IL44023A - Fractionation of coagulation factor depleted blood serum and plasma - Google Patents

Fractionation of coagulation factor depleted blood serum and plasma

Info

Publication number
IL44023A
IL44023A IL44023A IL4402374A IL44023A IL 44023 A IL44023 A IL 44023A IL 44023 A IL44023 A IL 44023A IL 4402374 A IL4402374 A IL 4402374A IL 44023 A IL44023 A IL 44023A
Authority
IL
Israel
Prior art keywords
block copolymer
concentration
plasma
serum
supernatant
Prior art date
Application number
IL44023A
Other versions
IL44023A0 (en
Original Assignee
Baxter Travenol Lab
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Baxter Travenol Lab filed Critical Baxter Travenol Lab
Publication of IL44023A0 publication Critical patent/IL44023A0/en
Publication of IL44023A publication Critical patent/IL44023A/en

Links

Classifications

    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K35/00Medicinal preparations containing materials or reaction products thereof with undetermined constitution
    • A61K35/12Materials from mammals; Compositions comprising non-specified tissues or cells; Compositions comprising non-embryonic stem cells; Genetically modified cells
    • A61K35/14Blood; Artificial blood
    • A61K35/16Blood plasma; Blood serum

Landscapes

  • Health & Medical Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Cell Biology (AREA)
  • Hematology (AREA)
  • Engineering & Computer Science (AREA)
  • Biomedical Technology (AREA)
  • Biotechnology (AREA)
  • Developmental Biology & Embryology (AREA)
  • Immunology (AREA)
  • Virology (AREA)
  • Zoology (AREA)
  • Chemical & Material Sciences (AREA)
  • Medicinal Chemistry (AREA)
  • Pharmacology & Pharmacy (AREA)
  • Epidemiology (AREA)
  • Animal Behavior & Ethology (AREA)
  • General Health & Medical Sciences (AREA)
  • Public Health (AREA)
  • Veterinary Medicine (AREA)
  • Medicines Containing Material From Animals Or Micro-Organisms (AREA)
  • Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
  • Peptides Or Proteins (AREA)
  • Medicines Containing Antibodies Or Antigens For Use As Internal Diagnostic Agents (AREA)

Abstract

1449333 Blood fractionation BAXTER LABORATORIES INC 25 Jan 1974 [30 Jan 1973] 3557/74 Heading A5B Blood protein fractions are prepared by (a) removing substantially all the blood coagulation factors (including fibrinogen, antihemophilic factor and prothrombin complex) from blood plasma or serum, (b) mixing with the treated plasma or serum 2-20 weight % of a block copolymer of ethylene oxide and propylene oxide containing at least 50 weight % of ethylene oxide residues and a poly(propylene oxide residue of molecular weight 950 or more and (c) recovering the blood protein fraction. In one embodiment, the plasma or serum is first treated with block copolymer at 10-20% concentration and pH 7 to 8 and the preciptate therefrom is treated with block copolymer at 3-13% concentration and pH 4 to 5 to provide an immunoglobulin complex. In another embodiment, the plasma or serum is first treated with the block copolymer at 10-20% concentration and pH 7 to 8 and the precipitate therefrom is treated with block copolymer at a concentration of 17-27% and a pH first of 7 to 8 and later of 4 to 5 to provide an albumin fraction. In a third embodiment, the plasma or serum is first treated with block copolymer at a concentration of 2-12% and a pH of 4 to 5 and the supernatant therefrom is treated with block copolymer at 14-24% to provide a precipitate for reconstitution to an organ perfusate. [GB1449333A]

