WO2015056681A1 - 多孔質セルロースビーズの製造方法およびそれを用いた吸着体 - Google Patents
多孔質セルロースビーズの製造方法およびそれを用いた吸着体 Download PDFInfo
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- WO2015056681A1 WO2015056681A1 PCT/JP2014/077362 JP2014077362W WO2015056681A1 WO 2015056681 A1 WO2015056681 A1 WO 2015056681A1 JP 2014077362 W JP2014077362 W JP 2014077362W WO 2015056681 A1 WO2015056681 A1 WO 2015056681A1
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- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/22—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof comprising organic material
- B01J20/24—Naturally occurring macromolecular compounds, e.g. humic acids or their derivatives
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- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01J—CHEMICAL OR PHYSICAL PROCESSES, e.g. CATALYSIS OR COLLOID CHEMISTRY; THEIR RELEVANT APPARATUS
- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/281—Sorbents specially adapted for preparative, analytical or investigative chromatography
- B01J20/282—Porous sorbents
- B01J20/285—Porous sorbents based on polymers
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- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/281—Sorbents specially adapted for preparative, analytical or investigative chromatography
- B01J20/286—Phases chemically bonded to a substrate, e.g. to silica or to polymers
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- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/30—Processes for preparing, regenerating, or reactivating
- B01J20/305—Addition of material, later completely removed, e.g. as result of heat treatment, leaching or washing, e.g. for forming pores
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- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/30—Processes for preparing, regenerating, or reactivating
- B01J20/3085—Chemical treatments not covered by groups B01J20/3007 - B01J20/3078
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- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/30—Processes for preparing, regenerating, or reactivating
- B01J20/32—Impregnating or coating ; Solid sorbent compositions obtained from processes involving impregnating or coating
- B01J20/3202—Impregnating or coating ; Solid sorbent compositions obtained from processes involving impregnating or coating characterised by the carrier, support or substrate used for impregnation or coating
- B01J20/3206—Organic carriers, supports or substrates
- B01J20/3208—Polymeric carriers, supports or substrates
- B01J20/3212—Polymeric carriers, supports or substrates consisting of a polymer obtained by reactions otherwise than involving only carbon to carbon unsaturated bonds
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- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
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- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/30—Processes for preparing, regenerating, or reactivating
- B01J20/32—Impregnating or coating ; Solid sorbent compositions obtained from processes involving impregnating or coating
- B01J20/3214—Impregnating or coating ; Solid sorbent compositions obtained from processes involving impregnating or coating characterised by the method for obtaining this coating or impregnating
- B01J20/3217—Resulting in a chemical bond between the coating or impregnating layer and the carrier, support or substrate, e.g. a covalent bond
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- 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
- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/30—Processes for preparing, regenerating, or reactivating
- B01J20/32—Impregnating or coating ; Solid sorbent compositions obtained from processes involving impregnating or coating
- B01J20/3231—Impregnating or coating ; Solid sorbent compositions obtained from processes involving impregnating or coating characterised by the coating or impregnating layer
- B01J20/3242—Layers with a functional group, e.g. an affinity material, a ligand, a reactant or a complexing group
- B01J20/3268—Macromolecular compounds
- B01J20/3272—Polymers obtained by reactions otherwise than involving only carbon to carbon unsaturated bonds
- B01J20/3274—Proteins, nucleic acids, polysaccharides, antibodies or antigens
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- 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
- B01J20/00—Solid sorbent compositions or filter aid compositions; Sorbents for chromatography; Processes for preparing, regenerating or reactivating thereof
- B01J20/30—Processes for preparing, regenerating, or reactivating
- B01J20/32—Impregnating or coating ; Solid sorbent compositions obtained from processes involving impregnating or coating
- B01J20/3291—Characterised by the shape of the carrier, the coating or the obtained coated product
- B01J20/3293—Coatings on a core, the core being particle or fiber shaped, e.g. encapsulated particles, coated fibers
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K17/00—Carrier-bound or immobilised peptides; Preparation thereof
- C07K17/02—Peptides being immobilised on, or in, an organic carrier
- C07K17/10—Peptides being immobilised on, or in, an organic carrier the carrier being a carbohydrate
- C07K17/12—Cellulose or derivatives thereof
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- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08B—POLYSACCHARIDES; DERIVATIVES THEREOF
- C08B15/00—Preparation of other cellulose derivatives or modified cellulose, e.g. complexes
- C08B15/10—Crosslinking of cellulose
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- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08J—WORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
- C08J9/00—Working-up of macromolecular substances to porous or cellular articles or materials; After-treatment thereof
- C08J9/16—Making expandable particles
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- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08J—WORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
- C08J9/00—Working-up of macromolecular substances to porous or cellular articles or materials; After-treatment thereof
- C08J9/28—Working-up of macromolecular substances to porous or cellular articles or materials; After-treatment thereof by elimination of a liquid phase from a macromolecular composition or article, e.g. drying of coagulum
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K1/00—General methods for the preparation of peptides, i.e. processes for the organic chemical preparation of peptides or proteins of any length
- C07K1/14—Extraction; Separation; Purification
- C07K1/145—Extraction; Separation; Purification by extraction or solubilisation
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K1/00—General methods for the preparation of peptides, i.e. processes for the organic chemical preparation of peptides or proteins of any length
- C07K1/14—Extraction; Separation; Purification
- C07K1/16—Extraction; Separation; Purification by chromatography
- C07K1/22—Affinity chromatography or related techniques based upon selective absorption processes
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- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08J—WORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
- C08J2201/00—Foams characterised by the foaming process
- C08J2201/02—Foams characterised by the foaming process characterised by mechanical pre- or post-treatments
- C08J2201/026—Crosslinking before of after foaming
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- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08J—WORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
- C08J2201/00—Foams characterised by the foaming process
- C08J2201/04—Foams characterised by the foaming process characterised by the elimination of a liquid or solid component, e.g. precipitation, leaching out, evaporation
- C08J2201/054—Precipitating the polymer by adding a non-solvent or a different solvent
- C08J2201/0545—Precipitating the polymer by adding a non-solvent or a different solvent from an aqueous solvent-based polymer composition
- C08J2201/0547—Precipitating the polymer by adding a non-solvent or a different solvent from an aqueous solvent-based polymer composition the non-solvent being aqueous
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- C—CHEMISTRY; METALLURGY
- C08—ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
- C08J—WORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
- C08J2301/00—Characterised by the use of cellulose, modified cellulose or cellulose derivatives
Definitions
- the present invention relates to a method for producing porous cellulose beads.
- Porous cellulose beads have the advantages of higher safety and less non-specific adsorption than when other synthetic polymers are used.
- various adsorbents such as various adsorbents for chromatography and affinity adsorbents due to the advantage that they have a high mechanical strength and contain many hydroxyl groups that can be used to introduce ligands that interact with the target substance to be adsorbed. It is used as a base material.
- affinity adsorbents have been utilized as medical adsorbents and antibody drug purifying adsorbents because they can efficiently purify target substances or reduce the concentration of unwanted substances.
- Non-Patent Document 1 Non-patent Document 1
- Patent Document 2 an adsorbent in which protein A is immobilized on a porous carrier as an affinity ligand has attracted attention
- an adsorbent in which protein A is immobilized on a porous carrier using an affinity ligand is attracting attention as an adsorbent for purifying antibody drugs that can specifically adsorb immunoglobulin (IgG).
- IgG immunoglobulin
- Patent Document 1 a method of dissolving and coagulating in a solvent such as an aqueous calcium thiocyanate solution that is highly corrosive and toxic and increases the difficulty of installation is disclosed. It is known that the cellulose solution used in this method exhibits unique behavior, and the porous cellulose beads obtained by this method have considerably large pores and a wide pore size distribution ( For example, Non-Patent Document 3).
- porous cellulose beads obtained by the method are used as an adsorbent such as an antibody, it cannot be expected to show a high adsorption performance because the specific surface area is small.
- a method of giving a substituent to the hydroxyl group of cellulose, dissolving in a general-purpose solvent, granulating, and removing the substituent after granulation to obtain a porous cellulose carrier (For example, Patent Document 2), however, the process is complicated, and the molecular weight is lowered in the process of adding or removing a substituent. There is a tendency that it is difficult to obtain an appropriate strength.
- Patent Documents 3 and 4 a method is disclosed in which cellulose can be dissolved in a low temperature sodium hydroxide aqueous solution (for example, Patent Documents 3 and 4).
- a mixture of cellulose and a hydrogen bond-cleaving solution is heated at 100 to 350 ° C. under pressure and then dissolved in an alkaline aqueous solution. Yes.
- Such a process is industrially disadvantageous.
- Patent Document 5 discloses cellulose that is soluble in an alkaline solution, but the cellulose has a microfibril diameter reduced to 1 ⁇ m or less and further refined to 500 nm or less. Such a refinement process is not suitable for industrial production.
- microbial cellulose is dissolved in an alkaline solution to prepare a cellulose solution, and after adding a dispersion solvent, particles are formed, and then the microbial cellulose particles are frozen and then washed.
- a method for obtaining cellulose beads is disclosed, the process is complicated and not suitable for an industrial production method.
- the present invention goes through a complicated process that is industrially disadvantageous without using highly toxic and corrosive auxiliary raw materials for cellulose beads having a good pore shape and pore size distribution suitable for an adsorbent and without using highly toxic and corrosive auxiliary materials.
- the object is to provide a simple and efficient method for production.
- the present inventors have intensively studied in view of the above problems. As a result, by adding a crosslinking agent to a cellulose fine dispersion prepared by mixing a low-temperature alkaline aqueous solution and cellulose powder, it is possible to produce porous cellulose beads with higher adsorption ability when the ligand is immobilized.
- the present invention has been completed by finding out what can be done.
