WO2015137531A1 - 면역글로불린의 정제방법 - Google Patents
면역글로불린의 정제방법 Download PDFInfo
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- WO2015137531A1 WO2015137531A1 PCT/KR2014/002021 KR2014002021W WO2015137531A1 WO 2015137531 A1 WO2015137531 A1 WO 2015137531A1 KR 2014002021 W KR2014002021 W KR 2014002021W WO 2015137531 A1 WO2015137531 A1 WO 2015137531A1
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- immunoglobulin
- exchange chromatography
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- anion exchange
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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
- C07K1/18—Ion-exchange chromatography
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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
- C07K1/30—Extraction; Separation; Purification by precipitation
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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
- C07K1/34—Extraction; Separation; Purification by filtration, ultrafiltration or reverse osmosis
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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
- C07K1/36—Extraction; Separation; Purification by a combination of two or more processes of different types
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/06—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies from serum
- C07K16/065—Purification, fragmentation
Definitions
- the present invention relates to a method for purifying immunoglobulins, and more particularly, after dissolving the plasma protein fraction I + II + III or fraction II + III containing the immunoglobulin. , Caprylate was added to precipitate and concentrated by dialysis to concentrate. Then, anion exchange resin and ceramic cation exchange resin purification techniques effectively remove the solvent and detergent added during virus inactivation, and eluate salt.
- the present invention relates to a method for purifying immunoglobulins, which maintains a low polymer content by maintaining a constant concentration.
- Immunoglobulins are plasma proteins that contain antibodies against various viruses and bacteria, and are used to prevent and treat diseases by administering them to people with innate antibody deficiencies or those who require artificial replenishment of antibodies due to viral or bacterial diseases. It is a medicine.
- immunoglobulin is not possible due to the limited dosage of 1) the mass injection, 2) the pain at the injection site during injection, and 3) the intrinsic immunoglobulin G (ImmunoglobulinG; IgG) content with antibody capability. 4, the globulin antibody value by the protease at the injection site is reduced, and 5) the maximum blood concentration reaching time is 24 hours or more.
- Intravenous injection of immunoglobulin has been attempted to solve the problem of intramuscular injection.
- intravenous administration of immunoglobulin preparations results in anaphylactic reactions due to aggregates with anticomplementary activity. Severe and a variety of immediate side effects from shortness of breath to circulatory shock. The above symptoms were mainly seen in patients with immunoglobulin deficiency, and especially side effects of severe hypersensitivity symptoms were observed in patients with antibodies to IgA.
- intravenous injection is not possible due to the above problem, development of intravenous preparations has been required, and methods have been developed that can remove such aggregates and / or prevent aggregate formation during the manufacturing process. Treated with proteolytic enzymes such as pepsin, papain, plasmin, or chemicals such as beta-propiolactone and altered the structure to prevent or destroy the formation of aggregates. Intravenous injections were made possible by lowering anticomplement activity.
- proteolytic enzymes such as pepsin, papain, plasmin, or chemicals such as beta-propiolactone
- IVIG Intravenous Immunoglobulin
- the process does not include a column chromatography step, and the manufactured product is lyophilized to remain stable for a suitable period of time, and used by dissolving immediately before use.
- some manufacturers' IVIG products have been shown to cause infections of viruses such as viral hepatitis C, which further includes one or more known virus inactivation and / or removal steps in the manufacturing process.
- a second generation IVIG with low anticomplement activity and higher stability was initiated in the mid 80s, which was purified through several chromatographic steps.
- Intravenous injections resolved the limitations of intramuscular immunoglobulin dosage, pain relief at the injection site, and reduced proglobin antibodies by protease. It became.
- the semen-injected immunoglobulin changes the structure and there is almost no inherent IgG having an antibody ability, and thus the complement binding capacity is reduced or the blood half-life is short as 4 to 12 days, which is satisfactory for the prevention and treatment of the disease.
- the first and second generation IVIG prepared in lyophilized powder form, requires further dissolution, and because of the slow dissolution rate, liquid IVIG products have been developed and improved to obtain more stable and pure IVIG products. A process was required.
- the method (3rd generation IVIG) introduced in German Patent No. 2,604,759 and US Patent No. 4.124,576 has a unique inherent ability to antibody using a nonionic surfactant such as polyethylene glycol, unlike gamma globulin for intravenous injection.
- a nonionic surfactant such as polyethylene glycol
- the development of a method of obtaining IgG of the present invention has the ability of complement binding and a long half-life of blood concentration, which is effective in preventing and treating diseases.However, these preparations prepared by polyethylene glycol treatment also have anti-complementary aggregates. It is difficult to completely remove the (anti-complement value is about 0.02 units / mg) there is a problem that the occurrence of side effects remain.
- Korean Patent Laid-Open Publication No. 1983-0007083 also prepared an immunoglobulin for intravenous injection through polyethylene glycol from cohn fraction II or fraction II + III isolated from human plasma, but the process was complicated and yield was low. There is this.
- immunoglobulins are purified using sodium caprylate precipitation, anion exchange chromatography, and cation exchange chromatography.