Description

Fractionation of coagulation factor depleted blood serum and plasma BAXTER TRAYENOL LABORATORIES, INC.
C:- 42199 This invention relates to a method of separating proteinaceous and lipid materials from blood serum and plasma. More particularly, the invention relates to fractionation of coagulation factor-depleted blood serum and plasma.
Blood comprises a fluid containing the red and the white blood cells and the blood platelets. The plasma, or fluid part of blood, contains about 90% water and 10% solids. These solids consist essentially of about 7-9% proteins, 1% salts, and the remainder lipids and other substances. Freshly drawn blood clots within a few minutes. Formation of the clot is a complex process in which the protein, fibrinogen, is converted into insoluble fibrin. Blood serum is plasma from which this fibrin has been removed.
Fractionation of blood plasma and serum and the laboratory and clinical use of the separated blood components is common practice today.
Among the various components separated from blood are albumin, -globulins, <λ 2 -globulins,^ -globulins, ^globulins, fibrinogen, prothrombin, antihemophilic globulin, lipoproteins, thromboplastin, complement components, isoagglutinins, cholesterol, phosphatides, and numerous enzymes, e. g. , amylase, fibrinolysin, esterase, and phosphatase. Various methods have been developed heretofore for separating and purifying the foregoing and other blood components. These methods generally comprise one or more of the following procedures : (a) fractional precipitation with ammonium sulfate and similar salts; (b) organic solvent precipitation with cold ethanol or acetone and other such alcohols and ketones; 44023/2 9 (c) selective adsorption on calcium phosphate gels or with barium sulfate; (d) isoelectric precipitation by pH adjustment to the point at which there is no net charge on a given protein; and (e) chromatography by use of adsorbents such as CM- or DEAE - cellulose or by "Sephadex" gel filtration.
Other more recently developed procedures for selectively fractionating and purifying blood proteins involve the use of amino acids such as glycine and beta alanine, water-soluble organic polymers such as polyethylene glycol and polypropylene glycol, and water-insoluble polyelectrolyte polymers containing basic amino groups such as the dimethylaminopropylimide group.
In accordance with the present invention, a new and improved method is provided for fractionating coagulation factor-depleted blood serum and plasma. The method comprises selective precipitation with certain block copolymers which are ethylene oxide -propylene glycol condensation products. Separation of various blood components with these block copolymers has been found to be substantially and significantly better than with the polymeric polyethylene glycol. These improvements consist of increased yield and higher purity of the precipitated protein substances, greater clarity and stability of the resulting liquid serum products, and more rapid separation of the desired components.
German Offenlegungschrift 2,231,676 discloses the broad use of ethylene oxide and propylene oxide block copolymers to fractionate blood serum and plasma products, in particular organ perfusion fluid, blood typing sera, anti-hemophilic factor, prothrombin complex and thromboplastin control. Certain of the reference procedures inherently effect the removal of coagulation factors from blood serum before the serum is further processed, but the reference taken as a whole would suggest that the block copolymers employed herein are not useful in the fractionation of the serum residue remaining after coagulation factors have been removed. Hence the present invention is characterized in that the subject block copolymers are employed to fractionate a particular starting material, i.e., coagulation factor-depleted blood plasma and serum.
The ethylene oxide-propylene glycol condensation products employed in this invention can be prepared by condensing ethylene oxide with polyoxypropylene polymer.
A further description of the preparation of these block copolymers is found in U.S. Patent 2,674,619.
These block copolymers can - 2a - 44023/2 be represented by the following structural formula : ^ HO ( CH CH20) a ( CHCH20) b ( CH2CH20) cH CH 3 For purposes of this invention , these block copolymers desirably contain at least 50 % ethylene oxide in the molecule and a polyoxypropylene hydrophobic base molecular weight of at least 950. In this respect , the block copolymers employed in this invention are related to and include materials used as blood plasma substituted and for priming heart-lung apparatus as described in U. S . Patents 3 , 450 , 502 , 3 , 577 , 522 and 3 , 590 , 125 , which are incorporated herein by reference .
Illustrative examples of suitable block copolymers are the F-38 and F-68 "PLURONIC" polyols sold by Wyandotte Chemicals Corp. F -38 contains 80% of polyoxyethylene hydrophilic units in the molecule and the polyoxypropylene hydrophobic base has a molecular weight of 950. F-68 also contains 80% of polyoxyethylene hydrophilic units in the molecule but the hydrophobic base has a molecular weight of 1750. The total molecular weight of these two "PLURONIC" polyols is 4750 and 8750, respectively. A further descriptio of these polyols is found in the bulletin of Wyandotte Chemicals Corp. "The Pluronic Grid", Sixth Edition, which is incorporated herein by reference.