- [1] a) A step of mixing a low-temperature alkaline aqueous solution and cellulose to prepare a cellulose fine dispersion, b) a step of adding a crosslinking agent to the cellulose fine dispersion to prepare a mixed solution; c) A step of producing an emulsion by dispersing the mixed liquid in a dispersion medium, d) A method for producing porous cellulose beads, comprising the step of bringing the emulsion into contact with a coagulation solvent.
- Adsorption characterized by immobilizing a ligand that interacts with a target substance on the beads obtained by the method for producing porous cellulose beads according to any one of [1] to [6] above body.
- An adsorbent comprising porous cellulose beads produced by the method according to any one of [1] to [6] above, and a ligand that interacts with a target product.
- the present invention has a pore shape and a pore size distribution suitable for an adsorbent simply and efficiently without using a complicated process that is industrially disadvantageous without using highly toxic and corrosive auxiliary materials.
- Cellulose beads having excellent adsorptivity can be produced.
- FIG. 1 is an enlarged SEM image of cellulose beads on Example 1 obtained according to the present invention.
- FIG. 2 is an SEM observation image of the surface of cellulose beads related to Comparative Example 1.
- FIG. 3 is a graph showing the relationship between the viscosity of the crosslinking agent added to the cellulose fine dispersion in Examples 2 to 6 according to the present invention and the median diameter of the obtained cellulose beads.
- FIG. 4 shows the viscosity radius and K av value of the marker used in the measurement of the gel phase partition coefficient (K av ) of the crosslinked porous cellulose beads obtained in Examples 2 to 5 and Comparative Example 2 according to the present invention. It is a graph which shows the relationship.
- FIG. 1 is an enlarged SEM image of cellulose beads on Example 1 obtained according to the present invention.
- FIG. 2 is an SEM observation image of the surface of cellulose beads related to Comparative Example 1.
- FIG. 3 is a graph showing the relationship between the viscosity of the crosslinking agent added to the
- FIG. 5 is a graph showing the relationship between the water content of the crosslinking agent added to the fine cellulose dispersion and the K av value of the obtained cellulose beads.
- FIG. 6 is a pore size distribution of the crosslinked porous cellulose beads obtained in Examples 2 to 5 and Comparative Example 2 according to the present invention.
- FIG. 7 is a graph showing the relationship between the water solubility of the crosslinking agent added to the cellulose fine dispersion and the average pore diameter of the obtained cellulose beads.
- FIG. 8 shows the viscosity radius and K av of the marker used in the measurement of the gel phase partition coefficient (K av ) of the crosslinked porous cellulose beads obtained in Examples 2, 7, and 8 and Comparative Example 2 according to the present invention.
- FIG. 9 is a graph showing the relationship between the amount of the crosslinking agent added to the fine cellulose dispersion and the K av value of the obtained cellulose beads.
- FIG. 10 is a pore size distribution of the crosslinked porous cellulose beads obtained in Examples 2, 7, and 8 and Comparative Example 2 according to the present invention.
- FIG. 11 is a graph showing the relationship between the amount of the crosslinking agent added to the fine cellulose dispersion and the average pore diameter of the obtained cellulose beads.
- FIG. 12 is a graph comparing the adsorption performance between the adsorbent of Example 12 and Reference Example 1 according to the present invention.
- FIG. 13 is a graph showing the relationship between the amount of protein A immobilized on the adsorbent and the amount of IgG adsorbed.
- FIG. 14 is a graph showing the relationship between the median particle size of the adsorbent and the IgG adsorption amount.
- the method for producing porous cellulose beads comprises: a) a step of preparing a cellulose fine dispersion by mixing a low-temperature alkaline aqueous solution and cellulose; b) adding a crosslinking agent to the cellulose fine dispersion and A step of producing, c) a step of producing an emulsion by dispersing the mixed liquid in a dispersion medium, and d) a step of obtaining porous cellulose beads by bringing the emulsion into contact with a coagulation solvent.
- porous cellulose can be obtained by dispersing cellulose in a low-temperature sodium hydroxide aqueous solution and bringing it into contact with a coagulation solvent.
- the present inventors conducted an experiment aiming at improving the mechanical strength of the porous cellulose beads by adding a crosslinking agent to the cellulose dispersion in the production process of the porous cellulose carrier using the low-temperature alkaline aqueous solution. It was. As a result, the reason is not clear, but surprisingly, it has been found that an adsorbent having a larger adsorption amount as well as mechanical strength can be obtained by adding a crosslinking agent to the cellulose dispersion. Perhaps it is because the cross-linking agent is suitably dispersed in the cellulose dispersion to form a microscopic area, and the cross-linking agent migrates to the coagulation solvent or washing solvent to form pores advantageous for adsorption. But this was not expected at all.
- the method of the present invention will be described step by step.
- Step a Preparation Step of Cellulose Fine Dispersion a cellulose fine dispersion is prepared by mixing a low-temperature alkaline aqueous solution and cellulose.
- low temperature refers to a temperature lower than normal temperature. If the temperature is lower than normal temperature, there is no major problem, but if it is -20 ° C or higher, it is preferable because the temperature control equipment is simple and the running cost is low. Moreover, if it is 10 degrees C or less, since coloring of a cellulose dispersion liquid decreases and the dispersibility and swelling property of a cellulose become high, it is preferable.
- the temperature is preferably ⁇ 10 ° C. or higher and 20 ° C. or lower. If it is ⁇ 10 ° C. or higher, freezing of the alkaline aqueous solution can be suppressed.
- a cellulose dispersion liquid can be prepared efficiently and coloring of a cellulose dispersion liquid can be suppressed.
- the temperature is preferably ⁇ 5 ° C. or higher, more preferably ⁇ 2 ° C. or higher, particularly preferably ⁇ 1 ° C. or higher, and is 0 ° C. or higher in view of the handling of water used in the cellulose dispersion and ease of temperature adjustment. Most preferred. Especially, 15 degrees C or less is more preferable, 9 degrees C or less is more preferable, 5 degrees C or less is more preferable, 4 degrees C or less is more preferable, 1 degrees C or less is more preferable. Moreover, if the said temperature is 9 degrees C or less, since the sphericity of the obtained porous cellulose bead becomes high, it is preferable.
- Alkali can be used without particular limitation as long as it shows alkalinity when it becomes an aqueous solution.
- Lithium hydroxide, sodium hydroxide and potassium hydroxide are preferable from the viewpoint of availability, and sodium hydroxide is most preferable from the viewpoint of product safety and price.
- the alkali concentration of the alkaline aqueous solution is not particularly limited, but is preferably 3 to 20% by weight. If the alkali concentration is within this range, the dispersibility / swellability of cellulose in an alkaline aqueous solution is increased, which is preferable.
- the concentration of alkali is more preferably 5 to 15% by weight, further preferably 7 to 10% by weight, and most preferably 8 to 10% by weight.
- the type of cellulose is not particularly limited.
- substituted cellulose such as cellulose into which a substituent for increasing solubility is introduced, and ordinary non-substituted cellulose is used as a raw material. it can.
- cellulose powder in order to efficiently disperse the cellulose in the alkaline aqueous solution, it is preferable to use cellulose powder as the cellulose.
- the molecular weight of the cellulose raw material used is not particularly limited, but the degree of polymerization is preferably 1000 or less. When the degree of polymerization is 1000 or less, the dispersibility / swellability in an aqueous alkali solution is increased, which is preferable. Moreover, since the mechanical strength of the obtained porous cellulose bead will become large if a polymerization degree is 10 or more, it is preferable.
- a more preferable range of the polymerization degree is 50 or more and 500 or less, more preferably 100 or more and 400 or less, particularly preferably 200 or more and 350 or less, and most preferably 250 or more and 350 or less.
- the concentration of cellulose in the cellulose fine dispersion is not particularly limited and may be appropriately adjusted. For example, it may be about 1% by weight or more and 20% by weight or less.
- the concentration is more preferably 2% by weight or more, further preferably 4% by weight or more, more preferably 15% by weight or less, and still more preferably 10% by weight or less.
- the method for preparing the cellulose fine dispersion may be in accordance with a conventional method. For example, what is necessary is just to stir violently, maintaining the mixture of aqueous alkali solution and a cellulose at low temperature.
- Step b Production Step of Mixed Liquid Containing Cellulose and Crosslinking Agent
- a mixed liquid is produced by adding a crosslinking agent to the cellulose fine dispersion.
- the “crosslinking agent” refers to one having two or more reactive groups capable of forming a covalent bond with a hydroxyl group on cellulose and capable of crosslinking between cellulose molecules.
- a conventionally well-known crosslinking agent can be used suitably.
- a cross-linking agent having a functional group capable of binding to a substituent of cellulose for example, a hydroxyl group in the case of unsubstituted cellulose is used. It is preferable to use it.
- the cross-linking reaction when the cross-linking reaction is performed after the formation of the porous beads (granulation), it is also preferable to use the same cross-linking agent used at that time.
- an epoxy group-containing compound is more preferable because it is easy to inactivate the functional group when the crosslinking agent remains, and nonspecific adsorption after the inactivation is small.
- the epoxy group-containing compound that can be used in the present invention is not particularly limited, and halohydrins such as epichlorohydrin, epibromohydrin, dichlorohydrin; bifunctional bisepoxides (bisoxiranes); polyfunctional polyepoxides ( Polyoxirane). Further, at least one of the epoxy group-containing compounds is a glycidyl ether compound, although the reason is not clear, but is preferable because the amount of adsorption becomes larger.