- An object of the present invention is to provide a method for purifying immunoglobulins that can efficiently remove impurities and thrombogenic substances in order to produce stable and high purity immunoglobulins.
- It provides a method for purifying immunoglobulin comprising a.
- Figure 1 is a schematic diagram showing the manufacturing process of the intravenous immunoglobulin according to the present invention.
- Figure 2 is the result of measuring the purity (Thrombin / IgG) of the production stage immunoglobulin.
- Figure 3 is the result of measuring the concentration of FXI (Human Coagulation Factor XI) contained in the filtrate or precipitate for each step by SDS-PAGE.
- FXI Human Coagulation Factor XI
- Plasma protein containing immunoglobulin of the present invention refers to cryoprecipitate-free plasma, various cones, from which various plasma proteins such as Factor IX and antithrombin are removed from human plasma or human placenta derived plasma. cohn) fractions and ammonium sulfate or PEG (Polson et al., Biochem Biophys Acta , 82: 463, 1964); Polson and Ruiz-Bravo, Vox Sang , 23: 107. Fractions obtained through precipitation by 1972).
- the plasma protein fraction may be Cone Fraction II, Cone Fraction I + II + III or Cone Fraction II + III.
- fraction I + II + III or fraction II + III obtained from human plasma was used and prepared according to the conventional corn plasma fractionation method. Subsequent purification processes were performed to remove various lipoproteins, fibrinogen, ⁇ -globulin, ⁇ -globulin and various coagulation factors contained in fraction I + II + III or fraction II + III.
- human plasma is a nucleic acid amplification test (NAT; Nucleic Acid Amplification Test for human immunodeficiency virus (HIV), hepatitis C virus (HCV), hepatitis B virus (HBV) and parvovirus B19 (parvovirus B19) US-derived plasma was used after biotest, including serological tests, and plasma stored at ⁇ 20 ° C. or below was stored in a jacketed vessel at 1 ° C. to 6 ° C. Reaction was dissolved for hours.
- NAT Nucleic Acid Amplification Test for human immunodeficiency virus (HIV), hepatitis C virus (HCV), hepatitis B virus (HBV) and parvovirus B19 (parvovirus B19) US-derived plasma was used after biotest, including serological tests, and plasma stored at ⁇ 20 ° C. or below was stored in a jacketed vessel at 1 ° C. to 6 ° C. Reaction was dissolved for hours.
- the plasma is melted to produce cryoprecipitate containing fibrinogen and coagulation factors, and the cryoprecipitation plasma is removed through centrifugation, and the frozen deficiency in which the cryopreserved plasma is removed. Cryopoor plasma was recovered. Thereafter, the precipitation and filtration were repeated to obtain fraction I + II + III.
- Filtration to separate the plasma containing immunoglobulin was added by adding a filter aid, and then mixed with the supernatant and sediment using a filter press, Celpure 300, Celpure 1000 was used as the filter aid.
- the dissolution of the fraction I + II + III or fraction II + III of step (a) is added so that the fraction I + II + III or fraction II + III: distilled water 1: 6 to 1: 10 Characterized in that, the distilled water may be used for injection distilled water.
- the plasma protein fraction is preferably suspended (dissolved) in water and / or buffer at substantially non-denaturing temperatures and pH.
- substantially unmodified means that the above-mentioned conditions do not cause a substantially irreversible loss of functional activity of immunoglobulin molecules, such as loss of antigen binding activity and / or biological Fc-action.
- the plasma protein fraction is dissolved in water acidified with one or more undenatured buffers at a volume of 6-10, preferably 7-8 times the volume of the plasma protein fraction, and the pH of the immunoglobulin-containing suspension is
- the pH is preferably maintained at pH 6.0 or lower, more preferably at 4.0 to 6.0, and most preferably at 4.1 to 4.3.
- Any acid known in the art may be used as the acid buffer, but preferably sodium phosphate, sodium acetate, sodium chloride, acetic acid, hydrochloric acid, water (distilled water), and the like, and distilled water or distilled water for injection was used in the present invention. .
- step (a) is a step of separating the supernatant and other substances containing the immunoglobulin through the precipitation reaction.
- the precipitant may use one or more materials selected from polyethylene glycol (PEG), caprylic acid and ammonium sulfate having various molecular weights, and an unmodified water-soluble protein precipitant known in the art may be used as a means of precipitation.
- PEG polyethylene glycol
- caprylic acid can be used.
- Precipitation reaction according to the step (a) is added so that the precipitant is 5 to 26mM, preferably 19 to 21mM and then the pH is adjusted to 4 to 6, preferably 4.5 to 5.5.
- the pH adjustment may include acetic acid or sodium hydroxide, but is not limited thereto, and it will be apparent to those skilled in the art that other materials that may be used for pH adjustment may be used.
- the precipitant is carried out for about 1 hour, preferably 50 minutes to 1 hour 10 minutes, until the precipitation reaction is equilibrated between the solid phase and the liquid phase. Throughout the precipitation reaction, the suspension is kept at low temperature, preferably at 2-6 ° C., and the most suitable temperature can be adjusted according to the properties of the protein precipitant.
