CA2069872A1 - Monoclonal antibody, hybridomas, their production and use - Google Patents
Monoclonal antibody, hybridomas, their production and useInfo
- Publication number
- CA2069872A1 CA2069872A1 CA002069872A CA2069872A CA2069872A1 CA 2069872 A1 CA2069872 A1 CA 2069872A1 CA 002069872 A CA002069872 A CA 002069872A CA 2069872 A CA2069872 A CA 2069872A CA 2069872 A1 CA2069872 A1 CA 2069872A1
- Authority
- CA
- Canada
- Prior art keywords
- bfgf
- arg
- asp
- antibody
- cell
- Prior art date
- Legal status (The legal status 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 status listed.)
- Abandoned
Links
Classifications
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/18—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans
- C07K16/22—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against growth factors ; against growth regulators
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P35/00—Antineoplastic agents
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/435—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- C07K14/475—Growth factors; Growth regulators
- C07K14/50—Fibroblast growth factors [FGF]
- C07K14/503—Fibroblast growth factors [FGF] basic FGF [bFGF]
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K38/00—Medicinal preparations containing peptides
Abstract
Disclosed are (1) a monoclonal antibody which immuno-neutralizes the activity of a bFGF protein and highly sensitively combines with the bFGF protein; (2) a cloned hybridoma for (1); (3) a method for producing the cloned hybridoma (2); (4) a method for producing the monoclonal (1); (5) a method for purifying the bFGF
protein, which comprises using the monoclonal antibody (1); and (6) a method for detecting or determining the bFGF protein, which comprises using the monoclonal antibody (1).
protein, which comprises using the monoclonal antibody (1); and (6) a method for detecting or determining the bFGF protein, which comprises using the monoclonal antibody (1).
Description
WO91/09X75 PCT/JP9OtO1726 ~ 5~ 7 DESCRIPTION
MONOCLONAL ANTIBODY, HYBRIDOMAS, THEIR PRODUCTION AND USE
Technical Field The present invention relates to monoclonal antibodies `~
5 which immuno-neutralize the biological activity of basic `~
fibroblast growth factor ~also briefly referred to as bFGF
in the present specification) proteins and have high binding sensitivity with bFGF proteins, hybridomas secreting the same, their production and use thereof.
Backqround Art bFGF is a basic polypeptide hormone having an affinity for heparin and a molecular weight of about 17,000 ~D.
Gospodarowicz, Nature 249, 123 (1974)]. It is now known that bFGF exhibits growth promoting action on almost all cells derived from mesoblast, and acts as a differentiating factor to a mesoblast system. For example, bFGF induces the proliferation of nerve cells, the proliferation of vascular endothelial cells to cause angiogenesis, and the proliferation of cancer cells. Coupled with these functions, therefore, bFGF is involved in diseases such as tumors. Accordingly, a monoclonal antibody which inhibits the actlvity of bFGF would be useful as a therapeutic drugs for such diseases. However, this possibility has not been recognized till now. Further, as a means for diagnosing 25 these diseases, the determination of blood bFGF `::
concentrations is considered. It is however impossible to detect bFGF with great sensitivity by previously known methods.
WO91/09875 pCT/JP90/01726 z~ 2 -As discussed above bFGF is involved in diseases such as cancer, so that the inhibition of the growth promoting - activity of bFGF to the cancer cells presents the possibility of use as a cancer therapy.
In addition, there is the potential that bFGF itself may have application as a therapeutic drug for traumas and burns. In this case, the determination of fundamental information regarding bFGF is essential for the development of bFGF as a medicine. Also in the diseases in which bFGF
is invollved, such as cancer, the diagnosis of the disease becomes possible by tracing the blood bFGF concentrations.
However, since bFGF is adsorbed by heparan sulfate existing among vascular endothelial cells, bFGF exists in blood only in trace amounts. Accordingly, there is a need in the art to develop a highly sensitive quantitative assay for measuring bFGF in the blood.
SummarY of the Invention In view of the above-mentioned circumstances, the present inventors prepared monoclonal antibodies which
MONOCLONAL ANTIBODY, HYBRIDOMAS, THEIR PRODUCTION AND USE
Technical Field The present invention relates to monoclonal antibodies `~
5 which immuno-neutralize the biological activity of basic `~
fibroblast growth factor ~also briefly referred to as bFGF
in the present specification) proteins and have high binding sensitivity with bFGF proteins, hybridomas secreting the same, their production and use thereof.
Backqround Art bFGF is a basic polypeptide hormone having an affinity for heparin and a molecular weight of about 17,000 ~D.
Gospodarowicz, Nature 249, 123 (1974)]. It is now known that bFGF exhibits growth promoting action on almost all cells derived from mesoblast, and acts as a differentiating factor to a mesoblast system. For example, bFGF induces the proliferation of nerve cells, the proliferation of vascular endothelial cells to cause angiogenesis, and the proliferation of cancer cells. Coupled with these functions, therefore, bFGF is involved in diseases such as tumors. Accordingly, a monoclonal antibody which inhibits the actlvity of bFGF would be useful as a therapeutic drugs for such diseases. However, this possibility has not been recognized till now. Further, as a means for diagnosing 25 these diseases, the determination of blood bFGF `::
concentrations is considered. It is however impossible to detect bFGF with great sensitivity by previously known methods.
WO91/09875 pCT/JP90/01726 z~ 2 -As discussed above bFGF is involved in diseases such as cancer, so that the inhibition of the growth promoting - activity of bFGF to the cancer cells presents the possibility of use as a cancer therapy.
In addition, there is the potential that bFGF itself may have application as a therapeutic drug for traumas and burns. In this case, the determination of fundamental information regarding bFGF is essential for the development of bFGF as a medicine. Also in the diseases in which bFGF
is invollved, such as cancer, the diagnosis of the disease becomes possible by tracing the blood bFGF concentrations.
However, since bFGF is adsorbed by heparan sulfate existing among vascular endothelial cells, bFGF exists in blood only in trace amounts. Accordingly, there is a need in the art to develop a highly sensitive quantitative assay for measuring bFGF in the blood.
SummarY of the Invention In view of the above-mentioned circumstances, the present inventors prepared monoclonal antibodies which
2~ highly sensitive determination of bFGF proteins, as well as immuno-neutralize the activity of the bFGF. The present invention conducted further researches based thereon, thus completing the present invention.
The present invention provides:
~l) a monoclonal antibody which has the following characteristics, it immuno-neutralizes the activity of a bFGF protein and has high binding sensitivity with the bFGF
: . :
., ., ... . . . ~ .. :: .. : .. . :: . ~ - . :
WO 91to9~7~; PC'r/JI~O/û1726 0~ ~
protein:
(a) it has a molecular weight of about 140,000 to 160,000, (b) it does not cross-react with acidic fibroblast growth factor, ~ c) it belongs to immunoglobulin class IyGl, (d) it binds with rhbFGF mutein CS23 (a mutein in which the cysteine residues at positions 70 and 88 of hbFGF are substituted for serine residues), (e) it completely inhibits proliferation of a human unbilical vein endothelial (HUVE) cell by addition of 50 : :
ng/ml thereof in the presence of 2 ng/ml of bFGF, and (f) it can detect 20 pg/ml of the bFGF protein by a sandwich enzyme-linked immunosorbent assay (ELISA) using monoclonal antibody MoAbl2 (solid phase) and a peroxidase-labeled antibody;
~ 2) a cloned hybridoma derived from a mammalian spleen cell and a homogenic or heterogenic lymphoid cell, said mammal being immunized with a mutein in which at least one ~:
cysteine residue of bFGF is substituted for a serine ; residue;
The present invention provides:
~l) a monoclonal antibody which has the following characteristics, it immuno-neutralizes the activity of a bFGF protein and has high binding sensitivity with the bFGF
: . :
., ., ... . . . ~ .. :: .. : .. . :: . ~ - . :
WO 91to9~7~; PC'r/JI~O/û1726 0~ ~
protein:
(a) it has a molecular weight of about 140,000 to 160,000, (b) it does not cross-react with acidic fibroblast growth factor, ~ c) it belongs to immunoglobulin class IyGl, (d) it binds with rhbFGF mutein CS23 (a mutein in which the cysteine residues at positions 70 and 88 of hbFGF are substituted for serine residues), (e) it completely inhibits proliferation of a human unbilical vein endothelial (HUVE) cell by addition of 50 : :
ng/ml thereof in the presence of 2 ng/ml of bFGF, and (f) it can detect 20 pg/ml of the bFGF protein by a sandwich enzyme-linked immunosorbent assay (ELISA) using monoclonal antibody MoAbl2 (solid phase) and a peroxidase-labeled antibody;
~ 2) a cloned hybridoma derived from a mammalian spleen cell and a homogenic or heterogenic lymphoid cell, said mammal being immunized with a mutein in which at least one ~:
cysteine residue of bFGF is substituted for a serine ; residue;
(3) a method for producing a cloned hybridoma which comprises fusing a spleen cell from a mammal and a homogenic or heterogenic lymphoid cell, said mammal being immunized with a mutein in which at least one cysteine residue of bFGF
is substituted for a serine residue, and selecting the desired hybridoma, followed by cloning;
WO9~ 7s pCT/JP9~/01726 t Q`~ 4
is substituted for a serine residue, and selecting the desired hybridoma, followed by cloning;
WO9~ 7s pCT/JP9~/01726 t Q`~ 4
(4) a method for producing the monoclonal antibody described in the above item (1), which comprises culturing a ~`
cloned hybridoma comprising a spleen cell from a mammal and a homogenic or heterogenic lymphold cell in a liquid culture medium or in a peritoneal cavity of the mammal to produce the monoclonal antibody, said mammal being immunized with a mutein in which at least one cysteine residue of bFGF is substituted for a serine residue, and recovering the monoclonal antibody;
cloned hybridoma comprising a spleen cell from a mammal and a homogenic or heterogenic lymphold cell in a liquid culture medium or in a peritoneal cavity of the mammal to produce the monoclonal antibody, said mammal being immunized with a mutein in which at least one cysteine residue of bFGF is substituted for a serine residue, and recovering the monoclonal antibody;
(5) a method for purifying a bFGF protein, which comprises contacting the monoclonal antibody described in the above item (1) with a sample containing bFGF protein;
and
and
(6) a method for detecting or measuring a bFGF protein, which comprises using the monoclonal antibody described in the above item (1).
- Brief Description of Drawinq_ Fig. 1 shows a cDNA se~uence of human aFGF used in Reference Example l;
Fig. 2 is a schematic representation showing the construction of plasmid pTB975 obtained in Reference Example l;
Figs. 3 to S show elution pat~erns obtained in Reference Example 1;
Fig. 6 is a graph showing the affinity of monoclonal antibody 3H3 of the present invention obtained in Example 4 for rhbFGF mutein CS23;
`~
:`
., .. , .,, . .. . . ..... .,, . . . .. . ~. . .