The coagulation factor -depleted blood serum and plasma employed in this invention is blood serum and plasma from which essentially all the blood coagulation factors have been removed, especially fibrinogen (Factor I), antihemophilic factor (Factor VIII), and the prothrombin complex factors (Factors II, VII, IX, and X). Methods for removing these factors from blood serum and plasma are known and described, for example, in U. S. Patents 3, 415, 804; 3, 560, 475; 3, 631, 018; 3, 652, 530; and 3, 682, 881.
In accordance with the present invention, fractionation of coagulation factor-depleted blood serum or plasma is carried out to provide improved immunoglobulin preparations, albumin-containing fractions, and organ perfusates. The immunoglobulin preparations include immunoglobulin complex (IgM, IgA, o<2-macroglobulin, and plasminogen), immune serum globulin and the intravenous gamma globulin disclosed in co-pending Israel Patent Application No. 43643. The albumin-containing fractions include normal serum albumin, plasma protein fractions (containing 83-90 % albumin and the balance The selective precipitation of the present invention is carried out by the following sequency of steps : The starting coagulation factor-depleted blood serum or plasma is diluted with water or other aqueous media to a protein concentration of from about 0. 5% to about 2. 5%. The diluted material is adjusted to a pH of from about 7 to about 8 and thoroughly mixed with the block copolymer to a concentration of from about 10% to about 20%. The resulting precipitate is further fractionated to provide the above -defined immunoglobulin preparations, and the supernatant is further fractionated to provide the aforementioned albumin-containing fractions. Alternatively, the diluted coagulation factor-depleted blood serum or plasma starting material can be fractionated as hereinbelow described to provide an organ perfusate.
The precipitate collected from, the initial fractionation with the block copolymer at 10% - 20% concentration may contain residual amounts of prothrombin and/or albumin which are first removed. Residual prothrombin is removed by diluting the precipitate with physiologically normal saline (0. 9% NaCl) to a protein concentration of from about 0. 5% to about 2. 5%. The diluted material is adjusted to a pH of from about 6. 7 to about 7. 7 and thoroughly mixed with a suitable adsorbent, such as calcium phosphate, to a concentration of from about 0. 5% to about 1. 5%. The resulting precipitate is separated from the supernatant and discarded.
Residual albumin is then removed by adjusting the supernatant to a pH of from about 6. 5 to about 7. 5 and thoroughly mixing with the block copolymer to a concentration of from about 9% to about 19%. The resulting precipitate is retained for further treatment to obtain the immunoglobulin preparations of the present invention and the supernatant is discarded.
The precipitate collected from the treatment for removal of residual prothrombin and albumin is diluted with normal saline to a protein concentration of from about 0. 5% to about 2. 5%. The diluted material is adjusted to a pH of from about 4 to about 5 and thoroughly mixed ith the block copolymer to a concentration of from about 3% to about 13%. The resulting precipitate is collected and retained as the desired immunoglobulin complex and the supernatant is retained for further treatment to provide immune serum globulin and intravenous gamma globulin products.
The supernatant from the immunoglobulin complex separation is adjusted to a pH from about 4. 5 to about 5. 5 and thoroughly mixed with the block copolymer to a concentration of from about 4% to about 14%. The resulting precipitate is discarded. The supernatant is adjusted to a pH of to a concentration of from about 10% to about 20%. The resulting precipitate is collected and retained as a fraction containing greater than 90% gamma globulin. It can be resuspended in buffered aqueous solution to a protein concentration of 15. 5% - 17. 5% as an immune serum globulin for intramuscular use or at a protein concentration of 5% - 7% for intravenous use.
The albumin-containing supernatant collected from the initial fractionation with the block copolymer at 10% - 20% concentration, maintained at a pH of from about 7 to about 8, is thoroughly mixed with the block copolymer to a concentration of from about 17% to about 27%. The resulting precipitate is discarded. The supernatant is adjusted to a temperature of from about 0° C. to about 10° C. , to a pH of from about 4 to about 5, and thoroughly mixed in acetate buffer (4 molar acetic acid, 0. 8 molar sodium acetate, pH 4. 0). The resulting precipitate is collected and retained for further treatment to provide serum albumin and plasma protein fractions and the supernatant is discarded.
A purified serum albumin solution for therapeutic use can be made by first heat treating the collected precipitate to remove alpha and beta globulins as described, for example, in U. S. Patent 2, 765, 299. The precipitate is dissolved in normal saline to a protein concentration of from about 4% to about 8%. Sodium caprylate is added to a concentration of from about 0. 0075 to about 0. 02 molarity and the pH is adjusted to from about 5 to about 5. 2. This suspension is heated from about one to about four hours at a temperature of from about 65° to about 75° C. with constant stirring.