- the glycidyl ether compound is not particularly limited, but 1,4-butanediol diglycidyl ether, cyclohexanedimethanol diglycidyl ether, resorcinol diglycidyl ether, neopentyl glycol diglycidyl ether, 1,6-hexanediol diglycidyl Ether, hydrogenated bisphenol A diglycidyl ether, glycerol diglycidyl ether, trimethylolpropane diglycidyl ether, diglycidyl terephthalate, diglycidyl orthophthalate, ethylene glycol diglycidyl ether, diethylene glycol diglycidyl ether, propylene glycol diglycidyl ether, glycerol Polyglycidyl ether, pentaerythritol polyglycidyl ether, jig Se roll polyglycidyl ether, polyglycerol polyg
- sorbitol polyglycidyl ether (Denacol EX-611, EX-612, EX-614, EX-614B, EX-622, etc. manufactured by Nagase ChemteX Corporation), polyglycerol polyglycidyl ether ( Nagase ChemteX Denacol EX-512, EX-521, etc.), diglycerol polyglycidyl ether (Nagase ChemteX Denacol EX-421, etc.), glycerol polyglycidyl ether (Nagase Chemtex Denacol EX-313, EX) -314 etc.), polypropylene glycol diglycidyl ether (“Denacol EX-920” etc. manufactured by Nagase ChemteX Corporation) can be suitably used.
- the water content of the crosslinking agent used in the present invention is preferably 50% or more.
- the water solubility refers to the ratio of the crosslinking agent actually dissolved in water when an operation of dissolving 10 parts of the crosslinking agent in 90 parts of water at room temperature is performed.
- the water solubility of the crosslinking agent is 50% or more, the compatibility with the cellulose dispersion which is the process of the present invention is improved, and the sphericity of the beads is easily maintained.
- the water content of the crosslinking agent is preferably 60% or more and 100% or less.
- the crosslinking agent having a water solubility of 50% or more is not particularly limited.
- glycerol polyglycidyl ether Nagase Chemtex Denacol EX-313, EX-314, etc.
- diglycerol polyglycidyl ether Nagase Chemtex) Denacol EX-421, etc.
- polyglycerol polyglycidyl ether Nagase ChemteX Denacol EX-512, EX-521, etc.
- sorbitol polyglycidyl ether Nagase Chemtex Denacol EX-614, EX-614B, etc.
- Ethylene glycol diglycidyl ether Nagase ChemteX Denacol EX-810, EX-811, etc.
- diethylene glycol diglycidyl ether Nagase Chemtex Denacol EX-850, EX-851, etc.
- the viscosity of the crosslinking agent used in the present invention is preferably 100 mPa ⁇ s or more and 50000 mPa ⁇ s or less. The reason is not clear, but if the viscosity of the cross-linking agent is within this range, the amount of adsorption may be larger, and details are unknown, but pores advantageous for adsorption are likely to be formed in the beads. thinking. Further, although the reason is not clear, it is preferable to use a cross-linking agent of 100 mPa ⁇ s or more because the obtained beads do not have a too large particle size.
- a more preferable range of the viscosity is 100 mPa ⁇ s or more and 30000 mPa ⁇ s or less, more preferably 150 mPa ⁇ s or more and 25000 mPa ⁇ s or less, and particularly preferably 150 mPa ⁇ s or more and 5500 mPa ⁇ s or less.
- the viscosity can be measured with a Heppler viscometer.
- the cross-linking agent having a viscosity of 100 mPa ⁇ s or more and 50000 mPa ⁇ s or less is not particularly limited.
- resorcinol diglycidyl ether eg Denacol EX-201 manufactured by Nagase ChemteX
- neopentyl glycol diglycidyl ether Nagase
- 1,6-hexanediol diglycidyl ether Nagase ChemteX Denacol EX-212, etc.
- hydrogenate bisphenol A diglycidyl ether Nagase Chemtex Denacol EX-) 252
- glycerol polyglycidyl ether Nagase ChemteX Denacol EX-313, EX-314, etc.
- trimethylolpropane polyglycidyl ether Nagase Chemtex Denacol EX-321, etc.
- Pentaerythritol polyglycidyl ether Denakol EX-411 manufactured by Nagase ChemteX
- the amount of the crosslinking agent used in this step is not particularly limited as long as it is appropriately adjusted. For example, it can be 0.5 to 10 times the cellulose contained in the cellulose dispersion. .
- the amount of the crosslinking agent in the mixed liquid of the cellulose fine dispersion and the crosslinking agent is preferably 1% by mass or more and 20% by mass or less. As the said ratio, 2 mass% or more is more preferable, and 15 mass% or less is more preferable.
- the method for adding the crosslinking agent to the cellulose dispersion is not particularly limited.
- a crosslinking agent may be added to the cellulose dispersion after production, or a crosslinking agent may be added during production of the cellulose dispersion.
- the crosslinking agent is liquid or solid, it may be added as it is, dissolved in a solvent and added as a solution, or added as a dispersion or slurry.
- the solvent or dispersion medium there is no particular limitations on the solvent or dispersion medium in this case, and an organic solvent or water can be used.
- the temperature conditions at the time of addition of a crosslinking agent it is preferable from a viewpoint of preventing coloring that it is 25 degrees C or less.
- it is 0 degreeC or more, since expression of the effect as a crosslinking agent can be anticipated, it is preferable.
- cross-linking agent is not necessarily uniformly dispersed or dissolved in the cellulose dispersion, but when it is desired to uniformly disperse or dissolve, operations such as natural diffusion, stirring, and shaking can be performed.
- Step c Emulsion Preparation Step
- an emulsion is prepared by dispersing the mixed liquid in a dispersion medium.
- Examples of the dispersion medium constituting the emulsion include animal and vegetable oils and fats, hydrogenated animal and vegetable oils and fats, fatty acid glycerides, aliphatic hydrocarbon solvents, and aromatic hydrocarbon solvents.
- a surfactant such as a nonionic surfactant may be used.
- palm oil, shea fat, monkey fat, iripe fat, pork fat, beef tallow, rapeseed oil, rice oil, peanut oil, olive oil, corn oil, soybean oil, perilla oil, cottonseed oil, sunflower oil, evening primrose oil, Sesame oil, safflower oil, coconut oil, cacao butter, palm kernel oil, fish oil, wakame oil, kombu oil and the like can be mentioned.
- hydrogenated animal and vegetable oils and fats mention may be made of hardened palm oil, hardened palm oil, hardened rapeseed oil, hardened rapeseed oil, hardened soybean oil, hardened tallow fat, hardened fish oil and the like.
- the fatty acid glyceride may be any of tri-, di-, and mono-glycerides, and examples thereof include stearic glyceride, palmitic glyceride, and lauric glyceride.
- examples of the aliphatic hydrocarbon solvent include beeswax, candelilla wax, rice bran wax and the like.
- examples of the aromatic hydrocarbon solvent include benzene, toluene, chlorobenzene, dichlorobenzene and the like.
- a surfactant In order to prepare an emulsion, an appropriate amount of a surfactant may be added.
- the surfactant include sorbitan fatty acid esters such as sorbitan laurate, sorbitan stearate, sorbitan oleate, and sorbitan trioleate.
- the amount of the dispersion medium used may be an amount that can sufficiently disperse the liquid mixture droplets. For example, it can be 1 mass times or more with respect to the said liquid mixture. On the other hand, if the amount of the dispersion medium is too large, the amount of waste liquid may increase excessively, and the ratio is preferably 10 times by mass or less. As the said ratio, 2 mass times or more are more preferable, 4 mass times or more are more preferable, 8 mass times or less are more preferable, 7 mass times or less are more preferable.
- the emulsion may be prepared by a conventional method. For example, it can be prepared by vigorously stirring the mixed solution containing the mixed solution, the dispersion medium and the surfactant.
- Step d Coagulation Step Next, the emulsion is brought into contact with a coagulation solvent to extract the solvent from the droplets of the cellulose fine dispersion to obtain porous cellulose beads.
- the coagulation solvent is not particularly limited as long as it has an affinity for the solvent of the fine cellulose dispersion, and examples thereof include alcohol solvents and mixed solvents of water and alcohol solvents.
- the alcohol solvent include C 1-4 alcohols such as methanol, ethanol, n-propanol, isopropanol, n-butanol, isobutanol, s-butanol, and t-butanol.
- the amount of the coagulation solvent to be used is not particularly limited and may be adjusted as appropriate.
- the coagulation method is not particularly limited, but since the emulsion may be unstable, it is preferable to add the coagulation solvent with vigorous stirring so that the droplets do not bind to each other.
- the coagulated porous cellulose beads may be separated by filtration or centrifugation, and washed with water or alcohol.
- the obtained porous cellulose beads may be classified using a sieve or the like in order to make the particle diameter uniform.
- Step e Crosslinking Step of Porous Cellulose Beads
- the crosslinking agent in the preparation step b of the mixed liquid containing cellulose and the crosslinking agent it is preferable to crosslink to form a crosslinked porous cellulose bead.
- crosslinking conditions there are no particular limitations on the crosslinking conditions and the crosslinking agent.
- the method described in WO2008 / 146906 can be used.
- crosslinking agent examples include halohydrins such as epichlorohydrin, epibromohydrin and dichlorohydrin; bifunctional bisepoxides (bisoxiranes); and polyfunctional polyepoxides (polyoxiranes).
- a crosslinking agent may be used individually by 1 type, and may use 2 or more types together.
- the solvent for the reaction for cross-linking the porous cellulose beads with a cross-linking agent may be selected as appropriate.
- water miscibility such as alcohol solvents such as methanol, ethanol and isopropanol, and nitrile solvents such as acetonitrile, etc. Mention may be made of organic solvents. Further, two or more crosslinking reaction solvents may be mixed and used.
- the crosslinking reaction may be performed a plurality of times, and the reaction solvent and the crosslinking agent may be changed each time.
- the first crosslinking reaction may be performed in a water-miscible organic solvent
- the final crosslinking reaction may be performed in water.
- the intermediate solvent composition may be the same as or different from either the first time or the last time, or may be an intermediate composition thereof.
- all rounds may be carried out in an aqueous solvent. The same applies to the crosslinking agent.
- a base may be added to the reaction solution.
