CA1204058A - Dual microcapsules - Google Patents
Dual microcapsulesInfo
- Publication number
- CA1204058A CA1204058A CA000422820A CA422820A CA1204058A CA 1204058 A CA1204058 A CA 1204058A CA 000422820 A CA000422820 A CA 000422820A CA 422820 A CA422820 A CA 422820A CA 1204058 A CA1204058 A CA 1204058A
- Authority
- CA
- Canada
- Prior art keywords
- mini
- microcapsules
- liquid
- dual
- microcapsule
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired
Links
Classifications
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- 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
- A61K9/5073—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 having two or more different coatings optionally including drug-containing subcoatings
-
- A—HUMAN NECESSITIES
- A01—AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
- A01N—PRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
- A01N25/00—Biocides, pest repellants or attractants, or plant growth regulators, characterised by their forms, or by their non-active ingredients or by their methods of application, e.g. seed treatment or sequential application; Substances for reducing the noxious effect of the active ingredients to organisms other than pests
- A01N25/26—Biocides, pest repellants or attractants, or plant growth regulators, characterised by their forms, or by their non-active ingredients or by their methods of application, e.g. seed treatment or sequential application; Substances for reducing the noxious effect of the active ingredients to organisms other than pests in coated particulate form
- A01N25/28—Microcapsules or nanocapsules
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01J—CHEMICAL OR PHYSICAL PROCESSES, e.g. CATALYSIS OR COLLOID CHEMISTRY; THEIR RELEVANT APPARATUS
- B01J13/00—Colloid chemistry, e.g. the production of colloidal materials or their solutions, not otherwise provided for; Making microcapsules or microballoons
- B01J13/02—Making microcapsules or microballoons
- B01J13/025—Applications of microcapsules not provided for in other subclasses
-
- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01J—CHEMICAL OR PHYSICAL PROCESSES, e.g. CATALYSIS OR COLLOID CHEMISTRY; THEIR RELEVANT APPARATUS
- B01J13/00—Colloid chemistry, e.g. the production of colloidal materials or their solutions, not otherwise provided for; Making microcapsules or microballoons
- B01J13/02—Making microcapsules or microballoons
- B01J13/06—Making microcapsules or microballoons by phase separation
- B01J13/12—Making microcapsules or microballoons by phase separation removing solvent from the wall-forming material solution
- B01J13/125—Making microcapsules or microballoons by phase separation removing solvent from the wall-forming material solution by evaporation of the solvent
Abstract
Abstract of the Disclosure Dual microcapsules are disclosed. The outer membrane encapsulates a liquid having one or more smaller microcapsules (mini-microcapsules) suspended therein. The mini-microcapsules contain a complex or a reaction product of a drug which dif-fuses into the liquid in which mini-microcapsules are suspended. The suspending liquid contains an enzyme which reacts with drug complex or reaction product to regenerate or release the drug. The drug diffuses through the outer membrane into a host.
Description
2 6 4 9 D, - 6 6 ~2~
DUAL MICROC~PSULES
Background of the Invent;on An increasingly importan~ process for delivering a functlonal material to a particular locus involves the use of microcapsules. As the term is used in the art, a microcapsule is a functional material encapsulated in a membrane.
An important application of microcapsules is in the medlcal arts. In this field of application, a functional drug is encapsulated in a membrane that is semipermeable to the drug.
When the drug is administered to the host, the drug is transported across the semipermeable membrane to release the drug to the hos~.
While the use of microcapsules for drug administration is widely employed, the method suffers from certain shortcomings which limits its further application in this art. Specifically, the rate at which the drug is released to the patient is control-led by the ra-te at which the drug i5 transported across the semi-permeable membrane. While many types of polymeric materials providing different diffusion rates can be employed as the semi-permeable membrane~ each membrane has â limited range of permeabil-:it~
6260 (1) CAN
~ 1 --which effec~ively controls the rate at which a drug of interest is released to the host. For many pur-poses; the drug release rate may be too slow or too rapid to provide the desired drug release rate~
Accordingly r there is a need in the art for more refined and structurally modified microcapsules haviny ~he ability to release drugs to a host over a wide range of preselected rates.
Summar of the Invention ,~ ~
The invention is directed to certain novel microcapsules which can be employed to release a wide variety oF d~ùgs to a host over a wide range of preselected drug release rates. The microcapsules of the invention are hereinafter characterized as dual microcapsules in that they include an outer semipermeable membrane which encapsulates ~wo sepa-rate and distinct encapsulated componentsO One encapsulated component is a liquid material. The second encapsulated component is a smaller microcap-sule, hereinafter referred to as a mini-microcapsule.
The mini-microcapsule has a functional material encapsulated therein.
In a preferred embodiment of the invention, the two separately encapsulated components~ one encapsulated by the outer membrane and the other encapsulated by the membrane of the mini~microcap-sule, are reactive with each other. The component encapsulated within the mini-microcapsule diffuses across the wall of the mini-microcapsule to co~tact the component encapsulated within the outer membrane of the microcapsule. The two components ~hen inter~
act to generate a new entity not originally present per se in either of the two encapsula~ed components.
The new entity then diffuses through ~h~ outer mem-brane and i5 released to the host.
In another embodiment of the invention, a single component is encapsulated in the mini-micro-capsule with the second component encapsulated by the outer membrane serving ~olely or principally a transport medium for the agent encapsulated within the mini-mlcrocapsule. The two membranes included in the dual micxocapsule will be fabricated from differen~ polymeric materials a~d will have diEEerent diffusion rates for the component encapsulated within the mini-microcapsule.
The invention also is directed to methods for preparing the dual microcapsules of the inven-tion.
The invention is further directed ~o methods for preparing certain mini-microcapsules employed in the manufacture of the dual microcapsules o the invention.
Brief Descri tion of the Dra~in s P ~
Fig. l is a sectional view of a dual micro~
capsule of the invention.
Fig. l~ is a sectional view of the dual microcapsule of Fig. l which has been dehydxated to remove the bulk of the water from the aqueous media orig~nally present within the dual microcapsule, including the encapsulated mini-microcapsule.
Flg. 2 is a sectional view of a dual micro-capsule having two different mini-microcapsules encapsulated therein~
Defined Terms As an aid in interpreting the descriptions of the inventions which follow, the following terms will have the special meanings set forth below.
"Microcapsule" i5 an article of manufacture havins a Functional Core Material encapsulated within a polymeric membrane. While Microcapsules may have essentially any physical form, they customarily are essentially spherical in shape and customarily have average diameters in the range of about 1 m to 2,000 m.
"Functional Core Material" is any solid or liquid material, other than a Mini~Microcapsule, encapsulated in a Microcapsule.
"Dual Microcapsule" is a special Microcap-sule having at least ~wo components encapsulated within the exterîor membrane oE the capsule. At least one of the t~Jo components will be a Microcap~
sule having a diameter smaller than the external membrane of the Dual Microcapsule, such small encap-sulated microcapusles hereafter being identified as Mini-Microcapsules~ A ~ual Microcapsule may have two or more different types of Mini-Microcapsules encapsulated therein.
?5 "Mini-Microcapsule" is a Microcapsule suf-ficiently small to be encapsulated within the inte-rior of a Dual Microcapsule~
"Encapsulating Process" is any process for encapsulating a Functional-Core Material in a poly-meric membrane~
'IPhase Separation Encapsula~ion Process" is a process for preparing Microcapsules in which the Functional Core Material to be encapsulated is dis-persed, customarily by stirring, in a solvent solu-tion of a polymer/ While continuing stirring ~o keep the Functional Core Material uniformly dispersed throughout the polymer solution, a nonsolven~ liquid is added to the polymer solution to change ~he poly-mer solubility in the medium and cause a phase sepa-ration of the dissolved polymer. Depending upon the specific polymer/solvent system, the polymer either precipitates from the solution or two immiscible liquid phases are produced, one of which is rich in polymer and polymer solvent and poor in nonsolvent, and the second of which i5 rich in nonsolvent and poor in solvent and polymer. Under certain condi-tions, the polymer rich phase will migrate to the interface between the dispersed droplets/particles and the continuous phase (non-solvent rich dispersing medium). The suspended particles of ~he Functional Core Ma~erial are encapsulated with the polymer and are subsequently hardened and recovered from the solvent/nonsolvent medium.
"Conjugate" is a product formed between two materials, one characterized as the "Functional Agent" and the second as the "Carrier", both of these terms being subsequent defined. The Conjugate is an entity separate and distinct from the Func-tional Agent and the CarrierO The Conjugate can be either a true chemical reaction product of the Func-tional Agent and the Carrrier or can be any type of complex formed therebetween~ In either event, the Conjugate can be subsequently treated with another material characterized as a Deconjugating Agent (subsequently described) to reform at least a portion of the originally employed Functional Agent.
"Functional Agent" is an entity which per-forms a specific identifiable function.
"Carrier" is a material which will reac~
with or form a complex with a Functional Agent.
"Drug" is a Functional Agent having a desir-able beneficial physiological efect upon a host.
"Drug Conjugate" is a Conjugate in which the Functional Agent included therein is a Drug.
"Prodrug" is a term sometimes used inter-changeably with Drug Conjugate, usually to define a Conjugate which is formed by effecting a chemical reaction between a Drug and a Carrier.
"Deconjugatinq Agent~' is an agent capable of interacting ~ith a Con~ugate to liberate or reform at least a portion of the Functional Agent employed in the preparation of the Conjugate.
"CAB" is a cellulose acetate butyrate poly-mer. Such polymers are known in the art, are de-scribed in numerous patents and publications and are 2~ commercially avallable from multiple sources includ-ing Eastman Chemicals. `
"PLA" is a polymer of lactic acid~ Such polymers are known in the art. See U.S. 3,991,7760 "Dalton" is a term becoming increasingly popular in the art to designate molecular weight. A
Dalton number is numerically equivalen~ to a gram molecular weigh~. By way of example, the Dalton number of sucrose is 342~
"Solvent" is an organic liquid having the power to dissolve at least 0.1 weight ~ of a desig-nated polymer of interest at ambient tempera~ure.
"Nonsolven~" is an or~anic liquid miscible with a solvent and having little or no solvent power ~f~
~7--for a designated polymer of interest at ambient temperature.
"Crenate Shape" is the shape assumed by an article having a flexible membrane supported by an internal fluid after the supporting fluid is evacu~
ated from the membrane. The shape assumed by a deflated basketball bladder after the bulk of the air has diffused therefrom is a prime example of a Crenate Shape.
Detailed Description of the Invention _ Fig. 1 represents an embodiment of the invention containin~ a single mini-capsule encapsu-lated within another larger capsule to form a dual capsule~ The structure conta~ns an outer polymeric membrane 10. A first liquid 12 is encapsulated within membrane lOo A mini-microcapsule having a polymeric membrane 14 is encapsulated within membrane 10~ A second liquid 16 is encapsulated within mem-brane 140 In the most preferred embodiment of the invention, liquids 12 and 16 are aqueous liquids, with liquid 16 having a Conjugate dissolved or dis-persed therein and liquid 12 having a Deconjugating Agent dissolved or dispersed therein. The membrane 14 will be semipermeable with respect to the Conju-gate within liquid 160 Upon diffusing through mem-brane 14 and contacting the Deconjugating Agent within liquid 12, an interaction takes place to regenerate the Functional ~gent. The Functional Agent then diffuses through membrane 10 into the system of the host. The structure shown in Fig. 1 is the structure of the dual capsule as it is pre-pared.
In one of the preferred embodiments of the invention, the membranes 10 and 14 shown in Fig~ 1 are semipermeable to water and can be dehydrated by processes subsequently described so as to remove the bulk of the water ~rom bo~h a~ueous li~uid 12 and aqueous liquid 15~ The approximate Crenate Shape that the dehydrated dual capsule takes is shown in Fig. lA. The bulk of the solids of original liquid 16 is maintained within membrane 14. The bulk of 10 the solids originally present in liquid 12 is main tained in the space between membranes 10 and 14.
When the dehydrated dual capsule of Fig. lA is placed in contact wlth water, it imbi~es water so as to dissolve or disperse the solids encapsulated within membranes 10 and 14 to reform the dual capsule in substantially the form illustrated in FigO 1.