WO91/~987~ PCTIJP90/01726 Fig. 7 is a graph s~o~ing the human bFGF-neutralizing activity of monoclonal antibody 3H3 of the present invention obtained in Example 6;
Figs. 8~a) and 8(b) are yraphs showing the proliferation inhibition effect of monoclonal antibody 3~3 of the present invention obtained in Example 6 for HUVE
cells, in which Fig. 8(a) shows the results of cultivation for 3 days and Fig. 8(b) shows the results of cultivation for 5 days;
Fig. 9 is a graph showing the relationship between the concentration and the absorbance of hbFGF, obtained in Example '~;
Fig. 10(1) and 10~2) are graphs showins the influence of heparin in a hbFGF determination system, obtained in Example 10, in which Fig. 10(1) shows the results when MAbl2 is fixed, and Fig. 10(2) shows the results when a 50-50 mixture of MAb52 and MAb98 is fixed;
Fig. 11(1) and 11(2) are graphs showing the reaction in a hbFGF determination system, obtained in Example 11, in which Fig. 11(1) shows the results when MAbl2 is solidified, and Fig. 11(2) shows the results when a 50-50 mixture of MAbS2 and MAb98 is fixed;
Fig. 12 is a graph showing the anti-tumor effect of an antibody of the present invention, obtained in Example 13;
and Fig. 13 is a schematic representation showing the construction of plasmid p'rB1000 obtained in Reference Example 2.
~:
~ 6 -Detailed Descri~tion of the_Invention The bFGF proteins of the present invention include bFGFs and muteins in which at least one cysteine residue of bFGF is substituted for a serine residue and which have bFGF
activity.
As the bFGF proteins, there are preferably used polypeptides containing the amino acid sequence represented ~:
by formula (I):
Phe-Phe-Leu-Arg-Ile-~is-Pro-Asp-Gly-Arg-Val- `
lOAsp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro tI) The bFGFs of the present invention include bFGFs derived from mammals. The mammals include humans, monkeys, pigs, bovines, sheep and horses.
The bFGFs also include bFGFs extracted from various lS organs existence of which is already clarified, such as brains and pituitary glands.
The bFGF proteins may be produced by recombinant DNA
techniques.
Examples of amino acid sequences of the bFGFs include the amino acid sequence represented by formula tII):
Pro-Ala-Leu-Pro-Glu-Asp-Gly-Gly-Ser-Gly-Ala-Phe-Pro-Pro-Gly-His-Phe-Lys-Asp-Pro-Lys-Arg-Leu-Tyr-Cys-Lys-Asn-Gly-Gly-Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-25Val-Asp-Gly-Val-Arg-Glu Lys-Ser-Asp-Pro-His-Ile-Lys-Leu-Gln-Leu-Gln-Ala-Glu-Glu-Arg-Gly-Val-Val-Ser-Ile-Lys-Gly-Val-Cys-WO91/o9875 PCT/JP90/01726 ~ ;'``;~.7~
Ala-Asn-Arg-Tyr-Leu~Ala-Met-Lys-Glu-Asp-Gly-Arg-Leu-Leu-Ala-Ser-Lys-Cys-Val-Thr-Asp-Glu-Cys-Phe-Phe-Phe-Glu-Arg-Leu-Glu-Ser-Asn-Asn-Tyr-Asn-Thr-Tyr-Arg-Ser-Arg-Lys-Tyr-X -Ser-Trp-Tyr-Val-Ala-Leu-Lys-Arg-Thr-Gly-Gln-Tyr-Lys-Leu-Gly-Y Lys-Thr-Gly-Pro-Gly-~ln-Lys-Ala-Ile-Leu-Phe-Leu-Pro-Met-Ser-Ala-Lys-Ser (II) wherein X represents Thr or Ser, and Y represents Ser when X
is Thr, an~ Y represents Pro when X is Ser.
As the bFGF, human bFGF is preferable. The human bFGF
has the amino acid sequence in which X is Thr and Y is Ser in the above formula (II).
The muteins in which at least one cysteine residue of the above bFGF is substituted for a serine residue include, for example, the muteins described in Seno et al., BiophYs.
Res. Commun. 151, 701 (1988) and European Patent Publication No. 281,822.
In particular, there is preferably used recombinant human bFGF mutein CS23 (hereinafter also briefly referred to as rhbFGF mutein CS23) in which each of the cysteine residues at positions 70 and 88 of the human bFGF is substituted for a serine residue. With respect to the number of the positions of the above amino acids, in the amino acid sequence in which Met is added to the N-terminus of the peptide in which X is Thr and Y is Ser in the above formula ~II), the Met is numbered as the first.
~'`', ' :
~091/09M75 PCT/JP90/01726 ~ 8 --In thè bFGFs produced by the above-mentioned genetic engineering techniques, examples of the human bFGF include bFGF produced by the methods described, for example, in FEBS
Letters 213, 189 (1987), ~E~y___Res. Commun. 146, 470 (1987) and European Patent Publication No. 237,966.
When mammals are immunized with the bFGF proteins or protein conjugates, there are used experimental animals such as sheep, goat, rabbits, guinea pigs, rats and mice, as the mammals to be immunized. In order to obtain monoclonal antibodies, however, it is preferred to use rats or mice for immunization.
When mice are immunized, for example, they can be immunized by any of the subcutaneous, intraperitoneal, intravenous, intramuscular and intracutaneous routes.
However, subcutaneous, intraperitoneal and intravenous injections are preferably used. In particular, subcutaneous injection is preferable. The immunizing interval and the immunizing dose are widely variable, and various methods are available. For example, methods in which immunization is carried out about 2 to 6 times at intervals of 2 weeks and spleen cells are removed after about 1 to 5 days, preferably about 2 to 4 days from the final immunization are frequently used. As the immunizing dose, it is preferred to use about 0.1 ~g or more, preerably about 10 to 300 ~g of the peptide per one immunization of a mouse. Further, it is desirable to carry out the fusion process using the spleen cells after confirmation of an increase in antibody titer in blood by WOgltO9875 PCT/JP9~/~t726 jJ?
collecting a portion o~ blood and measuring the antibody titer before removal of the spleens.
The above spleen cells are then fused wlth lymphoid cells. For example, the spleen cells removed from the mice ~
5 are fused with lymphoid cell strains such as suitable ~ ;
myeloma cells [for example, P3-X-63-Ag-8UI ~Ichimori et al., J. Immun. Method 80, 55 ~1985))~ of the same kind or a different kind (preferably ~he same kind) having markers such as hypoxanthine-guanine-phosphoribosyl-transferase 10 deficient (HGPRT ) and thymidine kinase deficient (TK ).
For example, begin a new paragraph the fused cells are produced in accordance with the method of Kohler and Milstein [~ature 256, 495 (1975)1. For example, myeloma _ cells and spleen cells in a ratio of about 1:5 are suspended 15 in a medium prepared by mixing Iskov medium and Ham F-12 medium in a 1:1 ratio (hereinafter referred to as IH
medium), and a fusion accelerator such as Sendai virus or polyethylene glycol (PEG) is added thereto. It is of course possible to add other fusion accelerators such as dimethyl 20 sulfoxide (DMSO). The polymerization degree of PEG is ?
usually about 1,000 to 6,000, the fusion time is about 0.5 to 30 minutes, and the concentration of the suspension is about 10 to 80%. As a preerred condition, the fusion is carried out efficiently by using PEG 6,000 in a concentration of about 35 to 55% for about 4 to 10 minutes.
The fused cells can be selectively proliferated using hypoxanthine-aminopterin-thymidine medium ~HAT medium) ~ ' ' WO 91/09875 PCr/JP90/01726 ,~ f --[Nature, 256, 4~5 (1975) ].
_ _ The culture supernatant of the proliferated cells is then screened for the production of the desired antibody.
Screening of the antibody titer can be carried out in the following manner. First, the presence or absence of the antibody production by peptide immunization is examined by radio immunoassays (RIAs) or enzyme immunoassays (EIAs).
For these methods, various modified me~hods are also available.
As a preferred example of the assays, a method using the EIA is described below. A rabbit anti-mouse immunoglobulin antibody is coupled with a carrier such as cellulose beads according to conventional methods, and then a culture supernatant or mouse serum to be assayed is added thereto, followed by reaction at a constant temperature (about 4 to 40C, the same applied hereinafter) for a definite time. After the reaction product is thoroughly washed, an enzyme-labeled peptide (a peptide is coupled with an enzyme according to conventional methods, followed by purification) is added thereto, followed by reaction at a constant temperature for a specified time. After the reaction product is thoroughly washed, an enzyme substrate is added thereto, followed by reaction at a constant temperature for a speciied time. Then, the absorbance or fluorescence of the color-produced product is measured.
As to the culture supernatant of the proliferated cells, the screening of the neutralizing activity to the ,. .
. ~:
wogl/0987~ 7~ PCT/JP9OtO1726 bFGF proteins can be carried out in the following manner.
In this case, the neutralizing activity can be examined using cells whcse proliferation is induced by the bFGF
proteins. As such cells, there can be used vascular endothelial cells, fibroblasts, nerve cells and the like.
It is however desirable to know whether or not the additional effect of the bFGF proteins is inhibited by ; measuring the number of cells, using the vascular endothelial cells begin a new paragraph.
Methods for measuring the number of cells include a method for measuring directly the number of cells, a method or determining radioactivity by using tritium thymidine and a method for measuring colorimetrically using (4,5-dimethyl-; 2-thiazoly)-2,5-diphenyl-2H-tetrazolium bromide (MTT) (MTT
method). As one example of the preferred assays, there is ; hereinafter described a method for assaying cell proliferation by the MTT method using human umbilical vein-derived endothelial cells. After the cells are seeded, the bFGF protein and the culture supernatant to be assayed are added thereto, followed by cultivation at a constant temperature (37C) at a low concentration of oxygen ~about
- Brief Description of Drawinq_ Fig. 1 shows a cDNA se~uence of human aFGF used in Reference Example l;
Fig. 2 is a schematic representation showing the construction of plasmid pTB975 obtained in Reference Example l;
Figs. 3 to S show elution pat~erns obtained in Reference Example 1;
Fig. 6 is a graph showing the affinity of monoclonal antibody 3H3 of the present invention obtained in Example 4 for rhbFGF mutein CS23;
`~
:`
., .. , .,, . .. . . ..... .,, . . . .. . ~. . .
WO91/~987~ PCTIJP90/01726 Fig. 7 is a graph s~o~ing the human bFGF-neutralizing activity of monoclonal antibody 3H3 of the present invention obtained in Example 6;
Figs. 8~a) and 8(b) are yraphs showing the proliferation inhibition effect of monoclonal antibody 3~3 of the present invention obtained in Example 6 for HUVE
cells, in which Fig. 8(a) shows the results of cultivation for 3 days and Fig. 8(b) shows the results of cultivation for 5 days;
Fig. 9 is a graph showing the relationship between the concentration and the absorbance of hbFGF, obtained in Example '~;
Fig. 10(1) and 10~2) are graphs showins the influence of heparin in a hbFGF determination system, obtained in Example 10, in which Fig. 10(1) shows the results when MAbl2 is fixed, and Fig. 10(2) shows the results when a 50-50 mixture of MAb52 and MAb98 is fixed;
Fig. 11(1) and 11(2) are graphs showing the reaction in a hbFGF determination system, obtained in Example 11, in which Fig. 11(1) shows the results when MAbl2 is solidified, and Fig. 11(2) shows the results when a 50-50 mixture of MAbS2 and MAb98 is fixed;
Fig. 12 is a graph showing the anti-tumor effect of an antibody of the present invention, obtained in Example 13;
and Fig. 13 is a schematic representation showing the construction of plasmid p'rB1000 obtained in Reference Example 2.
