Title of Invention

"CELL SEPARATION COMPOSITION"

Abstract The invention provides compositions and methods for cell separation. These reagents and techniques specially agglutinate cells via surface recognition and can be used to recover even rare cell types in high yield.
Full Text The present invention relates to a cell separation compositions.
BACKGROUND
Many conventional blood cell isolation procedures include a preliminarybulk separation of erythrocytic and granulocytic components by density-gradient sedimentation. Density-gradient separation relies on small differences in the density of different cell types causing them to segregate at different levels in a fluid medium of variable density. Differences in density between the cell types can be small, and individual cells types can be heterogeneous in size and density. Consequently, particular cell types can become distributed throughout a density-gradient" medium rather than precisely segregating at a discrete area in the density medium. This phenomenon can result in poor recovery of desired cells and/or contamination with tmdesired cell types. In procedures that enrich for rare blood cell types such as hematopoietic progenitor cells density-gradient sedimentation generally results in poor yields. For example, using conventional density-gradient methods to isolate progenitor cells (e.g., CD34+ hematopoietic stem cells) from umbilical cord blood reportedly results in a significant loss of the desired stem cells. See e.g., Wagner, J. E., Am J Ped Hematol Oncol 15:169 (1993). As another example, using conventional density-gradient methods to isolate lymphocytes reportedly results in selective loss of particular lymphocyte subsets. See e.g., Collins, D.P.. J Immunol Methods 243:125 (2000).
Increasing the recovery of rare cell types from donor tissue could dramatically improve the success of transplant and immune therapies (e.g.bone marrow transplants, stem cell-based gene therapy, and immune cell therapy), the success of which apparently is related to the actual number of the cells being used for therapy.
SUMMARY
The invention provides compositions and methods for separating cells. The disclosed compositions and methods can be used, for example, to efficiently prepare cells for tissue culture, immunophenotypic characterization, other diagnostic testing, further purification, and therapeutic administration.
Methods of the invention include contacting a blood cell-containing sample (e.g., peripheral blood sample, umbilical cord sample, and bone marrow sample) with a cell separation composition. Without being bound by a particular mechanism, compositions of the invention can selectively agglutinate cells via interaction with cell surface antigens and/or by stimulating cell-cell adherence (e.g., via increased expression of cell surface adhesion factors). Agglutinated cells partition away from unagglutinated cells, which remain in solution. Cells can be recovered from either or both the agglutinate or the supernatant phase.
The disclosed compositions and methods can be used to isolate and enrich for a variety of cell types, including, for example, T lymphocytes, T helper cells, T suppressor cells, B cells, hematopoietic stem cells, circulating fetal cells in maternal circulation, and circulating metastatic tumor cells. The disclosed compositions and methods can be used in the context of allogenic and autologous transplantation. In the context of autologous transplantation, the disclosed compositions and methods can be used, for example, to remove undesired cells such as metastatic cancer cells from a patient's blood or bone marrow. Desirable cells (e.g., hematopoietic stem cells) then can be returned back to a patient without, or substantially free of, life-threatening tumor cells. The disclosed compositions and methods can be applied to cells of any mammal, including humans, non-human primates, rodents, swine, bovines and equines.
Cell separation compositions can contain dextran, anti-glycophorin A antibody, as well as one or more antibodies against cell surface antigens such as CD9, CD15, CD2, CD3, CD4, CD8, CD72, CD16, CD41a, HLA Class I, HLA-DR, CD29, CDlla, CDllb, CDllc, CD19, CD20, CD23, CD39, CD40, CD43, CD44, CDw49d, CD53, CD54, CD62L, CD63, CD66, CD67, CD81, CD82, CD94, CD99, CD100, CD161, Leu-13, TPA-1, or surface Ig, and combinations thereof.
For example, a composition can include dextran, anti-glycophorin A antibody, anti-CD 15 antibody, anti-CD9 antibody, anti-CD94 antibody, and anti-CD161 antibody. In some embodiments, such a composition further can include an anti-CD72 antibody or anti-CD2 antibody. In other embodiments, such a composition further can include anti-CD4 antibody, anti-CD16 antibody, and anti-CD19 antibody, or anti-CD8 antibody, anti-CD 16 antibody, and anti-CD 19 antibody.
Cell separation compositions can contain antibodies against surface antigens of other types of cells (e.g., cell surface proteins of tumor cells).
Antibodies against cell surface antigens can be included in a cell separation composition in either or both soluble and substrate-bound forms. Antibodies can be bound to substrates such as latex microparticles, acid-etched glass particles, aggregated polypeptides, polysaccharides, avidin particles, or biotinylated agarose gel particles. Antibodies in cell separation compositions can be monoclonal and can be IgM or IgG antibodies. In some embodiments, a cell separation composition contains anti-human antibody. The concentration of a soluble antibody in a cell separation composition can be about 0.01 mg/L to about 15 mg/L. Substrate-bound antibodies can be included in a cell separation composition at a concentration between about 0.1 and about 50.0 x 109 particles/1.
Cell separation compositions also can contain heparin, divalent cations (e.g., Ca+2, Mg+2), and phosphate buffered saline. In some embodiments, compositions have a pH between 6.8 to 7.8 (e.g., between 7.2 to 7.4).
The invention also provides kits containing components of a cell separation composition and packaging material. Kits can include a blood collection vessel such as a blood bag or a vacuum tube.
Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention pertains. Although methods and materials similar or equivalent to those described herein can be used to practice the invention, suitable methods and materials are described below. All publications, patent applications, patents, and other references mentioned herein are incorporated by reference in their entirety. In case of conflict, the
present specification, including definitions, will control. In addition, the materials, methods, and examples are illustrative only and not intended to be limiting.
Other features and advantages of the invention will be apparent from the following detailed description, and from the claims.
DESCRIPTION OF THE DRAWINGS
FIG. 1 is a graph of the percent recovery of CD4 T cells from blood samples.
FIG. 2 is a graph of the percent purity of CD4 T cells recovered from blood samples.
FIG. 3 is a graph of the percent recovery of CD8 T cells from blood samples.
FIG. 4 is a graph of the percent purity of CD8 T cells recovered from blood samples.
DETADLED DESCRIPTION