In other embodiments of the invention, the liquid 16 may be a simple solution or dispersion of a Functional Agent in a suitable liquid~ usually water, and liquid 12 will contain no material react-able with the Functional Agent and will serve princi-pally as a transport medium for the Functional ~gent~
In such embodiments, membranes 10 and 14 will be fabricated from different polymeric materials so that the membranes will have different diffusion rates for the Functional Agent, with membrane 14 being signiicantly les5 permeable than membrane 10.
Fig. 2 illustrates another embodiment of the invention in which the dual microcapsule contains
DUAL MICROC~PSULES
Background of the Invent;on An increasingly importan~ process for delivering a functlonal material to a particular locus involves the use of microcapsules. As the term is used in the art, a microcapsule is a functional material encapsulated in a membrane.
An important application of microcapsules is in the medlcal arts. In this field of application, a functional drug is encapsulated in a membrane that is semipermeable to the drug.
When the drug is administered to the host, the drug is transported across the semipermeable membrane to release the drug to the hos~.
While the use of microcapsules for drug administration is widely employed, the method suffers from certain shortcomings which limits its further application in this art. Specifically, the rate at which the drug is released to the patient is control-led by the ra-te at which the drug i5 transported across the semi-permeable membrane. While many types of polymeric materials providing different diffusion rates can be employed as the semi-permeable membrane~ each membrane has â limited range of permeabil-:it~
6260 (1) CAN
~ 1 --which effec~ively controls the rate at which a drug of interest is released to the host. For many pur-poses; the drug release rate may be too slow or too rapid to provide the desired drug release rate~
Accordingly r there is a need in the art for more refined and structurally modified microcapsules haviny ~he ability to release drugs to a host over a wide range of preselected rates.
Summar of the Invention ,~ ~
The invention is directed to certain novel microcapsules which can be employed to release a wide variety oF d~ùgs to a host over a wide range of preselected drug release rates. The microcapsules of the invention are hereinafter characterized as dual microcapsules in that they include an outer semipermeable membrane which encapsulates ~wo sepa-rate and distinct encapsulated componentsO One encapsulated component is a liquid material. The second encapsulated component is a smaller microcap-sule, hereinafter referred to as a mini-microcapsule.
The mini-microcapsule has a functional material encapsulated therein.
In a preferred embodiment of the invention, the two separately encapsulated components~ one encapsulated by the outer membrane and the other encapsulated by the membrane of the mini~microcap-sule, are reactive with each other. The component encapsulated within the mini-microcapsule diffuses across the wall of the mini-microcapsule to co~tact the component encapsulated within the outer membrane of the microcapsule. The two components ~hen inter~
act to generate a new entity not originally present per se in either of the two encapsula~ed components.
The new entity then diffuses through ~h~ outer mem-brane and i5 released to the host.
In another embodiment of the invention, a single component is encapsulated in the mini-micro-capsule with the second component encapsulated by the outer membrane serving ~olely or principally a transport medium for the agent encapsulated within the mini-mlcrocapsule. The two membranes included in the dual micxocapsule will be fabricated from differen~ polymeric materials a~d will have diEEerent diffusion rates for the component encapsulated within the mini-microcapsule.
The invention also is directed to methods for preparing the dual microcapsules of the inven-tion.
The invention is further directed ~o methods for preparing certain mini-microcapsules employed in the manufacture of the dual microcapsules o the invention.
Brief Descri tion of the Dra~in s P ~
Fig. l is a sectional view of a dual micro~
capsule of the invention.
Fig. l~ is a sectional view of the dual microcapsule of Fig. l which has been dehydxated to remove the bulk of the water from the aqueous media orig~nally present within the dual microcapsule, including the encapsulated mini-microcapsule.
Flg. 2 is a sectional view of a dual micro-capsule having two different mini-microcapsules encapsulated therein~
Defined Terms As an aid in interpreting the descriptions of the inventions which follow, the following terms will have the special meanings set forth below.
"Microcapsule" i5 an article of manufacture havins a Functional Core Material encapsulated within a polymeric membrane. While Microcapsules may have essentially any physical form, they customarily are essentially spherical in shape and customarily have average diameters in the range of about 1 m to 2,000 m.
"Functional Core Material" is any solid or liquid material, other than a Mini~Microcapsule, encapsulated in a Microcapsule.
"Dual Microcapsule" is a special Microcap-sule having at least ~wo components encapsulated within the exterîor membrane oE the capsule. At least one of the t~Jo components will be a Microcap~
sule having a diameter smaller than the external membrane of the Dual Microcapsule, such small encap-sulated microcapusles hereafter being identified as Mini-Microcapsules~ A ~ual Microcapsule may have two or more different types of Mini-Microcapsules encapsulated therein.
?5 "Mini-Microcapsule" is a Microcapsule suf-ficiently small to be encapsulated within the inte-rior of a Dual Microcapsule~
"Encapsulating Process" is any process for encapsulating a Functional-Core Material in a poly-meric membrane~
'IPhase Separation Encapsula~ion Process" is a process for preparing Microcapsules in which the Functional Core Material to be encapsulated is dis-persed, customarily by stirring, in a solvent solu-tion of a polymer/ While continuing stirring ~o keep the Functional Core Material uniformly dispersed throughout the polymer solution, a nonsolven~ liquid is added to the polymer solution to change ~he poly-mer solubility in the medium and cause a phase sepa-ration of the dissolved polymer. Depending upon the specific polymer/solvent system, the polymer either precipitates from the solution or two immiscible liquid phases are produced, one of which is rich in polymer and polymer solvent and poor in nonsolvent, and the second of which i5 rich in nonsolvent and poor in solvent and polymer. Under certain condi-tions, the polymer rich phase will migrate to the interface between the dispersed droplets/particles and the continuous phase (non-solvent rich dispersing medium). The suspended particles of ~he Functional Core Ma~erial are encapsulated with the polymer and are subsequently hardened and recovered from the solvent/nonsolvent medium.
"Conjugate" is a product formed between two materials, one characterized as the "Functional Agent" and the second as the "Carrier", both of these terms being subsequent defined. The Conjugate is an entity separate and distinct from the Func-tional Agent and the CarrierO The Conjugate can be either a true chemical reaction product of the Func-tional Agent and the Carrrier or can be any type of complex formed therebetween~ In either event, the Conjugate can be subsequently treated with another material characterized as a Deconjugating Agent (subsequently described) to reform at least a portion of the originally employed Functional Agent.
"Functional Agent" is an entity which per-forms a specific identifiable function.
"Carrier" is a material which will reac~
with or form a complex with a Functional Agent.
"Drug" is a Functional Agent having a desir-able beneficial physiological efect upon a host.
"Drug Conjugate" is a Conjugate in which the Functional Agent included therein is a Drug.
"Prodrug" is a term sometimes used inter-changeably with Drug Conjugate, usually to define a Conjugate which is formed by effecting a chemical reaction between a Drug and a Carrier.
"Deconjugatinq Agent~' is an agent capable of interacting ~ith a Con~ugate to liberate or reform at least a portion of the Functional Agent employed in the preparation of the Conjugate.
"CAB" is a cellulose acetate butyrate poly-mer. Such polymers are known in the art, are de-scribed in numerous patents and publications and are 2~ commercially avallable from multiple sources includ-ing Eastman Chemicals. `
"PLA" is a polymer of lactic acid~ Such polymers are known in the art. See U.S. 3,991,7760 "Dalton" is a term becoming increasingly popular in the art to designate molecular weight. A
Dalton number is numerically equivalen~ to a gram molecular weigh~. By way of example, the Dalton number of sucrose is 342~
"Solvent" is an organic liquid having the power to dissolve at least 0.1 weight ~ of a desig-nated polymer of interest at ambient tempera~ure.
"Nonsolven~" is an or~anic liquid miscible with a solvent and having little or no solvent power ~f~
~7--for a designated polymer of interest at ambient temperature.
"Crenate Shape" is the shape assumed by an article having a flexible membrane supported by an internal fluid after the supporting fluid is evacu~
ated from the membrane. The shape assumed by a deflated basketball bladder after the bulk of the air has diffused therefrom is a prime example of a Crenate Shape.
Detailed Description of the Invention _ Fig. 1 represents an embodiment of the invention containin~ a single mini-capsule encapsu-lated within another larger capsule to form a dual capsule~ The structure conta~ns an outer polymeric membrane 10. A first liquid 12 is encapsulated within membrane lOo A mini-microcapsule having a polymeric membrane 14 is encapsulated within membrane 10~ A second liquid 16 is encapsulated within mem-brane 140 In the most preferred embodiment of the invention, liquids 12 and 16 are aqueous liquids, with liquid 16 having a Conjugate dissolved or dis-persed therein and liquid 12 having a Deconjugating Agent dissolved or dispersed therein. The membrane 14 will be semipermeable with respect to the Conju-gate within liquid 160 Upon diffusing through mem-brane 14 and contacting the Deconjugating Agent within liquid 12, an interaction takes place to regenerate the Functional ~gent. The Functional Agent then diffuses through membrane 10 into the system of the host. The structure shown in Fig. 1 is the structure of the dual capsule as it is pre-pared.
In one of the preferred embodiments of the invention, the membranes 10 and 14 shown in Fig~ 1 are semipermeable to water and can be dehydrated by processes subsequently described so as to remove the bulk of the water ~rom bo~h a~ueous li~uid 12 and aqueous liquid 15~ The approximate Crenate Shape that the dehydrated dual capsule takes is shown in Fig. lA. The bulk of the solids of original liquid 16 is maintained within membrane 14. The bulk of 10 the solids originally present in liquid 12 is main tained in the space between membranes 10 and 14.
When the dehydrated dual capsule of Fig. lA is placed in contact wlth water, it imbi~es water so as to dissolve or disperse the solids encapsulated within membranes 10 and 14 to reform the dual capsule in substantially the form illustrated in FigO 1.
In other embodiments of the invention, the liquid 16 may be a simple solution or dispersion of a Functional Agent in a suitable liquid~ usually water, and liquid 12 will contain no material react-able with the Functional Agent and will serve princi-pally as a transport medium for the Functional ~gent~
In such embodiments, membranes 10 and 14 will be fabricated from different polymeric materials so that the membranes will have different diffusion rates for the Functional Agent, with membrane 14 being signiicantly les5 permeable than membrane 10.
Fig. 2 illustrates another embodiment of the invention in which the dual microcapsule contains
3~ encapsulated therein two different mini-microcap sules. The second mini~microcapsule will include a polymeric membrane 18 encapsulatng a third liquid 20. The membrane 18 and the liquid 20 customarily r ~
_g_ will diEfer in at least minor respects from the corresponding elements of the other mini-microcap-sule 7 The physical size of the dual microcapsule6 is not ordinarily a matter of critical importance in the practice of the invention. Customarily, the dual microcaps~les will have outer diameters in the range of from about 20 ~m to 2 mm. The physical size of the mini-microcapsules will be such that they easily fit within the outer meinbrane of the dual microcapsules. Typically, the mini-microcap-sules will have diameters in the range of from about 1 ~m to 1 mm.
The dual microcapsules can be prepared by a modification of the Phase Separation Encapsulation Process defined earlier herein. In this process, the liquid material to be encapsulated and the mini-microcapsules are suspended and stirred in the poly-mer solution to uniformly disperse the liquid mate~
rial and the mini-microcapsules as a fine dispersion throughout the polymer solutionO It is observed that the liquid material tends to cling to the outer mem~ranes of the mini-microcapsules. While continu-ing stirring to keep the liquid material and the mini^microcap ules uniformly dispersed throughout the polymer solution1 a nonsolvent liquid is added to th~ polymer solution ~o change the polymer solu-bility in the medium and cause a phase separation of the dissolved polymer. A~ earlier noted, the polymer either precipitates ~rom the solution or two immisci~
ble liquid phases are produced, one of which i5 rich in polymer and polymer solvent and poor in nonsol~
vent, and the second of which is rich in the nonsol-vent and poor in solvent and polymerO By this means,the suspended particles o the liquid and the mini-microcapsules are encapsulated with the polymerwhich forms the outer membrane of the dual microcap-sules. The entire suspension then i5 added to alarye volume of the nonsolvent which precipitates any remaining dissolved polymer and hardens the outer membrane of the dual microcapsule. The dual microcapsules then are recovered, optionally given a surface treatment to modify the permeability charac-teristics of the outer membrane, and dried.
