Patent Publication Number: US-3880989-A

Title: Production of antisera comprising fractionating plasma or serum with an ethylene oxide-polyoxypropylene block copolymer

Description:
United States Patent Garcia [4 1 Apr. 29, 1975 PRODUCTION OF ANTISERA COMPRISING FRACTIONATING PLASMA OR SERUM WITH AN ETHYLENE OXlDE-POLYOXYPROPYLENE BLOCK COPOLYMER Luis A. Garcia, Huntington Beach. Calif.  
 Baxter Laboratories, lnc., Morton Grove, 111.  
 Filed: Jan. 30, 1973 Appl. No.: 327,894  
 Inventor:  
 Assignee:  
 U.S. C1 424/11; 210/53; 260/112 B;  
  424/12; 424/85; 424/101 Int. Cl. A6lk 23/02; C08h 7/00 Field of Search 260/1 12 B, 11; 424/85,  
 Primary E.\&#39;aminerl-1oward E. Schain Attorney, Agent, or Firm-Scott J. Meyer; Louis Altman [57] ABSTRACT A process for the preparation of a stable and concentrated antiserum comprising sequentially fractionating blood plasma or serum with block copolymers of ethylene oxide and polyoxypropylene polymer at selected concentrations and pHs.  
 2 Claims, No Drawings PRODUCTION OF ANTISERA COMPRISING FRACTIONATING PLASMA OR SERUM WITH AN ETHYLENE OXIDE-POLYOXYPROPYLENE BLOCK COPOLYMER This invention relates to a method for the production of antisera. More particularly, the invention relates to the preparation of stable and concentrated antisera by fractional precipitation of blood serum or plasma.  
  Mammalian antisera to the most diversified antigens are widely used as immunochemical tools in industry, clinical laboratories and hospitals throughout the world.  
  Blood grouping and typing sera are among these widely used antisera. They are generally produced by rabbit or other animal immunization, trial bleedings, assay of raw materials and subsequent preparation of a suitable pool of product through blending to any desired specification.  
  Concentration of the antibody fraction of such sera is then commonly carried out such as by (NH SO, and/or Rivanol (6,9-diamino-Z-ethoxyacridine lactate monohydrate) precipitation.  
  In accordance with the invention, an improved method for the preparation of a stable and concentrated antiserum is provided. Normal human or animal plasma or serum, or plasma or serum from immunized humans or animals is fractionated into two major fractions. One fraction consists of high molecular weight proteins including the antibodies, and the other fraction comprises albumin and the lower molecular weight globulins. By further treatment, the high molecular weight fraction is delipidated and reprecipitated to render a highly concentrated antibody paste. The lower molecular weight fraction is further treated to yield a stable protein solution consisting of primarily albumin and aand B-globulins of lower molecular weight, which can be used as a diluent for antibodies and other biological material, for priming heart-lung apparatus and as an organ perfusate.  
  Each of the foregoing two major fractions can be used as such, but preferably a blended material is made in which the antibody paste is reconstituted with the above-prepared lower molecular weight protein solution to about one-fourth to one-fifth the original volume of the starting material. The antisera thus prepared has a lto 4-fold greater antibody potency than in the starting material. It is free of particulate matter and remains clear upon storage at temperatures ranging from 5 to 40 C. The method of the present invention is thereby especially useful for the production of high titer group typing sera.  
  In the method of the invention, the starting material is subjected to selective precipitation at appropriate pH levels with certain block copolymers which are ethylene oxide-propylene glycol condensation products.  
