AU701440B2 - Spray-dried microparticles as therapeutic vehicles - Google Patents
Spray-dried microparticles as therapeutic vehicles Download PDFInfo
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- AU701440B2 AU701440B2 AU35302/95A AU3530295A AU701440B2 AU 701440 B2 AU701440 B2 AU 701440B2 AU 35302/95 A AU35302/95 A AU 35302/95A AU 3530295 A AU3530295 A AU 3530295A AU 701440 B2 AU701440 B2 AU 701440B2
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- Prior art keywords
- microparticles
- water
- microparticles according
- microcapsules
- particles
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Classifications
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- A61K9/0012—Galenical forms characterised by the site of application
- A61K9/007—Pulmonary tract; Aromatherapy
- A61K9/0073—Sprays or powders for inhalation; Aerolised or nebulised preparations generated by other means than thermal energy
- A61K9/0075—Sprays or powders for inhalation; Aerolised or nebulised preparations generated by other means than thermal energy for inhalation via a dry powder inhaler [DPI], e.g. comprising micronized drug mixed with lactose carrier particles
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- A61K49/22—Echographic preparations; Ultrasound imaging preparations ; Optoacoustic imaging preparations
- A61K49/222—Echographic preparations; Ultrasound imaging preparations ; Optoacoustic imaging preparations characterised by a special physical form, e.g. emulsions, liposomes
- A61K49/223—Microbubbles, hollow microspheres, free gas bubbles, gas microspheres
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- A61K9/14—Particulate form, e.g. powders, Processes for size reducing of pure drugs or the resulting products, Pure drug nanoparticles
- A61K9/16—Agglomerates; Granulates; Microbeadlets ; Microspheres; Pellets; Solid products obtained by spray drying, spray freeze drying, spray congealing,(multiple) emulsion solvent evaporation or extraction
- A61K9/1682—Processes
- A61K9/1688—Processes resulting in pure drug agglomerate optionally containing up to 5% of excipient
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- A—HUMAN NECESSITIES
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- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/14—Particulate form, e.g. powders, Processes for size reducing of pure drugs or the resulting products, Pure drug nanoparticles
- A61K9/16—Agglomerates; Granulates; Microbeadlets ; Microspheres; Pellets; Solid products obtained by spray drying, spray freeze drying, spray congealing,(multiple) emulsion solvent evaporation or extraction
- A61K9/1682—Processes
- A61K9/1694—Processes resulting in granules or microspheres of the matrix type containing more than 5% of excipient
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- A61K9/48—Preparations in capsules, e.g. of gelatin, of chocolate
- A61K9/50—Microcapsules having a gas, liquid or semi-solid filling; Solid microparticles or pellets surrounded by a distinct coating layer, e.g. coated microspheres, coated drug crystals
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- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/48—Preparations in capsules, e.g. of gelatin, of chocolate
- A61K9/50—Microcapsules having a gas, liquid or semi-solid filling; Solid microparticles or pellets surrounded by a distinct coating layer, e.g. coated microspheres, coated drug crystals
- A61K9/5089—Processes
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- A—HUMAN NECESSITIES
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- Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
Description
WO 96/09814 PCT/GB95/02279 1 SPRAY-DRIED MICROPARTICLES AS THERAPEUTIC VEHICLES Field of the Invention This invention relates to spray-dried microparticles and their use as therapeutic vehicles. In particular, the invention relates to means for delivery of diagnostic and therapeutic agents and biotechnology products, including therapeutics based upon rDNA technology.
Background of the Invention The most commonly used route of administration of therapeutic agents, oral or gastrointestinal, is largely inapplicable to peptides and proteins derived from the rDNA industry. The susceptibility of normally blood-borne peptides and proteins to the acidic/proteolytic environment of the gut, largely precludes this route for administration. The logical means of administration is intravenous, but this presents problems of poor patient compliance during chronic administration and very often rapid first-pass clearance by the liver, resulting in short iv lifetimes.
Recently, the potential for delivery by mucosal transfer has been explored. Whilst nasal delivery has been extensively explored, the potential delivery of peptides via the pulmonary airways is largely unexplored.
Alveolar cells, in their own right, provide an effective barrier. However, even passage of material to the alveolar region represents a significant impediment to this method of administration. There is an optimal size of particle which will access the lowest regions of the pulmonary airways, i.e. an aerodynamic diameter of <5 Am.
Particles above this size will be caught by impaction in the upper airways, such that in standard commercial suspension preparations, only 10-30% of particles, from what are normally polydispersed suspensions, reach the lowest airways.
Current methods of aerosolising drugs for inhalation include nebulisation, metered dose inhalers and dry powder systems. Nebulisation of aqueous solutions requires large WO 96/09814 PCT/GB95/02279 2 volumes of drugs and involves the use of bulky and nonportable devices.
The most common method of administration to the lung is by the use of volatile propellant-based devices, commonly termed metered dose inhalers. The basic design is a solution of propellant, commonly CFC 11, 12 or 114, containing either dissolved drug or a suspension of the drug in a pressurised canister. Dosing is achieved by depressing an actuator which releases a propellant aerosol of drug suspension or solution which is carried on the airways. During its passage to the lung, the propellant evaporates to yield microscopic precipitates from solution or free particles from suspension. The dosing is fairly reproducible and cheap, but there is growing environmental pressure to reduce the use of CFCs. Furthermore, the use of CFC solvents remains largely incompatible with many of the modern biotechnology drugs, because of their susceptibility to denaturation and low stability.
Concurrently, there is a move toward dry powder devices which consist of dry powders of drugs usually admixed with an excipient, such as lactose or glucose, which facilitates the aerosolisation and dispersion of the drug particles. The energy for disaggregation is often supplied by the breath or inspiration of air through the device.
Drugs are currently micronised, to reduce particle size. This approach is not applicable for biotechnology products. In general, biotechnology products are available in low quantity and, furthermore, are susceptible to the methods currently employed to dry and micronise prior to mixing with excipient. Further, it is particularly difficult to provide blends of drug and excipient which are sufficiently free-flowing that they flow and dose reproducibly in the modern multiple dose inhalers such as the Turbohaler (Astra) and Diskhaler (Glaxo). Studies have revealed that, contrary to expectation, spray-dried (spherical) salbutamol microparticles showed greater forces WO 96/09814 PCT/GB95/02279 3 of cohesion and adhesion than similarly-sized particles of micronised drug. Electron micrographs of the spray-dried material revealed the particles to possess pitted, rough surfaces.