The invention features compositions and methods for separating cells. Compositions of the invention can be used to selectively agglutinate cells from blood cell-containing samples. Without being bound by a particular mechanism, compositions of the invention can agglutinate cells via interaction with cell surface antigens and/or by stimulating expression of cell surface adhesion factors such as LFA-1 (Lymphocyte Function-Associated Antigen-1, CDlla/CD18) and ICAM-1 (Intercellular Adhesion Molecule-1, CD54). Agglutinated cells partition away from unagglutinated cells, which remain in solution. Cells can be recovered from the supernatant or from the agglutinate.
Cell Separation Compositions
A cell separation composition in accord with the invention can contain dextran and one or more antibodies against (i.e., that have specific binding affinity for) a cell surface antigen.
Dextran is a polysaccharide consisting of glucose units linked predominantly in alpha (1 to 6) mode. Dextran can cause stacking of erythrocytes (i.e., rouleau formation) and thereby facilitate the removal of erythroid cells from solution. Typically, the concentration of dextran in a cell separation composition is 10 to 20 g/L (e.g., 20 g/L).
Antibodies against cell surface antigens can facilitate the removal of blood cells from solution via homotypic agglutination (i.e., agglutination of cells of the same cell type) and/or heterotypic agglutination (i.e., agglutination of cells of different cell types).
Cell separation compositions can contain antibodies against blood, cell surface antigens including, for example, glycophorin A, CD15, CD9, CD2, CD3, CD4, CD8, CD72, CD16, CD41a, HLA Class I, HLA-DR, CD29, CDlla, CDllb, CDllc, CD19, CD20, CD23, CD39, CD40, CD43, CD44, CDw49d\ CD53, CD54, CD62L, CD63, CD66, CD67, CD81, CD82, CD94, CD99, CD100, CD161, Leu-13, TPA-1, surface Ig, and combinations thereof. Thus, cell separation compositions can be formulated to selectively agglutinate particular types of blood cells.
In some embodiments, a cell separation composition includes antibodies against glycophorin A. Typically, the concentration of anti-glycophorin A antibodies in a cell separation composition ranges from 0.1 to 15 mg/L (e.g., 0.1 to 10 mg/L, 1 to 5 mg/L, or 1 mg/L). Anti-glycophorin A antibodies can facilitate the removal of red cells from solution by at least two mechanisms. Anti-glycophorin A antibodies can cause homotypic agglutination of erythrocytes since glycophorin A is the major surface glycoprotein on erythrocytes. In addition, anti-glycophorin A antibodies also can stabilize dextran-mediated rouleau formation. Exemplary monoclonal anti-glycophorin A antibodies include, without limitation, 107FMN (Murine IgGl Isotype), YTH89.1 (Rat IgG2b Isotype), and E4 (Murine IgM Isotype). See e.g., M. Vanderlaan et al., Molecular Immunology 20:1353 (1983); Telen M. J. and Bolk, T. A., Transfusion 27: 309 (1987); and Outram S. et al., Leukocyte Research 12:651 (1988).
In some embodiments, a cell separation composition includes antibodies against CD15. The concentration of anti-CD15 antibodies in a cell separation composition can range from 0.1 to 15 mg/L (e.g., 0.1 to 10,1 to 5, or 1 mg/L). Anti-CD 15 antibodies can cause homotypic agglutination of granulocytes by crosslinking CD 15 molecules that are present on the surface of granulocytes. Anti CD 15 antibodies also can cause homotypic and heterotypic agglutination of granulocytes with monocytes, NK-cells and B-cells by stimulating expression of adhesion molecules (e.g., L-selectin and beta-2 integrin) on the surface of granulocytes that interact with adhesion molecules on monocytes, NK-cells and B-cells. Heterotypic agglutination of these cell types can facilitate the removal of these
cells from solution along with, red cell components. Exemplary monoclonal anti-CD 15 antibodies include, without limitation, AHN1.1 (Murine IgM Isotype), FMC-10 (Murine IgM Isotype), BU-28 (Murine IgM Isotype), MEM-157 (Murine IgM Isotype), MEM-158. (Murine IgM Isotype), MEM-167 (Murine IgM Isotype). See e.g., Leukocyte typing IV (1989); Leukocyte typing II (1984); Leukocyte typing VI (1995); Sorter D. et al., Proc. Natl. Acad. Sci. USA 75:5565 (1978); Kannagi, R. et al., J. Biol. Chem. 257:14865 (1982); Magnani, J. L. et al., Archives of Biochemistry and Biophysics 233:501 (1984); Eggens, I. et al.. J. Biol. Chem. 264:9476 (1989).
In some embodiments, a cell separation composition includes antibodies against CD9 (e.g., at a concentration ranging from 0.1 to 15, 0.1 to 10^ 1 to 5, or 1 mg/L). Anti-CD9 antibodies can cause homotypic agglutination of platelets. Anti-CD9 antibodies also can cause heterotypic agglutination of granulocytes and monocytes via platelets that have adhered to the surface of granulocytes and monocytes. CD9 antibodies can promote the expression of platelet 1-selectin, which facilitates the binding of platelets to leukocyte cell surfaces. Thus, anti-CD9 antibodies can promote multiple cell-cell linkages and thereby facilitate agglutination and removal from solution. Exemplary monoclonal anti-CD9 antibodies include, without limitation, MEM-61 (Murine IgGl Isotype), MEM|-62 (Murine IgGl Isotype), MEM-192 (Murine IgM Isotype), FMC-8 (Murine IgG2a Isotype), SN4 (Murine IgGl Isotype), BU-16 (Murine IgG2a Isotype). See e.g., Leukocyte typing VI (1995); Leukocyte typing II (1984); Von dem Bourne A. E. G. Kr. and Moderman P. N. (1989) In Leukocyte typing IV (ed. W. Knapp, et al), pp. 989 - 92. Oxford University Press, Oxford; Jennings, L. K, et al. In Leukocyte typing V. ed. S. F. Schlossmann et al., pp. 1249 - 51. Oxford University Press, Oxford (1995); Lanza, F. et al., J.Biol.Chem.266:10638 (1991); Wright et al., Immunology Today 15:588 (1994); Rubinstein, E. et al.. Seminars in Thrombosis and Hemostasis 21:10 (1995).
In some embodiments, a cell separation composition contains antibodies against CD41, which can selectively agglutinate platelets. In some embodiments, a cell separation composition contains antibodies against CD3, which can selectively agglutinate T-cells. In some embodiments, a cell separation composition contains antibodies against CD2, which can selectively agglutinate T-cells and NK cells. In some embodiments, a cell separation composition contains antibodies against CD72, which can
selectively agglutinate B-cells. In some embodiments, a cell separation composition contains antibodies against CD 16, which can selectively agglutinate NK cells and neutrophilic granulocytes. The concentration of each of these antibodies can range from 0.01 to 15 mg/L.
In other embodiments, a cell separation composition includes antibodies against CD94 and CD161, which can selectively agglutinate subsets of NK cells. Clone HP-3D9 is an example of a suitable anti-CD94 antibody. Clone B199.2 is an example of a suitable anti-CD161 antibody. Monoclonal anti-CD94 and anti-CD161 antibodies are particularly useful. Typically, the concentration of each of these antibodies ranges from 0.01 mg/L to 10 mg/L (e.g., 0.1 to 5,0.1 to 2.5,0.1 to 1.5 mg/L). For example, the concentration of anti-CD94 antibody can be 0.125 to 0.25 mg/L. The concentration of an anti-CD161 antibody can be 0.25 to 1 mg/L.