~:
~ 6 -Detailed Descri~tion of the_Invention The bFGF proteins of the present invention include bFGFs and muteins in which at least one cysteine residue of bFGF is substituted for a serine residue and which have bFGF
activity.
As the bFGF proteins, there are preferably used polypeptides containing the amino acid sequence represented ~:
by formula (I):
Phe-Phe-Leu-Arg-Ile-~is-Pro-Asp-Gly-Arg-Val- `
lOAsp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro tI) The bFGFs of the present invention include bFGFs derived from mammals. The mammals include humans, monkeys, pigs, bovines, sheep and horses.
The bFGFs also include bFGFs extracted from various lS organs existence of which is already clarified, such as brains and pituitary glands.
The bFGF proteins may be produced by recombinant DNA
techniques.
Examples of amino acid sequences of the bFGFs include the amino acid sequence represented by formula tII):
Pro-Ala-Leu-Pro-Glu-Asp-Gly-Gly-Ser-Gly-Ala-Phe-Pro-Pro-Gly-His-Phe-Lys-Asp-Pro-Lys-Arg-Leu-Tyr-Cys-Lys-Asn-Gly-Gly-Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-25Val-Asp-Gly-Val-Arg-Glu Lys-Ser-Asp-Pro-His-Ile-Lys-Leu-Gln-Leu-Gln-Ala-Glu-Glu-Arg-Gly-Val-Val-Ser-Ile-Lys-Gly-Val-Cys-WO91/o9875 PCT/JP90/01726 ~ ;'``;~.7~
Ala-Asn-Arg-Tyr-Leu~Ala-Met-Lys-Glu-Asp-Gly-Arg-Leu-Leu-Ala-Ser-Lys-Cys-Val-Thr-Asp-Glu-Cys-Phe-Phe-Phe-Glu-Arg-Leu-Glu-Ser-Asn-Asn-Tyr-Asn-Thr-Tyr-Arg-Ser-Arg-Lys-Tyr-X -Ser-Trp-Tyr-Val-Ala-Leu-Lys-Arg-Thr-Gly-Gln-Tyr-Lys-Leu-Gly-Y Lys-Thr-Gly-Pro-Gly-~ln-Lys-Ala-Ile-Leu-Phe-Leu-Pro-Met-Ser-Ala-Lys-Ser (II) wherein X represents Thr or Ser, and Y represents Ser when X
is Thr, an~ Y represents Pro when X is Ser.
As the bFGF, human bFGF is preferable. The human bFGF
has the amino acid sequence in which X is Thr and Y is Ser in the above formula (II).
The muteins in which at least one cysteine residue of the above bFGF is substituted for a serine residue include, for example, the muteins described in Seno et al., BiophYs.
Res. Commun. 151, 701 (1988) and European Patent Publication No. 281,822.
In particular, there is preferably used recombinant human bFGF mutein CS23 (hereinafter also briefly referred to as rhbFGF mutein CS23) in which each of the cysteine residues at positions 70 and 88 of the human bFGF is substituted for a serine residue. With respect to the number of the positions of the above amino acids, in the amino acid sequence in which Met is added to the N-terminus of the peptide in which X is Thr and Y is Ser in the above formula ~II), the Met is numbered as the first.
~'`', ' :
~091/09M75 PCT/JP90/01726 ~ 8 --In thè bFGFs produced by the above-mentioned genetic engineering techniques, examples of the human bFGF include bFGF produced by the methods described, for example, in FEBS
Letters 213, 189 (1987), ~E~y___Res. Commun. 146, 470 (1987) and European Patent Publication No. 237,966.
When mammals are immunized with the bFGF proteins or protein conjugates, there are used experimental animals such as sheep, goat, rabbits, guinea pigs, rats and mice, as the mammals to be immunized. In order to obtain monoclonal antibodies, however, it is preferred to use rats or mice for immunization.
When mice are immunized, for example, they can be immunized by any of the subcutaneous, intraperitoneal, intravenous, intramuscular and intracutaneous routes.
However, subcutaneous, intraperitoneal and intravenous injections are preferably used. In particular, subcutaneous injection is preferable. The immunizing interval and the immunizing dose are widely variable, and various methods are available. For example, methods in which immunization is carried out about 2 to 6 times at intervals of 2 weeks and spleen cells are removed after about 1 to 5 days, preferably about 2 to 4 days from the final immunization are frequently used. As the immunizing dose, it is preferred to use about 0.1 ~g or more, preerably about 10 to 300 ~g of the peptide per one immunization of a mouse. Further, it is desirable to carry out the fusion process using the spleen cells after confirmation of an increase in antibody titer in blood by WOgltO9875 PCT/JP9~/~t726 jJ?
collecting a portion o~ blood and measuring the antibody titer before removal of the spleens.
The above spleen cells are then fused wlth lymphoid cells. For example, the spleen cells removed from the mice ~
5 are fused with lymphoid cell strains such as suitable ~ ;
myeloma cells [for example, P3-X-63-Ag-8UI ~Ichimori et al., J. Immun. Method 80, 55 ~1985))~ of the same kind or a different kind (preferably ~he same kind) having markers such as hypoxanthine-guanine-phosphoribosyl-transferase 10 deficient (HGPRT ) and thymidine kinase deficient (TK ).
For example, begin a new paragraph the fused cells are produced in accordance with the method of Kohler and Milstein [~ature 256, 495 (1975)1. For example, myeloma _ cells and spleen cells in a ratio of about 1:5 are suspended 15 in a medium prepared by mixing Iskov medium and Ham F-12 medium in a 1:1 ratio (hereinafter referred to as IH
medium), and a fusion accelerator such as Sendai virus or polyethylene glycol (PEG) is added thereto. It is of course possible to add other fusion accelerators such as dimethyl 20 sulfoxide (DMSO). The polymerization degree of PEG is ?
usually about 1,000 to 6,000, the fusion time is about 0.5 to 30 minutes, and the concentration of the suspension is about 10 to 80%. As a preerred condition, the fusion is carried out efficiently by using PEG 6,000 in a concentration of about 35 to 55% for about 4 to 10 minutes.
The fused cells can be selectively proliferated using hypoxanthine-aminopterin-thymidine medium ~HAT medium) ~ ' ' WO 91/09875 PCr/JP90/01726 ,~ f --[Nature, 256, 4~5 (1975) ].
_ _ The culture supernatant of the proliferated cells is then screened for the production of the desired antibody.
Screening of the antibody titer can be carried out in the following manner. First, the presence or absence of the antibody production by peptide immunization is examined by radio immunoassays (RIAs) or enzyme immunoassays (EIAs).
For these methods, various modified me~hods are also available.
As a preferred example of the assays, a method using the EIA is described below. A rabbit anti-mouse immunoglobulin antibody is coupled with a carrier such as cellulose beads according to conventional methods, and then a culture supernatant or mouse serum to be assayed is added thereto, followed by reaction at a constant temperature (about 4 to 40C, the same applied hereinafter) for a definite time. After the reaction product is thoroughly washed, an enzyme-labeled peptide (a peptide is coupled with an enzyme according to conventional methods, followed by purification) is added thereto, followed by reaction at a constant temperature for a specified time. After the reaction product is thoroughly washed, an enzyme substrate is added thereto, followed by reaction at a constant temperature for a speciied time. Then, the absorbance or fluorescence of the color-produced product is measured.
As to the culture supernatant of the proliferated cells, the screening of the neutralizing activity to the ,. .
. ~:
wogl/0987~ 7~ PCT/JP9OtO1726 bFGF proteins can be carried out in the following manner.
In this case, the neutralizing activity can be examined using cells whcse proliferation is induced by the bFGF
proteins. As such cells, there can be used vascular endothelial cells, fibroblasts, nerve cells and the like.
It is however desirable to know whether or not the additional effect of the bFGF proteins is inhibited by ; measuring the number of cells, using the vascular endothelial cells begin a new paragraph.
Methods for measuring the number of cells include a method for measuring directly the number of cells, a method or determining radioactivity by using tritium thymidine and a method for measuring colorimetrically using (4,5-dimethyl-; 2-thiazoly)-2,5-diphenyl-2H-tetrazolium bromide (MTT) (MTT
method). As one example of the preferred assays, there is ; hereinafter described a method for assaying cell proliferation by the MTT method using human umbilical vein-derived endothelial cells. After the cells are seeded, the bFGF protein and the culture supernatant to be assayed are added thereto, followed by cultivation at a constant temperature (37C) at a low concentration of oxygen ~about
7% is preferable) for a definite time. Then, the culture solution are replaced by a medium containing MTT, and cultivation is further continued, whereby MTT is reduced to a formazan, a colorimetric material, in intracellular endogenous mitochondria.
After a specified time has elapsed, SDS is added ~ 12 -thereto to dissolve the cellsl and the concentration of the formazan is made even, the absorbance at 590 nm is measured.
The proliferative property of cells correlates with the absorbance. Hence, if the solution containing the hybridoma supernatant is decreased in absorbance compared with a solution not containing the hybridoma supernatant, the antibody contained in the supernatant can be said to have bFGF neutralizing activity.
It is desirable that the cells in wells which proliferate in a selective medium and which produce antibodies with immuno-neutralizing activity to the peptide used for immunization be cloned by a limiting dilution analysis. The supernatant of the cloned cells is similarly screened, and the selected cells which show a high antibody titer are proliferated, whereby monoclonal antibody-producing hybridoma clones showing the reactivity with the immunized peptide can be obtained.
The hybridoma cells thus cloned are proliferated in a liquid medium. Specifically, for example, the hybridoma ce}ls are cultivated in the liquid medium such as a medium prepared by adding about 0.1-40% bovine serum to RPMI-1640 [G. E. Moore et al., J. Am. Med. Assoc. 199, 549 ~1967)], for about 2 to 10 days, preferably for 3 to 5 days, whereby the monoclonal antibody can be obtained from the culture solution. The antibody can further be obtained by intraperitoneally inoculating mammals with the hybridoma cells, thereby proliferating the cells and then collecting :
WO91t09875 PCT/JP90/01726 - 13 - ,~r,~h~ ~
the ascites. In the case o a mouse, for example, about l X
104 to l X 107, preferably 5 X 105 to 2 X 106 of the hybridoma cells are intraperitoneally inoculated into a mouse such as BALB/c preliminarily inoculated with mineral oil and the like, and the ascites is collected after about 7 to 20 days, preferably after about lO to 14 days. The monoclonal antibody formed and accumulated in the ascites can be easily isolated as pure immunoglobulin by ammonium sulfate fractionation, DEAE-cellulose column chromatography or the like.
The monoclonal antibodies of ~he present invention have high binding sensitivity not only with the immunogen peptides, but also with the bFGF proteins, and further exhibit the neutralizing activity to the bFGF proteins.
As a result of this high binding sensitivity, the monoclonal antibodies of the present invention are very useful as reagents for assaying the bFGF proteins and for purifying the bFGF proteins. ;
The bFGF proteins can be assayed to 20 pg/ml by the 20 assays using the monoc}onal antibodies of the present !~
invention. The ability to assay such an extremely small amount of bFGF in vivo is an important development in the art. As diseases induced by overproduction of bFGF, tumors are mentioned. For the tumors, there are the case that cancer cells proliferate directly by bFGF and the case that vascular endothelial cells react with bFGF produced from the ;~
tumors to proliferate and induce n-w formed blood vessels " ~:
~: .
w ~ n9B75 Pcr which supply nutritive substances to the tumors, which results in enlarged tumor masses. In these cases, these diseases can be anticipated by measuring the amount of the bFGF overproduced. Since bFGF easily adheres to the inner walls of blood vessels, it is therefore important to have a detecting or determining assay method as sensitive as possible.