Haghpanah et al reported, at the 1994 British Pharmaceutical Conference, that albumin microparticles incorporating salbutamol, had been produced by spray-drying and were of a suitable size for respiratory drug delivery, i.e. 1-5 gm. The aim was to encapsulate salbutamol, for slow release. It does not appear that the product is of substantially uniformly spherical or smooth microparticles that have satisfactory flow properties, for multi-dose dry powder inhalers.
Diagnostic agents comprising hollow microcapsules have been used to enhance ultrasound imaging. For example, EP- A-458745 (Sintetica) discloses a process of preparing airor gas-filled microballoons by interfacial polymerisation of synthetic polymers such as polylactides and polyglycolides. WO-A-9112823 (Delta) discloses a similar process using albumin. Wheatley et al (1990) Biomaterials 11:713-717, disclose ionotropic gelation of alginate to form microbubbles of over 30 gm diameter. WO-A-9109629 discloses liposomes for use as ultrasound contrast agents.
Przyborowski et al, Eur. J. Nucl. Med. 7:71-72 (1982), disclose the preparation of human serum albumin (HSA) microspheres by spray-drying, for radiolabelling, and their subsequent use in scintigraphic imaging of the lung. The microspheres were not said to be hollow and, in our repetition of the work, predominantly poorly formed solid microspheres are produced. Unless the particles are hollow, they are unsuitable for echocardiography.
Furthermore, the microspheres were prepared in a one-step process which we have found to be unsuitable for preparing microcapsules suitable for echocardiography; it was necessary in the prior process to remove undenatured albumin from the microspheres, and a wide size range of WO 96/09814 PCT/GB95/02279 4 microspheres was apparently obtained, as a further sieving step was necessary.
Przyborowski et al refer to two earlier disclosures of methods of obtaining albumin particles for lung scintigraphy. Aldrich Johnston (1974) Int. J. Appl. Rad.
Isot. 25:15-18, disclose the use of a spinning disc to generate 3-70 gm diameter particles which are then denatured in hot oil. The oil is removed and the particles labelled with radioisotopes. Raju et al (1978) Isotopenpraxis 14(2):57-61, used the same spinning disc technique but denatured the albumin by simply heating the particles. In neither case were hollow microcapsules mentioned, and the particles prepared were not suitable for echocardiography.
EP-A-0606486 (Teijin) describes the production of powders in which an active agent is incorporated into small particles, with carriers comprised of cellulose or cellulose derivatives. The intention is to prevent drug particles from adhering to the gelatin capsules used in a unit dose dry powder inhaler. Page 12 of this publication refers to the spray-drying of "medicament and base", to obtain particles of which 80% or more were 0.5-10 jm in size. No directions are given as to what conditions should be used, in order to obtain such a product.
EP-A-0611567 (Teijin) is more specifically concerned with the production of powders for inhalation, by spraydrying. The carrier is a cellulose, chosen for its resistance to humidity. The conditions that are given in Example 1 (ethanol as solvent, 2-5% w/v solute) mean that there is no control of surface morphology, and Example 4 reports a poor lower airway respirable fraction indicating poor dispersion properties. Spherical particles are apparently obtained at high drug content, indicating that particle morphology is governed by the respective drug and carrier contents.
Conte et al (1994) Eur. J. Pharm. Biopharm. 40(4):203- 208, disclose spray-drying from aqueous solution, with a WO 96/09814 PCT/GB95/02279 maximum solute concentration of High drug content is required, in order to obtain the most nearly spherical particles. This entails shrunken and wrinkled particle morphology. Further, after suspension in butanol, to facilitate Coulter analysis, sonication is apparently necessary, implying that the particles are not fully dry.
It is an object behind the present invention to provide a therapeutic delivery vehicle and a composition that are better adapted than products of the prior art, for delivery to the alveoli in particular.
Summary of the Invention According to the present invention, it has surprisingly been found that, in microparticles (and also microcapsules and microspheres) that are also suitable as an intermediate product, i.e. before fixing, in the production of air-containing microcapsules for diagnostic imaging, e.g. as disclosed in WO-A-9218164 as "intermediate microcapsules", the wall-forming material is substantially unaffected by spray-drying. Thus, highly uniform microparticles, microspheres or microcapsules of heatsensitive materials such as enzymes, peptides and proteins, e.g. HSA, and other polymers, may be prepared and formulated as dry powders, for therapeutic or diagnostic use.
By contrast to the prior art, it has also now been found that effective, soluble carriers for therapeutic and diagnostic agents can be prepared, by spray-drying, and which are free-flowing, smooth, spherical microparticles of water-soluble material, e.g. human serum albumin (HSA), having a mass median particle size of 1 to 10 mm. More generally, a process for preparing microcapsules of the invention comprises atomising a solution (or dispersion) of a wall-forming material. A therapeutic or diagnostic agent may be atomised therewith, or coupled to the microcapsules thus produced. Alternatively, the material may be an active agent itself. In particular, it has been found that, under the conditions stated herein, and more WO 96/09814 PCT/GB95/02279 6 generally described by Sutton et al (1992), e.g. using an appropriate combination of higher solute concentrations and higher air:liquid flow ratios than Haghpanah et al, and shell-forming enhancers, remarkably smooth spherical microparticles of various materials may be produced. The spherical nature of the microparticles can be established by means other than mere maximum size analysis, i.e. the laser light diffraction technique described by Haghpanah et al. Moreover, the particle size and size distribution of the product can be controlled within a tighter range, and with greater reproducibility. For example, by Coulter analysis, 98% of the particles can be smaller than 6 Am on a number basis, within an interquartile range of 2 Am, and with less than 0.5 Am mean size variation between batches.
Furthermore, when tested in a dry powder inhaler under development, reproducible dosing was achieved, and subsequent aerosolisation under normal flow conditions 1/min) resulted in excellent separation of microparticles from excipient.
Unfixed capsules of this invention, composed of nondenatured HSA or other spray-dryable material, possess highly smooth surfaces and may be processed with relatively low levels of excipients to produce free-flowing powders ideal for dry powder inhalers. Using this approach, it is possible to produce heterogeneous microcapsules which are comprised of a suspending excipients and active principle.
This has the advantage of yielding free-flowing powder of active principles which may be further processed to give powders that dose and aerosolise with excellent reproducibility and accuracy.
In addition, the process of spray-drying, in its current form, gives rise to relatively little denaturation and conversion to polymers in the production of the freeflowing powder. In all cases, the size of the microcapsule suspension can be such that 90% of the mass lies within the desired size, e.g. the respirable region of 1-5 Mm.