In the process, the preferred solvents for use are halogenated hydrocarbons having boiling points less than about 65 C and ester~ prepared from alkanol~ containing 1-4 carbon atoms and alka-noic acids containing 1-4 carbon atoms. Particularly suitable solvents are methylene chloride, chloroform and ethyl acetate. Suitable nonsolvents are li~uid hydrocarbons such as hexane, heptane, nonane cyclo-hexane, certain fluorocarbons such as Freon TF,and the like.
The mini-microcapsules employed in the preparation oE the dual microcapsules can be prepared by any of the processes known and reported in the art. When the mini microcapsules employed have a PL,A membrane, they preferably are prepared by ~he novel modified pro~esses subsequently described.
The membrane employed as the outer member of the dual cap~ule and the membrane of the mini~
microcapsule can be fabricated from any polymeric material cu~tomarily employed for such purposes.
Typical polymeric materials which can be employed include cellulose acetate butyrate ICAB), d,l-poly _ * Registered Trademark of E.I. Dupont.
actide ~PLA)~ including its copolymers, cellulose ethers and esters, polyesters, polylactones, poly-amides, silicone rubbers, collagen, and the like.
The polymeric material employed will be selected to be semipermeable to the Conjugate and/or Functional Agent to be encapsulated and/or formed within the Dual Microcapsules. When the dual microcapsules are to be employed for injection into or ingestion by a host, it is desirable to employ in the membranes polymeric materials which are nontoxic to the host, particularly CAB and PLA.
The diffusion rates of materials encapsu-lated within the dual microcapsules are a func~ion both of the encapsulated materials and the polymeric material from which the membranes are fabricated.
The diffusion rates can be modified by giving the membranes a physical or chemical treatment subsequent to their preparation. This can be done by suspending the capsules in a nonsolvent medium containing a chemical reactive with the polymeric material includ-ed in the membrane. Diisocyanates such as TDI can be employed for this purpose, particularly when the polymeric membrane contains reactive hydrogen atoms.
The inclusion of a mini-microcapsule in a dual microcapsule makes possible significantly greater control of the time period over which a drug can be released to a host. Drug-containing microcap-sules presently employed in the medical arts have so-called "zero-order solute release rates"~ That is to say~ the drug delivery Lhrough the membrane is essentially independent of the amount of drug within the microcapsule. With such microcapsules, the time period over which the drug is released thererom is ~ 7~
~12-controlled nearly exclusively by the solubility of the drug included within the microcapsule and the wall permeabili~y to ~he drug.
By employment of the dual capsules of the invention, the effective period over which a drug can be released to a host can be controlled by either or both of two mechanisms~ One mechanism consists of encapsulating the drug within a mini-microcapsule having a membrane with low permeability for the encapsulated drug. The li~uid in which the mini-microcapsule is suspended and the outer membrane of the dual microcapsule will he selected so that the drug diffusion rate through the outer membrane is significantly greater than the corresponding rate through the membrane of the mini-microcapsule. As readily perceived, the effective drug release rate to the host is controlled by the diffusion rate of the drug through the mini microcapsulels membrane.
In this type of dual microcapsule, the medium in which the mini-microcapsule is suspended serves principally as a transpor~ medium for the drug~
A more sophisticated and preferred mechanism involves the use of Conjugate/Deconj~gate Agent systems. In this embodiment of the invention, a Drug Conjugate is encapsulated within the mini-micro-capsuleO The mini-microcapsule is suspended in a liquid containing a Deconjugating AgentO
As earller noted7 a Drug Conjugate is either a reaction product of a Drug and a Carrie~ or a complex formed between the Drug and the Carrier.
The diffu~ion rate of the Drug ~onjugate through the mini-microcapsule 1 5 membrane ordinarily will be considerably lo~er than the diffusion rate of the free drug through the mini-capsule's membrane. When the Drug Conjugate enters the liquid containing the Deconjugating Ayent, the two materials will inter-react with each other to reform or release the drug.
The free drug then diffuses through the outer mem-brane of the dual microcapsule into the host~ As can be readily recognized, the overall drug release rate to the host is controlled by two other rates, specifically, the diffusion rate of the Drug Conju-gate through the mini-microcapsule's membrane and the rate at which the Drug Conjugate reacts with the Deconjugating AgentO
A Drug Conjugate system well suited for use with the dual microcapsules of the invention is a Drug Conjugate formed by reacting a Drug containing a carboxyl group with a monoor diglyceride fatty acid ester~ A typical drug-glyceride conjugate of this type is the ester obtained by reacting aspirin with glyceryl distearate. This conjugate has a molecular weight 786 as compared with the molecular weight of 180 for aspirin. The preparation of such conju~ates is shown by G. Jones, Cb~ist~v ~d In~
~, June 7, 1980, page 452. The aspirin can be esterified with the diglyceride in the presence of triphenyl phosphine and diethyl azo-dicarboxylate as described by R. Aneja et al., r~ n~ <t~e.~
Chemical Communications, 1974, page 963.
The intermediate glyceryl distearate can be prepared by tbe method described by P.H. Bentley and W.
McCrae, ~ , 35, 2082 (1970).
A number of enzyme systems will function as Deconjugating Agents for the above-described drug-glyceride conjugates. Two effective enzymes are serum esterases and pancreatic lipase~ These enzymes cleave the drug -- also ~he ~atty acid ~- from the glyceride. The freed drug, ~he lower molecular weight bound drug fragments (principally the ester between the drug and either glycerine or glyceryl monostearate) and possibly minor quantities of the original Drug Conjugate will diffuse across the outer membrane of ~he dual capsule to enter the host. The original conjugate and its fragments containing still-bound drug will be further cleaved by the enzyme systems in the host to release the drug~
Ano~her Drug Conjugate system of interest for use in the dual microcapsules of the invention are conjugates formed between drugs containing a hydroxyl ~roup or an amine group and a polymeric acid such as polyglutamic acid, Several enzyme systems including gamma-glutaminase and carboxypeptiw dase Y function as effective De~on~ugating Agents for such Drug Conjugates.
Polyglutamic acid is commercially available as the sodium salt in a range of molecular weights from about 2,000 to 100,000 daltons~ Polyglutamic acid has a pendant car~oxyl group for each monomer unit of the polymerO Drugs containing hydroxyl or amine groups can be reacted with the pendant carboxyl groups to form the Drug Conjugate~ A broad range of drug loadings can be provided, which allows for the tailoring of the level of drug loading with the rate of enzymatic deconjugation so as to optimize the drug release rate.
A ~rug Conjugate of this type which can be employed in the dual microcapsules of ~he in~ention to lower systemic blood pressure is the conjugate -15~
formed between dopamine and a polyglu~amic acid having a molecular weight in the range of 2,000 to 15,000. The dopamine is reacted wi~h the polyglu-tamic acid in an aqueous medium containing l-ethyl-3-(3' dimethyl amino propyl) carbodiimide. The reac-tion conditions are selected so that one molecule of dopamine is reacted for each 10-20 glutamic groups present in the polyglutamic acid, Another Drug Conjugate system of interest is the conjugate that can be formed between 17-alpha hydroxyprogesterone and polyglutamic acid. The hydroxyprogesterone is reacted with pendant carboxyl groups of the polyglutamic acid. Th2 chemical link age between the two components, of course, i5 an ester group. The esterification can be carried out employing mixed-pha~e reaction systems of the type reported in the literature. The reaction conditions will be selected so that one molecule of the hydro-xyprogesterone is reacted for each 10 20 pendant carboxyl groups of the polyglutamic acid~
The enzyme gamma-glutaminase i5 very effi-cient at hydroly~ing the gamma glutaminyl amide of dopamine, but not the aspartyl, succinyl or glutaryl amides of dopamine. The enzyme, carboxypeptidase Y
(CPY) is an exopeptidase/ and cleaves peptide bonds sequentially to release individual amino acids from the C~t~rminus of the polypeptide The broad speci-icity of CPY permits it to accept as subskrates, polypeptides having modified side chains (R-groups) containing the drug moiety The CPY removes all L-amino acids f rom most C~terminal sequences. In the event the drug confers a distinctly basic charac-ter upon the drug-polypeptide conjugate~ carboxypep-tidase B may be substituted for CPY
Yet another Drug C,onjugate ~ystem of inker~
est is the class of products that can be prepared ~o~:
1~ A polymeric alcohol containing a plur ality of hydroxyl groups, eOg., dex~ran or polyvinyl alcohol, 2. Chloroacetic or alpha-chloropropionic acid, and 3. A Drug containing a functional group reactive wi~h a bydroxyl group.
An ester is first formed between the poly-meric alcohol and the chloracetic or the alpha-chlor-opropionic acid. The chloro group of the resulting ester then is converted to a hydroxyl group by rou~es known in the art. Finally, a drug having a carboxyl group (or chemical equivalent) is esterified with the resulting pendant hydroxyl group. Drug Conju-gates of this type can be prepared from alpha-methyl DOP~ or gamma-aminoisobutyric acid (GA~A~.
Chymotrypsin and serum esterases can be used to cleave these D~ug Conjugates. Chymotrypsin will cleave the Drug Conjuga~e at the ester carbonyl of the drug quite readily. The serum esterases will cleave at the ester carbonyl of the glycolic acid moiety equally well. Either position of cleavage will lead to low molecular weight products that permeate the outer wall of the dual microcapsules.
Other Conjugate systems can be deYeloped which are stakle above or below a given pH maintained within the mini-microcapsule, Examples of such Con~ugates are salts formed from Drugs containing a basic functlon such as an amino group and a polymeric acid such as polyacrylic acid, an ethylene-maleic anhydride copolymer, an acidic ion-exchange resin .
and the like~ Alternatively, the Conjugate ~an be formed between a Drug containing an acidic function and a high molecular weight base. An aqueous medium buffered to a selected pH can function as a Deconju-gating Agent for such Conjugates.
PLA microcapsules are one of the preferredembodimen~s of the invention. Such PLA microcapsules are difficult to prepare by the Phase Separation Encapsulation Process defined earlier hereinO Speci-fically, when the nonsolven~ liquid is added ~o thePLA-containing solvent solution to encapsulate the core material, it is ob~erved that the PLA-encapsu-lated product appears to have a tacky exterior coat-ingO The encapsulated spheres tend to agglomerate into oversized clusters that are too large for use.
One of the aspects of the present invention is to provide a reliable process for preparing PLA
microcapsules~ In the first step of this process, the PLA is dissolved in a miscible mixture of a solvenk and a nonsolventO The solvent and nonsolvent will be employed in a ratio such that the resulting PLA solution prepared therefrom is very close to its phase separation point. As will be readily recog-nized, the precise ratio of the solvent and nonsol-vent employed will depend both upon the specificsolvent and nonsolvent employed as well as the con-centration of PLA desired in the solution at its phase separation point. A convenient way to prepare the PLA solution i5 to dissolve the PLA in pure solvent9 add sufficient nonsolvent to cause incipient PLA phase separation, and then add the smallest quantity of solvent to redissolve the small quantity of separated PLA.
~18-For reasons which will become apparent from the subsequent descriptions, it is import~nt that the solvent employed have a vapor pressure signifi-cantly higher than the vapor pressure of the nonsol-vent at the temperature employed ts precipitate PLAin the third step of the pro~ess subsequently de-scrib~d.
In the second step of the process; the PLA-containing homogeneous solution prepared in the first step of the process is vigorously agitated and the functional core material is added. The agitation provided will be sufficient to disperse these mate-rials uniformly throughout the continuous PLA-con taining solvent solution as a fine suspension.
In the third step of the process, agitation is continued to maintain the core material dispersed throughout the PLA-containing solvent solution.
Conditions are established to vaporize solvent and nonsolvent from the suspension. While both solvent and nonsolvent will be vaporized and removed from ~he suspension, the solvent will be removed in greater quantities than the nonsolvent by reason of the solvent's higher vapor pressure. The preferen-tial removal of solvent from the system, of course, changes the ratio of the solvent and nonsolvent liquid in which the PLA is dissolved. Since the PLA-containing solution as prepared is near its saturation point Eor PLA, as the composition of the solvent/nonsolvent medium is changed, the PLA will undergo a phase separation. The phase separa~ed PLA
migrates to the surface of the finely dispersed core droplets or particles and begins encapsulation there-of. After a sufficient quantity of PLA has encapsu-~ 4 Qd5 8 ~19--lated the core droplets or particles, the resultingcomplex dispersion is ready for transfer to the fourth step of the process.