- the precipitate precipitated by the precipitation reaction contains a large amount of aggregated protein material, and the supernatant contains immunoglobulin, so only the supernatant can be purified to purify the immunoglobulin, and the immunoglobulin-containing supernatant is a large aggregate, a filter.
- a filtration step can be further performed to remove aids, residual non-dissolved pastes, and the like. The filtration is preferably performed using a depth filter and is performed using C150 AF, AF 2000 or AF 1000 (SChenk), 30 LA (Cuno) or similar filters. If desired, removal of aggregates, filter aids, residual non-dissolved protein material may also be performed by centrifugation.
- fraction I + II + III paste protein concentration extracted by adding distilled water or WFI (injection distilled water) so that distilled water is 1: 6 to 10 Was adjusted to 15 mg / ml, the pH was adjusted to 4.2 ⁇ 0.1 with 1M acetic acid, and then the fraction I + II + III paste was extracted.
- WFI injection distilled water
- 1M sodium caprylate solution was added to the extract so that the concentration of caprylate was 20 ⁇ 1.0 mM, and then 1M acetic acid or 0.5M sodium hydroxide (NaOH) was used. The pH was adjusted to 5.1 ⁇ 0.1, and precipitation reaction was performed at 4 ° C. for 1 hour ⁇ 10 minutes. The supernatant was recovered and the immunoglobulin solution was filtered through a depth filter.
- step (b) is a step of concentrating the immunoglobulin and removing impurities, through which the concentration of the immunoglobulin is adjusted to 10 to 50, preferably 20 to 30 mg / ml, Anion exchange chromatography is performed at a pH of 5.0 to 6.0, flow rate of 95 to 145 cm / hr, and fractions not attached to the anion exchange chromatography are obtained at 1.6 to 2.0 Loading Volume (LV). .
- the pH is adjusted to 5.4 to 5.8, most preferably 5.5 to 5.7.
- Concentrated immunoglobulin-containing solutions can be subjected to anion and cation exchange chromatography in one or more steps to remove precipitants and other plasma proteins, including immunoglobulin A (IgA), albumin, aggregates.
- Anion exchange chromatography was performed to remove caprylic acid and other plasma proteins contained in the immunoglobulin containing solution.
- the anion exchange resin in the anion exchange chromatography step may be substituted with diethylaminoethyl (DEAE) or quaternary ammonium groups, but is not limited thereto.
- DEAE diethylaminoethyl
- quaternary ammonium groups but is not limited thereto.
- either one of a group having a strong basic quaternary ammonium group or an anion exchange resin having a weakly basic diethylaminoethyl (DEAE) group can be selected and used.
- strong basic anion exchange resins include Q Sepharose Fast Flow, Q Sepharose High Performance, Resource Q, Source 15Q, Source 30Q, Mono Q, Mini Q, Capto Q, Capto Q ImpRes, Q HyperCel, Q Cermic HyperD F , Nuvia Q, UNOsphere Q, Macro-Prep High Q, Macro-Prep 25 Q, Fractogel EMD TMAE (S), Fractogel EMD TMAE Hicap (M), Fractogel EMD TMAE (M), Eshmono Q, Toyopearl QAE-550C, Toyopearl SuperQ-650C, Toyopearl GigaCap Q-650M, Toyopearl Q-600C AR, Toyopearl SuperQ-650M, Toyopearl SuperQ-650S, TSKgel SuperQ-5PW 30, TSKgel SuperQ-5PW 20, TSKgel SuperQ-5PW etc.
- the present invention is not limited thereto, and an anion
- the appropriate volume of resin used in anion exchange chromatography is reflected by the column dimensions, ie the diameter of the column and the height of the resin, and depends, for example, on the amount of immunoglobulin solution in the solution applied and the binding performance of the resin used.
- the anion exchange resin is preferably equilibrated with a buffer so that the resin can bind to its counter ions.
- Q sepharose FF Q sepharose Fast Flow
- column buffer an equalization buffer known in the art such as sodium phosphate buffer, citric acid buffer, acetic acid buffer, Wash buffers and elution buffers may be used.
- the column for in anion exchange chromatography was equilibrated with 25 ⁇ 0.5 mM sodium acetate (NaOAc) buffer to pH 5.6 ⁇ 0.1 and the flow rate of the mobile phase was adjusted to 120 ⁇ 25 cm / hr.
- the loading amount of the concentrated immunoglobulin solution was loaded to the column to be 90.0 ⁇ 20 mg / mLr.
- the step (c) is to inactivate a virus such as a lipid enveloped virus in a solution containing an immunoglobulin and, after inactivation, to remove a substance used for inactivation.
- virus-inactivating agents preferably solvents and / or detergents, most preferably solvent-cleaner mixtures, can be used.
- step (c) potential lipid enveloped viruses such as HIV1 and HIV2, hepatitis type C and non ABC, HTLV1 and 2, herpes virus group, CMV and Epstein Barr virus can be inactivated, thereby enhancing the safety of the final product.
- HIV1 and HIV2 hepatitis type C and non ABC, HTLV1 and 2, herpes virus group, CMV and Epstein Barr virus
- CMV and Epstein Barr virus can be inactivated, thereby enhancing the safety of the final product. have.