WO 96/09814 PCT/GB95/02279 7 In essence therefore we have defined how to produce microparticles which are: predominantly 1-5 Am in size; smooth and spherical; gas-containing; and composed of undamaged protein molecules and which may be stored and shipped prior to other processing steps. In preparing intermediate microcapsules for ultrasound imaging, we have defined those characteristics of a process and the resulting powder which are essential for the production of superior powders for dry powder inhalers (DPI's). We find that many of the assays which have been developed for the echocontrast agent are suitable for defining those parameters of the particles which are advantageous for DPI powders, namely; echogenicity and pressure resistance of cross-linked particles defining perfectly formed microparticles; microscopic evaluation in DPX or solvents, defining sphericity and gas-containing properties of soluble intermediate capsules; size and size distribution analysis and also the monomeric protein assay to define the final level of fixation of the product.
Especially for use in therapy, considerable care is necessary in order to control particle size and size distribution. We have chosen a biocompatible polymer which when cross-linked remains innocuous and also learned how to reproducibly cross-link this molecule. In order to achieve controlled cross-linking, we have divorced the processes of microparticle formation and cross-linking which other emulsion and solvent evaporation process do not. This means that the initial step of the process does not damage the wall-forming material. We have defined the particular parameters which are important for complete particle formation and further defined more advantageous conditions which yield more intact particles. In choosing HSA as a particularly favourable polymer we have also chosen a potential carrier molecule which may: protect labile molecules; enhance uptake of peptides across the lung; bind low molecular weight drug through natural binding affinities; and be covalently modified to carry drugs WO 96/09814 PCT/GB95/02279 8 across cellular barriers to the systemic circulation and beyond.
When researchers have used spray-drying to produce microparticles of small dimensions, they have tended to use volatile solvents, which encourages rapid droplet shrinkage. Alternatively, researchers have used feedstocks with low solute content in order to keep the solution viscosity low, to enhance smaller droplet production. In both cases, when the microparticles are produced, the process has little impact on the final morphology; rather this is dictated by the components used to form the particles. We have taken the extensive learning of how to produce controlled sized particles from HSA and applied this to many other materials including active drugs. We are able to use relatively high solute contents, e.g. w/v as opposed to to produce microparticles comprising low molecular weight active with lactose; active alone: peptides with HSA and modified polymeric carriers with active. We now find that it is the process which dictates the final particle morphology rather than the composition of the solutes. Further, we are able to use combinations of aqueous and water-miscible solvents to enhance particle morphology. Thus we have a "process" driven methodology which allows beneficial production of smooth, spherical controlled sized particles suitable for pulmonary delivery.
It has been found that the process of the invention can be controlled in order to obtain microspheres with desired characteristics. Thus, the pressure at which the protein solution is supplied to the spray nozzle may be varied, for example from 1.0-10.0 x 105 Pa, preferably 2-8 x 105 Pa, and most preferably about 7.5 x 105 Pa. Other parameters may be varied as disclosed below. In this way, novel microspheres may be obtained.
A further aspect of the invention provides hollow microspheres in which more than 30%, preferably more than 50%, or 60%, of the microspheres have a diameter WO 96/09814 PCT/GB95/02279 9 within a 2 Am range and at least 90%, preferably at least or 99%, have a diameter within the range 1.0-8.0 Mm.
The interquartile range may be 2 jm, with a median diameter of 3.5, 4.0, 4.5, 5.0, 5.5, 6.0 or 6.5 Am.
Thus, at least 30%, 40%, 50% or 60% of the microspheres may have diameters within the range 1.5-3.5 Am, 2.0-4.0 Am, 3.0-5.0 Lm, 4.0-6.0 jm, 5.0-7.0 Am or im. Preferably a said percentage of the microspheres have diameters within a 1.0 Am range, such as 1.5-2.5 pm, 2.0-3.0 Am, 3.0-4.0 Am, 4.0-5.0 Am, 5.0-6.0 Am, 6.0-7.0 Am or 7.0-8.0 Am.
A further aspect of the invention provides hollow microspheres with proteinaceous walls in which at least preferably at least 95% or 99%, of the microspheres have a diameter in the range 1.0-8.0 m; at least preferably at least 95% or 99%, of the microspheres have a wall thickness of 40-500 nm, preferably 100-500 nm.
Description of the Invention The wall-forming material and process conditions should be so chosen that the product is sufficiently nontoxic and non-immunogenic in the conditions of use, which will clearly depend on the dose administered and duration of treatment. The wall-forming material may be a starch derivative, a synthetic polymer such as tert-butyloxycarbonylmethyl polyglutamate (US-A-4888398) or a polysaccharide such as polydextrose.
Generally, the wall-forming material can be selected from most hydrophilic, biodegradable physiologically compatible polymers, as described in more detail in WO-A- 9218164.
Preferably, the wall-forming material is proteinaceous. For example, it may be collagen, gelatin or (serum) albumin, in each case preferably of human origin derived from humans or corresponding in structure to the human protein). Most preferably, it is human serum albumin (HSA) derived from blood donations or, ideally, from the fermentation of microorganisms (including cell WO 96/09814 PCT/GB95/02279 lines) which have been transformed or transfected to express HSA. Further detail is given in WO-A-9218164.
The protein solution or dispersion is preferably 0.1 to 50% w/v, more preferably about 5.0-25.0% protein, particularly when the protein is albumin. About 20% is optimal. Mixtures of wall-forming materials may be used, in which case the percentages in the last two sentences refer to the total content of wall-forming material.
The preparation to be sprayed may contain substances other than the wall-forming material and solvent or carrier liquid. Again, reference may be made to WO-A-9218164.
The protein solution or dispersion (preferably solution), referred to hereinafter as the "protein preparation", is atomised and spray-dried by any suitable technique which results in discrete microspheres or microcapsules of 1 to 10 Am diameter. These figures refer to at least 90% of the population of microcapsules, the diameter being measured with a Coulter Master Sizer II.
The term "microcapsules" means hollow particles enclosing a space, which space is filled with a gas or vapour but not with any solid materials. Honeycombed particles resembling the confectionery sold in the UK as Maltesers® are not formed.
The atomising comprising forming an aerosol of the protein preparation by, for example, forcing the preparation through at least one orifice under pressure into, or by using a centrifugal atomiser in a chamber of warm air or other inert gas. The chamber should be big enough for the largest ejected drops not to strike the walls before drying. The gas or vapour in the chamber is clean preferably sterile and pyrogen-free) and nontoxic when administered into the bloodstream in the amounts concomitant with administration of the microcapsules in use. The rate of evaporation of the liquid from the protein preparation should be sufficiently high to form hollow microcapsules but not so high as to burst the microcapsules. The rate of evaporation may be controlled WO 96/09814 PCT/GB95/02279 11 by varying the gas flow rate, concentration of protein in the protein preparation, nature of liquid carrier, feed rate of the solution and, more importantly, the temperature of the gas encountered by the aerosol. With an albumin concentration of 15-25% in water, an inlet gas temperature of at least about 100 0 C, preferably at least 110 0 C, is generally sufficient to ensure hollowness and the temperature may be as high as 250 0 C without the capsules bursting. About 180-240 0 C, preferably about 210-230°C and most preferably about 220 0 C, is optimal, at least for albumin. Since the temperature of the gas encountered by the aerosol will depend also on the rate at which the aerosol is delivered and on the liquid content of the protein preparation, the outlet temperature may be monitored to ensure an adequate temperature in the chamber.