As mentioned above, cell separation compositions can be formulated to selectively agglutinate particular blood cells. As an example, a cell separation composition containing dextran and antibodies against glycophorin A, CD 15, and CD9 can facilitate the agglutination of erythrocytes, granulocytes, NEC cells, B cells, and platelets. T cells, NK cells and rare precursor cells then can be recovered from solution. If the formulation also contained an antibody against CD3, T cells also could be agglutinated, and NK cells and rare precursors could be recovered from solution. In otber embodiments, a cell separation composition includes dextran and antibodies against glycophorin A, CD 15, CD9, CD94, and CD161 such that erythrocytes, granulocytes, NK cells, B cells, and platelets are agglutinated and T cells and rare precursor cells can be recovered from the solution. To obtain purified populations of CD4 T cells, anti-CD8 antibodies, anti-CD16 antibodies, and anti-CD 19 antibodies can be included in the composition. To obtain purified populations of CD8 T cells, anti-CD4 antibodies, anti-CD16 antibodies, and anti-CD19 antibodies can be included in the composition. Non-limiting examples of suitable anti-CD4 antibodies include clones QS4120, RPA-T4, S3.5, M-T441, RFT-4, and 13B8.2. Non-limiting examples of suitable anti-CD8 antibodies include clones HIT8a, UCHT4, and RPA-T8. Clone 3G8 is an example of a suitable anti-CD 16 antibody. Non-limiting examples of suitable anti-CD 19 antibodies includes clones HB19 and BU12.
Cell separation compositions can contain antibodies against surface antigens of other types of cells (e.g., cell surface proteins of tumor cells). Those of skill in the art can use routine methods to prepare antibodies against cell surface antigens of blood, and other, cells from humans and other mammals, including, for example, non-human primates, rodents (e.g., mice, rats, hamsters, rabbits and guinea pigs), swine, bovines, and equines.
Typically, antibodies used in the composition are monoclonal antibodies, which are homogeneous populations of antibodies to a particular epitope contained within an antigen. Suitable monoclonal antibodies are commercially available, or can be prepared using standard hybridoma technology. In particular, monoclonal antibodies can be obtained by techniques that provide for the production of antibody molecules by continuous cell lines in culture, including the technique described by Kohler, G. et al., Nature, 1975,256:495, the human B-cell hybridoma technique (Kosbor et al., Immunology Today 4:72 (1983); Cole et al., Proc. Natl. Acad. Sci. USA 80:2026 (1983)), and the EBV-hybridoma technique (Cole et al, "Monoclonal Antibodies and Cancer Therapy," Alan R. Liss, Inc., pp. 77-96 (1983)).
Antibodies can be of any immunoglobulin class including IgG, IgM, IgE, IgA, IgD, and any subclass thereof. Antibodies of the IgG and IgM isotypes are particularly useful in cell separation compositions of the invention. Pentameric IgM antibodies contain more antigen binding sites than IgG antibodies and can, in some cases (e.g., anti-glycophorin A and anti-CD 15), be particularly useful for cell separation reagents. In other cases (e.g., anti-CD9 antibodies), antibodies of the IgG isotype are particularly useful for stimulating homotypic and/or heterotypic agglutination.
Antibodies against cell surface antigens can be provided in liquid phase (i.e., soluble) or can be provided in association with a solid phase (i.e., substrate-bound). Liquid phase antibodies typically are provided in a cell separation composition at a concentration between about 0.01 and about 15 mg/L (e.g., between 0.25 to 10, 0.25 to 1, 0.5 to 2,1 to 2, 4 to 8, 5 to 10 mg/L). Substrate-bound antibodies typically are provided in a cell separation composition at a concentration between about 0.1 and about 50.0 x 109 particles/L (e.g., between 0.25 to 10.0 x 109,1 to 20.0 x 109,2 to 10.0 x 109, 0.5 to 2 x
109,2 to 5 x 109,5 to 10 x 109, and 10 to 30 x iO9 particles/L), where particles refers to solid phase particles having antibodies bound thereto.
Antibodies against different cell surface antigens can be covalently linked to a solid phase to promote crosslinking of cell surface molecules and activation of cell surface adhesion molecules. The use of substrate-bound antibodies can facilitate cell separation (e.g., by virtue of the mass that the particles contribute to agglutinated cells, or by virtue of properties useful for purification).
In some embodiments, the solid phase with which an substrate-bound antibody is associated is particulate. In some embodiments, an antibody is bound to a latex microparticle such as a paramagnetic bead (e.g., via biotin-avidin linkage, covalent linkage to COO groups on polystyrene beads, or covalent linkage to NH2 groups on modified beads). In some embodiments, an antibody is bound to an acid-etched glass particle (e.g., via biotin-avidin linkage). In some embodiments, an antibody is bound to an aggregated polypeptide such as aggregated bovine serum albumin (e.g., via biotin-avidin linkage, or covalent linkage to polypeptide COO groups or NH2 groups). In some embodiments, an antibody is covalently linked to a polysaccharide such as high molecular weight (e.g., >1,000,000 Mr) dextran sulfate. In some embodiments, biotinylated antibodies are linked to avidin particles, creating tetrameric complexes having four antibody molecules per avidin molecule, In some embodiments, antibodies are bound to biotinylated agarose gel particles (One Cell Systems, Cambridge, MA, U.S.A.) via biotin-avidin-biotinylated antibody linkages. Such particles typically are about 300-500 microns in size, and can be created in a sonicating water bath or in a rapidly mixed water bath. ,
Cell-substrate particles (i.e., particles including cells and substrate-bound antibodies) can sediment from solution as an agglutinate. Cell-substrate particles also can be removed from solution by, for example, an apphed magnetic field, as when the particle is a paramagnetic bead.
Cell separation compositions also can contain divalent cations (e.g., Ca+2 and Mg+2). Divalent cations can be provided, for example, by a balanced salt solution (e.g., Hank's balanced salt solution). Ca+2 ions may be important for selectin-mediated and integrin-mediated cell-cell adherence.
Cell separation compositions of the invention also can contain an anticoagulant such as heparin. Heparin can prevent clotting and non-specific cell loss associated with clotting in a high calcium environment. Heparin also promotes platelet clumping. Clumped platelets can adhere to granulocytes and monocytes and thereby enhance heterotypic agglutination more so than single platelets. Heparin can be supplied as a heparin salt (e.g., sodium heparin, lithium heparin, or potassium heparin).
Cell Separation Methods
The disclosed compositions can be used, for example, to efficiently prepare cells for tissue culture, immunophenotypic characterization, diagnostic testing, further purification, and therapeutic administration. Without being bound by a particular mechanism, compositions of the invention can selectively agglutinate cells via interaction with cell surface antigens and/or by stimulating cell-cell adherence (e.g., via increased expression of cell surface adhesion factors). Agglutinated cells partition away from unagglutinated cells, which remain in solution.
After agglutination, unagglutinated cells can be recovered from the solution phase (i.e., the supernatant). In embodiments in which one or more biotinylated antibodies are used, the supernatant can be contacted with a composition containing avidin or streptavidin coated particles (e.g., magnetic beads) to further deplete the supernatant of undesired cells. After mixing the supernatant and composition, the beads can be separated from the supernatant (e.g., by applying a magnet) and cells can be removed from the supernatant.