In the fourth step of the process, the complex suspension from the third step of the process is transferred into an agitated mass of nonsolvent.
Upon contacting the nonsolvent ~o which the suspen-sion is added, any PLA remaining dissolved in the initial solvent solution is precipitated. A second phenomenon which is believed to occur is the extrac~
tion of the residual solvent from the PLA mem~rane.
In carrying out ~he process, the solvent/
nonsolven~ mixture employed in the ~irst step of ~he process should have the requisite solubility ~o dissolve a convenient quantity of PLA. It is desir-able to employ solvent/nonsolvent mixtures which will dissolve at least about 0,3 part by weight of PLA per 100 parts by volume of solvent/nonsolvent mixture at ambient temperature. It also is desirable to employ solvent/nonsolvent mi~tures having rela-tively sharp changes in PLA solubility capacity with temperature~ The presently preferred solvents for use in the process are halogenated hydrocarbons having an atmospher.ic ~oiling point o~ less than about 65 C. and esters ormed between alkanols con-taining 1-4 carbon atoms and alkanoic acids contain-ing 1-4 carbon atoms. Suitable halogenated hydrocar-bons of this class include methylene chloride and chloroformO The preferred ester is ethyl acetate.
The nonsolvents presently preferred for use in the process are hexane, cyclohexane, heptane, selected mineral spirits, nonane 9 Freon TF and ~he like~
* Registered Trademark of EoI~ Dupont.
p~
~2Q-In the third step of the process~ after the core materials are uniformly dispersed ~hroughout the polymer solution, conditions are established to vaporize ~he solvent and nonsolv2nt from the suspen-sion, This can be done by reducing the pressure onthe suspension by drawing a slight vacuum on the system or suppl~i~g heat to the suspension, or both.
In the em~odiment of the invention in which methylene chloride or chloroform is employed as the solvent and an aliphatic hydrocarbon, such as hexane or heptane, is employed as the nonsolvent, vigorous agitation is sufficient to supply the small quantity of energy required to vaporize the requisi~e quantity of solvent to initiate phase separation of the PLAo In carrying out the fourth step of the process, care should be exercised to transfer the entire suspension from the third step of the process into the agitated nonsolvent before the encapsulated core materlals begin a~glomeration into oversized aggregates, presumably by reason of the somewhat tacky nature of the encapsulating PLA membrane at this stage of the process~ The appropriate point at which the suspension should be transferred to the agitated nonsolvent can be readily established wi~h a minimum of experimentation. It has been the appli-cant's observation that in preparing batches of the si~e subsequently described in the workin~ examples, the suspension should be transerred to the agitated nonsolvent in a time period of between 3 and 10 and preferably 4-7 minutes after the initial phase sepa-ration of the PLA i5 observed in the th.ird step of the process.
~21~
In the final step of the process, it is desirable ~o transfer the suSpension from ~he third step of the process into a large excess of the no~-solvent, e.g~, 3-20 times the ~o~al volume of the solvent solution employed in the f irst step of the process.
The process described above is carried out under essenti~lly isothermal condltions and prefera-bly at ambient temperatures.
Although not presently preferred, it is possi~le to heat the PLA solution in the first step of the process to a temperature somewhat above am~
bient temperature. As the temperature drops in carrying out the second and third steps of the pro-cess, the lowering of the temperature accelerates the phase separation of the ~A.
Cellulose acetate bu~yrate (CAB) is one of the preferred polymeric materials for use in prepar-ing the membrane o~ the mini-microcapsules and the outer membrane of the dual microcapsules. Mini-microcapsules and dual microcapsules including such CAB membranes can be prepared by ~he Phase Separa~ion Encapsulation Process described earlier herein.
It has been noted, however, that minor dif f iculties are encountered which lengthen the process cycle for preparing ei.her of the above-type caps~ules from CAB. Specifically, C~B is somewhat difficult to dissolve in the chlorinated hydrocabon solvents preferred for use in the process~ Specifi~
cally, when the particulate CAB is added to the solvent, the CAB particles swell, ~ecome agglomerated with each other~ and take relatively long periods of time to dissolve to form the true solutions required -~2-in the capsule forma~ion process. This difficulty can be significantly ameliorated by first suspending the CAB particles in a small volume of the nonsolven~
to be su~sequently used in the process~ preerably a liquid hydrocarbon such as hexane, heptane or octane.
When the CAB solvent, e.g~ methylene chloride, is added to the suspension wi~h stirring, the CAB parti-cles readily dissolve~ Thereafter, the remaining steps of the process are conventional.
The following examples are set forth to illustrate certain principles and practices of the inven~ion to those skilled in the art. The examples have ~een run to illustrate the fundamental principle of controlling the release rate of a Functional Agent from the dual microcapsules. Details of the action of ~he ultimately t-ransferred Functional Agent upon the host are not set forth, since such action per se i5 known.
Example 1 This example illustrates the preparation of a dual microcapsule in which a mini-microcapsule having India Ink encapsulated in a CAB membrane and a saline solution are encapsulated in a CAB membrane.
A charge of lo 6 grams of particulate CAB was made to a 400 ml extraction flask which contained 40 ml of n-hexane. A charge of 130 ml of methylene chloride ldichloromethane, MDC) was added to the dispersion.
The sys~em was continuously agitated with a GT21 variable speed laboratory stirrer and stirring rod set at a speed of 2~5 ~fast drive gear ratio~. The polymer tCAB) dissolved in less than a minute, at which time 15 grams of an aqueous core material were added~ The aqueous core was composed of 13 grams of phosphate buffered saline solution plus 2 grams (wet weight) of previously prepared mini microcapsules, having aVeEage diameters of less than 105 ~m, and having an India Ink suspension encapsulated therein.
The India Ink containing mini-microcapsules were used to allow the formed dual microcapsules to be photographed. After the aqueous core droplets were dispersed, 86 ml of n-hexane was added gradually over a thirty minute period (about 3 ml/minute).
The action caused phase separation of the CAB and encapsulation of the mini-microcapsules and ~he saline solution. The dispersion was then siphoned into a beaker which contained 800 ml of n-hexane.
lS During this transfer, both the dispersion and the n-hexane were being s~irred with the GT21 variable speed stirrer and stirring rod set at a speed setting of 2O5 (fast drive gear ratio). After fifteen min-utes of stirring, the product was filtered u~ing a Buchner funnel (about 20 cm diameter)~ filter paper (#589 Black ribbon) and an aspirator. The filtered product was humid air-dried for about 24 hours~ The product was then bottled and stored at room tempera-ture.
Example_2 This example illustrates the preparation of a dual microcapsule in which a mini~microcapsule having India Ink encapsulated in a CAB membrane and a sallne solution are encapsulated in a PLA membrane~
Make a charge of 1.1 grams of particulate PLA (code 35614-19) to a 250 ml extraction flask containing 75 ml of methylene chloride (dichloromethane, MDC).
Agitate the system using a GT21 variable speed labo-ratory stirrer and stirring rod set at a stirrer speed of 2~5 (fast drive gear ra~io). After the PLA
has completely dissolved, add nonane to the solution until a cloud-point develops (i.e., ~o the point where the polymer begins to precipitate)A Approxi-mately 78 ml will be required. Then add MDC dropwise with stirring until the solution is clarified. ~dd an aqueous core containing ten grams of phosphate-bufered saline solution plus 1 gm (wet weight) ofpreviously prepared mini-microcapsules containing the India Ink ~uspension. Continue ~igorous stirring until PLA first precipita~es ~y reason of MDC evapo-ration. Stir for an additional 6 minutes and siphon the resulting slurry into a beaker containing 3,S00 ml of n-heptane and surfactant. Stir the n-hep~ane and the surfactant during transfer using similar stirring equipment and a stirrer speed of 2.5 (fast drive gear ratio~ 5tir for an additional 5 minutes, then recover and dry the dual microcapsules as de~
scribed in Example lo To demonstrate the effectiveness of the dual microcapsules of the invention, employing Conju-gate/Deconjug~ting Agents therein, in controlling the diffusion rate of a Functional Agent from the microcapsules, experiments were run employing glucose ~MW = 180 daltons) or glucose precursors as the Functional Agent.
Four lots of dual microcapsules were pre-30 paredO In all experiments, CAB was used in both themini-microcapsule membranes and the outer membranesO
In lot "A" a 10% glucose solution was included in the mini-microcapsules with the suspending liquid ~25-being a phosphate buffered saline solution (ph =
7.3). Lot l'BI' differed rom lot "A" in that a 10%
dispersion of potato starch sold under the trade designation DIFC0 was included in the mini-microcap-sules. Lot "C" differed from lot "B" in that asmall quantity of alpha amylase was included within the mini-microcapsules to slowly convert the starch to reducing sugars. Lot l'D" differed from lot 'IC"
in that a small quantity of gluco-amylase was includ-ed in the ~uspending saline solution. This enzymewill convert reducing sugars to glucose.
The construction of the dual microcapsules are summarized in Table I together with the pro-duct(s~ expected to be obtained by diffusion of their contents through the outer membrane into an aqueous mediumu TABLE I
Interior ~x~erior Capsule Capsule Capsule Expected System Contents Contents ~esults "A" 10% glucose buffer rapid glucose re-only lease 'IB" 10~ potato buffer no glucose re-s~arch only lease; no reduc-ing sugars re-lease "C" 10% potato buffer no glucose re-starch & only lease; slow re-alpha-amylase ducing sugars re-lease "D" 10~ potato gluco prolonged glu-starch & amylase cose release;
alpha~amylase maybe slow reduc-ing sugars re-lease The dual microcapcules were evaluated in in vitro experiments. Two grams of capsules were placed in f ive milliliters of aqueous test solution (pH 5.5 buffer). The solutions were iltered and assayed for the presene of glucose and reducing sugars.
25 Fresh test solution was added back to the capsules at each predetermined time point. In this experi-men~, the reducing suyar test quantifies glucose plus higher polysaccharides combined, but the slucose meter used is specif ic for glucose only. The results of the experiment are shown in Table 2.
13.~
-26a-~ oo~O
~ _ ~ ~i .~ oo~pO
1/, 1 .~,, ~ o~
~ ~Oq :-.
c~ a ~` ~2~
~ 27--The results show that:
1~ Glucose was rapidly released from the "A" capsules as expected.
2 No carbohydrate was released from the "B" capsules either as glucose or higher poly-saccharides, as expected.
3. The addition of alpha-amylase in the "C" capsules caused the slow release of the higher polysaccharides without producing glucose.
_g_ will diEfer in at least minor respects from the corresponding elements of the other mini-microcap-sule 7 The physical size of the dual microcapsule6 is not ordinarily a matter of critical importance in the practice of the invention. Customarily, the dual microcaps~les will have outer diameters in the range of from about 20 ~m to 2 mm. The physical size of the mini-microcapsules will be such that they easily fit within the outer meinbrane of the dual microcapsules. Typically, the mini-microcap-sules will have diameters in the range of from about 1 ~m to 1 mm.
The dual microcapsules can be prepared by a modification of the Phase Separation Encapsulation Process defined earlier herein. In this process, the liquid material to be encapsulated and the mini-microcapsules are suspended and stirred in the poly-mer solution to uniformly disperse the liquid mate~
rial and the mini-microcapsules as a fine dispersion throughout the polymer solutionO It is observed that the liquid material tends to cling to the outer mem~ranes of the mini-microcapsules. While continu-ing stirring to keep the liquid material and the mini^microcap ules uniformly dispersed throughout the polymer solution1 a nonsolvent liquid is added to th~ polymer solution ~o change the polymer solu-bility in the medium and cause a phase separation of the dissolved polymer. A~ earlier noted, the polymer either precipitates ~rom the solution or two immisci~
ble liquid phases are produced, one of which i5 rich in polymer and polymer solvent and poor in nonsol~
vent, and the second of which is rich in the nonsol-vent and poor in solvent and polymerO By this means,the suspended particles o the liquid and the mini-microcapsules are encapsulated with the polymerwhich forms the outer membrane of the dual microcap-sules. The entire suspension then i5 added to alarye volume of the nonsolvent which precipitates any remaining dissolved polymer and hardens the outer membrane of the dual microcapsule. The dual microcapsules then are recovered, optionally given a surface treatment to modify the permeability charac-teristics of the outer membrane, and dried.