- Solvents and cleaning agents that can be used in step (c) can be used without limitation as long as they have properties that can inactivate viruses, particularly lipid enveloped viruses.
- the detergent may be selected from the group consisting of nonionic and ionic detergents, preferably substantially unmodified.
- a nonionic detergent is preferred, and the solvent is most preferably tri-n-butyl phosphate (TNBP) as disclosed in US Pat. No. 4,764,369, but It is not limited.
- TNBP tri-n-butyl phosphate
- virus-inactivating agents for carrying out the present invention are, but are not limited to, mixtures of one or more selected from TNBP and polysorbate 80 (Tween 80), Triton X-100 and Triton X-45. .
- Preferred solvent / detergent mixtures are added such that the concentration of TNBP in the immunoglobulin containing solution is within 0.2 to 0.6% by weight, preferably 0.24 to 0.36% by weight, and the concentration of Tween 80 is within the range of 0.8 to 1.5% by weight, preferably Add to the concentration of 0.8 to 1.2% by weight.
- the virus-inactivation step is performed under conditions that inactivate the lipid envelope virus, resulting in an immunoglobulin containing solution that is substantially free of virus risk.
- the reaction temperature in the above conditions is preferably 4 to 30 °C, more preferably 19 to 28 °C, most preferably 24 to 26 °C, the reaction time is preferably 1 to 24 hours, more preferably 4 to 12 hours, most preferably about 8 hours, sufficient to ensure virus inactivation.
- the cation exchange chromatography of step (c) is characterized in that the pH is carried out under conditions of 4.5 to 5.5, flow rate 110 to 130cm / hr, preferably the pH is adjusted to 4.9 to 5.1 do.
- the immunoglobulin loaded into the cation exchange resin is 90 to 130 mg per ml cation exchange resin, more preferably 95 to 105 mg per ml resin. Immunoglobulins are adsorbed and then washed with equilibration buffer.
- the equilibration buffer used for washing in the above conditions can be washed using a volume of at least 3 times, preferably at least 5 times the volume of the column, and after washing the immunoglobulin with at least 8 times the elution buffer of the column volume. Elution.
- the cation exchange resin may be Sephadex, Sepharose, HyperCell, or Source, but is not limited thereto, and cation exchange resins known in the art may be used. .
- a ceramic series CM hyper D gel was used as the cation exchange resin, and as the column buffer, an equalization buffer known in the art such as sodium phosphate buffer, citric acid buffer, acetic acid buffer, Washing buffer and elution buffer were used.
- Elution of the immunoglobulin from the cation exchange resin is performed with a substantially non-denaturing buffer with sufficient pH and ionic strength to cause efficient elution of the immunoglobulin to recover the immunoglobulin containing eluate.
- Efficient elution means that at least 75%, at least 80%, and the like, such as at least 85%, of the immunoglobulin solution loaded on the cation exchange resin are eluted from the cation exchange resin.
- the cation exchange chromatography of step (c) may be carried out at a salt concentration of the elution buffer high enough to replace the immunoglobulin in the cation exchange resin, salt concentration of 400 to 600 mM, preferably It can be carried out at a salt concentration of 500mM.
- step (d) finally removes impurities once more.
- the salt concentration of the cation exchange chromatography eluate maintained at 50 to 150 mM in order to maintain the polymer content during dialysis and / or concentration.
- the elution method of maintaining a low salt in the protein elution step can minimize the polymer content of the immunoglobulin to purify the immunoglobulin of improved quality.
- the cation exchange resin eluate maintained a salt concentration of 100 mM or less to maintain the polymer content.
- the dialysis and / or concentration of the step (d) is characterized in that using the ultrafiltration / diafiltration (Ultrafiltration / Diafiltration; UF / DF) system, the osmosis is carried out at 10 mOsmol / kg or less, It is characterized by adjusting the pH to 5.5 to 6.5. That is, the eluate eluted in cation exchange chromatography is dialyzed and concentrated, and diafiltration and ultrafiltration by diafiltration and concentration are performed in one step.
- Membranes used for dialysis / ultrafiltration advantageously have an official weight cutoff in the range of 50,000 Da.
- diafiltration was performed to remove low molecular ions from the cation exchange chromatography eluate, and the osmotic pressure of the UF / DF system was 10 mOsmol / kg or less.
- Dialysis and / or concentrated immunoglobulin was confirmed to have been concentrated to 1.5 ⁇ 0.1 by the test results of a refractometer (T / S meter).
- the anion exchange chromatography of the step (d) is carried out under the conditions of pH 5.5 to 6.5, flow rate 90 to 150cm / hr, loading fractions not attached to the anion exchange chromatography 0.8 to 1.2 loading volume (Loding Volume; LV).
- the pH is adjusted to 5.78 to 6.30, most preferably 6.0 to 6.2, and fractions not attached to the anion exchange chromatography may be recovered to preferably 0.96 to 1.04 loading volume (LV).
- the pH of the fraction that is not attached to the anion exchange chromatography in the step (d) is characterized in that it is adjusted to 4.0 to 5.5, preferably acid, preferably 1M sulfuric acid, so that the pH is 4.3 to 4.7, By addition of hydrochloric acid or acetic acid.