Cells also can be recovered from the agglutinate. Agglutinated cells can be dissociated by, for example, transferring the cells into buffers that contain divalent cation chelators such as EDTA or EGTA. Cells recovered from the agglutinate can be further separated by using antibodies against cell surface antigens. Cells can be recovered from a gel microparticle-antibody-cell agglutinate by heating the agglutinate to a temperature just above the melting point.
The disclosed compositions can be used to separate cells from a variety of blood-cell containing samples, including peripheral blood (e.g., obtained by venipuncture), umbilical cord blood (e.g., obtained post-gravida), and bone marrow (e.g., from aspirate).
Blood ceH-containing samples can be contacted with a cell separation composition to cause agglutination of particular types of cells. For example, erythrocytes and differentiated myeloid blood constituents can be selectively agglutinated using cell separation compositions containing antibodies to surface antigens of these cells. The disclosed compositions and methods can be used to isolate and enrich for a variety of cell types, including, for example, T lymphocytes, T helper cells, T suppressor cells, B cells, hematopoietic stem cells, circulating fetal cells in maternal circulation, and circulating metastatic tumor cells. The disclosed compositions can be used to agglutinate cells of any mammal, including humans, non-human primates, rodents, swine, bovines, and equines.
The disclosed compositions and methods can be used in the context of allogenic and autologous transplantation. In the context of autologous transplantation, the disclosed compositions and methods can be used, for example, to remove undesired cells such as metastatic cancer cells from a patient's blood or bone marrow. Desirable cells (e.g., hematopoietic stem cells) then can be returned back to a patient without, or substantially free of, life-threatening tumor cells.
Cell separation compositions containing antibodies against cell surface proteins of tumor cells can be used to purge tumor cells from a patient's blood or bone marrow. Such compositions also can be used for diagnostic procedures to, for example, obtain and detect tumor cells in an agglutinate, where they are concentrated and are therefore more easily detectable than in circulating blood or in bone marrow. A cell separation composition containing antibodies against the receptor for epithelial growth factor can be used to agglutinate tumor cells derived from epithelial tumors (e.g., head and neck tumors). A cell separation composition containing antibodies against estrogen receptors can be used to agglutinate tumor cells derived from breast and ovarian tumors. A cell separation composition containing antibodies against surface immunoglobulins can be used to agglutinate tumor cells associated with chronic lymphocytic leukemia, plasmacytoma, and multiple myeloma. Breast carcinoma cells express CD 15 on their cell surface, and can be purged from bone marrow using cell separation compositions that contain antibodies against CD15. Other formulas can be made on the basis of cell type and cell surface proteins to obtain or deplete metastatic tumor cells derived from other
carcinomas (e.g., erythroleukemia, endothelial carcinoma, or gastrointestinal carcinoma) from a patient's blood or bone marrow.
Cell Separation Kits
A cell separation composition can be combined with packaging material and sold as a kit. The components of a cell separation composition can be packaged individually or in combination with one another. In some embodiments, the packaging material includes a blood collection vessel (e.g., blood bag, vacuum tube). The packaging material included in a kit typically contains instructions or a label describing how the cell separation composition can be used to agglutinate particular types of cells. Components and methods for producing such kits are well known.
The invention is further described in the following examples, which do not limit the scope of the invention described in the claims.
EXAMPLES Example 1: Separating blood cells.
This example describes the general method by which cells were separated using the cell separation reagelits described below. An equal volume of a cell separation reagent (i.e., 25 ml) was combined with an equal volume of an emylenediaminetetraacetic acid (EDTA) anti-coagulated heparinized peripheral blood sample (i.e., 25 ml) in a 50 ml conical tube. Samples containing white blood cell counts greater than 20 x 10 cells / ml were combined one part blood with two parts cell separation reagent. Tubes were gently mixed on a rocker platform for 20 to 45 minutes at room temperature. Tubes were stood upright in a rack for 30 to 50 minutes to permit agglutinated cells to partition away from unagglutinated cells, which remained in solution. Without disturbing the agglutinate, a pipette was used to recover unagglutinated cells from the supernatant. Recovered cells were washed in 25 ml PBS and centrifuged at 500 x g for 7 minutes. The cell pellet was resuspended in 4 ml PBS.
In embodiments in which one or more of the antibodies are biotinylated, avidin coated magnetic beads were added to the supernatant (1 mL beads/mL of starting sample). Beads and supernatant were mixed on a platform rocker for 20 minutes. Beads
and beads bound to undesired cells were removed by placing the tube containing the mixture in a PrepaMag™ for 5 minutes. Beads and beads bound to undesired cells were drawn to the sides of the tube. A pipet was used to draw the fluid from the center and bottom of each tube, with care taken not to disturb the beads and cells on the sides of the tube.
Cells also were recovered from the agglutinate using a hypotonic lysing solution containing EDTA and ethylene glycol-bis(2-aminoethylether)-N,N,N',N'-tetraacetic acid (EGTA). Agglutinated cells were treated with 25 ml VitaLyse™ (BioErgonomics, St. Paul, MN) and vortexed. After 10 minutes, cells either were exposed to an applied magnetic field to recover cells associated with antibodies bound to paramagnetic beads, or were centrifuged at 500 x g for 7 minutes and the supernatant was removed. In either case, cells were resuspended in 4 ml PBS.
Recoveries of erythrocytes, leukocytes, lymphocytes, monocytes, granulocytes, T cells, B cells, and NK cells were determined by flow cytometry and immunophenotyping. Prior to flow cytometry, leukocyte recovery (i.e., white blood cell count) was determined using a Coulter Onyx Hematology Analyzer, and samples were adjusted with PBS to a cell count of 1 x 107 cells/mL. 100 ul aliquots of volume-adjusted sample were stained at room temperature in the dark for 15 to 30 minutes with either FITC labeled anti-CD3 antibodies (reactive to T cells), PE labeled anti-CD 19 antibodies (reactive to B cells), or PE labeled anti-CD16 antibodies (reactive to NK cells). 2 ml of PBS was added to each sample, and the sample then was vortexed and centrifuged to pellet cells. Supematants were discarded, and cell pellets were vortexed and resuspended in 0.5 ml PBS. Stained and unstained cells were analyzed by flow cytometry using a Coulter XL flow cytometer. Erythrocytes, leukocytes, lymphocytes, monocytes, granulocytes and platelets were identified on the basis of diagnostic forward and side light scatter properties. B cells, T cells, and NK cells were identified on the basis of light scattering and staining by labeled antibodies.
Example 2: Erythrocyte agglutination.
The reagent described in Table 1 was used to separate cells according to the method described in Example 1.
Table 1
(Table Removed)