In the process, the preferred solvents for use are halogenated hydrocarbons having boiling points less than about 65 C and ester~ prepared from alkanol~ containing 1-4 carbon atoms and alka-noic acids containing 1-4 carbon atoms. Particularly suitable solvents are methylene chloride, chloroform and ethyl acetate. Suitable nonsolvents are li~uid hydrocarbons such as hexane, heptane, nonane cyclo-hexane, certain fluorocarbons such as Freon TF,and the like.
The mini-microcapsules employed in the preparation oE the dual microcapsules can be prepared by any of the processes known and reported in the art. When the mini microcapsules employed have a PL,A membrane, they preferably are prepared by ~he novel modified pro~esses subsequently described.
The membrane employed as the outer member of the dual cap~ule and the membrane of the mini~
microcapsule can be fabricated from any polymeric material cu~tomarily employed for such purposes.
Typical polymeric materials which can be employed include cellulose acetate butyrate ICAB), d,l-poly _ * Registered Trademark of E.I. Dupont.
actide ~PLA)~ including its copolymers, cellulose ethers and esters, polyesters, polylactones, poly-amides, silicone rubbers, collagen, and the like.
The polymeric material employed will be selected to be semipermeable to the Conjugate and/or Functional Agent to be encapsulated and/or formed within the Dual Microcapsules. When the dual microcapsules are to be employed for injection into or ingestion by a host, it is desirable to employ in the membranes polymeric materials which are nontoxic to the host, particularly CAB and PLA.
The diffusion rates of materials encapsu-lated within the dual microcapsules are a func~ion both of the encapsulated materials and the polymeric material from which the membranes are fabricated.
The diffusion rates can be modified by giving the membranes a physical or chemical treatment subsequent to their preparation. This can be done by suspending the capsules in a nonsolvent medium containing a chemical reactive with the polymeric material includ-ed in the membrane. Diisocyanates such as TDI can be employed for this purpose, particularly when the polymeric membrane contains reactive hydrogen atoms.
The inclusion of a mini-microcapsule in a dual microcapsule makes possible significantly greater control of the time period over which a drug can be released to a host. Drug-containing microcap-sules presently employed in the medical arts have so-called "zero-order solute release rates"~ That is to say~ the drug delivery Lhrough the membrane is essentially independent of the amount of drug within the microcapsule. With such microcapsules, the time period over which the drug is released thererom is ~ 7~
~12-controlled nearly exclusively by the solubility of the drug included within the microcapsule and the wall permeabili~y to ~he drug.
By employment of the dual capsules of the invention, the effective period over which a drug can be released to a host can be controlled by either or both of two mechanisms~ One mechanism consists of encapsulating the drug within a mini-microcapsule having a membrane with low permeability for the encapsulated drug. The li~uid in which the mini-microcapsule is suspended and the outer membrane of the dual microcapsule will he selected so that the drug diffusion rate through the outer membrane is significantly greater than the corresponding rate through the membrane of the mini-microcapsule. As readily perceived, the effective drug release rate to the host is controlled by the diffusion rate of the drug through the mini microcapsulels membrane.
In this type of dual microcapsule, the medium in which the mini-microcapsule is suspended serves principally as a transpor~ medium for the drug~
A more sophisticated and preferred mechanism involves the use of Conjugate/Deconj~gate Agent systems. In this embodiment of the invention, a Drug Conjugate is encapsulated within the mini-micro-capsuleO The mini-microcapsule is suspended in a liquid containing a Deconjugating AgentO
As earller noted7 a Drug Conjugate is either a reaction product of a Drug and a Carrie~ or a complex formed between the Drug and the Carrier.
The diffu~ion rate of the Drug ~onjugate through the mini-microcapsule 1 5 membrane ordinarily will be considerably lo~er than the diffusion rate of the free drug through the mini-capsule's membrane. When the Drug Conjugate enters the liquid containing the Deconjugating Ayent, the two materials will inter-react with each other to reform or release the drug.
The free drug then diffuses through the outer mem-brane of the dual microcapsule into the host~ As can be readily recognized, the overall drug release rate to the host is controlled by two other rates, specifically, the diffusion rate of the Drug Conju-gate through the mini-microcapsule's membrane and the rate at which the Drug Conjugate reacts with the Deconjugating AgentO
A Drug Conjugate system well suited for use with the dual microcapsules of the invention is a Drug Conjugate formed by reacting a Drug containing a carboxyl group with a monoor diglyceride fatty acid ester~ A typical drug-glyceride conjugate of this type is the ester obtained by reacting aspirin with glyceryl distearate. This conjugate has a molecular weight 786 as compared with the molecular weight of 180 for aspirin. The preparation of such conju~ates is shown by G. Jones, Cb~ist~v ~d In~
~, June 7, 1980, page 452. The aspirin can be esterified with the diglyceride in the presence of triphenyl phosphine and diethyl azo-dicarboxylate as described by R. Aneja et al., r~ n~ <t~e.~
Chemical Communications, 1974, page 963.
The intermediate glyceryl distearate can be prepared by tbe method described by P.H. Bentley and W.
McCrae, ~ , 35, 2082 (1970).
A number of enzyme systems will function as Deconjugating Agents for the above-described drug-glyceride conjugates. Two effective enzymes are serum esterases and pancreatic lipase~ These enzymes cleave the drug -- also ~he ~atty acid ~- from the glyceride. The freed drug, ~he lower molecular weight bound drug fragments (principally the ester between the drug and either glycerine or glyceryl monostearate) and possibly minor quantities of the original Drug Conjugate will diffuse across the outer membrane of ~he dual capsule to enter the host. The original conjugate and its fragments containing still-bound drug will be further cleaved by the enzyme systems in the host to release the drug~
Ano~her Drug Conjugate system of interest for use in the dual microcapsules of the invention are conjugates formed between drugs containing a hydroxyl ~roup or an amine group and a polymeric acid such as polyglutamic acid, Several enzyme systems including gamma-glutaminase and carboxypeptiw dase Y function as effective De~on~ugating Agents for such Drug Conjugates.
Polyglutamic acid is commercially available as the sodium salt in a range of molecular weights from about 2,000 to 100,000 daltons~ Polyglutamic acid has a pendant car~oxyl group for each monomer unit of the polymerO Drugs containing hydroxyl or amine groups can be reacted with the pendant carboxyl groups to form the Drug Conjugate~ A broad range of drug loadings can be provided, which allows for the tailoring of the level of drug loading with the rate of enzymatic deconjugation so as to optimize the drug release rate.
A ~rug Conjugate of this type which can be employed in the dual microcapsules of ~he in~ention to lower systemic blood pressure is the conjugate -15~
formed between dopamine and a polyglu~amic acid having a molecular weight in the range of 2,000 to 15,000. The dopamine is reacted wi~h the polyglu-tamic acid in an aqueous medium containing l-ethyl-3-(3' dimethyl amino propyl) carbodiimide. The reac-tion conditions are selected so that one molecule of dopamine is reacted for each 10-20 glutamic groups present in the polyglutamic acid, Another Drug Conjugate system of interest is the conjugate that can be formed between 17-alpha hydroxyprogesterone and polyglutamic acid. The hydroxyprogesterone is reacted with pendant carboxyl groups of the polyglutamic acid. Th2 chemical link age between the two components, of course, i5 an ester group. The esterification can be carried out employing mixed-pha~e reaction systems of the type reported in the literature. The reaction conditions will be selected so that one molecule of the hydro-xyprogesterone is reacted for each 10 20 pendant carboxyl groups of the polyglutamic acid~
The enzyme gamma-glutaminase i5 very effi-cient at hydroly~ing the gamma glutaminyl amide of dopamine, but not the aspartyl, succinyl or glutaryl amides of dopamine. The enzyme, carboxypeptidase Y
(CPY) is an exopeptidase/ and cleaves peptide bonds sequentially to release individual amino acids from the C~t~rminus of the polypeptide The broad speci-icity of CPY permits it to accept as subskrates, polypeptides having modified side chains (R-groups) containing the drug moiety The CPY removes all L-amino acids f rom most C~terminal sequences. In the event the drug confers a distinctly basic charac-ter upon the drug-polypeptide conjugate~ carboxypep-tidase B may be substituted for CPY
Yet another Drug C,onjugate ~ystem of inker~
est is the class of products that can be prepared ~o~:
1~ A polymeric alcohol containing a plur ality of hydroxyl groups, eOg., dex~ran or polyvinyl alcohol, 2. Chloroacetic or alpha-chloropropionic acid, and 3. A Drug containing a functional group reactive wi~h a bydroxyl group.
An ester is first formed between the poly-meric alcohol and the chloracetic or the alpha-chlor-opropionic acid. The chloro group of the resulting ester then is converted to a hydroxyl group by rou~es known in the art. Finally, a drug having a carboxyl group (or chemical equivalent) is esterified with the resulting pendant hydroxyl group. Drug Conju-gates of this type can be prepared from alpha-methyl DOP~ or gamma-aminoisobutyric acid (GA~A~.
Chymotrypsin and serum esterases can be used to cleave these D~ug Conjugates. Chymotrypsin will cleave the Drug Conjuga~e at the ester carbonyl of the drug quite readily. The serum esterases will cleave at the ester carbonyl of the glycolic acid moiety equally well. Either position of cleavage will lead to low molecular weight products that permeate the outer wall of the dual microcapsules.
Other Conjugate systems can be deYeloped which are stakle above or below a given pH maintained within the mini-microcapsule, Examples of such Con~ugates are salts formed from Drugs containing a basic functlon such as an amino group and a polymeric acid such as polyacrylic acid, an ethylene-maleic anhydride copolymer, an acidic ion-exchange resin .
and the like~ Alternatively, the Conjugate ~an be formed between a Drug containing an acidic function and a high molecular weight base. An aqueous medium buffered to a selected pH can function as a Deconju-gating Agent for such Conjugates.
PLA microcapsules are one of the preferredembodimen~s of the invention. Such PLA microcapsules are difficult to prepare by the Phase Separation Encapsulation Process defined earlier hereinO Speci-fically, when the nonsolven~ liquid is added ~o thePLA-containing solvent solution to encapsulate the core material, it is ob~erved that the PLA-encapsu-lated product appears to have a tacky exterior coat-ingO The encapsulated spheres tend to agglomerate into oversized clusters that are too large for use.
One of the aspects of the present invention is to provide a reliable process for preparing PLA
microcapsules~ In the first step of this process, the PLA is dissolved in a miscible mixture of a solvenk and a nonsolventO The solvent and nonsolvent will be employed in a ratio such that the resulting PLA solution prepared therefrom is very close to its phase separation point. As will be readily recog-nized, the precise ratio of the solvent and nonsol-vent employed will depend both upon the specificsolvent and nonsolvent employed as well as the con-centration of PLA desired in the solution at its phase separation point. A convenient way to prepare the PLA solution i5 to dissolve the PLA in pure solvent9 add sufficient nonsolvent to cause incipient PLA phase separation, and then add the smallest quantity of solvent to redissolve the small quantity of separated PLA.
~18-For reasons which will become apparent from the subsequent descriptions, it is import~nt that the solvent employed have a vapor pressure signifi-cantly higher than the vapor pressure of the nonsol-vent at the temperature employed ts precipitate PLAin the third step of the pro~ess subsequently de-scrib~d.
In the second step of the process; the PLA-containing homogeneous solution prepared in the first step of the process is vigorously agitated and the functional core material is added. The agitation provided will be sufficient to disperse these mate-rials uniformly throughout the continuous PLA-con taining solvent solution as a fine suspension.
In the third step of the process, agitation is continued to maintain the core material dispersed throughout the PLA-containing solvent solution.
Conditions are established to vaporize solvent and nonsolvent from the suspension. While both solvent and nonsolvent will be vaporized and removed from ~he suspension, the solvent will be removed in greater quantities than the nonsolvent by reason of the solvent's higher vapor pressure. The preferen-tial removal of solvent from the system, of course, changes the ratio of the solvent and nonsolvent liquid in which the PLA is dissolved. Since the PLA-containing solution as prepared is near its saturation point Eor PLA, as the composition of the solvent/nonsolvent medium is changed, the PLA will undergo a phase separation. The phase separa~ed PLA
migrates to the surface of the finely dispersed core droplets or particles and begins encapsulation there-of. After a sufficient quantity of PLA has encapsu-~ 4 Qd5 8 ~19--lated the core droplets or particles, the resultingcomplex dispersion is ready for transfer to the fourth step of the process.