An outlet temperature of 40-150 0 C has been found to be suitable. Controlling the flow rate has been found to be useful in controlling the other parameters such as the number of intact hollow particles.
The microcapsules comprise typically 96-98% monomeric
HSA.
More particularly, microparticles of the invention preferably have a maximum interquartile range of 3 jAm, more preferably 2 Am, and most preferably 1.5 Am, with respect to their mass median particle size. The mass median particle diameter is determined by Coulter counter with a conversion to a volume-size distribution. This is achieved by spray-drying in which there is a combination of low feed stock flow rate with high levels of atomisation and drying air. The effect is to produce microcapsules of very defined size and tight size distribution.
Several workers have designed equations to define the mean droplet size of pneumatic nozzles; a simple version of the various parameters which affect mean droplet size is as follows: D A/( 2 a B. (Mair/Miq) 'b WO 96/09814 PCT/GB95/02279 12 Where D Mean droplet size A Constant related to nozzle design B Constant related to liquid viscosity V Relative air velocity between liquid and nozzle d Air density Mair and Mq Mass of air and liquid flow a and b Constants related to nozzle design Clearly, for any given nozzle design, the droplet size is most affected by the relative velocity at the nozzle and concurrently the mass ratio of air to liquid. For most common drying use, the air to liquid ratio is in the range of 0.1-10 and at these ratios it appears that the average droplet size is 15-20 Atm. For the production of microparticles in the size range described herein we use an air to liquid ratio ranging from 20-1000:1. The effect is to produce particles at the high ratios which are exceedingly small by comparative standards, with very narrow size distributions. For microparticles, produced at the lower ratios of air to liquid, slightly larger particles are produced, but they still nevertheless have tight size distributions which are superior to microparticles produced by emulsion techniques.
The amount of added active principle is not critical; the microparticles may comprise at least 50, more preferably 70 or 80, and most preferably 90, by weight HSA or other carrier material. For use in an inhaler device, the microparticles may be formulated with a conventional excipient such as lactose or glucose.
The microparticles may comprise therapeutic agent and carrier, or a compound which alone is therapeuticallyactive. The amount of the active principle will be chosen having regard to its nature and activity, to the mode of administration and other factors known to those skilled in the art. By way of example only, the number of particles administered may be such as to deliver 100 mg/day a-l anti- WO 96/09814 PCT/GB95/02279 13 trypsin, or 0.1 mg/day of an active material such as beclomethasone.
The active principle may be, for example, a diagnostic substance or a classical pharmaceutical entity which may or may not bind, covalently or otherwise, to the carrier material. The therapeutic agent may be a proteinaceous material such as insulin, parathyroid hormone, calcitonin or similar bioactive peptide, albuterol, salicylate, naproxen, augmentin or a cytotoxic agent. For experimental purposes, a marker such as lysine-fluorescein may be included.
Microparticles of the invention may comprise an antagonist or receptor-binding component in addition to the therapeutic or diagnostic agent. For example, a sugar or other molecule may be included in the molecular vehicle, with a view to directing administration of the vehiclebound drug to a given receptor at or beyond the alveoli.
HSA is used herein as an illustrative example of water-soluble carrier materials for use in the invention.
Other materials that can be used include simple and complex carbohydrates, simple or complex amino- or polyamino-acids, fatty acid or fatty acid esters, or natural or recombinant human proteins or fragments or short forms thereof.
The invention allows for the nature of the dry microcapsules to be manipulated, in order to optimise the flow or vehicle properties, by changing and reducing the forces of cohesion and adhesion within the microcapsule preparation. For example, if so required, the microcapsules may be made predominantly positive or negative by the use of highly-charged monomeric or polymeric materials, e.g. lysine or poly-lysine and glutamate or poly-glutamate in systems without HSA or heterogeneous systems including HSA and active principles.
A further embodiment of the invention is the co-spraydrying of the active principle with HSA in order to facilitate stabilisation of the active principle during formulation, packing and, most importantly, during WO 96/09814 PCT/GB95/02279 14 residence on the alveolar lining. In this environment, there can be intense proteolytic activity. Whilst protease inhibitors can be used to protect peptide drugs, there may well be contra-indications to this approach. By using HSA, both as excipient and vehicle, it can offer a large excess of alternative substrate on which the locally-active proteases may act. A further advantage is that, since HSA has been shown to cross the alveolar barrier, by receptoror non-receptor-mediated transcytotic mechanisms, it may be used as a vehicle to facilitate the passage of an active principle across the epithelial lining.
In a further embodiment, active principle may be covalently linked to HSA via cleavable linkages prior to spray-drying. This embodiment represents a method of carrying active principles all the way from device to bloodstream, and possibly to targets within the body. The formation of particles with optimal aerodynamic size means that the "physical" vehicle delivers the active principle to the site of absorption. Once deposited upon the alveoli, the "molecular" vehicle then protects and facilitates passage into the bloodstream and, once in the bloodstream, can further enhance circulatory half-life and even direct the active principle to certain sites within the body on the basis of receptor-mediated events.
A suitable linker technology is described in WO-A- 9317713 (Rijksuniversiteit Groningen). Esterase-sensitive polyhydroxy acid linkers are described. Such technology, used in the derivatisation of HSA prior to spray-drying, enables the production of a covalent carrier system for delivery of drugs to the systemic vasculature. This utilises the potential of HSA to cross the alveoli to carry drugs over a prolonged period whilst protecting potentially unstable entities.
Although the active principle used in this invention may be imbibed into or otherwise associated with the microparticles after their formation, it is preferably formulated with the HSA. The microparticles may be at WO 96/09814 PCT/GB95/02279 least partly coated with a hydrophobic or water-insoluble material such as a fatty acid, in order to delay their rate of dissolution and to protect against hydroscopic growth.
The following Examples illustrate the invention. The spray dryer used in the Examples, available from A/S Niro Atomizer, Soeborg, Denmark, under the trade name "Mobile Minor", is described in detail in WO-A-9218164.