Results of a separation are shown in Table 2. Erythrocytes were depleted 99.7% from the supernatant. Lymphocytes (T cells, B cells, and NEC cells) were enriched in the supernatant relative to the monocytes and granulocytes.
Table 2
(Table Removed)
Example 3: Erythrocyte and CD2+ cell agglutination.
The reagent described in Table 3 was used to separate cells according to the method described in Example 1.
Table 3
(Table Removed)
Results of a separation are shown in Table 4. In the supernatant, erythrocytes were depleted 99.7%, T cells were depleted 95.1%, and NK cells were depleted 69.1%. B cells were enriched in the supernatant relative to other cells.
Table 4
(Table Removed)
Example 4: Erythrocyte and CD72+ cell agglutination.
The reagent described in Table 5 was used to separate cells according to the method described in Example 1.
Table 5
(Table Removed)
Results of a separation are shown in Table 6. In the supernatant, erythrocytes were depleted 99.5%, and B cells were depleted 81.6%.
Table 6
(Table Removed)
Example 5: Erythrocyte, CD15+ cell, and CD9+ cell agglutination.
The reagent described in Table 7 was used to separate cells according to the method described in Example 1.
Table 7
(Table Removed)
Results of a separation are shown in Table 8. In the supernatant, erythrocytes were depleted 99.9%, monocytes and granulocytes were depleted 99.8%, B cells were depleted 74%, and NK cells were depleted 64.9%. In addition, platelets, present in the supernatant at 226 x 106 /ml before separation, were depleted to 1.4 x 106/ml for 99.4% depletion.
Table 8
(Table Removed)
Example 6: Erythrocyte, CD15+ cell, CD9+ cell, and CD2+ cell agglutination.
The reagent described in Table 9 was used to separate cells according to the method described in Example 1.
Table 9
(Table Removed)
Results of a separation are shown in Table 10. In the supernatant, erythrocytes were depleted 99.9%, monocytes and granulocytes were depleted 99.9%, B cells were depleted 16.8%, NK cells were depleted 29%, and T cells were depleted 91.5%. In addition, platelets, present in the supernatant at 226 x 106 /mL before separation, were depleted to 0.3 x 106/mL for 99.9% depletion.
Table 10
(Table Removed)
Example 7: Erythrocyte, CD15+ cell, CD9+ cell, and CD72+ cell agglutination.
The reagent described in Table 11 was used to separate cells according to the method described in Example 1.
Table 11