In the fourth step of the process, the complex suspension from the third step of the process is transferred into an agitated mass of nonsolvent.
Upon contacting the nonsolvent ~o which the suspen-sion is added, any PLA remaining dissolved in the initial solvent solution is precipitated. A second phenomenon which is believed to occur is the extrac~
tion of the residual solvent from the PLA mem~rane.
In carrying out ~he process, the solvent/
nonsolven~ mixture employed in the ~irst step of ~he process should have the requisite solubility ~o dissolve a convenient quantity of PLA. It is desir-able to employ solvent/nonsolvent mixtures which will dissolve at least about 0,3 part by weight of PLA per 100 parts by volume of solvent/nonsolvent mixture at ambient temperature. It also is desirable to employ solvent/nonsolvent mi~tures having rela-tively sharp changes in PLA solubility capacity with temperature~ The presently preferred solvents for use in the process are halogenated hydrocarbons having an atmospher.ic ~oiling point o~ less than about 65 C. and esters ormed between alkanols con-taining 1-4 carbon atoms and alkanoic acids contain-ing 1-4 carbon atoms. Suitable halogenated hydrocar-bons of this class include methylene chloride and chloroformO The preferred ester is ethyl acetate.
The nonsolvents presently preferred for use in the process are hexane, cyclohexane, heptane, selected mineral spirits, nonane 9 Freon TF and ~he like~
* Registered Trademark of EoI~ Dupont.
p~
~2Q-In the third step of the process~ after the core materials are uniformly dispersed ~hroughout the polymer solution, conditions are established to vaporize ~he solvent and nonsolv2nt from the suspen-sion, This can be done by reducing the pressure onthe suspension by drawing a slight vacuum on the system or suppl~i~g heat to the suspension, or both.
In the em~odiment of the invention in which methylene chloride or chloroform is employed as the solvent and an aliphatic hydrocarbon, such as hexane or heptane, is employed as the nonsolvent, vigorous agitation is sufficient to supply the small quantity of energy required to vaporize the requisi~e quantity of solvent to initiate phase separation of the PLAo In carrying out the fourth step of the process, care should be exercised to transfer the entire suspension from the third step of the process into the agitated nonsolvent before the encapsulated core materlals begin a~glomeration into oversized aggregates, presumably by reason of the somewhat tacky nature of the encapsulating PLA membrane at this stage of the process~ The appropriate point at which the suspension should be transferred to the agitated nonsolvent can be readily established wi~h a minimum of experimentation. It has been the appli-cant's observation that in preparing batches of the si~e subsequently described in the workin~ examples, the suspension should be transerred to the agitated nonsolvent in a time period of between 3 and 10 and preferably 4-7 minutes after the initial phase sepa-ration of the PLA i5 observed in the th.ird step of the process.
~21~
In the final step of the process, it is desirable ~o transfer the suSpension from ~he third step of the process into a large excess of the no~-solvent, e.g~, 3-20 times the ~o~al volume of the solvent solution employed in the f irst step of the process.
The process described above is carried out under essenti~lly isothermal condltions and prefera-bly at ambient temperatures.
Although not presently preferred, it is possi~le to heat the PLA solution in the first step of the process to a temperature somewhat above am~
bient temperature. As the temperature drops in carrying out the second and third steps of the pro-cess, the lowering of the temperature accelerates the phase separation of the ~A.
Cellulose acetate bu~yrate (CAB) is one of the preferred polymeric materials for use in prepar-ing the membrane o~ the mini-microcapsules and the outer membrane of the dual microcapsules. Mini-microcapsules and dual microcapsules including such CAB membranes can be prepared by ~he Phase Separa~ion Encapsulation Process described earlier herein.
It has been noted, however, that minor dif f iculties are encountered which lengthen the process cycle for preparing ei.her of the above-type caps~ules from CAB. Specifically, C~B is somewhat difficult to dissolve in the chlorinated hydrocabon solvents preferred for use in the process~ Specifi~
cally, when the particulate CAB is added to the solvent, the CAB particles swell, ~ecome agglomerated with each other~ and take relatively long periods of time to dissolve to form the true solutions required -~2-in the capsule forma~ion process. This difficulty can be significantly ameliorated by first suspending the CAB particles in a small volume of the nonsolven~
to be su~sequently used in the process~ preerably a liquid hydrocarbon such as hexane, heptane or octane.
When the CAB solvent, e.g~ methylene chloride, is added to the suspension wi~h stirring, the CAB parti-cles readily dissolve~ Thereafter, the remaining steps of the process are conventional.
The following examples are set forth to illustrate certain principles and practices of the inven~ion to those skilled in the art. The examples have ~een run to illustrate the fundamental principle of controlling the release rate of a Functional Agent from the dual microcapsules. Details of the action of ~he ultimately t-ransferred Functional Agent upon the host are not set forth, since such action per se i5 known.
Example 1 This example illustrates the preparation of a dual microcapsule in which a mini-microcapsule having India Ink encapsulated in a CAB membrane and a saline solution are encapsulated in a CAB membrane.
A charge of lo 6 grams of particulate CAB was made to a 400 ml extraction flask which contained 40 ml of n-hexane. A charge of 130 ml of methylene chloride ldichloromethane, MDC) was added to the dispersion.
The sys~em was continuously agitated with a GT21 variable speed laboratory stirrer and stirring rod set at a speed of 2~5 ~fast drive gear ratio~. The polymer tCAB) dissolved in less than a minute, at which time 15 grams of an aqueous core material were added~ The aqueous core was composed of 13 grams of phosphate buffered saline solution plus 2 grams (wet weight) of previously prepared mini microcapsules, having aVeEage diameters of less than 105 ~m, and having an India Ink suspension encapsulated therein.
The India Ink containing mini-microcapsules were used to allow the formed dual microcapsules to be photographed. After the aqueous core droplets were dispersed, 86 ml of n-hexane was added gradually over a thirty minute period (about 3 ml/minute).
The action caused phase separation of the CAB and encapsulation of the mini-microcapsules and ~he saline solution. The dispersion was then siphoned into a beaker which contained 800 ml of n-hexane.
lS During this transfer, both the dispersion and the n-hexane were being s~irred with the GT21 variable speed stirrer and stirring rod set at a speed setting of 2O5 (fast drive gear ratio). After fifteen min-utes of stirring, the product was filtered u~ing a Buchner funnel (about 20 cm diameter)~ filter paper (#589 Black ribbon) and an aspirator. The filtered product was humid air-dried for about 24 hours~ The product was then bottled and stored at room tempera-ture.
Example_2 This example illustrates the preparation of a dual microcapsule in which a mini~microcapsule having India Ink encapsulated in a CAB membrane and a sallne solution are encapsulated in a PLA membrane~
Make a charge of 1.1 grams of particulate PLA (code 35614-19) to a 250 ml extraction flask containing 75 ml of methylene chloride (dichloromethane, MDC).
Agitate the system using a GT21 variable speed labo-ratory stirrer and stirring rod set at a stirrer speed of 2~5 (fast drive gear ra~io). After the PLA
has completely dissolved, add nonane to the solution until a cloud-point develops (i.e., ~o the point where the polymer begins to precipitate)A Approxi-mately 78 ml will be required. Then add MDC dropwise with stirring until the solution is clarified. ~dd an aqueous core containing ten grams of phosphate-bufered saline solution plus 1 gm (wet weight) ofpreviously prepared mini-microcapsules containing the India Ink ~uspension. Continue ~igorous stirring until PLA first precipita~es ~y reason of MDC evapo-ration. Stir for an additional 6 minutes and siphon the resulting slurry into a beaker containing 3,S00 ml of n-heptane and surfactant. Stir the n-hep~ane and the surfactant during transfer using similar stirring equipment and a stirrer speed of 2.5 (fast drive gear ratio~ 5tir for an additional 5 minutes, then recover and dry the dual microcapsules as de~
scribed in Example lo To demonstrate the effectiveness of the dual microcapsules of the invention, employing Conju-gate/Deconjug~ting Agents therein, in controlling the diffusion rate of a Functional Agent from the microcapsules, experiments were run employing glucose ~MW = 180 daltons) or glucose precursors as the Functional Agent.
Four lots of dual microcapsules were pre-30 paredO In all experiments, CAB was used in both themini-microcapsule membranes and the outer membranesO
In lot "A" a 10% glucose solution was included in the mini-microcapsules with the suspending liquid ~25-being a phosphate buffered saline solution (ph =
7.3). Lot l'BI' differed rom lot "A" in that a 10%
dispersion of potato starch sold under the trade designation DIFC0 was included in the mini-microcap-sules. Lot "C" differed from lot "B" in that asmall quantity of alpha amylase was included within the mini-microcapsules to slowly convert the starch to reducing sugars. Lot l'D" differed from lot 'IC"
in that a small quantity of gluco-amylase was includ-ed in the ~uspending saline solution. This enzymewill convert reducing sugars to glucose.
The construction of the dual microcapsules are summarized in Table I together with the pro-duct(s~ expected to be obtained by diffusion of their contents through the outer membrane into an aqueous mediumu TABLE I
Interior ~x~erior Capsule Capsule Capsule Expected System Contents Contents ~esults "A" 10% glucose buffer rapid glucose re-only lease 'IB" 10~ potato buffer no glucose re-s~arch only lease; no reduc-ing sugars re-lease "C" 10% potato buffer no glucose re-starch & only lease; slow re-alpha-amylase ducing sugars re-lease "D" 10~ potato gluco prolonged glu-starch & amylase cose release;
alpha~amylase maybe slow reduc-ing sugars re-lease The dual microcapcules were evaluated in in vitro experiments. Two grams of capsules were placed in f ive milliliters of aqueous test solution (pH 5.5 buffer). The solutions were iltered and assayed for the presene of glucose and reducing sugars.
25 Fresh test solution was added back to the capsules at each predetermined time point. In this experi-men~, the reducing suyar test quantifies glucose plus higher polysaccharides combined, but the slucose meter used is specif ic for glucose only. The results of the experiment are shown in Table 2.
13.~
-26a-~ oo~O
~ _ ~ ~i .~ oo~pO
1/, 1 .~,, ~ o~
~ ~Oq :-.
c~ a ~` ~2~
~ 27--The results show that:
1~ Glucose was rapidly released from the "A" capsules as expected.
2 No carbohydrate was released from the "B" capsules either as glucose or higher poly-saccharides, as expected.
3. The addition of alpha-amylase in the "C" capsules caused the slow release of the higher polysaccharides without producing glucose.
4. With ~he "D" capsules, glucose was released, but not over the entire 20-hour period.
The experiment demonstrates the operating principle of the dual microcapsules. The failure to release glucose from the "D" capsules over the entire 15 20-hour period doubtlessly resulted from inadequate glucoamylase activity for the continued hydrolysis of the higher polysaccharides. This shor~coming can be corrected by modifying enzyme activity within the exterior capsule of khe "~" capsules.
As earlier noted, the preferred embodiments of the invention have a Conjugate (usually dispersed in an aqueous medium) encapsulated within the mini-microcapsules and have the Deconjugating Agent dis-persed in an aqueous medium in the space intermediate of the mini-microcapsule membrane and the outer membraneO The Conjugate will diffuse throu~h the mini microcapsule membrane whenever the dual micro-capsules contain water. As earlier noted~ to prolong ~he effective shelf-life of the dual capsules/ short-ly after their preparation they should be dehydrated to form the Crenate Shape earlier discussed and ustrated in Fig. lA. The dehydration step can be carried out by mild heating, drying in a vacuum oven, or in some cases, simply upon standing in air ~~ ~
-2~-where the membranes are very permeable to water.
The dual micxocapsules, after being dehydrated, should be stored in sealed containers and preerably under anhydrous conditions. Shortly before usel the dehydrated dual microcapsules will be rehydrated by being steeped in water.
Al~ernate means can be employed to extend the shelf-life of the dual microcapsules. One such techni~ue is to encapsulate the Functional Agent within a mini-microcapsule whose membrane is essen-tially totally impermeable to the Functional Agent.