Example 1 A 20% solution of sterile, pyrogen-free HSA in pyrogen-free water (suitable for injection) was pumped to the nozzle of a two-fluid nozzle atomizer mounted in the commercial spray-drying unit described above. The peristaltic pump speed was maintained at a rate of approximately 10 ml/minute such that with an inlet air temperature of 220 0 C the outlet air temperature was maintained at 95 0
C.
Compressed air was supplied to the two fluid atomising nozzle at 2.0-6.0 Bar (2.0-6.0 x 105 Pa). In this range microcapsules with a mean size of 4.25-6.2 Am are obtained.
Typically an increase in mean particle size (by reduced atomisation pressure) led to an increase in the amount of microcapsules over 10 Am in size (see Table 1).
Table 1 Effects of Atomisation Pressure on Frequency of Microcapsules Over 10 Am in Diameter Atomisation Pressure Frequency over 10 mm (xl0 5 Pa) 6.0 0.8 3.3 6.6 8.6 13.1 Under the conditions described above, i.e. the first step of Example 1 of WO-A-9218164, with a nozzle pressure WO 96/09814 PCT/GB95/02279 16 of 7.5 bar, microparticles were produced with a particle size of 4.7 lm. These soluble microparticles were smooth and spherical with less than 1% of the particles over a particle size of 6 Am. The microparticles were dissolved in aqueous medium and the molecular weight of the HSA determined by gel filtration chromatography. The resultant chromatograms for the HSA before and after spray-drying HSA are essentially the same. Further analysis of the HSA before and after spray-drying by means of tryptic peptide mapping with HPLC revealed that there were no observable differences in the peptides liberated. Both analyses show that, under the conditions of spray-drying described to produce microparticles of 4.7 Am, little or no structural damage is done to the protein.
Example 2 Alpha-1 antitrypsin derived from human serum was spray-dried under conditions similar to Example 1 with an inlet temperature of 150 0 C and an outlet temperature of 0 C. In all other respects the conditions for drying were the same as Example 1. The soluble microparticles produced had a mean size of 4.5 Am. The microparticles were dissolved in aqueous medium and analysed for retention of protein structure and normal trypsin inhibitory activity, then compared to the original freeze dried starting material. Analysis by gel permeation and reverse phase chromatography and capillary electrophoresis, revealed that there were no significant structural changes after spraydrying. Analysis of the inhibitory activity (Table 2) showed that within the experimental error, full retention of inhibitory activity had been achieved.
Table 2 Run Number Percentage of Activity Retained 1 84 2 222 3 148 WO 96/09814 PCT/GB95/02279 17 Example 3 Using the general method of Example 1, microcapsules composed of alcohol dehydrogenase (ADH) and lactose were prepared (ADH 0.1% w/w; Lactose 99.9% We find that optimisation of the spray-drying step is required to maximise the retention of enzyme activity. The general conditions of Example 1 were used, but the inlet and outlet temperature were changed to give conditions which allowed us to produce microparticles of the desired size (4-5 Am) that retained full activity after drying and reconstitution in aqueous media. The percentage. of activity retained compared with the original material is shown for each of the spray-drying conditions shown (Table The microcapsules were smooth and spherical and contained air as evidenced by their appearance in diphenylxylene (DPX) under light microscopy.
Table 3 Run Inlet Temp. Outlet Temp. Activity OC OC Remaining 1 220 73 57 2 175 71 98 Example 4 A series of experiments was performed under the conditions described in Example 1, to examine the influence of liquid feed rate on the yield of intact spherical particles. We find that, using the ability of gascontaining microparticles to reflect ultrasound, we are able to determine optimal condition for maximising the yield of intact smooth spherical microcapsules. The microparticles formed after spray-drying are heat-fixed, to render them insoluble, and then suspended in water to make the echo measurements. We find that increasing the liquid feed rate decreases the number of intact microparticles formed during the initial spray-drying (Table The mean particle size and overall pressure stability, i.e.
WO 96/09814 PCT/GB95/02279 18 thickness of the shell, do not change but the total echogenicity does, as the liquid flow rate is increased from 4 to 16 ml/min. We find that slower rates of evaporation (at higher liquid flow rates) lead to fewer intact spherical particles being formed.
Table 4 Flow Rates (ml/min) 4 8 12 16 Mean size (gm) 3.08 3.04 3.13 3.07 Echogenicity (video 22 21 14 density units) Echogenicity after 20 18 10 8 pressure (video density units) The assay was conducted by resuspending the heat-fixed microparticles at a concentration of 1x10 ml in 350 ml of water. This solution is stirred slowly in a 500 ml beaker above which is mounted an 3.5 MHz ultrasound probe attached to a Sonus 1000 medical imaging machine. The grey scale images obtained are captured by an image analyser and compared against a water blank to yield video density units of echo reflectance. The assay can also be adapted to examine the pressure resistance, by assessing the echoreflectance before and after exposure of the sample to cyclical bursts of pressure applied to the stock solution of particles. This analysis distinguishes incomplete particles which entrain air upon reconstitution, from fully spherical particles which "encapsulate" air within the shell. Incomplete particles do not show pressure resistance and lose the ability to reflect ultrasound immediately. The dose response for fixed albumin particles of Example 1 is c. 5, 9, 13, 20, 22 and 24 VDU's (backscatter intensity) at respective microcapsule concentrations of 0.25, 0.5, 1, 2, 3 and 4 x 106 per ml.
Example Significant experimentation to reduce the particle size and narrow the size distribution has been performed.
This was pursued to effectively increase the gas content of WO 96/09814 PCT/GB95/02279 19 the echocontrast agent and reduce the number of oversized particles. This exercise is also beneficial to respiratory formulations in that it maximises the potential number of respirable particles in the 1-5 gm range and produces inherently more smooth particles which will be less cohesive than non-spherical particles of similar size.
We find that it is possible to reduce particle size by lowering the solutes content of the feedstock. This effect, is in part, mediated by the effects of viscosity on droplet formation. However, we also find that by lowering the solute content under the conditions we use leads to a significant decrease in the number of intact particles. By further experimentation we have found that incorporation of water-miscible, volatile solvents in the feedstock, significantly increase the rate of shell formation during drying, with a concomitant increase in the number of intact particles or hollow particles (Table The assessment of hollowness is made by microscopic evaluation of particles floating to the surface of the coverslip on a haemocytometer versus particle count by Coulter counting.
Table Run HSA Content Ethanol Mean Percentage of Content of Particle of Hollow Feedstock Feedstock Size Particles (Am) 1 10 0 3.7 12.5 2 10 25 3.52 64.3 Example 6 A range of materials has been used to manufacture smooth spherical soluble microparticles. The range of microparticles produced includes inert materials such as HSA, lactose, mannitol, sodium alginate; active materials alone such as al-antitrypsin; and mixtures of active and inert carrier such as lactose/alcohol dehydrogenase, lactose/budesonide, HSA/salbutamol. In all cases, smooth, spherical and gas-containing particles are produced.