The denatured proteins are then removed by centrifugation and /or filtration and the protein concentration is adjusted to from about 0. 5% to about 2. 5% by mixing with normal saline.
Following this heat treatment, the block copolymer is added to a concentration of from about 15% to about 35%, the suspension is cooled to a temperature of from about 0° to about 10° C. , the pH is adjusted to from about 4 to about 5 with acetate buffer (as described hereinbefore), and the suspension thoroughly mixed. The resulting precipitate is retained and the supernatant is discarded. A 5% or 25% normal serum albumin solution is prepared by resuspending the precipitate in normal saline to the appropriate protein concentration. The ionic concentration is adjusted to 154 meq. /I. Na+, 124 meq. II. CI , and 0. 04 meq. II. K , or other suitable ionic levels.
Alternatively, a plasma protein fraction can be made by resuspending the collected precipitate in aqueous media to a protein concentration of from about 6% to about 7%. The suspension is heated for two hours at 55° - 65° C. and then clarified by centrifugation and /or filtration. The ionic concentration is adjusted to 100-120 meq. /I. Na , 45-55 meq. /I. CI , and not in excess of 2 meq. /I. K+, and the protein content adjusted to 5-5. 6 gm. %. This material can be used as a primary plasma volume expander.
An organ perfusate is prepared from the hereinbefore diluted coagulation factor-depleted blood serum or plasma starting material as follows.
The diluted material may contain residual amounts of prothrombin.
Residual prothrombin is removed by first adjusting the pH to a level of from about 5. 5 to about 6. 5. Fibrinogen is then thoroughly mixed with the suspension to a concentration of from about 0. 1% to about 1. 5%. The pH is adjusted to a level of from about 6. 7 to about 7. 7 and the suspension is then thoroughly mixed with a suitable adsorbent, such as calcium phosphate, to a concentration of from about 0. 5% to about 1. 5%. The resulting precipitate is separated from the supernatant and discarded.
The retained supernatant is adjusted to a pH of from about 4 to about 5 and the block copolymer thoroughly admixed therewith to a concentration of from about 2% to about 12%. The resulting precipitate, which is rich in lipoproteins, is separated from the supernatant and discarded. Additional proteinaceous material is removed from the remaining supernatant by thoroughly mixing with the block copolymer to a concentration of from about 14% to about 24%, cooling the suspension to a temperature of from about 0° C. to about 10° C. and adjusting the pH to a level of from about 4 to about 5 with acetate buffer (as hereinbefore described). The resulting precipitate is separated from the supernatant which is discarded. The precipitate is then resuspended in aqueous media to a protein concentration of from about 4% to about 8%, to provide the desired organ perfusate.
The following examples will further illustrate the invention although the invention is not limited to these specific examples.
EXAMPLE 1 Coagulation factors are removed from a pool of frozen normal human plasma by the following procedure. In this example the block copolymer is "PLURONIC" F-38. (a) The frozen plasma is quickly thawed and adjusted to pH 6. 88.
Sufficient glycine is added to bring the concentration to 2. 3 molar and the mixture is mechanically stirred for one to four hours at 2° C. and then centrifuged. The precipitate is retained and processed for the production of antihemophilic factor (AHF, Factor VIII) and fibrinogen, and the supernatant is processed for removal of prothrombin complex in part (b). (b> The supernatant from part (a) is diluted to double its volume with normal saline and adjusted to pH 6. Block copolymer is added to a concentration of 35% (weight basis) and the mixture is mechanically stirred for one to two hours at room temperature (20° C. ). The suspension is centrifuged and the supernatant is discarded. The precipitate is then suspended in normal saline to a protein concentration of 5% and the pH is adjusted to 7. 2. Tribasic calcium phosphate [ Ca10(OH)2 (PO^g] is added to a concentration of 0. 5% and the mixture is mechanically stirred for one hour at 20° C. and then centrifuged. The precipitate is retained and processed for the production of prothrombin complex, and the supernatant is processed for the production of immunoglobulin preparations, albumin-containing fractions and organ perfusates. (c) One part of the supernatant from part (b) is diluted with distilled water to a protein concentration of 1% and adjusted to pH 7. 5. Block copolymer is added to a concentration of 15% and the mixture is mechanically stirred for one to two hours and then centrifuged. The precipitate is retained as a high molecular weight protein fraction for separation of macroglobulins and immune serum globulin. The supernatant is retained as a lower molecular weight protein fraction for separation of albumin-containing fractions. (d) The precipitate from part (c) is suspended in normal saline to a protein concentration of 1%. Tribasic calcium phosphate is then added to the suspension to a concentration of 0. 