- bases include alkali metal hydroxides such as sodium hydroxide and potassium hydroxide; alkali metal hydrogen carbonates such as sodium hydrogen carbonate and potassium hydrogen carbonate; alkali metal carbonates such as sodium carbonate and potassium carbonate; triethylamine and pyridine.
- organic bases such as
- the crosslinked porous cellulose beads are insoluble, and may be washed with a solvent such as water.
- Step f Ligand Immobilization Step
- the porous cellulose beads according to the present invention can be made into an adsorbent by immobilizing a ligand that interacts with a target product. Since the adsorbent that can be obtained in the present invention has the characteristic that there is little nonspecific adsorption, it is possible to provide highly safe drugs and treatments, and also save labor in the intermediate washing step during purification and treatment. Can be realized.
- the “ligand” refers to an affinity ligand that has a specific affinity for an object to be purified by adsorbing to an adsorbent and interacts with the object.
- the target substance is an antibody
- antigens, proteins, peptide fragments and the like that specifically interact with the antibody can be exemplified.
- the ligand that can be used for the adsorbent according to the present invention is not particularly limited as long as it has a specific affinity for an object to be purified using the adsorbent according to the present invention.
- the method for immobilizing the ligand on the porous cellulose beads according to the present invention is not particularly limited, and a conventional method can be used.
- a conventional method can be used.
- cyanogen bromide method, trichlorotriazine method, epoxy Method immobilization of amino group-containing ligands using methods such as tresyl chloride method, periodate oxidation method, divinyl sulfonic acid method, benzoquinone method, carbonyldiimidazole method, acyl azide method; epoxy method, diazo coupling method, etc.
- a method of immobilizing a hydroxyl group-containing ligand using a method a method of immobilizing a thiol group-containing ligand using an epoxy method, a tresyl chloride method, a divinyl sulfonic acid method, etc .; a carboxylic acid-containing ligand or a formyl group on an amination carrier
- immobilization methods such as a method of immobilizing the contained ligand can be mentioned. The entire contents of this document are incorporated herein by reference.
- the adsorbent according to the present invention can be used as an adsorbent for purification, but can also be used as an adsorbent for purifying antibody drugs and a medical adsorbent that have attracted attention in recent years.
- the ligand when used in adsorbents for antibody drug purification, for example, antigens and proteins highly specific for antibodies, protein A, protein G, protein L and their variants, antibodies Examples thereof include amino group-containing ligands such as peptides having binding activity.
- an adsorbent capable of specifically adsorbing immunoglobulin (IgG) an adsorbent obtained by immobilizing protein A, protein G, or a variant thereof as a ligand on a porous carrier has attracted attention.
- the protein A or the like that can be used in the present invention is not particularly limited, and natural products and genetically modified products can be used without limitation.
- antibody binding domains, mutants thereof, those containing oligomers thereof, fusion proteins, and the like may be used.
- the number of polymerizations of the oligomer can be 2 or more and 10 or less.
- the adsorbent of the present invention in which protein A is immobilized can also be used as a therapeutic adsorbent that can be used for the treatment of dilated cardiomyopathy and the like.
- the adsorbent of the present invention in which dextran sulfate or the like is immobilized can be used as an adsorbent for treating hypercholesterolemia.
- the method for introducing the ligand into the porous cellulose beads can be selected from the various immobilization methods described above, but more preferably, the reaction between the formyl group contained in the porous particles and the amino group of the ligand is performed.
- the amount of ligand immobilized on the adsorbent of the present invention is not particularly limited, and can be, for example, 1 mg or more and 1000 mg or less per mL of porous cellulose beads. If the said ratio is 1 mg or more, since the adsorption amount with respect to a target object becomes large, it is preferable, since manufacturing cost can be suppressed if it is 1000 mg or less.
- the amount of ligand immobilized is preferably 2 mg or more, more preferably 4 mg or more, particularly preferably 5 mg or more, more preferably 500 mg or less, further preferably 250 mg or less, particularly preferably 200 mg or less per mL of porous cellulose beads. 100 mg or less is most preferable.
- the use of the adsorbent of the present invention is not particularly limited, but it is suitable for a medical adsorbent, especially a therapeutic adsorbent that adsorbs and removes large-sized pathogenic substances (such as LDL cholesterol) because the surface porosity can be improved. Can be used. Moreover, it can be used as various chromatographic carriers, especially industrial chromatographic carriers packed in large-diameter columns. In particular, when used as an adsorbent for antibody drug purification, which has been in great demand in recent years, the effect can be exhibited. From such a viewpoint, it can be suitably used as an adsorbent obtained by introducing protein A, protein G, or protein L into the porous beads of the present invention.
- the target product can be purified using the adsorbent according to the present invention.
- the adsorbent of the present invention may be brought into contact with a solution containing the target product.
- the contact method is not particularly limited, and the adsorbent according to the present invention may be added to a solution containing the target product.
- the column is packed with the adsorbent of the present invention to prepare a solution containing the target product.
- the target substance may be selectively adsorbed to the adsorbent of the present invention. Since the adsorbent according to the present invention has high strength, particularly when packed in a column, liquid can be passed at a high speed and the target product can be purified efficiently.
- the adsorbent of the present invention on which the target substance is selectively adsorbed is separated from the solution by filtration or centrifugation.
- the target product and other substances can be separated.
- the eluate is used to separate the object from the adsorbent of the present invention.
- an acidic buffer having a pH of about 2.5 or more and 4.5 or less can be used.
- Test Example 1 SEM Observation of Bead Surface
- Test Example 2 Dynamic adsorption amount measurement in RT (Residence time) 3 minutes (1) Solution preparation The following solutions were prepared.
- Liquid A pH 7.4 phosphate buffer (manufactured by Sigma)
- Solution B 35 mM sodium acetate at pH 3.5M (prepared with acetic acid, sodium acetate, RO water manufactured by Nacalai Tesque)
- Liquid C 1M acetic acid (prepared with acetic acid and RO water manufactured by Nacalai Tesque)
- Solution D 1 mg / mL human polyclonal IgG solution (prepared with 1500 mg / 10 mL of “gamma globulin NICHIYAKU” manufactured by NICHIYAKU and solution A)
- Liquid E 6M urea (prepared with urea and RO water manufactured by Kanto Chemical Co., Inc.) Each solution was degassed before use.
- Test Example 3 Measurement of Dynamic Adsorption Amount (1) Solution Preparation The following A to E solutions and neutralization solutions were prepared and degassed before use.
- PBS buffer solution having a pH of 7.4 was prepared using “Phosphor buffered saline” manufactured by Sigma and RO water (reverse osmosis membrane purified water).
- B liquid 35 mM sodium acetate aqueous solution of pH 3.5 was prepared using acetic acid, sodium acetate, and RO water.
- Solution D An aqueous IgG solution with a concentration of 3 mg / mL was prepared using Gamma Guard (polyclonal antibody) manufactured by Baxter and the solution A.
- Gamma Guard polyclonal antibody
- E solution 6M urea aqueous solution was prepared with urea and RO water.
- AKTAexplorer100 manufactured by GE Healthcare
- 3 mL of an adsorbent sample was placed in a column having a diameter of 0.5 cm and a height of 15 cm, and the linear velocity was 230 cm / h.
- a 2M NaCl aqueous solution (using RO water) was passed through for 15 minutes and filled.
- a 15 mL collection tube was set in the fraction collector, and the eluate collection tube was preliminarily filled with a neutralizing solution.
- the dynamic adsorption amount of IgG was determined from the amount of IgG adsorbed on the adsorbent and the adsorbent volume until IgG broke through 5%.
- the dynamic adsorption amount is referred to as 5% DBC.
- Test Example 4 20% Compressive Stress (1) Sample Preparation Pure water was added to the sample beads to prepare a slurry having a concentration of about 50% by volume. A homogenization / defoaming operation consisting of homogenization by stirring the slurry and subsequent defoaming by depressurization for 30 minutes or more was repeated three times to obtain a defoamed slurry. Separately from this operation, the object to be treated was changed to pure water, and the above homogenous / demethod operation was performed for 90 minutes or more to obtain defoamed water.
- the following dextran or glucose was used by dissolving in 50 mM phosphate buffer (pH 7.5) containing 1 M NaCl.
- K av (V R ⁇ V 0 ) / (V t ⁇ V 0 )
- V R represents the liquid passing amount (mL) to peak from the injection of the marker solution is observed
- V 0 is injected peaks from observation dextran solution having a molecular weight of 4 ⁇ 10 7
- V t indicates the volume of beads in the column (mL)]
- Test Example 6 Calculation of pore diameter distribution The viscosity radius of each marker and the value of K av obtained above were substituted into the following formula, and the radius of the pore where each marker entered the porous cellulose beads was determined.
- K av (1 ⁇ r m / r p ) 2 [Wherein, r m represents the viscosity radius (nm) of each marker, and r p represents the radius (nm) of the pore through which each marker enters the porous cellulose beads]
- the calculated pore radius of the porous cellulose beads is plotted on the horizontal axis, and the pore size distribution when the pore volume (V R ⁇ V 0 ) where a marker having a molecular weight of 180 has entered the beads is taken as 100% on the vertical axis. Plotted.
- Test Example 7 Calculation of Pore Diameter Distribution From the graph created in Test Example 6, the pore diameter when the cumulative pore volume was 50% was determined.
- Non-oriented control type Protein A used in the present invention has an amino acid sequence represented by SEQ ID NO: 1. This is a part of the protein A derived from Staphylococcus aureus excluding the signal sequence (S domain) and cell wall binding domain (X domain), and is described as SPA ′ in WO2006 / 004067.
- the said protein A was prepared according to the method as described in the Example of WO2006 / 004067. The entire contents of this WO2006 / 004067 are incorporated herein by reference.
- Orientation Controlled Alkali Resistant Protein A With reference to WO2012 / 133349, a modified C domain 5 conjugate described in WO2012 / 133349 was prepared as orientation controlled alkali resistant protein A.