Also in treating traumas and burns~ bFGF is considered to improve the symptoms thereof effectively. In this case, it is more effective to use a mutein in which at least one cysteine residue of the bFGF is substituted for a serine residue and which is higher in stability than the bFGF.
When the mutein is used as a therapeutic drug, the monoclonal antibodies of the present invention can be used as means for tracing the amount of the mutein in vivo, because the monoclonal antibodies also have high binding sensitivity with the mutein in which at least one cysteine residue is substituted for a serine residue.
As described above, many tumors are considered to be proliferated by bFGF in bodies. The monoclonal antibodies of the present invention inactivate the bFGF in vivo and exhibit antitumor activity, because of their strong immuno-neutralizing activity. }n this case, the monoclonal antibodies are administered in an amount of about 100 ~g/kg to 10 mg/kg. These monoclonal antibodies are also effective for treatment of enlarged tumors following angiogenesis.
Examples of the methads for detecting or assaying the ., . , . . . .
, -,. , ~ :
. . - . :
WOgl/0987~ P~T/JP90/01726 ~ ; J'-~J 7 ~
bFGF proteins include an immunoassay for assaying the bFGF
proteins by using an anti-bFGF antibody supported on a carrier and a conjugate ob~ained by combining an anti-bFGF
antibody directly with a labeling agent, the anti-bFGF
antibody differing from the antibody held on the carrier in an antigen determinant.
The carriers on which the antibody is held in the above-mentioned assay include, for example, gel particles such as agarose gels [for example, Sepharose 4B and`
Sepharose 6B (Pharmacia Fine Chemical, Sweden)~, dextran gels [for example, Sephadex G-75, Sephadex G-lO0 and Sephadex G-200 (Pharmacia Fine Chemical, Sweden)] and polyacrylamide gels [for example, Biogel P-30, Biogel P-60 and Biogel P-lO0 (Bio RAD Laboratories, U.S.A.)~; cellulose particles such as Avicel tAsahi Chemical Industry, Japan) and ion exchange cellulose (for example, diethylaminoethyl : cellulose and carboxymethyl cellulose); physical adsorbents such as glass (for example, glass balls, glass rods, aminoalkyl glass balls and aminoalkyl glass rods), silicone pieces, styrenic resins (for example, polystyrene balls and polystyrene particles) and plates for immunoassay ~for example, Nunc, Denmark); and ion exchange resins such as weakly acidic cation exchange resins lfor example, Amberlite IRC- 50 ~Rohm & Haas, U.S.A.) and Zeocurve 226 ~Permutit, West ~ermany)], and weakly basic anion exchange resins [for example, Amberlite IR-4B and Dowex (Dow Chemical, U.S.A.)].
In order to couple the antibody onto the carrier, , ~ `'`
WO91/09875 PcT/Jp9o/o172s ~ t~ ? ~ 16 - -methods k~own in th~ art are applied. Examples of such methods include the cyanogen bromide method and the glutaraldehyde method which are described in Metabolism, 8, 696 (1971). As a simpler method, the antibody may be physically adsorbed on the surface of the carrier.
The labeling agents with which the antibodies are combined include radioisotopes, enzymes, fluorescent substances and luminous substances. However, it is preferred to use the enzymes. As the enzymes, which are preferably stable and high in specific activity, there can be used peroxidases, alkaline phosphatases, ~-D-galactosidases, glucose oxidases and the like. In particular, peroxidases is preferably used. Peroxidases of various origins can be used. Examples of such peroxidases include peroxidases obtained from horseradishes, pineapples, figs, sweet potatoes, broad beans and cone. In particular, horseradish peroxidase (HRP) extracted from horseradishes is preferable.
In combining peroxidase with the antibody, the thiol group of Fab~ as the antibody molecule is utilized, and peroxidase into which a maleimide group is preliminarily introduced is conveniently used.
When a maleimide group is introduced into peroxidase, it can be introduced through an amino group of peroxidase.
For this purpose, N-succinimidyl-maleimide-carboxylate derivatives can be used. N-~y-maleimidobutyloXy)succinimide ~hereinafter also briefly referred to as GMBS) is preferably ' . r , ` . . ' . ' .. :., .. .. 1~ . ; ': ' ` . ' ~ . , ' ~ . ' . '.. ' ' . .. ' ' WO91J09X75 PCT/JP90/~17~6 - 17 ~ t'~ ~`, - ?
used. A certain group may therefore intervene between the maleimide group and perxidase.
G~BS is reacted with peroxidase in a buffer solution having a pH of 6 to 8 at about 10 to 50C for about 10 minutes to about 24 hours. The buffer solutions include, for example, 0.1 M phosphate buffer (pH 7.0). The maleimidated peroxidase thus obtained can be purified, for example, by gel chromatography. Examples of carriers used in the gel chromatography include Sephadex G-25 (Pharmacia Fine Chemical, Sweden) and Biogel P-2 (Bio RAD Laboratories, U.5.A.).
The maleimidated peroxidase can be reacted with the antibody molecule in a buffer solution at about 0 to 40C
for about 1 to 48 hours. The buffer solutions include, for `;
example, 0.1 M phosphate buffer (p~ 6.0) containing 5 mM
sodium ethylenediaminetetraacetate. The peroxidase labeled antibody thus obtained can be purified, for example, by gel chromatography. Examples of carriers used in the gel chromatography include Sephadex G-25 ~Pharmacia Fine Chemical, Sweden) and Biogel P-2 (Bio RAD Laboratories, U.S.A.).
A thiol group may be introduced into peroxidase to ~;
allow it to react with the maleimidated antibody molecule.
Enzymes other than peroxidases can be directly combined ;~
with the antibodies similarly to the methods of combining peroxidases, and known methods which achieve such combining include body fluids or, for example, the glutaraldehyde :
``~. , ,~, , "' ' ,- "., ~ ' . ',, , " ", !~
` ~ ~.' ': . ; ' ' ' . . , . : '' ,' ' ' ., . ' , ' ' ' ' . "``' . ' WO91/0~87~ PCT/JP90/~1726 ~ 18 -method, the periodic acid method and the water-soluble carbodiimide method.
Test samples used in the assay system of the present invention include humors such as urine, serum, plasma and cerebrospinal fluid, extracts of animal cells, and culture supernatants thereof.
As an example of the assays of the present invention, a case is hereinafter described in detail in which peroxidase is used as the labeling agent, but the present invention is not limited to peroxidase.
(1) First, a test sample containing the bFGF protein to be assayed is added to the antibody held on a carrier to conduct antigen-antibody reaction, and then the conjugate of the peroxidase with the anti-bFGF protein antibody obtained above is added thereto, followed by reaction.
(2) The substrate of the peroxidase is added to the reaction product obtained in (l), and then the absorbance or the fluorescent intensity of the resulting substance is measured, thereby knowing the enzyme activity of the above reaction product.
(3) The procedures described in ~l) and t2) are preliminarily carried out for the standard solution of the bFGF protein of a known amount to prepare a standard curve showing the relation between the amount of the bFGF protein and the absorbance or the fluorescent intensity thereof.
t4) The absorbance or the fluorescent intensity obtained for the test sample containing the bFGF protein of WO~1/098~ PCT/JP90/Ot726 - 19 - P~ r~ 7,~ ~.
an unknown amount is applied to the standard curve to determine the amount of the bFGF protein in the test sample.
In order to purify the bFGF protein, the purified antibody of the present invention is coupled with a suitable ~-~
carrier such as activated agarose gel beads according to conventional methods, and packed in a column. Then, a sample containing the crude bFGF protein, such as a culture supernatant or disrupted cells, is loaded onto the antibody affinity column to allow the sample to be adsorbed thereby, followed by washing. Then, elution is carried out with a chaotropic reagent such as potassium thiocyanate ~KSCN) or under such acescent conditions that the bFGF is not inactivated. Thus, the bFGF protein can be efficiently ~ ;
purified.
The antibody column can be prepared by coupling the monoclonal antibody of the present invention, which is, for ``
example, purified from ascites or other humors inoculated `~
with the hybridoma cells, with an appropriate carrier.
Any carrier may be used as long as the bFGF protein is 20 specifically efficiently adsorbed thereby after coupling and ~`
suitable elution is thereafter possible. Examples of such carriers include agarose gels, cellulose and acrylamide polymers. By way of example, polyacrylamide gel beads in which primary amines of the proteins are activated so as to be easily combinable, such as Af~i-Gel 10 ~Bio RAD), are conveniently used according to the following method. The antibody is reacted with Affi-Gel 10 in a buffer solution .. , : . ,- ,~ ,:: ::. :.. . ., , . , . . . . , : . , w09l~0987s PCT/JP90/~1726 such as a bicarbonate solution having a concentration of about 0.001 to l M, preferably about 0.1 M. The r~action is conducted at about 0 to 20C at a broad p~ range for about 10 minutes to about 24 hours, preferably at about 4C at a pH of about 3 to lO for about 4 hours. With respect to the mixing ratio of the antibody to Affi-Gel lO, the larger amount of antibody is mixed with Affi-Gel 10, the larger amount of antibody becomes combined therewith, within the range up to about 50 mg of antibody per 1 ml of Affi-Gel 10.
The antibody may ~herefore be mixed with Affi-Gel lO in any ratio within this range. However, about lO to 30 mg of the antibody is conveniently used, considering the combining efficiency and the purification efficiency in affinity chromatography. The antibody-carrier combined material thus formed is thoroughly washed with the buffer solution used for the reaction. Then, residual unreacted active groups are blocked by allowing the washed material to stand for several days, by adding a compound containing a primary amine such as ethanolamine-hydrochloric acid or glycine ~ thereto to a final concentration of about 0.05 to 0.10 M, followed by reaction at about 4C for about 1 to 4 hours, or by reacting a protein such as 1 to 5% bovine serum albumin ~SA) therewith at 4C overnight. ~he combined material thus treated is packed in an appropriate column to form the antibody column.
In purifying a sample with the above antibody column, the bFGF protein-containing sample is dissolved in a buffer WO91/09875 PCT/JP90/~1726 7~?
solution having a pH around neutrality such as phosphate buffer or Tris-hydrochloric acid buffer, followed by adsorption by the antibody column. Then, the column is washed with the same buf~er, and then the bFGF protein is S eluted. As eluents, the following solutions are commonly used: weakly acidic solutions such as acetic acid solutions, solutions containing polyethylene glycol, solutions containing peptides more easily combinable with the antibody than the sample, high concentration salt solutions and their ~;
combined solutions. Solutions which do not so promote the degradation of the bFGF protein are preferred.
Eluents are neutralized with buffer solutions by conventional methods. The above purification procedure can be repeated again as needed.
15Thus, the substantially pure bFGF protein substantially free from pyrogens and endotoxins can be obtained. The substantially pure bFGF protein of the present invention contains the bPGF protein in a concentration of 90% tw/w) or more, and preferably in a concentration of 95~ (w/w) or more.
The monoclonal antibodies of the present invention immuno-neutralize the biological activity of ~he bFGF
proteins at low concentrations and have high binding sensitivity with the bFGF proteins, so that they can be used as therapeutic drugs for treatment of diseases such as cancer, and as reagents for assaying the bFGF proteins.