5% and the pH is adjusted to 7. 2. The mixture is mechanically stirred for one hour^ followed by centrifugatxon. The precipitate is discarded and the supernatant is adjusted to pH 7, followed by addition of block copolymer to a concentration of 14%. Mechanical stirring is carried out for one to two hours at 20° C. followed by centrifu- gation. The supernatant, containing traces of albumin, is discarded and the precipitate is suspended in normal saline to a protein concentration of 1%. The suspension is adjusted to pH 4. 5, followed by the addition of block copolymer to a concentration of 8%. The mixture is mechanically stirred for one to two hours at room temperature, followed by centrifugation. The precipitate is retained as a crude immunoglobulin complex which contains e¾-macroglobulin, IgM, IgA, and plasminogen. (e) The supernatant from part (d) is adjusted to pH 5 and the block copolymer is added to a concentration of 9%. The mixture is mechanically stirred for one to two hours at room temperature, followed by filtration.
The precipitate, which contains complement factors, is discarded. The supernatant is adjusted to pH 7 and the block copolymer added to a concentration of 16%. The mixture is mechanically stirred for one to two hours, followed by centrifugation, and the resulting supernatant is discarded. The precipitate is suspended in glycine -saline solution (0. 3 molar glycine / 1% NaCl) to both 6% protein and 16. 5% protein levels, respectively. Samples of gamma globulin prepared by this process were shown to have the characteristics of immune serum globulin made by the Conn ethanol fractionation method, as determined by ultracentrifugation, Tiselius electrophoresis, immunoelectro-phoresis, and antibody content.
However, the product made by this process desirably had a substantially lower anti-complementary titer as compared to said Conn fractionated product. (f) The supernatant from part (c) is maintained at pH 7. 5 and mixed with the block copolymer to a concentration of 22% copolymer. The mixture is mechanically stirred for one to two hours at room temperature, followed by centrifugation. The precipitate, which contains traces of IgG and alpha and beta globulins, is discarded. The supernatant is mixed with normal saline to a concentration of 0. 9% NaCl, chilled to 5° C. , adjusted to pH 4. 5 with acetate buffer (0. 8 molar sodium acetate, 4 molar acetic acid, pH 4) and stirred for one to two hours, followed by centrifugation. The supernatant is discarded and one part of the precipitate is resuspended in normal saline to a protein concentration of 5%. This can be retained as a plasma protein fraction or further processed to obtain pure albumin. (g) Another part of the precipitate in part (f) is suspended in distilled water, adjusted to pH 5. 1, and heat treated at 70° C. with stirring for one to four hours in the presence of 0. 012 molar sodium caprylate. The resulting precipitate is discarded. The supernatant is mixed with normal saline to a concentration of 0. 9% NaCl and then mixed with the block copolymer to a concentration of 19% copolymer. After chilling the material to 5° C. , the pH is adjusted to 4. 5 with acetate buffer, the mixture is mechanically stirred for one to two hours and then centrifuged. The supernatant is discarded and the precipitate is suspended in saline to 5% and 25% protein concentrations, respectively. Samples of albumin solutions made by this process were shown to have the same physio-chemical characteristics of the albumin made by the Conn ethanol fractionation process, as determined by ultracentrifugation, Tiselius electrophoresis, immunoelectro-phoresis and osmolarity. (h) Another part of the supernatant from part (b) is diluted with normal saline to a protein concentration of 1% and adjusted to pH 6. Fibrinogen is then added to a concentration of 0. 5 grams per Kilogram of supernatant. The mixture is mechanically stirred for two hours at room temperature and the mixture then is adjusted to pH 7. 2. Tribasic calcium phosphate is added to a concentration of 0. 5%. After mixing for one to two hours, the mixture is centrifuged and the precipitate discarded. The supernatant is adjusted to pH 4. 5 and the block copolymer is added to a concentration of 7%. The mixture is stirred for one to two hours, followed by centrifugation. ς The resulting precipitate is discarded and the supernatant is mixed with the block copolymer to a concentration of 19%. The suspension is chilled to 5° C. and adjusted to pH 4. 5 with acetate buffer. After mixing two hours, the mixture is centrifuged and the supernatant is discarded. The precipitate is suspended in water to a protein concentration of 6% and the electrolytes are adjusted to that of plasma. This product is useful for organ perfusion at 5° C. without the formation of particulate matter.
EXAMPLE 2 The procedure of Example 1 is repeated except that "PLURONIC" F-68 is substituted for an equivalent amount of the "PLURONIC" F-38 with substantially similar results.
Various other examples and modifications of the foregoing examples will be apparent to those skilled in the art after reading the foregoing disclosure. All such further examples and modifications as come within the spirit and scope of the invention are included in the appended claims. 44023/2