  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. Pat. No. 2,674,619. The block copolymers can be represented by the following structural formula: I  
 no (ca ca m (cuca m (CH CH O) H For purposes of this invention, these block copolymers desirably contain at least 50 percent ethylene oxide in the molecule and a polyoxypropylene hydrophobic base molecular weight of at least 950. Materials containing less than 50 percent ethylene oxide are not sufficiently non-toxic and products having a hydrophobic base molecular weight less than 950 do not have the desired solubility characteristics. ln this respect, the block copolymers employed in this invention are related to and include materials used as blood plasma substitutes and for priming heart-lung apparatus as described in U.S. Pat. Nos. 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 percent of polyoxyethylene hydrophilic units in the molecule and the polyoxypropylene hydrophobic base has a molecular weight of 950. F-68 also contains 80 percent of polyoxyethylene hydrophilic units in the molecule but the hydrophobic base has a molecular weight of 1750. The total molecular weight of these two PLURONlC polyols is 4750 and 8750, respectively. A further description of these polyols is found in the bulletin of Wyandotte Chemicals Corp. The Pluronic Grid&#34;, Sixth Edition, which is incorporated herein by reference.  
  The selective precipitation of the present invention is carried out by the following sequence of steps:  
  The starting plasma or serum is diluted with water or other aqueous media to a protein concentration of from about 0.5 percent to about 2.5 percent. 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 12 to about 16 percent. The resulting precipitate consists of high molecular weight proteins including the antibodies, and the supernatant comprises albumin and the lower molecular weight globulins.  
  The high molecular weight fraction (precipitate) is separated from the supernatant and diluted with saline or other aqueous media to a protein concentration of from about 0.5 to about 2.5 percent. The diluted material is adjusted to a pH of from about 4.5 to about 5.5 and thoroughly mixed with the block copolymer to a concentration of from about 4.5 to about 5.5 percent. The resulting precipitate is separated from the supernatant and discarded. The supernatant, which contains the immuno globulins, is adjusted to a pH of from about 6 to 8 and thoroughly mixed with the block copolymer to a concentration of from about 14 to about 18 percent. The resulting precipitate (antibody paste) is collected and retained as the desired high molecular weight protein fraction and the supernatant is discarded.  
  The above-prepared lower molecular weight fraction (supernatant) which was initially separated from the high molecular weight fraction 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 20 to about 24 percent. The resulting precipitate is separated from the supernatant and discarded. The supernatant, which contains albumin and the aand B-globulins, is buffered at a pH of from about 4 to about 5 with thorough mixing while the block copolymer is held at a concentration of from about 20 to about 24 percent. In this step, the NaCl concentration preferably is brought to a molarity of 0.15. The resulting precipitate is then collected as the desired lower molecular weight protein fraction and the supernatant is discarded.  
  The above-prepared lower molecular weight protein fraction preferably is placed in solution form. This is achieved by diluting with water or other aqueous media to a concentration of from about 2 to about 4 percent protein, adjusting the pH to a level of from about 6.5 to about 7.5 and adjusting the electrolyte concentration to a level of from about 135 to about 155 milliequivalents of sodium per liter.  
  The thus-reconstituted lower molecular weight fraction preferably is clarified by treatment with a diatomaceous earth such as Celite&#34; and sterile filtered by passage through a Millipore filter using 0.22 micron pads.  
  Preferably, the antibody paste is then reconstituted by admixing with the thus-prepared lower molecular weight protein solution to about one-fourth to one-fifth the volume of the original starting material. This reconstituted material then also preferably is clarified and filtered as was done above for the lower molecular weight protein solution.  
  The following examples will further illustrate the invention although the invention is not limited to these specific examples.  
 EXAMPLE 1 a. Normal human blood plasma is diluted with distilled water to a protein concentration&#39;of l.5 gram percent (grams/lOO ml.) and the pH is adjusted to 7.5. PLURONIC R38 is added to the diluted plasma to a concentration of 14 gm. percent and mixed for 1-2 hours at 10-30 C. The resulting suspension is centrifuged and then both the precipitate and supernatant are collected. The supernatant is retained for further treatment in part (c), below.  
  b. The collected precipitate is suspended in normal physiological saline (0.85% NaCl) to a protein concentration of 1.5 gm. percent and the pH is adjusted to 5. PLURONIC F-38 is added to the diluted precipitate to a concentration of 5 gm. percent and mixed for l-2 hours at 30 C. The resulting suspension is centrifuged, the precipitate is discarded and the supernatant is adjusted to a pH of 7. PLURONlC F-38 is added to the retained supernatant to a concentration of 16 gm. percent and mixed for l-2 hours at 10-30 C. The resulting suspension is centrifuged, the precipitate (antibody paste) is collected and retained as the desired high molecular weight protein fraction while the supernatant is discarded.  