(Table Removed)
Results of a separation are shown in Table 12. In the supernatant, erythrocytes were depleted 99.9%, monocytes were depleted beyond detection, granulocytes were depleted 99.97%, B cells were depleted 97.2%, NK cells were depleted 54.9%. In addition, platelets, present in the supernatant at 226 x 106 /mL before separation, were depleted to 0.1 x 106/mL for 99.96% depletion.
Table 12
(Table Removed)
Example 8: Erythrocyte, CD15+ cell, CD9+ cell, CD19+ cell, and CD16+ cell agglutination.
The reagent described in Table 13 was used to separate cells according to the method described in Example 1. T cells and CD3+ cells were recovered from the supernatant. B cells and granulocytes are recovered from the agglutinate.
Table 13
(Table Removed)
Example 9: Erythrocyte, CD15+ cell, CD9+ cell, CD19+ cell, CD16+ cell, and CD4+ cell agglutination.
The reagent described in Table 14 was used to separate cells according to the method described in Example 1. CD8+ cells were recovered from the supernatant.
Table 14

(Table Removed)

Example 10: Erythrocyte, CD15+cell, CD9+cell, CD19+cell, CD16+cell, and CD8+ cell agglutination.
The reagent described in Table 15 is used to separate cells according to the
method described in Example 1. CD4+ cells are recovered from the supernatant.
Table 15