WO 96/09814 PCT/GB95/02279 We have assessed the success of the process in maintaining control over the morphology of the particles.
The particles are suspended in propanol and then visualised by microscopy. Those particles which contain gas appear to have an intense white core surrounded by an intact black rim whilst broken or miss-formed particles appear as ghosts. Microscopic evaluation of the following microparticles exemplifies the range of materials and actives which can be dried to produce smooth spherical particles:
HSA
Casein Haemoglobin Lactose ADH/lactose HSA/Peroxidase Lactose/Salbutamol Lactose/Budesonide Example 7 Lactose and Budesonide were spray-dried under the conditions described in the table below (Table 6).
Table 6 Parameter Setting Inlet Temperature 220 0
C
Outlet Temperature Atomisation Pressure 7.5 bar Damper Setting Feed Rate 3.88 g/min Stock Solution 9.3% w/v Budesonide, Ethanol 19% w/v lactose The resultant dry powder was blended with excipient grade lactose in a V type blender in the proportions outlined in Table 7. The blends were then loaded into gelatin capsules and discharged from a Rotahaler M into a twin stage impinger run at 60 1/min. The respirable fraction was calculated as the percentage deposited into the lower chamber.
WO 96/09814 PCT/GB95/02279 21 Table 7 Formulation Budesonide spray fast flow Respirable Number in spray dried lactose in fraction dried product in blend particles blend 1 9.3 10 90 42 2 9.3 15 85 29 3 9.3 20 80 34 4 5.7 30 70 36 The respirable fractions obtained are considerably superior to micronised product currently used in this device which are usually in the range of 10-20% maximum.
The Budesonide/Lactose formulations detailed in Example 7 were tested in an experimental gravity fed multidose DPI. The parameters examined were the variation of emitted dose over 30 shots and the respirable fraction in a four-stage impinger device. The results are shown below (Table 8).
Table 8 Formulation Dose Fine Particle CofV on Number (mg) (Respirable) Emitted Fraction Dose 1 4 52 2 4.2 42 2.8 3 3.7 58 8.1 For current DPI devices, the preliminary US Pharmacopoeia recommendation appears likely to be less than variation in the emitted dose. Clearly in all of the formulations tested so far we are within the current specifications and in the case of formulations 1 and 2 we are significantly under the current limits.
Example 8 To decrease the dissolution rate of soluble microcapsules as described in preceding Examples, microcapsules may be coated with fatty acids such as palmitic or behenic acids. The soluble microcapsules of WO 96/09814 PCT/GB95/02279 22 Example 1 were coated by suspending a mixture of soluble HSA microcapsules and glucose (50% w/w) in an ethanolic solution containing 10% palmitic or behenic acid. The solution was evaporated and the resultant cake milled by passage through a Fritsch mill.
The efficacy of coating was assessed by an indirect method derived from our previous ultrasound studies.
Ultrasound images were gathered from a beaker of water containing 1 x 106 microcapsules/ml using a HP Sonus 1000 ultrasound machine linked to an image analyser. Video intensity over a blank reading (VDU). was measured over time (Table 9).
The uncoated microcapsules very quickly lost all air and thus the potential to reflect ultrasound. However, coated microcapsules retained their structure for a longer period and hence showed a prolonged signal over several minutes.
Table 9 Echogenicity of Coated HSA Microcapsules Time (min) Echogenicity (VDU) HSA only HSA/Palmitic HSA/Behenic Coated Coated 0 1.75 1.91 0.88 0.043 0.482 0.524 0 0 0.004 Example 9 Soluble mannitol microcapsules were prepared as set out in Example 1 (15% aqueous mannitol spray-drying feedstock) and coated with palmitic acid and behenic acid as described in Example 8. A sample of each was suspended in water and the echogenicity measured. Ten minutes after the initial analysis, the echogenicity of the suspended samples was repeated (Table WO 96/09814 PCT/GB95/02279 23 Table Echogenicity of Coated Mannitol Microcapsules Time Echogenicity (VDU) (mi) Mannitol Palmitic Behenic 0 1.6 1.7 0.92 0.33 0.5 0.24 17 0 0.84 0 Example Soluble microcapsules with a model active (Lysine- Fluoroscein) contained within the matrix were prepared to allow the production of a free-flowing dry powder form of the "active" compound. On dissolution of the microcapsules, the active compound was released in its native form.
Using lysine as a model compound, the molecule was tagged with fluorescein isothiocyanate (FITC) to allow the compound to be monitored during the preparation of the soluble microcapsules and the subsequent release during dissolution.
3 g of lysine was added to FITC (0.5 g total) in carbonate buffer. After one hour incubation at 30 0 C, the resultant solution was tested for the formation of the FITC-lysine adduct by TLC. This showed the presence of a stable FITC-lysine adduct.
The FITC-lysine adduct was mixed with 143 ml of ethanol containing 100 mg/ml HSA to give the spray-drying feedstock. The spray-drying conditions used to form the microcapsules are detailed in Table 11 below. In the absence of ethanol we have found that only a small percentage of the particles are smooth and spherical.
The spray-drying process produced 17.21 g of microcapsules that did not dissolve when a sample was resuspended in ethanol. Moreover, no release of the FITClysine adduct was observed. However, when 10 ml water was added to the ethanol-suspended microcapsules, the WO 96/09814 PCT/GB95/02279 24 microcapsules dissolved and the FITC-lysine was released.
Analysis of the adduct using TLC before incorporation into the microcapsules and after release from the microcapsules on dissolution showed the model compound was unchanged.
Table 11 Spray-Drying Conditions Parameter Setting Inlet Temperature 220 0
C
Outlet Temperature 85 0
C
Atomisation Pressure 7.5 bar Damper Setting Feed Rate 3.88 g/min Stock Solution 25% v/v Ethanol, 10% w/v HSA The soluble microcapsules were sized in a non-aqueous system of ammonium thiocyanate and propan-2-ol using a Multisizer II (Coulter Electronics). The microcapsules had a mean size of 3.28 0.6 Am and with 90% of the mass within 2-5 Am.
The microcapsules were mixed with glucose (50% w/w microcapsules 50% w/w glucose), and milled by the passage of the mixture through a Fritsch mill three times. When a sample of the powder was added to water, the FITC-lysine was released intact when compared with its original form as determined by TLC analysis. This example shows the feasibility of making an amino acid or peptide formulation which could be used for respiratory formulations, which incorporates HSA within the formulation.