- Orientation-controlled alkali-resistant protein A has the amino acid sequence represented by SEQ ID NO: 2. The entire contents of WO2012 / 133349 are incorporated herein by reference.
- Example 1 Preparation of alkaline aqueous solution A 28.4 wt% aqueous sodium hydroxide solution was prepared using sodium hydroxide and distilled water manufactured by Wako Pure Chemical Industries, Ltd., and its temperature was adjusted to 4 ° C.
- glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corporation) as a crosslinking agent was added to the prepared cellulose dispersion, and the mixture was stirred at a speed of 500 rpm for 15 minutes.
- the obtained crosslinked beads twice were transferred to a container, distilled water was added to make the total volume 10 times the volume of crosslinked porous cellulose beads, and the mixture was heated at 120 ° C. for 60 minutes using an autoclave. After allowing to cool to room temperature, it was washed with distilled water at least 5 times the volume of the beads to obtain autoclaved twice-crosslinked beads to obtain crosslinked porous cellulose beads. Moreover, the SEM observation image of this bead surface was shown in FIG.
- Adsorbent preparation An adsorbent with protein A immobilized thereon was prepared according to the following procedure. RO water is added to 11.0 mL of the crosslinked porous cellulose beads obtained in (5) above to make the total volume 17.0 mL, and the mixture is placed in a 50 mL centrifuge tube. This is mixed rotor at 25 ° C. After mounting on the mix rotor MR-3 "), the mixture was stirred. Next, 6.0 mL of sodium periodate aqueous solution (sodium periodate dissolved in RO water, concentration: 8.64 mg / mL) was added and stirred at 25 ° C. for 1 hour.
- sodium periodate aqueous solution sodium periodate dissolved in RO water, concentration: 8.64 mg / mL
- the filtrate was washed with RO water on a glass filter (“11GP100” manufactured by Shibata Co., Ltd.) until the electric conductivity of the filtrate was 1 ⁇ S / cm or less to obtain formyl group-containing crosslinked porous cellulose beads.
- the electrical conductivity of the washing filtrate was measured with a conductivity meter (“ECTester 10 Pure +” manufactured by EUTECH INSTRUMENTS).
- the mixture was stirred using a mix rotor (“Mix Rotor MR-3” manufactured by ASONE). Subsequently, 0.39 mL of a 5.5% aqueous solution of dimethylamine borane (DMAB) (adjusted with dimethylamine borane manufactured by Kishida Chemical Co., Ltd. and RO water) was added and stirred at 6 ° C. for 1 hour. Thereafter, the reaction temperature was raised to 25 ° C., and the mixture was reacted at 25 ° C. for 18 hours with stirring using a mix rotor (“Mix Rotor MR-3” manufactured by ASONE).
- DMAB dimethylamine borane
- the amount of unreacted protein A was determined by measuring the UV absorbance at the absorption maximum near 278 nm of the reaction solution, and the amount of protein A immobilized was calculated by subtracting from the amount of charged ligand.
- the beads after the reaction were washed on a glass filter (“11GP100” manufactured by Shibata Co., Ltd.) with 3 times the volume of RO water of the beads.
- the solution was made 30 mL or more, put into a centrifuge tube, and washed with acid while stirring at 25 ° C. for 30 minutes.
- the beads were washed on a glass filter (“11GP100” manufactured by Shibata) with 3 times the volume of RO water of the beads, and then 3 times the volume of 0.05 M sodium hydroxide + 1 M sodium sulfate aqueous solution ( Nacalai Tesque sodium hydroxide, Kanto Chemical sodium sulfate and RO water) were added.
- 0.05 M sodium hydroxide + 1 M sodium sulfate aqueous solution was added to the beads to make the total volume 30 mL or more, put into a centrifuge tube, and washed with alkali while stirring at room temperature for 30 minutes.
- the beads were washed with 20 times volume of RO water on the glass filter (“11GP100” manufactured by Shibata). Next, 3 times the amount of beads, 0.5N trisodium citrate aqueous solution (prepared by Kanto Chemical Co., Ltd. trisodium citrate dihydrate + RO water) was added, and the filtrate was confirmed to be neutral. Then, the adsorbent which fixed the target protein A was obtained by wash
- the physical properties of the obtained adsorbent were evaluated according to Test Example 2. As a result, the amount of protein A introduced was 35 g / L (adsorbent volume), and 5% DBC at RT 3 minutes was 65 g / L (adsorbent filled volume). there were.
- Comparative Example 1 An adsorbent was prepared in the same manner as in Example 1 except that glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corporation) was not added as a cross-linking agent when preparing the cellulose dispersion.
- glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corporation) was not added as a cross-linking agent when preparing the cellulose dispersion.
- the amount of protein A introduced 35 g / L (adsorbent volume), and 5% DBC at RT 3 minutes was 49 g / L (adsorbent filled volume).
- FIG. 1 and FIG. 2 are compared, it can be seen that the surface pores of the porous cellulose beads of the present invention prepared by adding a crosslinking agent to a cellulose fine dispersion are clearly larger.
- Example 2 (1) Production of porous cellulose beads Porous cellulose beads were produced in the same manner as in Example 1. The median particle size of the obtained porous cellulose beads was 64 ⁇ m.
- the crosslinked cellulose beads obtained by the crosslinking reaction were transferred to a reaction vessel so that the total amount of cellulose beads and distilled water was 116.7 g. After 37.8 g of sodium sulfate was added and dissolved therein, 33 mL of epichlorohydrin was added and kept at 40 ° C. 21 mL of 17.0N NaOH aqueous solution was added to start the crosslinking reaction, and 5 mL of 17.0N NaOH aqueous solution was added 2.5 hours after the start of the reaction. After 5 hours from the start of the reaction, the gel was collected and washed with distilled water of 20 times volume or more of the beads. Table 3 shows the K av value of the crosslinked porous cellulose beads, FIG. 4 and FIG.
- FIG. 8 show the relationship between the viscosity radius of the marker and the K av value
- FIG. 5 shows the relationship between the water solubility of the crosslinking agent and the K av value
- Fig. 6 shows the pore size distribution and average pore size
- Fig. 6 and Fig. 10 show the pore size distribution
- Fig. 7 shows the relationship between the water content of the crosslinking agent and the average pore size
- Fig. 7 shows the crosslinking agent for cellulose fine dispersion.
- Table 5 and FIG. 9 show the addition amount and the Kav value of Table 1
- Table 6 and FIG. 11 show the addition amount and average pore diameter of the crosslinking agent to the cellulose fine dispersion.
- Example 3 Glycerol polyglycidyl ether (“Denacol EX-313” manufactured by Nagase ChemteX) was added as a cross-linking agent instead of glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corp.) when the cellulose dispersion was prepared. Except for the above, porous cellulose beads were obtained in the same manner as in Example 2. The median particle size of the obtained porous cellulose beads was 98 ⁇ m. Subsequently, classification and crosslinking were performed in the same manner as in Example 2 except that 38 ⁇ m and 150 ⁇ m sieves were used, to obtain crosslinked porous cellulose beads.
- Example 4 Polyglycerol polyglycidyl ether (“Denacol EX-521” manufactured by Nagase ChemteX) was added as a crosslinking agent in preparation of the cellulose dispersion instead of glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX). Except for this, porous cellulose beads were obtained in the same manner as in Example 2. The median particle size of the obtained porous cellulose beads was 65 ⁇ m. Subsequently, classification and crosslinking were performed in the same manner as in Example 3 to obtain crosslinked porous cellulose beads.
- Example 5 In addition to glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX) as a crosslinking agent, sorbitol polyglycidyl ether (“Denacol EX-614” manufactured by Nagase ChemteX) was added as a cross-linking agent when preparing the cellulose dispersion. Except for the above, porous cellulose beads were obtained in the same manner as in Example 2. The median particle size of the obtained porous cellulose beads was 63 ⁇ m. Subsequently, classification and crosslinking were performed in the same manner as in Example 3 to obtain crosslinked porous cellulose beads.
- glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX) as a crosslinking agent
- sorbitol polyglycidyl ether (“Denacol EX-614” manufactured by Nagase ChemteX)
- Example 6 Polypropylene glycol diglycidyl ether ("Denacol EX-920" manufactured by Nagase ChemteX) was added as a cross-linking agent instead of glycerol polyglycidyl ether ("Denacol EX-314" manufactured by Nagase ChemteX) as a cross-linking agent during the preparation of the cellulose dispersion. Except for this, porous cellulose beads were obtained in the same manner as in Example 2. The median particle size of the obtained porous cellulose beads was 244 ⁇ m.
- Example 7 Porous cellulose beads as in Example 2 except that the amount of glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corp.) added as a cross-linking agent during preparation of the cellulose dispersion was 6 g and the amount of water was increased by 6 g. Got. Subsequently, classification and crosslinking were performed in the same manner as in Example 3 to obtain crosslinked porous cellulose beads.
- Table 5 and FIG. 9 show the addition amount and Kav value of the crosslinking agent to the fine cellulose dispersion
- FIG. 10 shows the pore size distribution
- Table 6 shows the addition amount and average pore size of the crosslinking agent to the cellulose fine dispersion. As shown in FIG.
- Example 8 Porous cellulose beads in the same manner as in Example 2 except that the amount of glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corp.) added as a cross-linking agent was 18 g and the amount of water was reduced by 6 g when the cellulose dispersion was prepared. Got. Subsequently, classification and crosslinking were performed in the same manner as in Example 3 to obtain crosslinked porous cellulose beads.
- Table 5 and FIG. 9 show the addition amount and Kav value of the crosslinking agent to the fine cellulose dispersion
- FIG. 10 shows the pore size distribution
- Table 6 shows the addition amount and average pore size of the crosslinking agent to the cellulose fine dispersion. As shown in FIG.