Claims (10)

1. A process for the preparation of an immunoglobulin complex, an albumin-containing fraction and organ perfusates from coagulation factor-depleted blood serum and plasma comprising selective precipitation by admixing with block copolymers of ethylene oxide and polyoxypropylene polymer containing at least about 50% ethylene oxide in the molecule and a polyoxypropylene hydrophobic base molecular weight of at least about 950.
2. The process of Claim 1 in which the block copolymer contains about 80% of polyoxyethylene hydrophilic units in the molecule and the poly-oxypropylene hydrophobic base has a molecular weight of about 950.
3. The process of Claim 1 in which the block copolymer concentration employed is from about 10% to about 20% and the pH is from about 7 to about 8.
4. The process of Claim 3 in which the block copolymer contains about 80% of polyoxyethylene hydrophilic units in the molecule and the poly-oxypropylene hydrophobic base has a molecular weight of about 950.
5. The process of Claim 3 in which the precipitate resulting from the fractionation at 10% to 20% block copolymer concentration is further fractionated with from about 3% to about 13% of said copolymer at a pH of from about 4 to about 5 to provide an immunoglobulin complex.
6. The process of Claim 5 in which the block copolymer contains about 80% of polyoxyethylene hydrophilic units in the molecule and the polyoxypropylene hydrophobic base has a molecular weight of about 950.
7. The process of Claim 3 in which the supernatant resulting from the fractionation at 10% to 20% block copolymer concentration is further fractionated with from about 17% to about 27% of said copolymer at a pH of from about 7 to about 8 and then the resulting supernatant buffered to a pH of from about 4 to about 5 while holding the copolymer at said concentration to provide a concentrated albumin-containing fraction.
8. The process of Claim 7 in which the block copolymer contains about 80% of polyoxyethylene hydrophilic units in the molecule and the polyoxypropylene hydrophobic base has a molecular weight of about 950.
9. The process of Claim 1 in which the block copolymer concentration employed is from about 2% to about 12% and the pH is from about 4 to about 5 and then the concentration of said copolymer in the resulting supernatant is adjusted to from about 14% to about 24% to provide a precipitate for reconstitution to an organ perfusate.
10. The process of Claim 9 in which the block copolymer contains about 80% of polyoxyethylene hydrophilic units in the molecule and the polyoxypropylene hydrophobic base has a molecular weight of about 950.
IL44023A 1973-01-30 1974-01-20 Fractionation of coagulation factor depleted blood serum and plasma IL44023A (en)

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
US32789373A 1973-01-30 1973-01-30

Publications (2)

Publication Number Publication Date
IL44023A0 IL44023A0 (en) 1974-05-16
IL44023A true IL44023A (en) 1977-05-31