Example 11 500 mg beclomethasone was dissolved in ethanol and added to 50 ml HSA feedstock (10% w/v) and spray-dried using the conditions outlined in Example 10. The microcapsules hence formed were sized in the non-aqueous system as detailed in Example 10. The microcapsules had a mean size of 3.13 0.71 Am, 90% of which were between 2 and 5 im.
WO 96/09814 PCT/GB95/02279 The beclomethasone was extracted from the microcapsules by the precipitation of the HSA in 10% TCA, and the supernatant was extracted into ethanol. The ethanol extract was analysed using HPLC, at a wavelength 242 nm. The beclomethasone detected in this extract exists in the free state, but when the albumin pellet was extracted the presence of beclomethasone bound to native HSA was observed. It was found that although the majority of the active compound was in the free state, some was present in the albumin-bound state. Since albumin partitions only slowly into the bloodstream, this allows control over the release of the active compound over an extended period of time, compared to free drug.
Example 12 Whereas in Examples 10 and 11 at least, any binding of the active compounds was an effect of the intrinsic nature of albumin, this Example gives a product following initial cross-linking of the active compound, prior to spraydrying.
To a 10 mg/ml solution of methotrexate, 25 mg carbodiimide (EDCI) was added. The solution was stirred for 4 hours to initiate and ensure complete activation of the methotrexate. 50 mg HSA was added to the activated drug and stirred for 3 hours at room temperature. The methotrexate is chemically bound to the HSA via the amine groups on the albumin. This conjugate was then used as the spray-drying feedstock as detailed in Example The soluble microcapsules thus made were sampled, characterised and analysed for drug content. The microcapsules had a mean size of 3.2 0.6 pm with 90% by mass between 2-5 gm. The analysis of the drug content of the microcapsules showed that the microcapsules did not release drug; even after dissolution, drug was still bound to the HSA. Proteinase K digestion of the albumin released the bound drug which was shown to be linked to only a limited number of amino-acids and small peptides. It has been shown previously that the activity of doxorubicin WO 96/09814 PCT/GB95/02279 26 bound to polymeric carriers proves beneficial in tumours, showing the multidrug-resistant phenotype.
Example 13 Naproxen microcapsules were prepared as detailed in Examples 10 and 12 using a ratio of 1 to 5, drug to HSA.
The soluble microcapsules retained the active compound of a non-aqueous solvent. Moreover, on dissolution of the microcapsules in aqueous solution, the active compound was still bound to the albumin, as shown by HPLC analysis at 262 nm, as before. The naproxen was released from the albumin on digestion with proteinase K and esterases.
Example 14 Using samples of the microcapsules produced in Examples 8 to 13, an assessment of their behaviour in a dry powder inhaler was made. The dosing reproducibility of each formulation was assessed in conjunction with the aerolisation of the sample by microscopic evaluation.
A sample of each formulation was added to the storage funnel of an experimental dry powder inhaler (DPI). The dry powder inhaler used pressurised air to force the powder into a dosing measure. The dosing measure used was calibrated using spray-dried lactose.
Although the amounts dispensed into the dosing measure varied between samples as a function of their composition, the dosing reproducibility for each sample was very consistent; with a mean of 5.0 0.25 mg obtained for three dosing trials.
The aerolisation behaviour of the samples was tested by connecting the inhaler to a vacuum chamber; simulated inhalation was achieved by the release of the vacuum through the DPI and collection of the airborne dose was made on resin coated microscope slides. These slides were evaluated for dispersion of the particles. The slides showed that the DPI had deagglomerated the samples forming an even dispersion of microparticles on the microscope slides.
WO 96/09814 PCT/GB95/02279 27 Example The performance of the dry powder formulations from Examples 10 to 13 was analysed using the twin impinger method (Apparatus A for pressurised inhalations, British Pharmacopoeia 1988) following discharge from a Rotahaler (Glaxo UK) with 7 ml in stage 1 and 30 ml in stage 2 of distilled water. The formulations were delivered from size 3 gelatin capsules using a Rotahaler attached to the twin impinger using a rubber adapter. The vacuum pump was operated at 60 1/min for two 3 second bursts. The amount of each sample reaching stage 1 and stage 2 levels of the impinger was analysed. All samples showed the largest percentage deposition to occur in stage 2 of the impinger indicating optimal sized particles for alveoli delivery.
Example 16 A comparison of the dosing and deposition of fixed insoluble microcapsules and soluble microcapsules as produced in Example 10 was made in the lung of rabbits.
Anaethestised New Zealand white rabbits were dosed either with soluble microcapsules or fixed microcapsules.
The dosing was carried out using a computer controlled nebuliser (Mumed Ltd., UK). The soluble microcapsules were suspended in CFC 11 and the fixed particles were suspended in water. After dosing, the lungs of the rabbits were removed and an assessment of the deposition of the capsules made.
The fixed capsules were found intact in the alveoli tissue of the lung. This showed that the microcapsules were of the appropriate size for dispersion through the lungs. In comparison, no evidence of the presence of intact soluble microcapsules was found, the capsules having dissolved in the fluids of the lung. However, the presence of FITC-lysine adduct was observed in some of the alveoli tissue when studied using fluorescent microscopy. In addition, the presence of the adduct was also found the blood and urine of the animals, as opposed to that of the fixed capsules which showed no presence in either.
Q \OPER\JLR\35302 95 247 28/10/98 -27A- Throughout this specification and the claims which follow, unless the context requires otherwise, the word "comprise", and variations such as "comprises" and "comprising", will be understood to imply the inclusion of a stated integer or step or group of integers or steps but not the exclusion of any other integer or step or group of integers or steps.
o•
Claims (19)
1. Microparticles of a single water-soluble therapeutic or diagnostic material, which are smooth and spherical, and at least 90% of which have a particle size of 1 to 10 /tm, when used in therapy or diagnosis.
2. Microparticles of a mixture of a water-soluble therapeutic or diagnostic material and another water-soluble material, wherein the microparticles are smooth and spherical, and at least 90% of which have a particle size of 1 to 10 /m.
3. Microparticles according to claim 1 or claim 2, which are hollow.
4. Microparticles according to any one of the preceding claims, wherein said particle size is 1 to 5 pm.
Microparticles according to any one of the preceding claims, which have a maximum interquartile range of 3 /m.
6. Microparticles according to claim 5, which have a maximum interquartile range of 2
7. Microparticles according to any one of the preceding claims, which are sterile.
8. Microparticles according to any one of the preceding claims, which are at least partly coated with a water-insoluble material. o
9. Microparticles according to any one of the preceding claims, which additionally carry S* a receptor-binding component. s
10. Microparticles according to any one of the preceding claims, wherein the, either or Q.\OPER\JLR35302-95.2 4 7 27/10/98 -29- each water-soluble material is a carbohydrate.