Mouse 3H3 cells obtained in Example 2-~4) described .: .- .... . :: , - : : : . : , .. . - . - -, : . - . . .: ,.... . .. . .
,;,;,: : ' ~ ' : : :: : . : . : , '. ' ' :: : .:: .:: : : : . : , :: : ' : : . ., :: . : . :: :, : , , :,: . .
wosl/~98~5 PCT/JP9~/01726 ~ r~
below was deposited with the Institute for Fermentation, Osaka, Japan tIFO) under the accession number IFO 50216 on November 10, 1989. The above cells were also deposited with the Fermentation Research Institute, Agency of Industrial Science and Technology, Ministry of International Trade and Industry, Japan (FRI) under the accession number FERM BP-2658 on November 14, 1989.
Anti-bFGF monoclonal antibodies MAbl2, MAb52 and MAb98 described in the following Examples can be produced by the methods described in Hybridoma, 8, 209-221 (1989) and European Patent Publication No. 288,687 the disclosures of which are herein incorporated by reference. The recognition site of MAbl2 is included in the amino acid sequence of ~rom position 1 ~the N-terminus) to position 9 of bFGF, and the recognition sites of MAbS2 and MAb98 are included in the amino acid sequence of from position 14 to position 4~ of bFGF. Recombinant human aFGF which was produced by the methods described in Reference Example 1 was used.
Recombinant human bFGF (rhbFGF) which was produced by the methods described in Iwane et al., Biophys. Biochem.
~ Res. Commun. 146, 470 ~1987) and European Patent Publication ; No. 237,966 was used.
rhbFGF mutein CS23 which was produced using transformant Escherichia coli MM294/pT~762 (IFO 14613, FERM
BP-1645) by the methods described in Sano et al., BioPhys.
Biochem. Res. Commun. 151, 701 (1988) and European Patent Publication No. 281,822 was used. The above E. coli wosl/09~7s PC~/JP90~01726 MM294/pTB762 was deposited with IFO under the accession number IF0 14613 on May 27, 1987. This transformant was also deposited with FRI under the accession number FERM
P-9409 on June 11, 1987. This deposit was converted to the deposit under the ~udapest Treaty and the transformant is stored at the YRI under the accession number FERM BP-1645.
Escherichia coli MM294(DE3)/LysS,pTB762 which is . produced in Reference Example 1 was deposited with IF0 under the accession number IF0 14936 on September 12, 1989. This transformant was also deposited with FRI under the accession number FERM BP-2599 on September 20, 1989.
The following examples are given to illustrate embodiments of the present invention as it is presently preferred to practice. It will be understood that the examples are illustrative, and that the invention is not to be considered as restricted except as indicated in the appended claims.
Examples Reference Example 1 (Preparation of Recombinant Human aFGF) Human aFGF was produced by the ~ollowing method, with reference to the methods described in BiotechnoloqY, 5, 960 ~1987) and ICU5 Short Report, vol. 8, Advances in Gene Technology; Protein ~ngineering and Production, Proceedings of the 1988 Miami Bio/Technology Winter Symposium, page 11~, IRL Press.
(a) Construction o~ Expression Plasmid Plasmid pTB917 obtained by incorporating chemically .
~, , ...... . . . .
WO9l/~9875 . pCT/JPgo/01726 ~ 24 -synthesized human aFGF DNA (Fig. 1) into pUC18 [Methods in Enzymoloqy 101, 20-78 (1983)] was digested with BspMI, and the cleaved sites were changed to flush ends by reaction with DNA polymerase large ~ragment, followed by digestion with BamHI to produce a 0.45-kb DNA fragment.
As a vector DNA, there was used pET3c [F. W. Studier et al., J. Mol. Biol., 189, 113-130 (1986)] carrying a ~10 promoter for a T7 phage. pET3c was cleaved with NdeI and the termini thereof were made flush by treatment with large fragment. Then, an NcoI linker, 5'-CCATGG-3', was ligated thereto with T4 DNA ligase. The resulting plasmid was cleaved with NcoI, and the cleaved ites were made flush with DNA polymerase large fragments, followed by cleavage with Bam~I to remove the sequence of S10. Then, the above 0.45-kb blunt BspMI-BamHI fragment was incorporated thereinto with T4 DNA ligase to obtain pTB975 (Fig. 2).
~b) Expression of Human aFGF cDNA in E. coli ~Phage DE3 ~F. W. Studier et al., J. Mol. Biol. 189, 113-130 (1986)~ in which an RNA polymerase gene of the T7 phage was incorporated into E. coli strain MM294 was lysogenized, and plasmid pLysS [F. W. Studier et al., J.
Mol. Biol. 189, 113-130 ~1986)1 having a lysozyme gene of the T7 phage was further introduced thereinto to prepare E.
coli MM294~DE3)/pLysS. This strain was transformed with pTB975 to give E. coli MM294(DE3)/pLysS, pTB975~IFO 14936, FERM BP-2599).
This strain was cultivated in a medium containing 35 WO9l/~9875 PCT/3P9~/Ot726 - 25 ~
~g/ml of ampicillin and 10 ~g/ml oE chloramphenicol. When the turbidity reached 170 Kletts, isopropyl-~-D-thiogalactoside (IPTG) was added thereto to a final concentration of 0.5 mM, and cultivation was further continued for 3 hours. The cells were collected by centrifugation and washed with ice-cooled PBS. Then, the cells were collected again and stored at -20C until their `
use.
(c) Purification of Human aFGF
The cells collected from a one liter culture were suspended in 100 ml of an ice-cooled solution [10 mM
Tris-HCl tpH 7.4), 10 mM EDTA, 0.6 M NaCl, 10% sucrose, 0.25 mM PMSF], and egg white lysozyme was added thereto to a concentration of 0.5 mg/ml. The mixture was allowed to~
stand in ice for 1 hour, followed by incubation at 37C for 5 minutes. Then, the product was subjected to ultrasonication twice under ice cooling for 20 seconds, and then centrifuged at 18 Krpm at 4C for 30 minutes ~Sorvall) to obtain a supernatant. This supernatant was mixed with 200 ml of an ice-cooled solution [20 mM Tris-HCl ~pH 7.4), 1 mM EDTAI~ and the mixture was loaded onto a heparin Sepharose column (2.5 cm diameter X 4 cm) equilibrated with a buffer 120 mM Tris-HCl (pH 7.4), 1 mM EDTA]. The column was washed with 150 ml ~f a solution ~20 mM Tris-HCl (pH
7.4), 1 mM EDTA, 1.5 M NaCl], and then the protein was eluted with an eluting solution ~20 mM Tris-HCl (pH7.4~, 1 mM EDTA, 1.5 M NaCl]. The eluate was fractionated into 6 ml
After a specified time has elapsed, SDS is added ~ 12 -thereto to dissolve the cellsl and the concentration of the formazan is made even, the absorbance at 590 nm is measured.
The proliferative property of cells correlates with the absorbance. Hence, if the solution containing the hybridoma supernatant is decreased in absorbance compared with a solution not containing the hybridoma supernatant, the antibody contained in the supernatant can be said to have bFGF neutralizing activity.
It is desirable that the cells in wells which proliferate in a selective medium and which produce antibodies with immuno-neutralizing activity to the peptide used for immunization be cloned by a limiting dilution analysis. The supernatant of the cloned cells is similarly screened, and the selected cells which show a high antibody titer are proliferated, whereby monoclonal antibody-producing hybridoma clones showing the reactivity with the immunized peptide can be obtained.
The hybridoma cells thus cloned are proliferated in a liquid medium. Specifically, for example, the hybridoma ce}ls are cultivated in the liquid medium such as a medium prepared by adding about 0.1-40% bovine serum to RPMI-1640 [G. E. Moore et al., J. Am. Med. Assoc. 199, 549 ~1967)], for about 2 to 10 days, preferably for 3 to 5 days, whereby the monoclonal antibody can be obtained from the culture solution. The antibody can further be obtained by intraperitoneally inoculating mammals with the hybridoma cells, thereby proliferating the cells and then collecting :
WO91t09875 PCT/JP90/01726 - 13 - ,~r,~h~ ~
the ascites. In the case o a mouse, for example, about l X
104 to l X 107, preferably 5 X 105 to 2 X 106 of the hybridoma cells are intraperitoneally inoculated into a mouse such as BALB/c preliminarily inoculated with mineral oil and the like, and the ascites is collected after about 7 to 20 days, preferably after about lO to 14 days. The monoclonal antibody formed and accumulated in the ascites can be easily isolated as pure immunoglobulin by ammonium sulfate fractionation, DEAE-cellulose column chromatography or the like.
The monoclonal antibodies of ~he present invention have high binding sensitivity not only with the immunogen peptides, but also with the bFGF proteins, and further exhibit the neutralizing activity to the bFGF proteins.
As a result of this high binding sensitivity, the monoclonal antibodies of the present invention are very useful as reagents for assaying the bFGF proteins and for purifying the bFGF proteins. ;
The bFGF proteins can be assayed to 20 pg/ml by the 20 assays using the monoc}onal antibodies of the present !~
invention. The ability to assay such an extremely small amount of bFGF in vivo is an important development in the art. As diseases induced by overproduction of bFGF, tumors are mentioned. For the tumors, there are the case that cancer cells proliferate directly by bFGF and the case that vascular endothelial cells react with bFGF produced from the ;~
tumors to proliferate and induce n-w formed blood vessels " ~:
~: .
w ~ n9B75 Pcr which supply nutritive substances to the tumors, which results in enlarged tumor masses. In these cases, these diseases can be anticipated by measuring the amount of the bFGF overproduced. Since bFGF easily adheres to the inner walls of blood vessels, it is therefore important to have a detecting or determining assay method as sensitive as possible.
Also in treating traumas and burns~ bFGF is considered to improve the symptoms thereof effectively. In this case, it is more effective to use a mutein in which at least one cysteine residue of the bFGF is substituted for a serine residue and which is higher in stability than the bFGF.
When the mutein is used as a therapeutic drug, the monoclonal antibodies of the present invention can be used as means for tracing the amount of the mutein in vivo, because the monoclonal antibodies also have high binding sensitivity with the mutein in which at least one cysteine residue is substituted for a serine residue.
As described above, many tumors are considered to be proliferated by bFGF in bodies. The monoclonal antibodies of the present invention inactivate the bFGF in vivo and exhibit antitumor activity, because of their strong immuno-neutralizing activity. }n this case, the monoclonal antibodies are administered in an amount of about 100 ~g/kg to 10 mg/kg. These monoclonal antibodies are also effective for treatment of enlarged tumors following angiogenesis.
Examples of the methads for detecting or assaying the ., . , . . . .
, -,. , ~ :
. . - . :
WOgl/0987~ P~T/JP90/01726 ~ ; J'-~J 7 ~
bFGF proteins include an immunoassay for assaying the bFGF
proteins by using an anti-bFGF antibody supported on a carrier and a conjugate ob~ained by combining an anti-bFGF
antibody directly with a labeling agent, the anti-bFGF
antibody differing from the antibody held on the carrier in an antigen determinant.