Family

ID=23278536

Family Applications (1)

Application Number Title Priority Date Filing Date
IL44023A IL44023A (en) 1973-01-30 1974-01-20 Fractionation of coagulation factor depleted blood serum and plasma

Country Status (10)

Country Link
JP (1) JPS49102820A (en)
AU (1) AU6495474A (en)
BE (1) BE810217A (en)
CA (1) CA984748A (en)
DE (1) DE2403065A1 (en)
ES (1) ES422767A1 (en)
FR (1) FR2215241B1 (en)
GB (1) GB1449333A (en)
IL (1) IL44023A (en)
ZA (1) ZA74350B (en)

Families Citing this family (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3944391A (en) * 1974-12-27 1976-03-16 Preventive Systems, Inc. In vitro process for detecting endotoxin in a biological fluid
IL49752A (en) * 1975-07-09 1979-07-25 Kabi Ab Compositions having affinity for hepatitis virus and method for hepatitis virus removal or concentration
DK25877A (en) * 1977-01-21 1978-08-15 Nordisk Insulinlab PROCEDURE FOR EXTRACTING PURE ALBUMIN FROM BLOOD PLASMA
JPS5843369B2 (en) * 1977-09-10 1983-09-27 森六株式会社 Serum protein fractionation method
US4783441A (en) * 1979-04-30 1988-11-08 Hoechst Aktiengesellschaft Aqueous protein solutions stable to denaturation

Also Published As

Publication number Publication date
JPS49102820A (en) 1974-09-28
ZA74350B (en) 1974-11-27
DE2403065A1 (en) 1974-08-01
AU6495474A (en) 1975-07-31
CA984748A (en) 1976-03-02
ES422767A1 (en) 1976-06-01
FR2215241A1 (en) 1974-08-23
IL44023A0 (en) 1974-05-16
BE810217A (en) 1974-05-16
GB1449333A (en) 1976-09-15
FR2215241B1 (en) 1977-03-11

Similar Documents

Publication Publication Date Title
US3956259A (en) Fractionation of blood using block copolymer of ethylene oxide and polyoxypropylene polymer to recover fraction suitable for organ perfusate
US4073886A (en) Blood fractionation process using block copolymers of ethylene oxide and polyoxypropylene
US3770631A (en) Clarification of blood serum and plasma
Newman et al. Methods for the production of clinically effective intermediate and high‐purity factor‐VIII concentrates
CA2155630C (en) Low temperature albumin fractionation using sodium caprylate as a partitioning agent
US4188318A (en) Simplified method for preparation of high yield, high purity Factor VIII concentrate
US3682881A (en) Fractionation of plasma using glycine and polyethylene glycol
JP5178518B2 (en) Ultra high yield intravenous immunoglobulin preparation
CA1213214A (en) Preparation of highly purified human antihemophilic factor
AU2006287833B2 (en) An ultra-high yield intravenous immune globulin preparation
EP0176926B1 (en) Process for producing a high purity antihemophilic factor concentrate
US4876088A (en) Gamma-globulin injectable solutions containing sorbitol
US4087415A (en) Antithrombin III
AU549584B2 (en) Heat stabilization of plasma proteins
US3839314A (en) Clarification of blood serum and plasma using block copolymers of ethylene oxide and polyoxypropylene
US4025500A (en) Preparation of albumin by fractionation of blood plasma or serum
US4164495A (en) Method of recovering immunoglobulin using a polyol and an alkanoic acid
US8293242B2 (en) Ultra-high yield of alpha-1-anti-trypsin
USRE31268E (en) Method of recovering immunoglobulin using a polyol and an alkanoic acid
IL44023A (en) Fractionation of coagulation factor depleted blood serum and plasma
EP0011739A1 (en) Process for obtaining blood coagulation factor XIII derived from human placenta
US3893990A (en) Clarification of blood serum and plasma using a block copolymer of ethylene oxide and polyoxypropylene
US3893991A (en) Clarification of blood serum and plasma using block copolymers of ethylene oxide and polyoxypropylene
US4406886A (en) Purification of antihemophilia factor VIII by precipitation with zinc ions
IL44881A (en) Preparation of a blood fraction rich in albumin and alpha and beta-globulins