- Example 2 Porous cellulose beads were obtained in the same manner as in Example 2 except that glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corporation) was not added as a crosslinking agent during the preparation of the cellulose dispersion, and the amount of water was increased by 12 g. . Subsequently, classification and crosslinking were performed in the same manner as in Example 3 to obtain crosslinked porous cellulose beads. Table 3 shows the K av value of the crosslinked porous cellulose beads, FIG. 4 and FIG. 8 show the relationship between the viscosity radius of the marker and the K av value, and FIG.
- glycerol polyglycidyl ether (“Denacol EX-314” manufactured by Nagase ChemteX Corporation) was not added as a crosslinking agent during the preparation of the cellulose dispersion, and the amount of water was increased by 12 g. .
- classification and crosslinking were performed in
- FIG. 5 shows the relationship between the water solubility of the crosslinking agent and the K av value.
- Fig. 6 shows the pore size distribution and average pore size
- Fig. 6 and Fig. 10 show the pore size distribution
- Fig. 7 shows the relationship between the water content of the crosslinking agent and the average pore size
- Fig. 7 shows the crosslinking agent for cellulose fine dispersion.
- Table 5 and FIG. 9 show the addition amount and the Kav value of Table 1
- Table 6 and FIG. 11 show the addition amount and average pore diameter of the crosslinking agent to the cellulose fine dispersion.
- the Kav value that is, the pore volume in the cellulose beads
- the Kav value can be increased by adding a crosslinking agent to the fine cellulose dispersion and granulating.
- the Kav value that is, the pore volume in the cellulose beads was increased.
- the average pore diameter was the largest when the amount of the crosslinking agent in the mixed liquid of the cellulose fine dispersion and the crosslinking agent was 10%.
- Example 9 After obtaining crosslinked porous beads in the same manner as in Example 2, the crosslinked porous cellulose beads were subjected to wet classification using 38 ⁇ m and 90 ⁇ m sieves to obtain crosslinked porous cellulose beads having a median particle size of 65 ⁇ m. .
- the resulting crosslinked beads (3.5 mL) were placed in a centrifuge tube, and RO water was added to make a total volume of 6 mL. This was attached on a mix rotor (mix rotor MR-3, manufactured by AS ONE) at 25 ° C. and then stirred. Next, sodium periodate was dissolved in RO water, and 2.0 mL of 11.16 mg / mL sodium periodate aqueous solution was added, followed by stirring at 25 ° C. for 1 hour. After the reaction, the filtrate was washed with RO water until the electric conductivity of the filtrate was 1 ⁇ S / cm or less on a glass filter (manufactured by Shibata Co., Ltd. 11GP100) to obtain formyl group-containing crosslinked beads. The electrical conductivity of the washing filtrate was measured with a conductivity meter (“ECTester 10 Pure +” manufactured by EUTECH INSTRUMENTS).
- the obtained formyl group-containing crosslinked porous cellulose beads (3.5 mL) were placed in a centrifuge tube, and the liquid volume was adjusted with RO water so that the total volume was 7.5 mL.
- the mixture was stirred at 6 ° C. for 2 hours.
- 1.61 mL of 1.5 M trisodium citrate aqueous solution was added, and the pH was adjusted to 12 with 0.08 N sodium hydroxide aqueous solution.
- the mixture was reacted at 6 ° C. for 23 hours with stirring using a mix rotor (“Mix Rotor MR-3” manufactured by ASONE).
- reaction liquid 1 The liquid part contained in the beads was replaced with a buffer adjusted to pH 5 with 0.1 M trisodium citrate aqueous solution (using RO water) and 0.1 M citric acid aqueous solution, and then the total volume was 7 mL with the same buffer.
- the beads were returned to the centrifuge tube while adjusting so as to be, and stirred at 6 ° C. for 4 hours using a mix rotor (“Mix Rotor MR-3” manufactured by ASONE). Subsequently, after adding 1.93 mL of 5.5% by mass dimethylamine borane aqueous solution (using RO water) and stirring at 6 ° C.
- reaction liquid 2 a reaction liquid (hereinafter referred to as “reaction liquid 2”) was recovered.
- the UV absorbance of the reaction solution 1 and the reaction solution 2 at the absorption maximum near 278 nm was measured, and subtracted from the charged ligand amount, thereby calculating the protein A immobilized amount of the obtained beads.
- the beads were washed with 3 times volume RO water of beads on a glass filter (“11GP100” manufactured by Shibata). Next, 3 times volume of 0.1N citric acid aqueous solution (using RO water) is added, 0.1N citric acid aqueous solution (using RO water) is added to the beads to make the total volume 30 mL or more, put into a centrifuge tube, 25 Acid washing was performed while stirring at 30 ° C. for 30 minutes.
- the beads were washed on a glass filter ("11GP100" manufactured by Shibata) with 3 times the volume of RO water of the beads, and then 3 times the volume of 0.05 M sodium hydroxide and 1 M concentration of sodium hydroxide.
- An aqueous solution containing sodium sulfate (using RO water) was added.
- an aqueous solution containing 0.05 M sodium hydroxide and 1 M sodium sulfate is added to the beads to make the total volume 30 mL or more, put in a centrifuge tube, and washed with alkali while stirring at room temperature for 30 minutes. It was.
- the beads were washed with 20 times volume of RO water on the glass filter (“11GP100” manufactured by Shibata).
- the electric conductivity of the washing filtrate is increased using RO water. Washing was performed until the concentration became 1 ⁇ S / cm or less to obtain an adsorbent on which the target orientation controlled alkali-resistant protein A was immobilized.
- the conductivity of the washing filtrate was measured with a conductivity meter (“ECTester 10 Pure +” manufactured by EUTECH INSTRUMENTS).
- adsorption performance with respect to IgG was measured according to Test Example 3, and 20% compression stress was measured according to Test Example 4.
- Table 7 shows the adsorption performance and 20% compression stress
- FIG. 13 shows the relationship between the protein A immobilization amount and the IgG adsorption amount
- FIG. 14 shows the relationship between the median particle size and the IgG adsorption amount.
- Example 10 An adsorbent was obtained in the same manner as in Example 9 except that the amount of the aqueous solution containing the orientation controlled alkali-resistant protein A was changed to 1.10 g.
- adsorption performance with respect to IgG was measured according to Test Example 3, and 20% compression stress was measured according to Test Example 4.
- Table 7 shows the adsorption performance and 20% compression stress
- FIG. 13 shows the relationship between the protein A immobilization amount and the IgG adsorption amount
- FIG. 14 shows the relationship between the median particle size and the IgG adsorption amount.
- Example 11 An adsorbent was obtained in the same manner as in Example 9 except that the amount of the aqueous solution containing the orientation controlled alkali-resistant protein A was changed to 0.82 g.
- adsorption performance with respect to IgG was measured according to Test Example 3, and 20% compression stress was measured according to Test Example 4.
- Table 7 shows the adsorption performance and 20% compression stress
- FIG. 13 shows the relationship between the protein A immobilization amount and the IgG adsorption amount
- FIG. 14 shows the relationship between the median particle size and the IgG adsorption amount.
- Example 12 An adsorbent was obtained in the same manner as in Example 10 except that the crosslinked porous cellulose beads having a median particle size of 52 ⁇ m obtained by wet classification of the crosslinked porous cellulose beads using 38 ⁇ m and 63 ⁇ m sieves were used. It was.
- adsorption performance with respect to IgG was measured according to Test Example 3, and 20% compression stress was measured according to Test Example 4.
- the adsorption performance and 20% compression stress are shown in Table 7, and the comparison results of the adsorption performance with Reference Example 1 are shown in FIG.
- Example 13 An adsorbent was obtained in the same manner as in Example 10 except that the crosslinked porous cellulose beads having a median particle size of 71 ⁇ m obtained by wet classification of the crosslinked porous cellulose beads using 63 ⁇ m and 75 ⁇ m sieves were used. It was.
- adsorption performance with respect to IgG was measured according to Test Example 3, and 20% compression stress was measured according to Test Example 4.
- Table 7 shows the adsorption performance and 20% compressive stress.
- Reference example 1 The adsorption performance of “MabSelect SuRe LX” manufactured by GE Healthcare, which is known as an adsorbent for purifying high-performance antibody drugs with immobilized protein A having alkali resistance, was measured according to Test Example 3, and 20% compression was performed. The stress was measured according to Test Example 4. Table 7 shows the adsorption performance, and FIG. 12 shows the comparison results of the adsorption performance with Example 12.
- the adsorbent according to the present invention exhibits very high adsorption performance as compared with the conventional adsorbent product. Further, as shown in the results shown in FIG. 13, it was found that the adsorbent according to the present invention hardly deteriorates the adsorption performance even if the amount of ligand immobilized is small. Further, as shown in FIG. 14, it was found that the adsorbent according to the present invention hardly deteriorates the adsorption performance even when the median particle size is increased.
- the porous cellulose beads obtained by the present invention have good mass transfer, and it has been proved that if a ligand is immobilized, a very high performance adsorbent capable of adsorbing a target substance with high efficiency can be obtained. .