The carriers on which the antibody is held in the above-mentioned assay include, for example, gel particles such as agarose gels [for example, Sepharose 4B and`
Sepharose 6B (Pharmacia Fine Chemical, Sweden)~, dextran gels [for example, Sephadex G-75, Sephadex G-lO0 and Sephadex G-200 (Pharmacia Fine Chemical, Sweden)] and polyacrylamide gels [for example, Biogel P-30, Biogel P-60 and Biogel P-lO0 (Bio RAD Laboratories, U.S.A.)~; cellulose particles such as Avicel tAsahi Chemical Industry, Japan) and ion exchange cellulose (for example, diethylaminoethyl : cellulose and carboxymethyl cellulose); physical adsorbents such as glass (for example, glass balls, glass rods, aminoalkyl glass balls and aminoalkyl glass rods), silicone pieces, styrenic resins (for example, polystyrene balls and polystyrene particles) and plates for immunoassay ~for example, Nunc, Denmark); and ion exchange resins such as weakly acidic cation exchange resins lfor example, Amberlite IRC- 50 ~Rohm & Haas, U.S.A.) and Zeocurve 226 ~Permutit, West ~ermany)], and weakly basic anion exchange resins [for example, Amberlite IR-4B and Dowex (Dow Chemical, U.S.A.)].
In order to couple the antibody onto the carrier, , ~ `'`
WO91/09875 PcT/Jp9o/o172s ~ t~ ? ~ 16 - -methods k~own in th~ art are applied. Examples of such methods include the cyanogen bromide method and the glutaraldehyde method which are described in Metabolism, 8, 696 (1971). As a simpler method, the antibody may be physically adsorbed on the surface of the carrier.
The labeling agents with which the antibodies are combined include radioisotopes, enzymes, fluorescent substances and luminous substances. However, it is preferred to use the enzymes. As the enzymes, which are preferably stable and high in specific activity, there can be used peroxidases, alkaline phosphatases, ~-D-galactosidases, glucose oxidases and the like. In particular, peroxidases is preferably used. Peroxidases of various origins can be used. Examples of such peroxidases include peroxidases obtained from horseradishes, pineapples, figs, sweet potatoes, broad beans and cone. In particular, horseradish peroxidase (HRP) extracted from horseradishes is preferable.
In combining peroxidase with the antibody, the thiol group of Fab~ as the antibody molecule is utilized, and peroxidase into which a maleimide group is preliminarily introduced is conveniently used.
When a maleimide group is introduced into peroxidase, it can be introduced through an amino group of peroxidase.
For this purpose, N-succinimidyl-maleimide-carboxylate derivatives can be used. N-~y-maleimidobutyloXy)succinimide ~hereinafter also briefly referred to as GMBS) is preferably ' . r , ` . . ' . ' .. :., .. .. 1~ . ; ': ' ` . ' ~ . , ' ~ . ' . '.. ' ' . .. ' ' WO91J09X75 PCT/JP90/~17~6 - 17 ~ t'~ ~`, - ?
used. A certain group may therefore intervene between the maleimide group and perxidase.
G~BS is reacted with peroxidase in a buffer solution having a pH of 6 to 8 at about 10 to 50C for about 10 minutes to about 24 hours. The buffer solutions include, for example, 0.1 M phosphate buffer (pH 7.0). The maleimidated peroxidase thus obtained can be purified, for example, by gel chromatography. Examples of carriers used in the gel chromatography include Sephadex G-25 (Pharmacia Fine Chemical, Sweden) and Biogel P-2 (Bio RAD Laboratories, U.5.A.).
The maleimidated peroxidase can be reacted with the antibody molecule in a buffer solution at about 0 to 40C
for about 1 to 48 hours. The buffer solutions include, for `;
example, 0.1 M phosphate buffer (p~ 6.0) containing 5 mM
sodium ethylenediaminetetraacetate. The peroxidase labeled antibody thus obtained can be purified, for example, by gel chromatography. Examples of carriers used in the gel chromatography include Sephadex G-25 ~Pharmacia Fine Chemical, Sweden) and Biogel P-2 (Bio RAD Laboratories, U.S.A.).
A thiol group may be introduced into peroxidase to ~;
allow it to react with the maleimidated antibody molecule.
Enzymes other than peroxidases can be directly combined ;~
with the antibodies similarly to the methods of combining peroxidases, and known methods which achieve such combining include body fluids or, for example, the glutaraldehyde :
``~. , ,~, , "' ' ,- "., ~ ' . ',, , " ", !~
` ~ ~.' ': . ; ' ' ' . . , . : '' ,' ' ' ., . ' , ' ' ' ' . "``' . ' WO91/0~87~ PCT/JP90/~1726 ~ 18 -method, the periodic acid method and the water-soluble carbodiimide method.
Test samples used in the assay system of the present invention include humors such as urine, serum, plasma and cerebrospinal fluid, extracts of animal cells, and culture supernatants thereof.
As an example of the assays of the present invention, a case is hereinafter described in detail in which peroxidase is used as the labeling agent, but the present invention is not limited to peroxidase.
(1) First, a test sample containing the bFGF protein to be assayed is added to the antibody held on a carrier to conduct antigen-antibody reaction, and then the conjugate of the peroxidase with the anti-bFGF protein antibody obtained above is added thereto, followed by reaction.
(2) The substrate of the peroxidase is added to the reaction product obtained in (l), and then the absorbance or the fluorescent intensity of the resulting substance is measured, thereby knowing the enzyme activity of the above reaction product.
(3) The procedures described in ~l) and t2) are preliminarily carried out for the standard solution of the bFGF protein of a known amount to prepare a standard curve showing the relation between the amount of the bFGF protein and the absorbance or the fluorescent intensity thereof.
t4) The absorbance or the fluorescent intensity obtained for the test sample containing the bFGF protein of WO~1/098~ PCT/JP90/Ot726 - 19 - P~ r~ 7,~ ~.
an unknown amount is applied to the standard curve to determine the amount of the bFGF protein in the test sample.
In order to purify the bFGF protein, the purified antibody of the present invention is coupled with a suitable ~-~
carrier such as activated agarose gel beads according to conventional methods, and packed in a column. Then, a sample containing the crude bFGF protein, such as a culture supernatant or disrupted cells, is loaded onto the antibody affinity column to allow the sample to be adsorbed thereby, followed by washing. Then, elution is carried out with a chaotropic reagent such as potassium thiocyanate ~KSCN) or under such acescent conditions that the bFGF is not inactivated. Thus, the bFGF protein can be efficiently ~ ;
purified.
The antibody column can be prepared by coupling the monoclonal antibody of the present invention, which is, for ``
example, purified from ascites or other humors inoculated `~
with the hybridoma cells, with an appropriate carrier.
Any carrier may be used as long as the bFGF protein is 20 specifically efficiently adsorbed thereby after coupling and ~`
suitable elution is thereafter possible. Examples of such carriers include agarose gels, cellulose and acrylamide polymers. By way of example, polyacrylamide gel beads in which primary amines of the proteins are activated so as to be easily combinable, such as Af~i-Gel 10 ~Bio RAD), are conveniently used according to the following method. The antibody is reacted with Affi-Gel 10 in a buffer solution .. , : . ,- ,~ ,:: ::. :.. . ., , . , . . . . , : . , w09l~0987s PCT/JP90/~1726 such as a bicarbonate solution having a concentration of about 0.001 to l M, preferably about 0.1 M. The r~action is conducted at about 0 to 20C at a broad p~ range for about 10 minutes to about 24 hours, preferably at about 4C at a pH of about 3 to lO for about 4 hours. With respect to the mixing ratio of the antibody to Affi-Gel lO, the larger amount of antibody is mixed with Affi-Gel 10, the larger amount of antibody becomes combined therewith, within the range up to about 50 mg of antibody per 1 ml of Affi-Gel 10.
The antibody may ~herefore be mixed with Affi-Gel lO in any ratio within this range. However, about lO to 30 mg of the antibody is conveniently used, considering the combining efficiency and the purification efficiency in affinity chromatography. The antibody-carrier combined material thus formed is thoroughly washed with the buffer solution used for the reaction. Then, residual unreacted active groups are blocked by allowing the washed material to stand for several days, by adding a compound containing a primary amine such as ethanolamine-hydrochloric acid or glycine ~ thereto to a final concentration of about 0.05 to 0.10 M, followed by reaction at about 4C for about 1 to 4 hours, or by reacting a protein such as 1 to 5% bovine serum albumin ~SA) therewith at 4C overnight. ~he combined material thus treated is packed in an appropriate column to form the antibody column.
In purifying a sample with the above antibody column, the bFGF protein-containing sample is dissolved in a buffer WO91/09875 PCT/JP90/~1726 7~?
solution having a pH around neutrality such as phosphate buffer or Tris-hydrochloric acid buffer, followed by adsorption by the antibody column. Then, the column is washed with the same buf~er, and then the bFGF protein is S eluted. As eluents, the following solutions are commonly used: weakly acidic solutions such as acetic acid solutions, solutions containing polyethylene glycol, solutions containing peptides more easily combinable with the antibody than the sample, high concentration salt solutions and their ~;
combined solutions. Solutions which do not so promote the degradation of the bFGF protein are preferred.
Eluents are neutralized with buffer solutions by conventional methods. The above purification procedure can be repeated again as needed.
15Thus, the substantially pure bFGF protein substantially free from pyrogens and endotoxins can be obtained. The substantially pure bFGF protein of the present invention contains the bPGF protein in a concentration of 90% tw/w) or more, and preferably in a concentration of 95~ (w/w) or more.
The monoclonal antibodies of the present invention immuno-neutralize the biological activity of ~he bFGF
proteins at low concentrations and have high binding sensitivity with the bFGF proteins, so that they can be used as therapeutic drugs for treatment of diseases such as cancer, and as reagents for assaying the bFGF proteins.
Mouse 3H3 cells obtained in Example 2-~4) described .: .- .... . :: , - : : : . : , .. . - . - -, : . - . . .: ,.... . .. . .
,;,;,: : ' ~ ' : : :: : . : . : , '. ' ' :: : .:: .:: : : : . : , :: : ' : : . ., :: . : . :: :, : , , :,: . .
wosl/~98~5 PCT/JP9~/01726 ~ r~
below was deposited with the Institute for Fermentation, Osaka, Japan tIFO) under the accession number IFO 50216 on November 10, 1989. The above cells were also deposited with the Fermentation Research Institute, Agency of Industrial Science and Technology, Ministry of International Trade and Industry, Japan (FRI) under the accession number FERM BP-2658 on November 14, 1989.
Anti-bFGF monoclonal antibodies MAbl2, MAb52 and MAb98 described in the following Examples can be produced by the methods described in Hybridoma, 8, 209-221 (1989) and European Patent Publication No. 288,687 the disclosures of which are herein incorporated by reference. The recognition site of MAbl2 is included in the amino acid sequence of ~rom position 1 ~the N-terminus) to position 9 of bFGF, and the recognition sites of MAbS2 and MAb98 are included in the amino acid sequence of from position 14 to position 4~ of bFGF. Recombinant human aFGF which was produced by the methods described in Reference Example 1 was used.
Recombinant human bFGF (rhbFGF) which was produced by the methods described in Iwane et al., Biophys. Biochem.
~ Res. Commun. 146, 470 ~1987) and European Patent Publication ; No. 237,966 was used.
rhbFGF mutein CS23 which was produced using transformant Escherichia coli MM294/pT~762 (IFO 14613, FERM
BP-1645) by the methods described in Sano et al., BioPhys.