11. Microparticles according to any one of claims 1 to 9, wherein the, either or each water-soluble material is an amino- or polyamino-acid.
12. Microparticles according to any one of claims 1 to 9, wherein the, either or each water-soluble material is a fatty acid or ester thereof.
13. Microparticles according to any one of claims 1 to 9, wherein the, either or each water-soluble material is a protein, peptide or enzyme.
14. Microparticles according to claim 13, wherein the, either or each water-soluble material is a human protein or fragment, in natural or recombinant form.
Microparticles according to claim 14, wherein the or said other water-soluble material is human serum albumin.
16. Microparticles according to any one of the preceding claims, wherein the water- soluble material is chemically or enzymatically modified, prior to formation of the microparticles.
17. An inhaler device adapted to deliver a therapeutic agent via the pulmonary airways, which comprises the therapeutic agent in the form of microparticles according to any one of the preceding claims.
18. Use of a therapeutic agent for the manufacture of a medicament for treatment of a complaint on which the therapeutic agent acts on administration via the pulmonary airways, characterised in that the therapeutic agent is in the form of microparticles according to any one of claims 1 to 16. Q:\OPER\JLR\35302-95.247 11/12/98
19. In a method of treating a complaint by administration to a patient of an effective amount of a therapeutic agent that acts via pulmonary airways to treat the complaint, the improvement comprising administration of the therapeutic agent in the form of microparticles according to any one of claims 1 to 16. A microparticle according to any one of claims 1 to 16, or an inhaler device according to claim 17, or a use according to claim 18, or a method according to claim 19, substantially as hereinbefore described with reference to the Examples. DATED this 11th day of December 1998 ANDARIS LIMITED by its Patent Attorneys DAVIES COLLISON CAVE
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| EP94307126 | 1994-09-29 | ||
| PCT/GB1995/002279 WO1996009814A1 (en) | 1994-09-29 | 1995-09-26 | Spray-dried microparticles as therapeutic vehicles |
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| US6051256A (en) * | 1994-03-07 | 2000-04-18 | Inhale Therapeutic Systems | Dispersible macromolecule compositions and methods for their preparation and use |
| US5955108A (en) * | 1994-12-16 | 1999-09-21 | Quadrant Healthcare (Uk) Limited | Cross-linked microparticles and their use as therapeutic vehicles |
| GB9606188D0 (en) * | 1996-03-23 | 1996-05-29 | Danbiosyst Uk | Pollysaccharide microspheres for the pulmonary delivery of drugs |
| GB9606677D0 (en) * | 1996-03-29 | 1996-06-05 | Glaxo Wellcome Inc | Process and device |
| GB9607035D0 (en) * | 1996-04-03 | 1996-06-05 | Andaris Ltd | Spray-dried microparticles as therapeutic vehicles |
| GB9610341D0 (en) * | 1996-05-17 | 1996-07-24 | Andaris Ltd | Formulation for inhalation |
| JP4024302B2 (en) * | 1996-05-17 | 2007-12-19 | クアドラント、 ドラッグ、 デリバリー、 リミテッド | Microparticles and their use in wound treatment |
| US5855913A (en) * | 1997-01-16 | 1999-01-05 | Massachusetts Instite Of Technology | Particles incorporating surfactants for pulmonary drug delivery |
| US5874064A (en) * | 1996-05-24 | 1999-02-23 | Massachusetts Institute Of Technology | Aerodynamically light particles for pulmonary drug delivery |
| US6254854B1 (en) | 1996-05-24 | 2001-07-03 | The Penn Research Foundation | Porous particles for deep lung delivery |
| US5985309A (en) * | 1996-05-24 | 1999-11-16 | Massachusetts Institute Of Technology | Preparation of particles for inhalation |
| USRE37053E1 (en) | 1996-05-24 | 2001-02-13 | Massachusetts Institute Of Technology | Particles incorporating surfactants for pulmonary drug delivery |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| KR100277622B1 (en) * | 1992-06-12 | 2001-01-15 | 이타가키 히로시 | Inhalation ultrafine powder and its manufacturing method |
| EP0606486B1 (en) * | 1992-06-12 | 2001-08-29 | Teijin Limited | Pharmaceutical preparation for intra-airway administration |
-
1995
- 1995-09-26 BR BR9509171A patent/BR9509171A/en not_active Application Discontinuation
- 1995-09-26 MX MX9702357A patent/MX9702357A/en unknown
- 1995-09-26 PL PL95319600A patent/PL319600A1/en unknown
- 1995-09-26 RU RU97106769A patent/RU2147226C1/en not_active IP Right Cessation
- 1995-09-26 NZ NZ292980A patent/NZ292980A/en not_active IP Right Cessation
- 1995-09-26 WO PCT/GB1995/002279 patent/WO1996009814A1/en not_active Application Discontinuation
- 1995-09-26 KR KR1019970702043A patent/KR970705979A/en not_active Application Discontinuation
- 1995-09-26 EP EP95932122A patent/EP0783298A1/en not_active Ceased
- 1995-09-26 JP JP8511495A patent/JPH10506406A/en not_active Ceased
- 1995-09-26 AU AU35302/95A patent/AU701440B2/en not_active Ceased
- 1995-09-26 HU HU9702161A patent/HUT77373A/en unknown
- 1995-09-26 CA CA002199954A patent/CA2199954A1/en not_active Abandoned
- 1995-09-26 CZ CZ97924A patent/CZ92497A3/en unknown
- 1995-09-29 ZA ZA958239A patent/ZA958239B/en unknown
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1997
- 1997-03-26 NO NO971438A patent/NO971438D0/en not_active Application Discontinuation
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| BR9509171A (en) | 1997-09-16 |
| FI971332A (en) | 1997-04-01 |
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| RU2147226C1 (en) | 2000-04-10 |
| EP0783298A1 (en) | 1997-07-16 |
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| FI971332A0 (en) | 1997-04-01 |
| ZA958239B (en) | 1996-09-30 |
| KR970705979A (en) | 1997-11-03 |
| CZ92497A3 (en) | 1997-08-13 |
| AU3530295A (en) | 1996-04-19 |
| JPH10506406A (en) | 1998-06-23 |
| NO971438D0 (en) | 1997-03-26 |
| MX9702357A (en) | 1997-06-28 |
| CA2199954A1 (en) | 1996-04-04 |
| WO1996009814A1 (en) | 1996-04-04 |
| HUT77373A (en) | 1998-03-30 |
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