Abstract
Description
b)前記セルロース微分散液に架橋剤を加え混合液を作製する工程、
c)前記混合液を分散媒に分散させてエマルションを作製する工程、
d)前記エマルションを凝固溶媒に接触させる工程を含むことを特徴とする、多孔質セルロースビーズの製造方法。
本工程では、低温のアルカリ水溶液とセルロースとを混合してセルロース微分散液を作製する。
本工程では、前記セルロース微分散液に架橋剤を加え混合液を作製する。
本工程では、前記混合液を分散媒に分散させてエマルションを作製する。
次に、前記エマルションを凝固溶媒に接触させることによりセルロース微分散液の液滴から溶媒を抽出し、多孔質セルロースビーズを得る。
以上で得られた多孔質セルロースビーズは、強度を高めるために、前記セルロースと架橋剤を含む混合液の作製工程bにおける架橋剤の添加以外に、架橋剤により架橋して架橋多孔質セルロースビーズとすることが好ましい。
本発明に係る多孔質セルロースビーズは、目的物と相互作用するリガンドを固定化することにより、吸着体とすることができる。本発明で得ることができる吸着体は非特異吸着が少ないといった特性を有していることから、安全性が高い薬や治療の提供が可能で、さらには精製や治療時に中間洗浄工程等を省力化することが可能となる。
各製造例、実施例で得られたビーズを5倍体積量の30%エタノールで洗浄し、ビーズに含まれる液体部分を30%エタノールで置換した。次いで、50%エタノール、70%エタノール、90%エタノール、特級エタノール、特級エタノール、特級エタノールを順に用いてビーズを同様に処理し、液体部分をエタノールで置換した。さらにt-ブチルアルコール/エタノールが3/7の混合液を用いてビーズを同様に処理した。次いで、t-ブチルアルコール/エタノール=5/5、7/7、9/1、10/0、10/0、10/0の混合液を順に用いてビーズを処理し、液体部分をt-ブチルアルコールで置換した後、凍結乾燥した。凍結乾燥を行なったビーズに金/パラジウムを蒸着源とした蒸着処理を行い、SEM観察像を撮影した。
(1) 溶液作成
以下の溶液を調製した。
B液:pH3.5Mの35mM酢酸ナトリウム(ナカライテスク社製の酢酸、酢酸ナトリウム、RO水で調製)
C液:1M酢酸(ナカライテスク社製の酢酸とRO水で調製)
D液:1mg/mLのヒトポリクローナルIgG溶液(ニチヤク社製「ガンマグロブリンニチヤク」1500mg/10mLとA液で調製)
E液:6M尿素(関東化学社製の尿素とRO水で調製)
各溶液は、使用前に脱気した。
カラムクロマトグラフィー用装置として、AKTAexplorer 100(GEヘルスケア社製)を用い、直径0.5cm、高さ15cmのカラムに22μmのメッシュを取り付け、本発明の吸着体をそれぞれ3mL入れ、線速450cm/hで20%エタノール水溶液(和光純薬工業社製エタノールとRO水で調整)を1時間通液して充填した。フラクションコレクターに15mLの採取用チューブをセットした。この溶出液の採取用チューブについては、あらかじめ中和液を入れておいた。
A液を線速300cm/hで9mL通液し、次いでD液を、UVをモニターしながら、IgGが10%破過するまで線速300cm/hで通液した。ここで、5%破過した時のIgG負荷量をRT3分での5%DBCとした。次いで、A液を線速300cm/hで30mL通液し、B液を線速300cm/hで30mL通液してIgGを溶出させた。次にC液を線速300cm/hで9mL,E液を線速300cm/hで9mL通液し、再生処理を行った。
(1) 溶液調製
下記A~E液及び中和液を調製し、使用前に脱泡した。
カラムクロマトグラフィー用装置として、AKTAexplorer100(GEヘルスケア社製)を用い、直径0.5cm、高さ15cmのカラムに、吸着体試料を3mL入れ、線速230cm/hで0.2MのNaCl水溶液(RO水使用)を15分通液して充填した。フラクションコレクターに15mLの採取用チューブをセットし、溶出液の採取用チューブについては、あらかじめ中和液を入れておいた。
前記カラムにA液を15mL通液し、次いでD液を必要量通液した。次いで、A液を21mL通液後、B液を12mL通液してIgGを溶出させた。次にC液を6mL、E液を6mL、A液を15mL通液した。なお各液の流速は0.5mL/分または1mL/分とし、吸着体との接触時間が6分または3分となるようにした。
IgGが5%破過するまでに吸着体に吸着したIgG量と吸着体体積からIgGの動的吸着量を求めた。当該動的吸着量を5%DBCという。
(1) 試料調製
試料ビーズに純水を加え、濃度約50体積%のスラリーを調製した。このスラリーの攪拌による均質化と、それに続く30分以上の減圧による脱泡とからなる均質・脱泡操作を3回繰り返して実施し、脱泡スラリーを得た。この操作とは別に、処理対象を純水に変えて、前記均質・脱法操作を90分以上実施し、脱泡水を得た。
2.5mLのHANKE SASS WOLF社製ルアロック付ディスポーザブルシリンジ(商標名:NORM-JECT)の先端にディスポーザブルフィルター(孔径5.00μm、親水性)を取り付けた。シリンジのピストンを外し、シリンジ後端側から脱泡水を約2mL投入し、この脱泡水が0mLの標線を下回らないうちに、脱泡スラリーを投入した。ディスポーザブルフィルターの2次側にアスピレーターを接続し、液面がビーズ面を下まわらない様に注意しながら、前記脱泡スラリーを吸引した。ビーズ面の約0.5mL上まで液面が下がったところで吸引を停止した。以降の作業は、液面がビーズ面を下回らないよう、前記脱泡水を適宜追加しながら実施した。振動を与えながら前記脱泡スラリーを追加またはビーズを除去し、ビーズ面を1.5mLの標線に合わせ、振動を与えてもビーズ面が低下しないことを確認した。ビーズが舞わないようゆっくり脱泡水を溢れるまで追加し、気泡が入らないように注意しながらピストンを挿入した。以下、このシリンジを「ビーズ充填シリンジ」という。
レオテック社のFUDOH RHEO METERに10Kのロードセルを取り付け、変位速度のダイヤルを2cm/MINに合わせ、前記ビーズ充填シリンジをセットし、ピストンの変位を開始した。変位と応力との関係を記録し、下記式に基づき、20%圧縮応力を求めた。
試験例5 Kav:ゲル相分配係数の測定
多孔質セルロースビーズ22.8mLを蒸留水に分散させ、30分間脱気した。脱気した多孔質セルロースビーズをカラム(GEヘルスケア・ジャパン社製「Tricorn 10/300」)に充填した。島津製作所社製のサイズ排除クロマトグラフィーシステム(「DGU-20A3」、「RID-10A」、「LC-20AD」、「SIL-20AC」、「CTO-20AC」を含み、ソフトウェアとしては「LCSolution」を使用)を用いて測定を行った。
[式中、VRは各マーカー溶液を注入してからピークが観測されるまでの通液量(mL)を示し、V0は分子量4×107のデキストラン溶液を注入してからピークが観測されるまでの通液量(mL)を示し、Vtはカラム内のビーズの体積(mL)を示す]
試験例6 細孔径分布の計算
各マーカーの粘度半径と上記で求めたKavの値を下記式に代入し、各マーカーが多孔質セルロースビーズに侵入する細孔の半径を求めた。
[式中、rmは各マーカーの粘度半径(nm)を示し、rpは各マーカーが多孔質セルロースビーズに侵入する細孔の半径(nm)を示す]
算出された多孔質セルロースビーズの細孔半径を横軸に、分子量180のマーカーがビーズ内に侵入した細孔体積(VR-V0)を100%とした場合の細孔径分布を縦軸にプロットした。
試験例6で作成したグラフから累積細孔体積が50%の時の細孔径を求めた。
本発明で使用した無配向制御型プロテインAは、配列番号1で示されるアミノ酸配列を有する。これは、Staphylococcus aureus由来プロテインAからシグナルシーケンス(Sドメイン)及び細胞壁結合ドメイン(Xドメイン)を除いた部分にあたり、WO2006/004067においてSPA’として記載されているものである。当該プロテインAを、WO2006/004067の実施例に記載の方法に準じて調製した。なおこのWO2006/004067の全内容が、本願に参考のため援用される。
WO2012/133349を参照して、配向制御型アルカリ耐性プロテインAとして、WO2012/133349に記載の改変Cドメイン5連結体を調製した。配向制御型アルカリ耐性プロテインAは、配列番号2で示されるアミノ酸配列を有する。なお、このWO2012/133349の全内容が、本願に参考のため援用される。
(1) アルカリ水溶液の作製
和光純薬社製の水酸化ナトリウムと蒸留水を用いて、28.4wt%の水酸化ナトリウム水溶液を作製し、その温度を4℃に調整した。
セパラブルフラスコに79gの蒸留水と5.9gのセルロースを投入し、二段ディスクタービン(rushton turbine)翼を用いてスラリーの温度が4℃になるまで、150~200rpmで30分間攪拌した。次いで、4℃に冷却した28wt%の水酸化ナトリウム水溶液を36g添加し、500rpmの速度で攪拌しながら30分間保持した。その後、作製したセルロース分散液に架橋剤として12gのグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)を添加し、500rpmの速度で15分間撹拌を行った。
上記セルロース分散液に、1wt%のソルビタンモノオレエートが溶解した833gのo-ジクロロベンゼン溶液を投入し、4℃で600rpm、15分間撹拌することでセルロース液滴を分散させた。凝固溶剤としてメタノールを74mL添加し、4℃で600rpm、30分間攪拌した。その後、ガラスフィルター(TOP社製「26G-3」)で溶液を濾過し、次いでビーズの5倍体積量のメタノール、5倍体積量の蒸留水の順に洗浄を行ない、多孔質セルロースビーズを回収した。
得られた多孔質セルロースビーズを、38μmと90μmの篩を用いて湿式分級した。
分級後の多孔質セルロースビーズ20mLに蒸留水を加えて30mLとし、反応容器に移した。ここに架橋剤としてグリセロールポリグリシジルエーテルを含有するグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)を2.3g投入し、40℃に調整しながら攪拌を続けた。40℃に調整後、30分間攪拌した。次いで、2N NaOH水溶液(ナカライテスク社製水酸化ナトリウムと蒸留水で調製)7.1mLを用意し、1時間に1/4ずつ加えた。この間、温度を40℃に維持し、攪拌も継続した。最後の1/4量を添加後、同温度で1時間攪拌した。反応終了後、吸引濾過をしながら、ビーズの20倍体積量以上の蒸留水で洗浄し、架橋1回ビーズを得た。さらに得られた架橋1回ビーズに同じ架橋反応をもう1回実施し、架橋2回ビーズを得た。