- fractogel EMD TMAE Frractogel EMD TMAE
- NaOAc sodium acetate
- the flow rate of the bed was adjusted to 120 ⁇ 30 cm / hr.
- the loading amount of the dialysis and / or concentrated immunoglobulin solution was loaded to the column to be 110.0 ⁇ 10 mg / mLr, and the fraction not attached to the anion exchange chromatography was recovered to 1.0 ⁇ 0.04 loading volume, and then 1M acetic acid was added to The pH was adjusted to 4.5 ⁇ 0.2.
- the filtration of the step (e) is characterized by using a nanofiltration (nanofiltration) or ultrafiltration / diafiltration system, the nanofiltration is carried out at 2.0 to 3.0 bar pressure conditions, ultrafiltration / dialysis Filtration is carried out at an osmotic pressure of 10 mOsmol / kg or less, and then the pH is adjusted to 4.5 to 5.5.
- nanofiltration nanofiltration
- ultrafiltration / dialysis Filtration is carried out at an osmotic pressure of 10 mOsmol / kg or less, and then the pH is adjusted to 4.5 to 5.5.
- Nanofiltration is an important virus removal step, in which fractions that do not adhere to the secondary anion exchange chromatography are subjected to Pall DVD pre-filters and to no more than 2.5 ⁇ 0.5 bar pressure, preferably no more than 2.5 ⁇ 0.2 bar pressure.
- the virus contained in the immunoglobulin solution was removed by filtration through a DV20 virus filter, after which the ultrafiltration / Diafiltration (UF / DF) system was used to remove low molecular ions (10 mOsmol / kg or less). Diafiltration was carried out with.
- UF / DF ultrafiltration / Diafiltration
- step (e) it may further comprise the step of preparing an intravenous immunoglobulin by adding a stabilizer.
- the additional stabilizer is characterized in that at least one selected from sugar alcohol, maltose, sorbitol, mannose, glucose, trehalose, albumin, lysine, glycine PEG and Tween 80, preferably using glycine do.
- the stabilizer is characterized in that the addition to 200 to 300mM, and after adding the stabilizer, characterized in that to adjust the pH to 4.5 to 5.5.
- it can be done by adding an acid, preferably sulfuric acid or hydrochloric acid so that the pH is between 4.7 and 4.9.
- glycine glycine
- glycine is added to the dialysis and / or concentrated immunoglobulin solution to stabilize the immunoglobulin so that the final concentration is 250 ⁇ 50mM and thoroughly mixed, 0.5N hydrochloric acid so that the pH is 4.8 ⁇ 0.1
- the addition was controlled and sterilized using a 0.2 ⁇ m filter.
- the sterilized intravenous immunoglobulin preparation is characterized in that the protein concentration (purified immunoglobulin) is diluted or concentrated to 1 to 30% by weight of the total volume, in the present invention, the protein concentration is 40 to 60 g / L , Preferably diluted with WFI or concentrated by ultrafiltration to 45 to 55 g / l, more preferably 49.5 to 50.5 g / l, and then glycine is added to a final concentration of 250 ⁇ 50 mM and mixed thoroughly.
- the final formulation of the intravenous immunoglobulin preparation was prepared by adjusting hydrochloric acid to pH 4.8 ⁇ 0.1.
- the present invention relates to an intravenous immunoglobulin prepared by the method of the present invention.
- the immunoglobulin solution having a purity of 99% or higher as a result of measuring the purity (Thrombin / IgG) of the immunoglobulin solution at each stage of preparation and the concentration of Human Coagulation Factor XI (FXI) included in the filtrate or precipitate at each stage of preparation. It was confirmed that the purified (FIG. 2), it was confirmed that most of the thrombocoagulant FXI was also removed (Table 2 and Figure 3).
- Biotest Biotest is made, including the use of FDA approved plasma.
- US-derived plasma (Batch No. 600B0491) was used, and the plasma was stored at ⁇ 20 ° C. or lower until use.
- the bottle containing plasma was opened with a bottle cutting machine, and reacted for 12 to 72 hours in a jacketed vessel at 1 to 6 ° C. to dissolve the plasma.
- the plasma is melted to produce cryoprecipitate containing fibrinogen and coagulation factors, and the cryoprecipitation plasma is removed through centrifugation, and the frozen deficiency in which the cryopreserved plasma is removed. Cryopoor plasma was recovered.
- precipitation II + III steps were performed to further precipitate immunoglobulins (Immunoglpbulin) contained in the deficient plasma.
- the supernatant was named supernatant I + II + III (or II + III) and the precipitate was named fraction I + II + IIIw (or II + IIIw) (w; wash).
- Fraction I + II + IIIw (or II + IIIw) is used immediately or stored below -20 ° C.
- the extracted protein concentration was 15 mg / ml, and the pH was adjusted to 4.2 ⁇ 0.1 using 1M acetic acid, and then fraction I + II + for 11 ⁇ 0.5 hours at a temperature of 2 to 8 ° C. III paste was extracted.