The mini-microcapsule membrane in this embodiment will be prepared from a polymeric material different from the polymeri~ material employed to prepare the outer membrane of the dual microcapsule. ~he polymer included in the membrane of the mini-microcapsule will be fabricated from a material which can be ruptured or degradated by a treatment process having no corresponding effect upon the outer membrane of the dual microcapsule. Treatments of the ~ype ~is-ualized are microwave radiation, ultraviolet radia-tion, laser radiation, treatment with ultrasonic vibrations and the like. Alternatively, the membrane of the mini-microcapsules can be fabricated from a friable polymer while the outer membrane is fabri-cated from a flexible polymer. The mini microcap-sules' walls can be ruptured by application of a compressive force. In this embodiment of the inven-tion, of course, the rate of release of the Func-tional Rate to the host will be controlled solely byits diffusion rate through the outer membrane of the dual microcapsule.
The dual microcapsules of the invention can be employed to deliver various types of medication to mammals, including both man and domestic animals.
Materials which can be administered effectively include contraceptive materials, narcotic antago-nists~ cardiac axrhythmia agents/ chemo~herapeutic drugs and various veterinary products~
In a modification of the dual capsules previously described, they can be employed to remove a toxicant from a host. In this embodiment, the outer membrane of the dual microcapsule will be at least semipermeable to the toxicant in the host.
The liquid included within the dual microcapsule between the outer membrane of the capsule and the membrane of the mini-microcapsule will con~ain a Carrier which will react with the toxicant to form a first intermediate product, which can be either a true chemical reaction product or a complex formed between the toxicant and the CarrierO The first intermediate product then will diffuse through the membrane of the mini-microcapsule. The mini-micro-capsule will include therein a rnaterial which reacts with the first intermediate product to irreversibly convert the first intermediate produc~ and the ~oxi-cant contained therein to one or more materialsharmless to the hos~.
The dual microcapsules of the invention also can be employed to provide a prolonged release of Func~ional Agents other than drugs. Among the Functional Agents of the type that can ke delivered include herbicides, fertili.%ers, growth regulator substances, deodorizers, pheromones and other like materials.
-30~
While the processes and products herein described constitute preferred embodiments of the invention~ it is to be understood that the invention is not limited to these precise processes and pro-ducts, and that changes may be made therein withoutdepartiny from the scope of the invention which is defined in the appended claims.
What is claimed .is:
The experiment demonstrates the operating principle of the dual microcapsules. The failure to release glucose from the "D" capsules over the entire 15 20-hour period doubtlessly resulted from inadequate glucoamylase activity for the continued hydrolysis of the higher polysaccharides. This shor~coming can be corrected by modifying enzyme activity within the exterior capsule of khe "~" capsules.
As earlier noted, the preferred embodiments of the invention have a Conjugate (usually dispersed in an aqueous medium) encapsulated within the mini-microcapsules and have the Deconjugating Agent dis-persed in an aqueous medium in the space intermediate of the mini-microcapsule membrane and the outer membraneO The Conjugate will diffuse throu~h the mini microcapsule membrane whenever the dual micro-capsules contain water. As earlier noted~ to prolong ~he effective shelf-life of the dual capsules/ short-ly after their preparation they should be dehydrated to form the Crenate Shape earlier discussed and ustrated in Fig. lA. The dehydration step can be carried out by mild heating, drying in a vacuum oven, or in some cases, simply upon standing in air ~~ ~
-2~-where the membranes are very permeable to water.
The dual micxocapsules, after being dehydrated, should be stored in sealed containers and preerably under anhydrous conditions. Shortly before usel the dehydrated dual microcapsules will be rehydrated by being steeped in water.
Al~ernate means can be employed to extend the shelf-life of the dual microcapsules. One such techni~ue is to encapsulate the Functional Agent within a mini-microcapsule whose membrane is essen-tially totally impermeable to the Functional Agent.
The mini-microcapsule membrane in this embodiment will be prepared from a polymeric material different from the polymeri~ material employed to prepare the outer membrane of the dual microcapsule. ~he polymer included in the membrane of the mini-microcapsule will be fabricated from a material which can be ruptured or degradated by a treatment process having no corresponding effect upon the outer membrane of the dual microcapsule. Treatments of the ~ype ~is-ualized are microwave radiation, ultraviolet radia-tion, laser radiation, treatment with ultrasonic vibrations and the like. Alternatively, the membrane of the mini-microcapsules can be fabricated from a friable polymer while the outer membrane is fabri-cated from a flexible polymer. The mini microcap-sules' walls can be ruptured by application of a compressive force. In this embodiment of the inven-tion, of course, the rate of release of the Func-tional Rate to the host will be controlled solely byits diffusion rate through the outer membrane of the dual microcapsule.
The dual microcapsules of the invention can be employed to deliver various types of medication to mammals, including both man and domestic animals.
Materials which can be administered effectively include contraceptive materials, narcotic antago-nists~ cardiac axrhythmia agents/ chemo~herapeutic drugs and various veterinary products~
In a modification of the dual capsules previously described, they can be employed to remove a toxicant from a host. In this embodiment, the outer membrane of the dual microcapsule will be at least semipermeable to the toxicant in the host.
The liquid included within the dual microcapsule between the outer membrane of the capsule and the membrane of the mini-microcapsule will con~ain a Carrier which will react with the toxicant to form a first intermediate product, which can be either a true chemical reaction product or a complex formed between the toxicant and the CarrierO The first intermediate product then will diffuse through the membrane of the mini-microcapsule. The mini-micro-capsule will include therein a rnaterial which reacts with the first intermediate product to irreversibly convert the first intermediate produc~ and the ~oxi-cant contained therein to one or more materialsharmless to the hos~.
The dual microcapsules of the invention also can be employed to provide a prolonged release of Func~ional Agents other than drugs. Among the Functional Agents of the type that can ke delivered include herbicides, fertili.%ers, growth regulator substances, deodorizers, pheromones and other like materials.
-30~
While the processes and products herein described constitute preferred embodiments of the invention~ it is to be understood that the invention is not limited to these precise processes and pro-ducts, and that changes may be made therein withoutdepartiny from the scope of the invention which is defined in the appended claims.
What is claimed .is:
Claims (29)
1. Dual microcapsules having encapsulated therein at least two liquids and comprising:
(a) An outer polymeric membrane encapsu-lating a first liquid, and (b) At least one mini-microcapsule sus-pended in said first liquid, said mini-microcapsule(s) having polymeric membrane(s) encapsulating a second liquid;
said dual microcapsules being further characterized in that;
(c) The second liquid contains therein a Conjugate formed between a Functional Agent and a Carrier, (d) The first liquid contains therein a Deconjugating Agent, (e) The polymeric membrane(s) of the mini-microcapsule(s) are at least semipermeable with respect to the Conjugate so that said Conjugate can diffuse therethrough and into said first liquid at a controlled preselec-ted rate, (f) The Conjugate and the Deconjugating Agent are interactive with each other to release or reform the Functional Agent from the Conjugate, and (g) The outer polymeric membrane is at least semipermeable with respect to the Functional Agent so that said Functional Agent can diffuse therethrough at a con-trolled preselected rate.
(a) An outer polymeric membrane encapsu-lating a first liquid, and (b) At least one mini-microcapsule sus-pended in said first liquid, said mini-microcapsule(s) having polymeric membrane(s) encapsulating a second liquid;
said dual microcapsules being further characterized in that;
(c) The second liquid contains therein a Conjugate formed between a Functional Agent and a Carrier, (d) The first liquid contains therein a Deconjugating Agent, (e) The polymeric membrane(s) of the mini-microcapsule(s) are at least semipermeable with respect to the Conjugate so that said Conjugate can diffuse therethrough and into said first liquid at a controlled preselec-ted rate, (f) The Conjugate and the Deconjugating Agent are interactive with each other to release or reform the Functional Agent from the Conjugate, and (g) The outer polymeric membrane is at least semipermeable with respect to the Functional Agent so that said Functional Agent can diffuse therethrough at a con-trolled preselected rate.
2. Dual microcapsules of claim 1 in which the Conjugate is formed between a low molecular weight Functional Agent and a Carrier,
3. Dual microcapsules of claim 2 in which the low molecular weight Functional Agent has a molecular weight of less than about 1,000.
4. Dual microcapsules of claim 2 in which the Deconjugating Agent is a deconjugating enzyme.
5. Dual microcapsules of claim 4 in which the Conjugate is a Drug Conjugate.
6. Dual microcapsules of claim 1 in which the mini-microcapsules have diameters in the range of about 1 to about 1,000 µm.
7. Dual microcapsules of claim 6 which have diameters in the range of about 10 µm to about 2.00 mm.
8. Dual microcapsules having the capacity of removing a toxicant from a host, said microcapsules containing at least two functionally reactive mate-rials and comprising:
(a) An outer polymeric membrane encapsula-ting a liquid containing a first functional-ly reactive agent, and (b) At least one mini-microcapsule sus-pended in said first liquid, said mini-microcapsules having polymeric membrane(s) encapsulating a second functionally reactive agent;
said dual microcapsule(s) being further characterized in that;
(c) The outer membrane is at least semi-permeable to the toxicant in the host, (d) The first functionally reactive agent is reactive with the toxicant to generate at least one new entity, (e) The membrane(s) of the mini-microcap sule(s) are at least semipermeable to the new entity generated in step (d), and (f) The second functionally reactive agent within the mini-microcapsule(s) is reactable with the new entity generated in step (d) to irreversibly convert said entity to a product that Is harmless to the host.
(a) An outer polymeric membrane encapsula-ting a liquid containing a first functional-ly reactive agent, and (b) At least one mini-microcapsule sus-pended in said first liquid, said mini-microcapsules having polymeric membrane(s) encapsulating a second functionally reactive agent;
said dual microcapsule(s) being further characterized in that;
(c) The outer membrane is at least semi-permeable to the toxicant in the host, (d) The first functionally reactive agent is reactive with the toxicant to generate at least one new entity, (e) The membrane(s) of the mini-microcap sule(s) are at least semipermeable to the new entity generated in step (d), and (f) The second functionally reactive agent within the mini-microcapsule(s) is reactable with the new entity generated in step (d) to irreversibly convert said entity to a product that Is harmless to the host.
9. Dual microcapsules having encapsulated therein at least two materials and comprising an outer polymeric membrane encapsulating:
(a) At least one mini-microcapsule having encapsulated therein a substantially dry, but readily hydrateable Conjugate formed between a Functional Agent and a Carrier, and (b) A substantially dry but readily hydra-teable Deconjugating Agent between the membrane of the mini-microcapsule and the outer membrane;
said dual microcapsule being further characterized in that;
(c) The entire microcapsule, including the mini-microcapsule(s) encapsulated therein, has a Crenate Structure, (d) The outer membrane and the membrane(s) of the mini-microcapsules are at least semipermeable to water, and (e) The dual microcapsule will, when con-tacted with water, imbibe water so as to disperse both the Conjugate and the Deconju-gating Agent in aqueous media which are kept out of direct contact with each other by the membrane(s) of the mini-microcap-sule(s).
(a) At least one mini-microcapsule having encapsulated therein a substantially dry, but readily hydrateable Conjugate formed between a Functional Agent and a Carrier, and (b) A substantially dry but readily hydra-teable Deconjugating Agent between the membrane of the mini-microcapsule and the outer membrane;
said dual microcapsule being further characterized in that;
(c) The entire microcapsule, including the mini-microcapsule(s) encapsulated therein, has a Crenate Structure, (d) The outer membrane and the membrane(s) of the mini-microcapsules are at least semipermeable to water, and (e) The dual microcapsule will, when con-tacted with water, imbibe water so as to disperse both the Conjugate and the Deconju-gating Agent in aqueous media which are kept out of direct contact with each other by the membrane(s) of the mini-microcap-sule(s).
10. A dual microcapsule of claim 9 in which the Conjugate is formed between a Functional Agent and a Carrier.
11. A dual microcapsule of claim 10 in which the Conjugate is a Drug Conjugate and the Deconju-gating Agent is a deconjugating enzyme.
12. Dual microcapsules having encapsulated therein at least two materials and comprising:
(a) An outer polymeric membrane encapsu-lating a liquid which contains therein a Deconjugating Agent, and (b) At least one mini-microcapsule sus-pended in said liquid, said mini-microcap-sule having a polymeric membrane encapsu-lating a Conjugate formed between a Func-tional Agent and a Carrier;
said dual microcapsule being further characterized in that;
(c) The polymer included in the membrane(s) of the mini-microcapsule(s) is different from the polymer included in the outer polymeric membrane.
