffer.
4. The dissolution buffer of claim 1 wherein the amoφhous excipient is a sugar.
5. The dissolution buffer of claim 4 wherein the sugar is sucrose.
6. The dissolution buffer of claim 1 wherein the MenC immunogen is MenC-CRM 197.
7. A method for stabilizing one or more MenC immunogens upon lyophilization comprising;
(a) dissolving the MenC immunogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, and (b) lyophilizing the mixture.
8. The method of claim 7 wherein the MenC immunogen is MenC-CRM 197.
9. A lyophilized composition stabilized according to the method of claim 7 comprising at least one amoφhous excipient, at least one amoφhous buffer, and at least one MenC immunogen.
10. A method for storing one or more MenC immunogens comprising;
(a) dissolving the MenC immunogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, and (b) lyophilizing the mixture.
11. The method of claim 10 wherein the MenC immunogen is MenC-CRM 197.
12. A method for lyophilization of a MenC immunogen comprising; dissolving a MenC immunogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture; loading the mixture from about 10°C to about 20°C under from about 1000 Pa to about 2000 Pa of pressure; freezing the mixture from about 1 hour to about 4 hours to a temperature from about -70°C to about -50°C under from about 1000 Pa to about 2000 Pa of pressure; drying the mixture for from about 18 hours to about 30 hours at a temperature from about -50°C to about -35°C under a pressure from about 5 Pa to about 10 Pa; and drying the mixture for from 2 hours to about 12 hours at a temperature from about 10°C to about 20°C under a pressure from about 5 Pa to about 10 Pa.
13. The method of claim 12 wherein the MenC immunogen is MenC-CRM 197.
14. A method for lyophilization of a MenC immunogen comprising; dissolving a MenC immunogen in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture; loading the mixture at about 10°C under 1000 Pa of pressure; freezing the mixture for about 2 hours to a temperature of about -50°C under about 1000 Pa of pressure; drying the mixture for about 24 hours at a temperature of about -35°C under a pressure of about 5 Pa; and drying the mixture for about 8 hours at a temperature of about 20°C under a pressure of about 5 Pa.
15. The method of claim 14 wherein the immunogen is Men C-CRM 197.
16. A method for stabilizing a MenC vaccine upon lyophilization comprising; (a) dissolving the MenC vaccine in a dissolution buffer comprising at least one amoφhous excipient and an amoφhous buffer to form a mixture, and
(b) lyophilizing the mixture.
17. The method of claim 16 wherein the MenC vaccine is MenC-CRM 197.
18. A MenC vaccine stabilized according to the method of claim 16 comprising at least one amoφhous excipient and at least one amoφhous buffer.
PCT/US2000/042484 1999-12-02 2000-12-01 Compositions and methods for stabilizing biological molecules upon lyophilization WO2001041800A2 (en)

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CA2393298A1 (en) 2001-06-14
CY1108382T1 (en) 2014-02-12
CA2393298C (en) 2011-02-01
WO2001041800A9 (en) 2002-08-01
EP2292263A2 (en) 2011-03-09

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