- Anion exchange chromatography was performed to remove caprylic acid and other plasma proteins contained in the concentrated immunoglobulin solution obtained in Examples 1-4.
- the anion exchange resin was filled with Q sepharose FF (GE Healthcare, Catalog No. 17-0510) in the column, followed by an equalization buffer (25 ⁇ 0.5 mM sodium acetate (NaOAc), pH 5.6). Equilibrated to pH 5.6 ⁇ 0.1. Thereafter, the concentrated immunoglobulin solution obtained in Example 1-4 was loaded on the column at a flow rate of 120 ⁇ 25 cm / hr at 25 ° C. or higher, and the loading amount was 90.0 ⁇ 20 mg / mLr. Thereafter, the fractions not attached to anion exchange chromatography were recovered at 1.6 to 2.0 loading volume (LV).
- Q sepharose FF GE Healthcare, Catalog No. 17-0510
- an equalization buffer 25 ⁇ 0.5 mM sodium acetate (NaOAc), pH 5.6
- Equilibrated to pH 5.6 ⁇ 0.1 Thereafter, the concentrated immunoglobulin solution obtained in Example 1-4 was loaded on the column at a flow rate of 120 ⁇ 25 cm / h
- a step of treating the solvent and detergent was performed to inactivate the potential enveloped virus of the solution containing the immunoglobulin.
- the pH was adjusted to 5.0 ⁇ 0.1 by adding acetic acid to the fraction which was not attached to the anion exchange chromatography recovered in Example 1-5, and tri (en-butyl) -phosphate (Tri (n-butyl)- phosphate (TNBP) and Polysorbate 80 (Polysorbate 80; Tween 80) were added at a concentration of 0.3 ⁇ 0.06% and 1 ⁇ 0.2%, respectively, and then stirred at 200 ⁇ 50 RPM for 20-30 minutes. A portion of the TNBP and Tween 80 in the solution was homogeneously mixed and sampled to confirm that thereafter, stirring was continued at 200 ⁇ 50 RPM for 8 hours at 25 ⁇ 1.0 ° C.
- Tri (n-butyl)- phosphate (TNBP) and Polysorbate 80 Polysorbate 80; Tween 80
- CN exchange chromatography was performed to remove other impurities such as TNBP, Tween 80 and coagulation factor in the solvent / detergent immunoglobulin solution.
- the cation exchange resin is filled with a CM Hyper D gel (Pall Corporation; Catalog No. 20050), which is a ceramic material, to a column, and then has an pH of 5.0 using an equalization buffer (25 ⁇ 0.5 mM sodium acetate (NaOAc)). Equilibrate to ⁇ 0.1. Thereafter, the solvent / detergent treated immunoglobulin solution in Example 1-6 was loaded on the column at a flow rate of 120 ⁇ 10 cm / hr at 20 ⁇ 2 ° C., and the loading amount was 100.0 ⁇ 5 mg / mLr.
- CM Hyper D gel Pall Corporation; Catalog No. 20050
- immunoglobulin was eluted using at least 8 times the elution buffer of the column volume (elution buffer composition: 20 mM NaOAc pH 4.5 w / 0.5M NaCl).
- Diafiltration was performed to remove low molecular ions from the cation exchange chromatography eluate.
- Example 1-7 The eluate obtained in Example 1-7 was subjected to diafiltration at 10 mOsmol / kg or less using the ultrafiltration / Diafiltration (Millipore Pellicon 2 (50K)) system, and the UF / DF system maintained the polymer content. To this end, a cation exchange chromatography eluate was added to the calculated dialysis concentrate to maintain the concentration below 100 mM sodium chloride.
- the anion exchange resin was filled with a column of Fractogel EMD TMAEQ (Fractogel EMD TMAE; Merck-Millipore, Cat No. 116887), followed by an equalization buffer (20 ⁇ 0.5 mM sodium acetate (NaOAc), pH 6.1). To equilibrate to pH 6.1 ⁇ 0.1. Thereafter, the concentrated immunoglobulin solution obtained in Example 1-8 was loaded on the column at a flow rate of 120 ⁇ 30 cm / hr at 20 ⁇ 2 ° C., and the loading amount was 110.0 ⁇ 10 mg / mLr. Thereafter, the fractions not attached to the anion exchange chromatography were recovered at 1.0 ⁇ 0.04 loading volume (LV), and the pH was adjusted to 4.5 ⁇ 0.1 by adding hydrochloric acid.
- Fractogel EMD TMAEQ Fractogel EMD TMAE; Merck-Millipore, Cat No. 116887
- Nanofiltration is an important virus removal step, in which the immunoglobulin solution concentrated in dialysis in Examples 1-9 is filtered with a prefilter (Florodyne II prefilter, AB1DJL7PH4) not greater than 2.0 ⁇ 0.5 bar pressure and the virus under 2.0 ⁇ 0.5 bar pressure conditions.
- the virus contained in the immunoglobulin solution was removed by filtration through a filter (DV20, AB3DV207PH4).