Biochem. Res. Commun. 151, 701 (1988) and European Patent Publication No. 281,822 was used. The above E. coli wosl/09~7s PC~/JP90~01726 MM294/pTB762 was deposited with IFO under the accession number IF0 14613 on May 27, 1987. This transformant was also deposited with FRI under the accession number FERM
P-9409 on June 11, 1987. This deposit was converted to the deposit under the ~udapest Treaty and the transformant is stored at the YRI under the accession number FERM BP-1645.
Escherichia coli MM294(DE3)/LysS,pTB762 which is . produced in Reference Example 1 was deposited with IF0 under the accession number IF0 14936 on September 12, 1989. This transformant was also deposited with FRI under the accession number FERM BP-2599 on September 20, 1989.
The following examples are given to illustrate embodiments of the present invention as it is presently preferred to practice. It will be understood that the examples are illustrative, and that the invention is not to be considered as restricted except as indicated in the appended claims.
Examples Reference Example 1 (Preparation of Recombinant Human aFGF) Human aFGF was produced by the ~ollowing method, with reference to the methods described in BiotechnoloqY, 5, 960 ~1987) and ICU5 Short Report, vol. 8, Advances in Gene Technology; Protein ~ngineering and Production, Proceedings of the 1988 Miami Bio/Technology Winter Symposium, page 11~, IRL Press.
(a) Construction o~ Expression Plasmid Plasmid pTB917 obtained by incorporating chemically .
~, , ...... . . . .
WO9l/~9875 . pCT/JPgo/01726 ~ 24 -synthesized human aFGF DNA (Fig. 1) into pUC18 [Methods in Enzymoloqy 101, 20-78 (1983)] was digested with BspMI, and the cleaved sites were changed to flush ends by reaction with DNA polymerase large ~ragment, followed by digestion with BamHI to produce a 0.45-kb DNA fragment.
As a vector DNA, there was used pET3c [F. W. Studier et al., J. Mol. Biol., 189, 113-130 (1986)] carrying a ~10 promoter for a T7 phage. pET3c was cleaved with NdeI and the termini thereof were made flush by treatment with large fragment. Then, an NcoI linker, 5'-CCATGG-3', was ligated thereto with T4 DNA ligase. The resulting plasmid was cleaved with NcoI, and the cleaved ites were made flush with DNA polymerase large fragments, followed by cleavage with Bam~I to remove the sequence of S10. Then, the above 0.45-kb blunt BspMI-BamHI fragment was incorporated thereinto with T4 DNA ligase to obtain pTB975 (Fig. 2).
~b) Expression of Human aFGF cDNA in E. coli ~Phage DE3 ~F. W. Studier et al., J. Mol. Biol. 189, 113-130 (1986)~ in which an RNA polymerase gene of the T7 phage was incorporated into E. coli strain MM294 was lysogenized, and plasmid pLysS [F. W. Studier et al., J.
Mol. Biol. 189, 113-130 ~1986)1 having a lysozyme gene of the T7 phage was further introduced thereinto to prepare E.
coli MM294~DE3)/pLysS. This strain was transformed with pTB975 to give E. coli MM294(DE3)/pLysS, pTB975~IFO 14936, FERM BP-2599).
This strain was cultivated in a medium containing 35 WO9l/~9875 PCT/3P9~/Ot726 - 25 ~
~g/ml of ampicillin and 10 ~g/ml oE chloramphenicol. When the turbidity reached 170 Kletts, isopropyl-~-D-thiogalactoside (IPTG) was added thereto to a final concentration of 0.5 mM, and cultivation was further continued for 3 hours. The cells were collected by centrifugation and washed with ice-cooled PBS. Then, the cells were collected again and stored at -20C until their `
use.
(c) Purification of Human aFGF
The cells collected from a one liter culture were suspended in 100 ml of an ice-cooled solution [10 mM
Tris-HCl tpH 7.4), 10 mM EDTA, 0.6 M NaCl, 10% sucrose, 0.25 mM PMSF], and egg white lysozyme was added thereto to a concentration of 0.5 mg/ml. The mixture was allowed to~
stand in ice for 1 hour, followed by incubation at 37C for 5 minutes. Then, the product was subjected to ultrasonication twice under ice cooling for 20 seconds, and then centrifuged at 18 Krpm at 4C for 30 minutes ~Sorvall) to obtain a supernatant. This supernatant was mixed with 200 ml of an ice-cooled solution [20 mM Tris-HCl ~pH 7.4), 1 mM EDTAI~ and the mixture was loaded onto a heparin Sepharose column (2.5 cm diameter X 4 cm) equilibrated with a buffer 120 mM Tris-HCl (pH 7.4), 1 mM EDTA]. The column was washed with 150 ml ~f a solution ~20 mM Tris-HCl (pH
7.4), 1 mM EDTA, 1.5 M NaCl], and then the protein was eluted with an eluting solution ~20 mM Tris-HCl (pH7.4~, 1 mM EDTA, 1.5 M NaCl]. The eluate was fractionated into 6 ml
8~5 PCT/JPgO/01726 t ~ ., ~J ~
portions and OD28~ was monitored to collect the second peak fraction (8th to 11th, the total amount: 24 ml) ~Fig. 3).
Twenty-two ml of the eluate was mixed with an equal volume of solution 20 mM Tris HCl (pH 7.4), 1 mM EDTA, 2 M
(NH4)2SO~), and the mixture was loaded onto a phenyl Sepharose column (2.5 cm diameter X 8 cm) equilibrated with a buffer [20 mM Tris-HCl (pH 7.4), 1 mM EDTA, 1 M (~H4)2S04]
(flow rate: 0.5 ml/min). The column was washed with 20 ml of the same buffer, and eluted with a linear gradient of 0 to l M ammonium sulfate tflow rate: 0.5 ml/min, gradient time: 200 minutes). The eluted fractions 40 to 55 ~Fig. 4) were collected as purified human aFGF.
(d) Reverse-Phase C4 HPLC
A l.2 mg/ml solution of the purified human aFGF was mixed with 0.25 ml of 0.1% trifluoroacetic acid (TFA), and the mixture was applied to a reverse-phase C4 column lVYDAC). The column was eluted with a linear gradient of 0 to 90% acetonitrile in 0.1% TFA to examine an elution pattern. The flow rate was l ml/min and the gradient time was 60 minutes (Fig. 5).
le) Bioloqical Activity The activity of the human aFGF was determined by assaying the incorporation of ~3H] thymLdine as an indication o~ the DNA synthesis induction of mouse BALB/c3T3 cells (ATCC No. CRL 6587) according to the method of Sasada et al. [Sasada et al., Mol. Cell. Biol. 8, 588-594 11988)].
When the test sample was added, a heparin lSigma, Grade I) WO91/09B7S PCT/JP90~01726 - 27 ~ , 7( ~
solution was incorporated in the medium and the test sample as required.
Reference Example 2 ~ .
(a) Construction of Plasmid pTB1000 for ExPression of Human bFGF Mutein Plasmid pTB762, obtainable from E. coli MM294tDE3)/
Lys,pTB672 (IFO 14936, FERM BP-2599), and described in Japanese Patent Unexamined Publication (Laid-Open) ~o.
2-193/1990 (corresponding to European Patent Publication No.
281,822) was cleaved with restriction enzymes EcoRI and BamHI to obtain a 0.38-kb DNA fragment containing a region coding for human bFGF mutein CS23. Additionally, plasmid pTB503 described in ~apanese Patent Unexamined Publication . (Laid-Open) No. 62- 175182/1987 (corresponding to 15 EP-225,701) was cleaved with ClaI and EcoRI to obtain a 1.7-kb DNA fragment containing an LTR of a mouse leukemia virus (MuLV) region, an SV40-derived promoter and a splicing region and a leader sequence of human interleukin 2.
Further, plasmid pTB675 described in Japanese Patent ~ Unexamined Publication (Laid-Open) No. 2-193/1990 ~corresponding to EP-281,822) was cleaved with ClaI and BamHI to obtain a 3.4-kb DNA fragment containing a region coding for the C-terminal side of the human bFGF, a 3'-untranslated region thereof, a pLasmid pBR322-derived ampicillin-re5lstant gene and a replicator in E. coli.
These three DNA fragments were ligated using T4 DNA ligase to obtain plasmid pTB1000 (Fig. 13).
. ~ "".
~ -~091/09~75 PCT/JP90/Ot726 (b) Transformation of Mouse BA~B/c3T3 Cell and Establishment of Transformed Cell Mouse BALB/c3T3 clone A31 cells ~T. ~akunaga et al.
Science, 209, 505-507 (1980)] were seeded on a 6 cm diameter dish for tissue culture having DMEM medium [Dulbecco et al. Viroloqy, 8, 396 (1959)] containing 10~
calf serum. The next day, the medium was exchanged for the same medium. After 4 hours, 10 ~g or 1 ~g of plasmid pTB1000 obtaine~ in the above (1) was transfected by the calcium phosphate method ~Graham et al., ViroloqY, 52, 456 (1973)]. After transfection, cultivation was continued in DMEM medium containing 5% calf serum. After about 3 weeks, the formed focuses (focus forming frequency: 10 to 20/~g DNA) were transferred into a new dish to cultivate them, and cloning was further conducted by the limiting dilution method. For the three transformed cell clone strains K1000-Fl, K1000-F2 and K1000-3 thus obtainedi the FGF
activity of the culture solution and a cell extract was assayed as D~A synthesis-promoting action to the A31 cells in a still state. The results are shown in the following table.
FGF activity ~ng FGF equivalent/dish) CellCulture solution Cell extract ~ , .
R1000-Fl 0.09 K1000-F2 0.16 11.3 X1000-F3 0.09 4.5 A31 ~ 0.05 < 0.2 Each of these transformed cells showed the form of a .; .
- 29 ~ ) !; `'l~'7?
malignant cell gland and formed colonies on a soft a~ar plate.
Example 1 (Immunization) BALB/c mice ~female, 8 weeks old) were intraperitoneally injected with 50 ~g of antigen rhbFGF
mutein CS23 (a mutein in which each of Cys residues at - positions 70 and 88 of human bFGF were substituted for a Ser residue) which was dissolved in Freund's complete adjuvant (Difco). Two weeks later, the mice were intraperitoneally given again 50 ~g of antigen rhbFGF mutein CS23 dissolved in 0.4 ml of Freund's complete adjuvant. Further 2 weeks later, the mice were additionally immunized with 50 ~g of antigen rhbFGF mutein CS23 dissolved in 0.4 ml of Freund's incomplete adjuvant. Two weeks after the additional immunization, S0 ~g of rhbFGF mutein CS23 dissolved in physiological saline was inoculated into the caudal veins of the mice.
ExamPle 2 (1) Cell Fusion Three days after the final inoculation, the spleens were removed from the mice immunized in Example 1 to obtain cells to be used for cell fusion. These cells were suspended in IH medium.
Mouse myeloma cells SP2/0-AG14 ~ATCC ~o. CRL 1581) were subcultured in DMEM medium containing 10% fetal calf serum under an atmosphere of 5% carbon dioxide and 95% air.
Cell fusion was carried out in accordance with the -~ , : - . , : . " .. .
W~91/0987~ PCT/3P90/~1726 method established by Kohler and Milstein [G. Kohler and C.