(Table Removed)
Example 11: Erythrocyte, CD15+ cell, CD9+ cell, CD19+ cell, and CD2+ cell agglutination.
The reagent described in Table 16 was used to separate cells according to the
method described in Example 1. CD34+ cells were recovered from the supernatant at
>50% purity and >80% yield.
Table 16
(Table Removed)
Example 12: Erythrocyte, CD15+ cell, CD9+ cell, CD2+ cell, and CD16+ cell agglutination.
The reagent described in Table 17 was used to separate cells according to the method described in Example 1. B cells were recovered from the supernatant.
Table 17
(Table Removed)
Example 13: Erythrocyte, Mature Myeloid Cells, NK cells, and B cell Agglutination.
The reagent described in Table 18 was used to separate cells according to the method described in Example 1. Hydrochloric acid (4N) or sodium hydroxide (4N) was used to adjust the pH to between 7.2 and 7.4. The ami-CD8, CD16, CD19, CD94, and CD161 antibodies were biotinylated. A cell suspension enriched for CD4 T cells was obtained from the supernatant. Approximately 75 to 94% of the CD4 cells were recovered from each whole blood sample (FIG. 1 provides representative data for five donors). In comparison, cell recovery was 50% or less in other commercially available products that used density-gradient separation. On average, purity of CD4 cells was 96.1% (see FIG. 2, representative data for 12 donors), whereas average purity was 86.7% for CD4 cells purified using other commercially available products that used density-gradient separation.
Table 18
(Table Removed)
Example 14: Erythrocyte, Mature Myeloid Cells, NE cells, and B cell Agglutination.
The reagent described in Table 19 was used to separate cells according to the method described in Example 1. Hydrochloric acid (4N) or sodium hydroxide (4N) was used to adjust the pH to between 7.2 and 7.4. The anti-CD4, CD16, CD19, CD94, and CD161 antibodies were biotinylated. A cell suspension enriched for CDS T cells was obtained from the supernatant. Approximately 53 to 81% of the CD8 cells were recovered from each whole blood sample (FIG. 3 provides representative data for five donors). In comparison, cell recovery was less than 52% using other commercially available products that required density-gradient separation, and more typically, cell recovery was less than 35%. On average, purity of CD8 cells was 93.9% (see FIG. 4, representative data for 12 donors), whereas average purity was 84.2% for CDS cells purified by other commercially available products.
Table 19
(Table Removed)
OTHER EMBODIMENTS
While the invention has been described in conjunction with the foregoing detailed description and examples, the foregoing description and examples are intended to illustrate and not to limit the scope of the invention, which is defined by the scope of the appended claims. Other aspects, advantages, and modifications are within the scope of the claims.