- glycine was added to the dialysis and / or concentrated immunoglobulin solution to a final concentration of 250 ⁇ 50 mM and thoroughly mixed. The pH of the stabilized immunoglobulin solution was measured and the pH was 4.8 ⁇ . 0.5N hydrochloric acid was added and adjusted to 0.1. The filtrate was then sterilized using a 0.2 ⁇ m filter and transferred to a stainless steel storage tank.
- Immunoglobulin formulations were sterilized after pH adjustment, transferred to a filling room for filling, and prepared at product, then stored at 2-8 ° C.
- Example 2 Thromboembolic risk measurement in immunoglobulin solution according to preparation step (Generated Thrombin / IgG)
- the purity (Thrombin / IgG) of the immunoglobulin preparations sampled for each preparation step of Example 1 was measured.
- Thromboembolic risk measurement in the immunoglobulin solution according to the preparation step of Example 1 in the present invention is the Thrombin Generation protocol (CBER Thrombin Generation protocol 01 Experiment (100916) of the Center for Biologics Evaluation and Research (CBER), one of six analytical organizations under FDA) It was carried out according to a).
- the immunoglobulin purification process of the present invention is accompanied by a cone plasma fractionation method and an ion chromatography purification method, and as shown in FIG. 2 and Table 1, cation exchange resin chromatography in caprylic acid precipitation process and chromatography purification method. And secondary anion exchange resin chromatography was confirmed that the amount of generated thrombin caused by the thrombus generating material can be effectively removed.
- the concentration of Human Coagulation Factor XI (FXI) included in the filtrate or precipitate of each step of preparation of Example 1 was measured using an ELISA (AsayMax Human Factor XI (FXI) ELISA Kit; ssaypro, Catalog No. EF1011-1) and SDS-PAGE.
- ELISA AssayMax Human Factor XI (FXI) ELISA Kit; ssaypro, Catalog No. EF1011-1) and SDS-PAGE.
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Abstract
Description
단계 (process) | 비고 | 트롬빈(Thrombin) nM |
1. 페이스트 추출 (paste extraction) | 266.4 | |
2. 카프릴산 침전(caprylate precipitation) | 56.9 | |
3. 1차 음이온 교환 크로마토그래피(1st AEX chromatography) | 로딩부분 | 71.9 |
통과액 부분 | 40.0 | |
4. 양이온 교환 크로마토그래피(CEX chromatography) | 로딩 부분 | 37.6 |
용출 부분 | 29.4 | |
5. 2차 음이온 교환 크로마토그래피(2nd AEX chromatography) | 로딩 부분 | 25.5 |
통과액 부분 | 7.4 | |
6. 나노여과 (nanofilitration) | 9.1 | |
7. 농축 (concentration) | 7.7 | |
8. 크루드 용액 (crude solution) | 14.5 |
단계 (process) | 비고 | FXI(EIA) | |
(ng/mL) | |||
1 | 페이스트 추출 (paste extraction) | 732.77 | |
2 | 카프릴산 침전 (caprylate precipitation) | 1.76 | |
3 | 1차 음이온 교환 크로마토그래피(1st AEX chromatography) | 로딩부분 | 4.16 |
4 | 통과액 부분 | 1.02 | |
5 | 양이온 교환 크로마토그래피(CEX chromatography) | 로딩 부분 | 1.93 |
6 | 용출 부분 | 2.16 | |
7 | 2차 음이온 교환 크로마토그래피 (2nd AEX chromatography) | 로딩 부분 | 0.31 |
8 | 통과액 부분 | 2.67 | |
9 | 나노여과 (nanofilitration) | 6.46 | |
10 | 농축 (concentration) | 4.89 | |
11 | 크루드 용액 (crude solution) | N.D |
Claims (20)
- 다음 단계를 포함하는 면역글로불린의 정제방법:(a) 면역글로불린을 함유하는 혈장 단백질 분획 I+II+III(fraction I+II+III) 또는 분획 II+III(fraction II+III)를 용해시킨 다음, 침전제를 첨가하여 침전반응을 수행하는 단계;(b) 상기 침전물을 제거하고 면역글로불린이 포함된 상층액을 여과시킨 다음, 여과액을 농축하고 음이온교환 크로마토그래피를 수행하고, 음이온교환 크로마토그래피 컬럼에 부착되지 않은 분획을 수득하는 단계;(c) 바이러스 불활성화를 위하여 상기 수득된 분획에 용매/세정제를 처리한 후, 상기 용매/세정제를 제거하기 위하여 양이온교환 크로마토그래피를 수행하는 단계;(d) 상기 양이온교환 크로마토그래피 용출액을 투석 및/또는 농축시키고, 음이온교환 크로마토그래피를 수행하여 음이온교환 크로마토그래피 컬럼에 부착되지 않은 분획을 수득하는 단계; 및(e) 상기 수득된 분획을 바이러스 필터에 여과하고 투석 및/또는 농축하여 정제된 면역글로불린을 수득하는 단계.