(a) An outer polymeric membrane encapsu-lating a liquid which contains therein a Deconjugating Agent, and (b) At least one mini-microcapsule sus-pended in said liquid, said mini-microcap-sule having a polymeric membrane encapsu-lating a Conjugate formed between a Func-tional Agent and a Carrier;
said dual microcapsule being further characterized in that;
(c) The polymer included in the membrane(s) of the mini-microcapsule(s) is different from the polymer included in the outer polymeric membrane.
13. Dual microcapsules of claim 12 in which the membrane(s) of the mini-microcapsules are decomposa-ble by a treatment which will not decompose the outer membrane.
14. Dual microcapsules of claim 13 in which the membrane(s) of the mini-microcapsules are decomposa-ble by exposure to laser, microwave or ultraviolet radiation.
15. Dual microcapsules of claim 13 in which the membranes of the mini-microcapsules are friable and the outer membranes are flexible so that a compres-sive force will rupture the mini-microcapsules' membranes without rupturing the outer membranes.
16. Dual microcapsules of claim 13 in which the membrane(s) of the mini-microcapsules are decomposa-ble by exposure to ultrasonic vibrations,
17. A process for preparing dual microcapsules having encapsulated therein both a Conjugate formed between a Functional Agent and a Carrier and a Decon-jugating Agent which comprises:
(a) Agitating a solution of a polymer in an organic solvent therefore and adding thereto a mixture of;
(1) an aqueous liquid which is im-miscible with said polymer solution and includes therein a Deconjugating Agent, and (2) mini-microcapsules having a Con-jugate encapsulated therein, so as to uniformly disperse said aqueous liquid and said mini-microcapsules through-out said polymer solution, and (b) Agitating the suspension of step (a) and adding thereto an organic liquid which is miscible with the polymer solvent and has little or no solvent power for said polymer in an amount sufficient to cause phase separation of the polymer and encap-sulation of the aqueous liquid and the mini-microcapsule(s).
(a) Agitating a solution of a polymer in an organic solvent therefore and adding thereto a mixture of;
(1) an aqueous liquid which is im-miscible with said polymer solution and includes therein a Deconjugating Agent, and (2) mini-microcapsules having a Con-jugate encapsulated therein, so as to uniformly disperse said aqueous liquid and said mini-microcapsules through-out said polymer solution, and (b) Agitating the suspension of step (a) and adding thereto an organic liquid which is miscible with the polymer solvent and has little or no solvent power for said polymer in an amount sufficient to cause phase separation of the polymer and encap-sulation of the aqueous liquid and the mini-microcapsule(s).
18. The process of claim 17 in which the polymer solvent employed is a halogenated hydrocarbon or an ester formed between an alkanol containing 1-4 carbon atoms and an alkanoic acid containing 1-4 carbon atoms.
19. The process of claim 18 in which the solvent is methylene chloride, chloroform or ethyl acetate.
20. The process of claim 18 in which the organic liquid employed in step (b) is a liquid hydrocarbon.
21. The process of claim 19 in which the organic liquid employed in step (b) is a liquid hydrocarbon.
22. The process of claim 17 in which the product of step (b) is added to an agitated mass of an or-ganic liquid having little or no solvent power for the polymer to precipitate any remaining dissolved polymer and harden the polymer which has encapsulated the aqueous liquid and the mini-microcapsule(s).
23. The process of claim 22 in which the polymer solvent employed is a halogenated hydrocarbon or an ester formed between an alkanol containing 1-4 carbon atoms and an alkanoic acid containing 1-4 carbon atoms and the organic liquid having little or no solvent power for the polymer is a liquid hydrocar-bon.
24. The process of claim 23 in which the solvent is methylene chloride, chloroform or ethyl acetate.
25. A process for preparing a microcapsule having a functional core material encapsulated in a d,l-polylactide (PLA) which comprises;
(a) Dissolving PLA in a mixture of two miscible organic liquids, the first being a liquid having solvent power for PLA and the second having little or no solvent power for PLA, the two liquids being present in a ratio such that the solution is near its saturation point for PLA, the liquid having solvent power for PLA having a vapor pres-sure significantly higher than the vapor pressure of the second liquid, (b) Agitating the solution of step (a) and adding thereto a functional core material so as to uniformly disperse the functional core material as a fine suspension through-out the continuous liquid phase having the PLA dissolved therein, and (c) Vaporizing the liquid having solvent power for PLA from the suspension of step (b) while continuing agitation so as to cause phase separation of the PLA and encap-sulation of the finely dispersed functional core material with PLA, and (d) Transferring the dispersion of step (c) into an agitated mass of an organic liquid having little or no solvent power for PLA to precipitate any remaining dis-solved PLA and harden the PLA which has encapsulated the functional core material.
(a) Dissolving PLA in a mixture of two miscible organic liquids, the first being a liquid having solvent power for PLA and the second having little or no solvent power for PLA, the two liquids being present in a ratio such that the solution is near its saturation point for PLA, the liquid having solvent power for PLA having a vapor pres-sure significantly higher than the vapor pressure of the second liquid, (b) Agitating the solution of step (a) and adding thereto a functional core material so as to uniformly disperse the functional core material as a fine suspension through-out the continuous liquid phase having the PLA dissolved therein, and (c) Vaporizing the liquid having solvent power for PLA from the suspension of step (b) while continuing agitation so as to cause phase separation of the PLA and encap-sulation of the finely dispersed functional core material with PLA, and (d) Transferring the dispersion of step (c) into an agitated mass of an organic liquid having little or no solvent power for PLA to precipitate any remaining dis-solved PLA and harden the PLA which has encapsulated the functional core material.
26. The process of claim 25 in which the liquid having solvent power for PLA is a halogenated hydro-carbon or an ester formed between an alkanol contain-ing 1-4 carbon atoms and an alkanoic acid containing 1-4 carbon atoms and the liquid having little or no solvent power for PLA is a liquid hydrocarbon.
27. The process of claim 26 in which the solvent is methylene chloride, chloroform or ethyl acetate.
28. The process of claim 26 in which each step of the process is carried out at essentially ambient temperature with the energy required to vaporize the solvent liquid in step (c) being provided by the agitation of the suspension.
29. The process of claim 27 in which each step of the process is carried out at essentially ambient temperature with the energy required to vaporize the solvent liquid in step (c) being provided by the agitation of the suspension.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US35486982A | 1982-03-04 | 1982-03-04 | |
| US354,869 | 1982-03-04 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1204058A true CA1204058A (en) | 1986-05-06 |
Family
ID=23395257
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA000422820A Expired CA1204058A (en) | 1982-03-04 | 1983-03-03 | Dual microcapsules |
Country Status (4)
| Country | Link |
|---|---|
| EP (1) | EP0102391A1 (en) |
| JP (1) | JPS58189031A (en) |
| CA (1) | CA1204058A (en) |
| WO (1) | WO1983003061A1 (en) |
Families Citing this family (25)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JPS60193917A (en) * | 1984-03-14 | 1985-10-02 | R P Shiila- Kk | Soft capsule of multiplet structure |
| DE3541304A1 (en) * | 1985-11-22 | 1987-05-27 | Scherer Gmbh R P | ORAL PREPARATIONS OF GARLIC AND METHOD FOR THEIR PRODUCTION |
| US5008112A (en) * | 1985-12-16 | 1991-04-16 | International Minerals & Chem. Corporation | Device for the extended delivery of diffusible agents |
| US4755180A (en) * | 1986-06-16 | 1988-07-05 | Alza Corporation | Dosage form comprising solubility regulating member |
| DE3721574A1 (en) * | 1987-06-30 | 1989-01-12 | Kettelhack Riker Pharma Gmbh | MEDICINAL PRODUCTS IN THE FORM OF PELLETS WITH ENZYMATICALLY CONTROLLED DRUG RELEASE |
| JP2754230B2 (en) * | 1989-03-23 | 1998-05-20 | 株式会社スリーボンド | Self-locking agents and fasteners |
| JP2733087B2 (en) * | 1989-03-29 | 1998-03-30 | 花王株式会社 | Hollow polymer fine particles, method for producing the same and use thereof |
| US5275943A (en) * | 1991-04-12 | 1994-01-04 | Dituro John W | Timed-release tablets for biological degradation of organic matter |
| JPH08507747A (en) * | 1992-12-30 | 1996-08-20 | クローバー コンソリデイテッド,リミテッド | Reusable macroencapsulation system that protects biologically active material packets and is biocompatible |
| JP3278273B2 (en) * | 1993-12-17 | 2002-04-30 | キヤノン株式会社 | Drug sustained release capsule |
| FR2725897B1 (en) * | 1994-10-24 | 1996-12-06 | Oreal | PRODUCT FOR TOPICAL APPLICATION CONTAINING A LIPASE AND AN ACTIVE PRECURSOR |
| FR2725898B1 (en) | 1994-10-24 | 1996-12-13 | Oreal | PRODUCT FOR TOPICAL APPLICATION CONTAINING A LIPASE AND A HYDROXYACID PRECURSOR |
| US6126936A (en) * | 1995-03-10 | 2000-10-03 | Biohybrid Technologies Llc | Microcapsules and composite microreactors for immunoisolation of cells |
| US6287558B1 (en) | 1997-08-01 | 2001-09-11 | Biohybrio Technologies Llc | Devices containing cells or tissue and an agent that inhibits damage by a host cell molecule |
| DE10359792A1 (en) * | 2003-12-19 | 2005-07-21 | Bayer Technology Services Gmbh | Multiphasic drug formulation |
| JP2007000772A (en) * | 2005-06-23 | 2007-01-11 | Casio Electronics Co Ltd | Dual microcapsule, method for preparing the same, and method for surface treatment of microcapsule |
| EP2120891B9 (en) * | 2006-12-28 | 2019-04-24 | Dow Silicones Corporation | Polynuclear microcapsules |
| US10688026B2 (en) | 2009-04-27 | 2020-06-23 | Premier Dental Products Company | Buffered microencapsulated compositions and methods |
| US9814657B2 (en) | 2009-04-27 | 2017-11-14 | Premier Dental Products Company | Buffered microencapsulated compositions and methods |
| AR081743A1 (en) * | 2010-03-26 | 2012-10-17 | Philip Morris Prod | MANUFACTURE OF NUCLEUS CAPSULES / CAPARAZON OF DIFFERENT GEOMETRICS AND TREATMENT FROM THE SAME |
| MX2012011142A (en) | 2010-03-26 | 2012-11-29 | Philip Morris Prod | Smoking article with heat resistant sheet material. |
| JP2013538855A (en) * | 2010-09-30 | 2013-10-17 | エボニック コーポレイション | Emulsion method for producing fine particles of low residual organic solvent |
| WO2014043385A2 (en) | 2012-09-14 | 2014-03-20 | Premier Dental Products Company | Buffered microencapsulated compositions and methods |
| AU2015377223A1 (en) | 2015-01-12 | 2017-08-31 | Nano Pharmaceutical Laboratories Llc | Layered sustained-release microbeads and methods of making the same |
| CN112716911B (en) * | 2021-02-04 | 2023-03-24 | 吉林省吴太感康药业有限公司 | Caffeine microcapsule, preparation method thereof and compound paracetamol and alkyl amine preparation |
Family Cites Families (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US3493652A (en) * | 1962-09-14 | 1970-02-03 | Charles W Hartman | Controlled release medicament |
| US3429827A (en) * | 1962-11-23 | 1969-02-25 | Moore Business Forms Inc | Method of encapsulation |
| US3773919A (en) * | 1969-10-23 | 1973-11-20 | Du Pont | Polylactide-drug mixtures |
| US4016099A (en) * | 1972-03-27 | 1977-04-05 | Xerox Corporation | Method of forming encapsulated toner particles |
| US4111201A (en) * | 1976-11-22 | 1978-09-05 | Alza Corporation | Osmotic system for delivering selected beneficial agents having varying degrees of solubility |
-
1983
- 1983-03-02 WO PCT/US1983/000285 patent/WO1983003061A1/en unknown
- 1983-03-02 EP EP19830902796 patent/EP0102391A1/en not_active Withdrawn
- 1983-03-03 CA CA000422820A patent/CA1204058A/en not_active Expired
- 1983-03-04 JP JP3572583A patent/JPS58189031A/en active Pending
Also Published As
| Publication number | Publication date |
|---|---|
| JPS58189031A (en) | 1983-11-04 |
| WO1983003061A1 (en) | 1983-09-15 |
| EP0102391A1 (en) | 1984-03-14 |
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