WE CLAIM:
1. A cell separation composition comprising:
a) dextran;
b) anti-glycophorin A antibody;
c) anti-CD 15 antibody;
d) anti-CD9 antibody;
e) anti-CD94 antibody, and
f) anti-CD 161 antibody;
wherein the concentration of said dextran is from 10 g/L to 20 g/L, the concentrations of said anti-glycophorin A antibody, said anti-CD 15 antibody, and said anti-CD9 antibody are from 0.1 mg/L to 15 mg/L, and the concentrations of said anti-CD94 antibody and said anti-CD 161 antibody are from 0.01 mg/L to 10 mg/L.
2. The composition as claimed in claim 1, said composition consisting of
anti-CD72 antibody at a concentration of from 0.01 mg/L to 15 mg/L.
3. The composition as claimed in claim 1, said composition consisting of
anti-CD4 antibody, anti-CD 16 antibody, and anti-CD 19 antibody,
wherein the concentrations of said anti-CD4 antibody, said anti-CD 16
antibody, and said anti-CD 19 antibody are from 0.01 mg/L to 15 mg/L.
4. The composition as claimed in claim 1, said composition consisting of anti-CD8 antibody, anti-CD 16 antibody, and anti-CD 19 antibody, wherein the concentrations of said anti CD8 antibody, said anti-CD 16 antibody, and said anti-CD 19 antibody are from 0.01 mg/L to 15 mg/L.
5. The composition as claimed in claim 1, said composition consisting of anti-CD2 antibody at a concentration of from 0.01 mg/L to mg/L.
6. The composition as claimed in any one of claims 1 to 5, consisting of heparin.
7. The composition as claimed in any one of claims 1 to 6, consisting of divalent cations.
8. The composition as claimed in claim 7, wherein said divalent cations are Ca+2 or Mg+2.
9. The composition as claimed in any one of claims 1 to 8, consisting of phosphate buffered saline.

10. The composition as claimed in any one of claims 1-8 or 9, wherein the pH of said composition is between 6.8 to 7.8.
11. The composition as claimed in claim 10, wherein the pH of said composition is between 7.2 to 7.4.
12. The composition as claimed in any one of claims 1-8 or 9-11, wherein said anti glycophorin A antibody, said anti-CD 15 antibody, or said anti-CD9 antibody is monoclonal.
13. The composition as claimed in any one of claims 1-8 or 9-12, wherein said anti glycophorin A antibody, said anti-CD 15 antibody, said anti-CD9 antibody, said anti-CD94 antibody, or said anti-CD 161 antibody is an lgM antibody, or an IgG antibody.
14. The composition as claimed in any one of claims 1-8 or 9-13, wherein said anti glycophorin A antibody, said anti-CD 15 antibody, said anti-CD9 antibody, said anti-CD94 antibody, or said anti-CD 161 antibody is an anti-human glycophorin A antibody.
15. The composition as claimed in any one of claims 1-8 or 9-14, wherein at
least one of said antibodies is biotinylated.
16. The composition as claimed in claim 15, wherein said anti-CD 16 antibody, said anti-CD 19 antibody, said anti-CD94 antibody, and said anti-CD 161 antibody are biotinylated.



Documents:

1351-delnp-2005-abstract.pdf

1351-delnp-2005-assignment.pdf

1351-DELNP-2005-Claims.pdf

1351-delnp-2005-complete specification (as files).pdf

1351-delnp-2005-complete specification (granted).pdf

1351-delnp-2005-correspondence-others.pdf

1351-delnp-2005-correspondence-po.pdf

1351-DELNP-2005-Description (Complete).pdf

1351-DELNP-2005-Drawings.pdf

1351-delnp-2005-form-1.pdf

1351-delnp-2005-form-18.pdf

1351-DELNP-2005-Form-2.pdf

1351-delnp-2005-form-3.pdf

1351-delnp-2005-form-5.pdf

1351-delnp-2005-gpa.pdf

1351-delnp-2005-pct-101.pdf

1351-delnp-2005-pct-210.pdf

1351-delnp-2005-pct-220.pdf

1351-delnp-2005-pct-304.pdf

1351-delnp-2005-pct-306.pdf

1351-delnp-2005-petition-137.pdf


Patent Number 243112
Indian Patent Application Number 1351/DELNP/2005
PG Journal Number 40/2010
Publication Date 01-Oct-2010
Grant Date 27-Sep-2010
Date of Filing 04-Apr-2005
Name of Patentee BIOE,INC.
Applicant Address 4280 CENTERVILLE ROAD, ST. PAUL, MINNESOTA-55127, UNITED STATES OF AMERICA.
Inventors:
# Inventor's Name Inventor's Address
1 DANIEL P. COLLINS 6656 PELICAN PLACE, LINO LAKES, MINNESOTA 55014, USA.
2 JOEL H. HAPKE 2401-55TH AVENUE NORTH, BROOKLYN CENTER, MINNESOTA 55430,USA.
3 CAROL A. BUCHERT 8110-173RD AVENUE NW, RAMSEY, MINNESOTA 55303, USA.
PCT International Classification Number C12N
PCT International Application Number PCT/US2003/030265
PCT International Filing date 2003-09-26
PCT Conventions:
# PCT Application Number Date of Convention Priority Country
1 60/414,692 2002-09-27 U.S.A.