- 제1항에 있어서, 상기 (a) 단계의 분획 I+II+III 또는 분획 II+III의 용해는 분획 I+II+III 또는 분획 II+III : 증류수가 1 : 6 내지 1 : 10이 되도록 첨가하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (a) 단계의 침전제는 카프릴산(caprylate)인 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (a) 단계 침전반응은 침전제가 5 내지 26mM이 되도록 첨가한 다음, pH가 4.0 내지 6.0이 되도록 조절하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (b) 단계의 음이온교환 크로마토그래피는 pH 5.0 내지 6.0, 유속 95 내지 145cm/hr의 조건에서 수행하며, 음이온교환 크로마토그래피에 부착되지 않은 분획을 1.6 내지 2.0 로딩볼륨(Loding Volume; LV)으로 수득하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (c) 단계의 용매는 트리(엔-부틸)-포스페이트 (TNBP, Tri-n-butyl phosphate)인 것을 특징으로 하며, 세정제는 폴리소르베이트 80, 트리톤 X-100 및 트리톤 X-45 중에서 선택되는 하나 이상인 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (c) 단계의 양이온교환 크로마토그래피는 400 내지 600 mM의 염 농도 조건에서 수행하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (c) 단계의 양이온교환 크로마토그래피는 pH 4.5 내지 5.5, 유속 110 내지 130cm/hr의 조건에서 수행하는 것을 특징으로 하는 면역글로불린의 제조방법.
- 제1항에 있어서, 상기 (c) 단계의 양이온교환 크로마토그래피에 흡착되는 면역글로불린의 흡착량은 양이온교환 수지 ㎖당 90 내지 130㎎/㎖인 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (c) 단계의 양이온교환 크로마토그래피는 세라믹 계열의 양이온교환 수지를 이용하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (d) 단계의 투석 및/또는 농축시 중합체 함량을 유지하기 위하여, 상기 (c) 단계의 양이온교환 크로마토그래피 용출액의 염 농도를 50 내지 150mM로 유지시키는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (d) 단계의 투석 및/또는 농축은 한외여과/투석여과 (Ultrafiltration/Diafiltration; UF/DF) 시스템을 이용하는 것을 특징으로 하며, 삼투압 10mOsmol/kg 이하에서 수행한 다음, pH를 5.5 내지 6.5로 조절하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (d) 단계의 음이온교환 크로마토그래피는 pH 5.5 내지 6.5, 유속 90 내지 150cm/hr의 조건에서 수행하며, 음이온교환 크로마토그래피에 부착되지 않은 분획을 0.8 내지 1.2 로딩볼륨(Loding Volume; LV)으로 수득하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (d) 단계에서 음이온교환 크로마토그래피에 부착되지 않은 분획의 pH는 4.0 내지 5.5가 되도록 조절하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (e) 단계의 여과는 나노여과(nanofiltration) 또는 한외여과/투석여과 시스템을 이용하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제15항에 있어서, 상기 나노여과는 2.0 내지 3.0 bar 압력 조건에서 수행하며, 상기 한외여과/투석여과는 삼투압 10mOsmol/kg 이하에서 수행한 다음, pH를 4.5 내지 5.5로 조절하는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제1항에 있어서, 상기 (e) 단계 이후, 안정화제를 첨가하여 정맥주사용 면역글로불린을 제조하는 단계가 추가로 포함되는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제17항에 있어서, 상기 안정화제는 슈가 알콜, 말토스, 소르비톨, 만노스, 글루코스, 트레할로스, 알부민, 리신, 글리신, PEG 및 Tween 80 중에서 선택되는 하나 이상인 것을 특징으로 하는 면역글로불린의 정제방법.
- 제17항에 있어서, 상기 안정화제는 200 내지 300mM이 되도록 첨가되는 것을 특징으로 하는 면역글로불린의 정제방법.
- 제17항에 있어서, 상기 안정화제를 첨가한 후, pH를 4.5 내지 5.5로 조절하는 것을 특징으로 하는 면역글로불린의 정제방법.
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CA2941232A CA2941232C (en) | 2014-03-11 | 2014-03-11 | Method for purifying immunoglobulin |
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EP14885344.3A EP3118210B1 (en) | 2014-03-11 | 2014-03-11 | Method for purifying immunoglobulin |
CN201480078536.3A CN106414476B (zh) | 2014-03-11 | 2014-03-11 | 用于纯化免疫球蛋白的方法 |
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2014
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AU2016231646B2 (en) * | 2016-09-26 | 2021-04-08 | Instituto Grifols, S.A. | Method for the preparation of immunoglobulins |
CN109627329A (zh) * | 2018-12-27 | 2019-04-16 | 成都蓉生药业有限责任公司 | 一种人免疫球蛋白制备时去除和灭活病毒的方法 |
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Publication number | Publication date |
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CN106414476B (zh) | 2019-12-31 |
CA2941232C (en) | 2020-08-25 |
EP3118210A4 (en) | 2017-11-15 |
KR101917197B1 (ko) | 2018-11-09 |
EP3118210B1 (en) | 2019-11-13 |
EP3118210A1 (en) | 2017-01-18 |
ES2769783T3 (es) | 2020-06-29 |
CN106414476A (zh) | 2017-02-15 |
US10414816B2 (en) | 2019-09-17 |
CA2941232A1 (en) | 2015-09-17 |
KR20160118299A (ko) | 2016-10-11 |
US20170015732A1 (en) | 2017-01-19 |
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