下記手順に従って、プロテインAを固定化した吸着体を作製した。上記(5)で得られた架橋多孔質セルロースビーズ11.0mLに、RO水を加えて全量を17.0mLとし、50mLの遠沈管に入れ、これを25℃にてミックスローター(アズワン社製「ミックスローターMR-3」)上に取り付けた後、攪拌した。次に過ヨウ素酸ナトリウム水溶液(過ヨウ素酸ナトリウムをRO水に溶解したもの、濃度:8.64mg/mL)6.0mLを加え、25℃で1時間攪拌した。反応後、グラスフィルター(シバタ社製「11GP100」)上で、濾液の電気伝導度が1μS/cm以下となるまでRO水で洗浄し、ホルミル基含有架橋多孔質セルロースビーズを得た。洗浄濾液の電気伝導度は、導電率計(EUTECH INSTRUMENTS社製「ECTester10 Pure+」)で測定した。得られたホルミル基含有架橋多孔質セルロースビーズ9.0mLをグラスフィルター(シバタ社製「11GP100」)上に移し、0.5Mクエン酸三ナトリウム二水和物(関東化学社製)+0.15M塩化ナトリウム(関東化学社製)バッファー30mLを通液してビーズ内の液体を前記クエン酸三ナトリウム水溶液に置換した。前記バッファーを用い、置換後のホルミル基含有架橋多孔質セルロースビーズを、遠沈管に入れた。ホルミル基含有多孔質セルロースビーズを沈降させた後、総体積量14mLとなるように上清を除去して調整した。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)を添加しないこと以外は、実施例1と同様に吸着体を作製した。得られた吸着体の物性評価を行った結果、プロテインA導入量:35g/L(吸着体体積)で、RT3分での5%DBCが49g/L(吸着体充填体積)であった。
(1) 多孔質セルロースビーズの作製
実施例1と同様に多孔質セルロースビーズの作製を行った。得られた多孔質セルロースビーズのメジアン粒径は64μmであった。
実施例1と同様に分級を行った。分級後の多孔質セルロースビーズに含まれる液体部分を100mLをエタノールで置換した後、反応容器に移し、セルロースビーズとエタノールの合計量が97gとなるようにした。そこに蒸留水28gとエピクロロヒドリン80mLを添加した。溶液温度を40℃に調整し、1.8N NaOH水溶液(ナカライテスク社製水酸化ナトリウムと蒸留水で調製)を96mL添加し、架橋反応を開始させた。反応開始から1.5時間後に17.0N NaOH水溶液を9.6mL添加し、反応開始から3時間後と4.5時間後にも17.0N NaOH水溶液を9.6mL添加した。反応開始から6時間後にゲルを回収し、ビーズの20倍体積量以上の蒸留水で洗浄した。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)の代わりに、グリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-313」)を添加したこと以外は、実施例2と同様に多孔質セルロースビーズを得た。得られた多孔質セルロースビーズのメジアン粒径は98μmであった。次いで、38μmと150μmの篩を用いたこと以外は、実施例2と同様に分級と架橋を行い、架橋多孔質セルロースビーズを得た。架橋後の多孔質セルロースビーズのKav値を表3に、マーカーの粘度半径とKav値との関係を図4に、架橋剤の水溶率とKav値との関係を図5に、細孔径分布と平均細孔径を表4に、細孔径分布を図6に、架橋剤の水溶率と平均細孔径との関係を図7に示す。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)の代わりに、ポリグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-521」)を添加したこと以外は、実施例2と同様に多孔質セルロースビーズを得た。得られた多孔質セルロースビーズのメジアン粒径は65μmであった。次いで、実施例3と同様に分級と架橋を行い、架橋多孔質セルロースビーズを得た。架橋後の多孔質セルロースビーズのKav値を表3に、マーカーの粘度半径とKav値との関係を図4に、架橋剤の水溶率とKav値との関係を図5に、細孔径分布と平均細孔径を表4に、細孔径分布を図6に、架橋剤の水溶率と平均細孔径との関係を図7に示す。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)の代わりに、ソルビトールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-614」)を添加したこと以外は、実施例2と同様に多孔質セルロースビーズを得た。得られた多孔質セルロースビーズのメジアン粒径は63μmであった。次いで、実施例3と同様に分級と架橋を行い、架橋多孔質セルロースビーズを得た。架橋後の多孔質セルロースビーズのKav値を表3に、マーカーの粘度半径とKav値との関係を図4に、架橋剤の水溶率とKav値との関係を図5に、細孔径分布と平均細孔径を表4に、細孔径分布を図6に、架橋剤の水溶率と平均細孔径との関係を図7に示す。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)の代わりに、ポリプロピレングリコールジグリシジルエーテル(ナガセケムテックス社製「デナコールEX-920」)を添加したこと以外は、実施例2と同様に多孔質セルロースビーズを得た。得られた多孔質セルロースビーズのメジアン粒径は244μmであった。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)の添加量を6gとし、水を6g増量した以外は、実施例2と同様に多孔質セルロースビーズを得た。次いで、実施例3と同様に分級と架橋を行い、架橋多孔質セルロースビーズを得た。セルロース微分散液への架橋剤の添加量とKav値を表5と図9に、細孔径分布を図10に、セルロース微分散液への架橋剤の添加量と平均細孔径を表6と図11に示す。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)の添加量を18gとし、水を6g減量した以外は、実施例2と同様に多孔質セルロースビーズを得た。次いで、実施例3と同様に分級と架橋を行い、架橋多孔質セルロースビーズを得た。セルロース微分散液への架橋剤の添加量とKav値を表5と図9に、細孔径分布を図10に、セルロース微分散液への架橋剤の添加量と平均細孔径を表6と図11に示す。
セルロース分散液作製時に架橋剤としてグリセロールポリグリシジルエーテル(ナガセケムテックス社製「デナコールEX-314」)を加えず、水を12g増量した以外は、実施例2と同様に多孔質セルロースビーズを得た。次いで、実施例3と同様に分級と架橋を行い、架橋多孔質セルロースビーズを得た。架橋後の多孔質セルロースビーズのKav値を表3に、マーカーの粘度半径とKav値との関係を図4と図8に、架橋剤の水溶率とKav値との関係を図5に、細孔径分布と平均細孔径を表4に、細孔径分布を図6と図10に、架橋剤の水溶率と平均細孔径との関係を図7に、セルロース微分散液への架橋剤の添加量とKav値を表5と図9に、セルロース微分散液への架橋剤の添加量と平均細孔径を表6と図11に示す。
実施例2と同様に架橋多孔質ビーズを得た後、架橋後の多孔質セルロースビーズを38μmと90μmの篩を用いて湿式分級を行ない、メジアン粒径が65μmの架橋多孔質セルロースビーズを得た。
配向制御型アルカリ耐性プロテインAの入った水溶液の添加量を1.10gに変更した以外は実施例9と同様に吸着体を得た。
配向制御型アルカリ耐性プロテインAの入った水溶液の添加量を0.82gに変更した以外は実施例9と同様に吸着体を得た。
架橋後の多孔質セルロースビーズを38μmと63μmの篩を用いて湿式分級を行なって得られたメジアン粒径52μmの架橋多孔質セルロースビーズを用いた以外は、実施例10と同様に吸着体を得た。
架橋後の多孔質セルロースビーズを63μmと75μmの篩を用いて湿式分級を行なって得られたメジアン粒径71μmの架橋多孔質セルロースビーズを用いた以外は、実施例10と同様に吸着体を得た。
アルカリ耐性のあるプロテインAを固定化した高性能な抗体医薬品精製用吸着体として知られているGEヘルスケア社製「MabSelect SuRe LX」の吸着性能を試験例3に従って測定し、また、20%圧縮応力を試験例4に従って測定した。吸着性能を表7に、実施例12との吸着性能の比較結果を図12に示す。
Claims (10)
- a)低温のアルカリ水溶液とセルロースとを混合してセルロース微分散液を作製する工程、
b)前記セルロース微分散液に架橋剤を加え混合液を作製する工程、
c)前記混合液を分散媒に分散させてエマルションを作製する工程、
d)前記エマルションを凝固溶媒に接触させる工程を含むことを特徴とする、多孔質セルロースビーズの製造方法。 - 前記a)の工程における前記アルカリ水溶液の液温が0~25℃であることを特徴とする請求項1に記載の製造方法。
- 前記架橋剤がエポキシ基含有化合物であることを特徴とする請求項1または2に記載の多孔質セルロースビーズの製造方法。
- 前記エポキシ基含有化合物がグリシジルエーテル系化合物であることを特徴とする請求項3に記載の多孔質セルロースビーズの製造方法。
- 前記架橋剤の水溶率が50%以上であることを特徴とする請求項1~4のいずれか一項に記載の多孔質セルロースビーズの製造方法。
- 前記架橋剤の粘度が100mPa・s以上50000mPa・s以下であることを特徴とする、請求項1~5のいずれか一項に記載の多孔質セルロースビーズの製造方法。
- 請求項1~6のいずれか一項に記載の多孔質セルロースビーズの製造方法で得られたビーズに、目的物と相互作用するリガンドを固定化したことを特徴とする吸着体。
- 請求項1~6のいずれか一項に記載の方法で製造された多孔質セルロースビーズ、および、目的物と相互作用するリガンドを含むことを特徴とする吸着体。
- 請求項1~6のいずれか一項に記載の方法で製造された多孔質セルロースビーズに、目的物と相互作用するリガンドを固定化することにより吸着体を得る工程を含むことを特徴とする吸着体の製造方法。
- 請求項7または8に記載の吸着体を用いることを特徴とする精製方法。
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