  c. The supernatant retained from part (a), above, is adjusted to a pH of 7.5. PLURONIC F-38 is added to a concentration of 22 gm. percent and mixed for l-2 hours at lO-30 C. The resulting suspension is centrifuged and the precipitate is discarded. The pH of the retained supernatant is buffered to 4.5 with a mixture of 0.8 molar sodium acetate and 4 normal acetic acid, the sodium chloride concentration is adjusted to 0.15 molarity, and PLURONIC F-38 is held at a concentration of 22 gm. percent while mixing for l-2 hours at 1030 C. The resulting suspension is centrifuged, the precipitate is collected and retained as the desired lower molecular weight protein fraction while the supernatant is discarded.  
  d. The final precipitate retained from part (c), above, is dissolved in distilled water to a protein concentration of 3 gm. percent. The pH of the solution is adjusted to 7 with normal sodium hydroxide and the electrolyte concentration adjusted to 145 milliequivalents of sodium per liter. The solution is then filtered through asbestos pads and sterile filtered to 0.22 micron.  
  e. The high molecular weight protein fraction (antibody paste) retained from part (b), above, is then mixed with sufficient solution of the lower molecular weight protein retained from part (d), above, to onefourth to one-fifth the original volume of the plasma starting material in part (a), above. The solution is clarified with Celite diatomaceous earth, cooled to 4 C and sterile filtered to 0.22 micron.  
  The final blended antisera from several runs made according to the above example using various plasma and serum starting materials were assayed and found to have the following characteristics:  
  1. The immunoelectrophoretic pattern resenbled that of the starting materials except that the immune serum globulin precipitant lines were sharper in the fractionated product.  
  2. The radial immunodiffusion determination showed that the fractionated product has a 3- to 4-fold greater content of IgG and lgM immunoglobulin content than that of the starting material.  
  3. Samples of the blended antisera made from group typing sera according to Example 1 were shown to have a 2 to 4-fold increase in both the saline and the Coombs isoagglutinin titers.  
  4. At least 80 percent of the total IgG and at least percent of the total lgM available in the starting material was retained in the final blended antisera.  
  5. The product was free of particulate matter upon storage at 5 C and 24 C for four months and no visible particulate matter was observed when agitated four hours on a mechanical shaker.  
 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 What is claimed is: I 1. A process for the preparation of a stable and concentrated antiserum comprising admixing A. the final product prepared from blood plasma or serum by fractionation with a compound of the formula c are integers such that the hydrophilic d by (CH CH O) constitutes at least of the molecule and b is an integer rophobic portion represented by wherein a and portion represente about 50 percent such that the hyd (CHC H 0) has a molecular weight of at least about 950 comprising admixing said plasma or serum with from about l2 to about 16 percent by weight of said compound at a pH of from about 7 to about 8, separating the precipitate from the resulting suspension and admixing with from about 4.5 to about 5.5 percent by weight of said compound at a pH of from about 4.5 to about 5.5, separating the supernatant from the resulting suspension and admixing with from about 14 to about 18 percent of said compound at a pH of from about 6 to about 8 and collecting the resulting precipitate with an aqueous solution of B. the final product prepared from blood plasma or serum by fractionation with said compound comprising admixing said plasma or serum with from about 12 to about 16 percent by weight of said compound at a pH of from about 7 to about 8, separating the supernatant from the resulting suspension and admixing with from about 20 percent to about 24 percent by weight of said compound at a pH of from about 7 to 8, separating the supernatant from the resulting suspension and admixing with buffer at a pH of from about 4 to about 5 while holding the concentration of said compound at about 20 percent to about 24% and collecting the resulting precipitate.  
  2. A process for the preparation of a stable and concentrated antiserum according to claim 1 in which said compound contains about percent of polyoxyethylene hydrophilic units in the molecule and the polyoxypropylene hydrophobic base has a molecular weight of about 950.