Milstein, Nature, 256, 995 (1975)]. The above myeloma cells (2 X 107 cells) were mixed with the immunized lymphocytes (1.5 X 108 cells) obtained by the above method, and the mixture was centrifused. Then, 1 ml of a 45% solution of polyethylene glycol 6000 (hereinafter referred to as PEG
6000) in IH medium was dropwise added thereto. The PEG 6000 solution was preheated to 37C and slowly added for 1 minute.
Then, 1 ml of IH medium was added for 1 minute, 1 ml for 1 minute and 8 ml for 3 minutes. The solution was thereafter centrifuged at room temperature at 1,000 rpm for 5 minutes to remove a supernatant. The resulting cell precipitate was suspended in 30 ml of IH medium containing 20% calf serum. The suspension was seeded on a 96-well microtiter plate (~unc) in an amount of 100 ~l/well. One day later, IH medium (containing 20% calf serum) supplemented with HAT (1 X 10 4 M hepoxanthine, 4 X 10 7 M
aminopterin, 1.6 X 10 5 M thymidine) was added to the microtiter plate in an amount of 100 ~l/well. The IH medium supplemented with HAT is hereinafter referred to as HAT
medium. Further every 3 days, one-half the amount of the medium was exchanged for HAT medium. The cells which thus grew were hybrid cells.
(2) Screening of Antibody-Producing Cells A fixing buffer [0.1 M sodium hydrogencarbonate (pH
portions and OD28~ was monitored to collect the second peak fraction (8th to 11th, the total amount: 24 ml) ~Fig. 3).
Twenty-two ml of the eluate was mixed with an equal volume of solution 20 mM Tris HCl (pH 7.4), 1 mM EDTA, 2 M
(NH4)2SO~), and the mixture was loaded onto a phenyl Sepharose column (2.5 cm diameter X 8 cm) equilibrated with a buffer [20 mM Tris-HCl (pH 7.4), 1 mM EDTA, 1 M (~H4)2S04]
(flow rate: 0.5 ml/min). The column was washed with 20 ml of the same buffer, and eluted with a linear gradient of 0 to l M ammonium sulfate tflow rate: 0.5 ml/min, gradient time: 200 minutes). The eluted fractions 40 to 55 ~Fig. 4) were collected as purified human aFGF.
(d) Reverse-Phase C4 HPLC
A l.2 mg/ml solution of the purified human aFGF was mixed with 0.25 ml of 0.1% trifluoroacetic acid (TFA), and the mixture was applied to a reverse-phase C4 column lVYDAC). The column was eluted with a linear gradient of 0 to 90% acetonitrile in 0.1% TFA to examine an elution pattern. The flow rate was l ml/min and the gradient time was 60 minutes (Fig. 5).
le) Bioloqical Activity The activity of the human aFGF was determined by assaying the incorporation of ~3H] thymLdine as an indication o~ the DNA synthesis induction of mouse BALB/c3T3 cells (ATCC No. CRL 6587) according to the method of Sasada et al. [Sasada et al., Mol. Cell. Biol. 8, 588-594 11988)].
When the test sample was added, a heparin lSigma, Grade I) WO91/09B7S PCT/JP90~01726 - 27 ~ , 7( ~
solution was incorporated in the medium and the test sample as required.
Reference Example 2 ~ .
(a) Construction of Plasmid pTB1000 for ExPression of Human bFGF Mutein Plasmid pTB762, obtainable from E. coli MM294tDE3)/
Lys,pTB672 (IFO 14936, FERM BP-2599), and described in Japanese Patent Unexamined Publication (Laid-Open) ~o.
2-193/1990 (corresponding to European Patent Publication No.
281,822) was cleaved with restriction enzymes EcoRI and BamHI to obtain a 0.38-kb DNA fragment containing a region coding for human bFGF mutein CS23. Additionally, plasmid pTB503 described in ~apanese Patent Unexamined Publication . (Laid-Open) No. 62- 175182/1987 (corresponding to 15 EP-225,701) was cleaved with ClaI and EcoRI to obtain a 1.7-kb DNA fragment containing an LTR of a mouse leukemia virus (MuLV) region, an SV40-derived promoter and a splicing region and a leader sequence of human interleukin 2.
Further, plasmid pTB675 described in Japanese Patent ~ Unexamined Publication (Laid-Open) No. 2-193/1990 ~corresponding to EP-281,822) was cleaved with ClaI and BamHI to obtain a 3.4-kb DNA fragment containing a region coding for the C-terminal side of the human bFGF, a 3'-untranslated region thereof, a pLasmid pBR322-derived ampicillin-re5lstant gene and a replicator in E. coli.
These three DNA fragments were ligated using T4 DNA ligase to obtain plasmid pTB1000 (Fig. 13).
. ~ "".
~ -~091/09~75 PCT/JP90/Ot726 (b) Transformation of Mouse BA~B/c3T3 Cell and Establishment of Transformed Cell Mouse BALB/c3T3 clone A31 cells ~T. ~akunaga et al.
Science, 209, 505-507 (1980)] were seeded on a 6 cm diameter dish for tissue culture having DMEM medium [Dulbecco et al. Viroloqy, 8, 396 (1959)] containing 10~
calf serum. The next day, the medium was exchanged for the same medium. After 4 hours, 10 ~g or 1 ~g of plasmid pTB1000 obtaine~ in the above (1) was transfected by the calcium phosphate method ~Graham et al., ViroloqY, 52, 456 (1973)]. After transfection, cultivation was continued in DMEM medium containing 5% calf serum. After about 3 weeks, the formed focuses (focus forming frequency: 10 to 20/~g DNA) were transferred into a new dish to cultivate them, and cloning was further conducted by the limiting dilution method. For the three transformed cell clone strains K1000-Fl, K1000-F2 and K1000-3 thus obtainedi the FGF
activity of the culture solution and a cell extract was assayed as D~A synthesis-promoting action to the A31 cells in a still state. The results are shown in the following table.
FGF activity ~ng FGF equivalent/dish) CellCulture solution Cell extract ~ , .
R1000-Fl 0.09 K1000-F2 0.16 11.3 X1000-F3 0.09 4.5 A31 ~ 0.05 < 0.2 Each of these transformed cells showed the form of a .; .
- 29 ~ ) !; `'l~'7?
malignant cell gland and formed colonies on a soft a~ar plate.
Example 1 (Immunization) BALB/c mice ~female, 8 weeks old) were intraperitoneally injected with 50 ~g of antigen rhbFGF
mutein CS23 (a mutein in which each of Cys residues at - positions 70 and 88 of human bFGF were substituted for a Ser residue) which was dissolved in Freund's complete adjuvant (Difco). Two weeks later, the mice were intraperitoneally given again 50 ~g of antigen rhbFGF mutein CS23 dissolved in 0.4 ml of Freund's complete adjuvant. Further 2 weeks later, the mice were additionally immunized with 50 ~g of antigen rhbFGF mutein CS23 dissolved in 0.4 ml of Freund's incomplete adjuvant. Two weeks after the additional immunization, S0 ~g of rhbFGF mutein CS23 dissolved in physiological saline was inoculated into the caudal veins of the mice.
ExamPle 2 (1) Cell Fusion Three days after the final inoculation, the spleens were removed from the mice immunized in Example 1 to obtain cells to be used for cell fusion. These cells were suspended in IH medium.
Mouse myeloma cells SP2/0-AG14 ~ATCC ~o. CRL 1581) were subcultured in DMEM medium containing 10% fetal calf serum under an atmosphere of 5% carbon dioxide and 95% air.
Cell fusion was carried out in accordance with the -~ , : - . , : . " .. .
W~91/0987~ PCT/3P90/~1726 method established by Kohler and Milstein [G. Kohler and C.
Milstein, Nature, 256, 995 (1975)]. The above myeloma cells (2 X 107 cells) were mixed with the immunized lymphocytes (1.5 X 108 cells) obtained by the above method, and the mixture was centrifused. Then, 1 ml of a 45% solution of polyethylene glycol 6000 (hereinafter referred to as PEG
6000) in IH medium was dropwise added thereto. The PEG 6000 solution was preheated to 37C and slowly added for 1 minute.
Then, 1 ml of IH medium was added for 1 minute, 1 ml for 1 minute and 8 ml for 3 minutes. The solution was thereafter centrifuged at room temperature at 1,000 rpm for 5 minutes to remove a supernatant. The resulting cell precipitate was suspended in 30 ml of IH medium containing 20% calf serum. The suspension was seeded on a 96-well microtiter plate (~unc) in an amount of 100 ~l/well. One day later, IH medium (containing 20% calf serum) supplemented with HAT (1 X 10 4 M hepoxanthine, 4 X 10 7 M
aminopterin, 1.6 X 10 5 M thymidine) was added to the microtiter plate in an amount of 100 ~l/well. The IH medium supplemented with HAT is hereinafter referred to as HAT
medium. Further every 3 days, one-half the amount of the medium was exchanged for HAT medium. The cells which thus grew were hybrid cells.
(2) Screening of Antibody-Producing Cells A fixing buffer [0.1 M sodium hydrogencarbonate (pH
9.6), 0.02~ sodium azide] containing 200 ng/ml of rhbFGF
, :
; - - :.,:.-. .-. .; . .
WO9l/~9875 - 31 - PCr/JP90/~1726 mutein cs23 was added in an amount of 100 ~l/well to a 96-well polystyrene microtiter plate (Nunc). After 2 hours, the microtiter plate was washed with a rinsing liquid (0.05 Tween 20, physiological phosphate buffer), and then 100 ~1 of the combined solution of 50 ~1 of the culture supernatant and S0 ~1 of a buffer for dilution (0.05 M Tris-HCl buffer pH 8.01, 1 mM magnesium chloride, 0.15 M sodium chloride, 0.05% Tween 20, 0.02% sodium azide, 0.3% gelatin) was added to the microtiter plate. After 2 hours, the culture
, :
; - - :.,:.-. .-. .; . .
WO9l/~9875 - 31 - PCr/JP90/~1726 mutein cs23 was added in an amount of 100 ~l/well to a 96-well polystyrene microtiter plate (Nunc). After 2 hours, the microtiter plate was washed with a rinsing liquid (0.05 Tween 20, physiological phosphate buffer), and then 100 ~1 of the combined solution of 50 ~1 of the culture supernatant and S0 ~1 of a buffer for dilution (0.05 M Tris-HCl buffer pH 8.01, 1 mM magnesium chloride, 0.15 M sodium chloride, 0.05% Tween 20, 0.02% sodium azide, 0.3% gelatin) was added to the microtiter plate. After 2 hours, the culture
10 supernatant was washed with a rinsing liquid, followed by - .
addition of the alkaline phosphatase-labeled anti-mouse IgG
goat antibody ~Bio RAD) as the second antibody. After 2 hours, the second antibody was washed with a rinsing liquid, and then coloring reaction was conducted by ~dding a }5 reaction substrate ~ELISA method). By this method, the rhbFGF mutein CS23 combining activity was observed in 4 wells.
~3) Screening of anti-bFGF Immuno-Neutralizing Antibody-Producing Cells Human umbilical vein-derived vascular endothe}ial cells was suspended in GI~ medium ~commercially available from .`
Wako Pure Chemical Industries, Ltd. Japan; a mammalian serum-derived composition for animal cell cultivation, produced by subjecting mammalian serum to purifying treatment including an inactivation process for cantaminant microorganisms and a salting-out/desalting process; cf. U.S.
Patent No. 4,654,304) containing 2.5~ feta} calf serum, .
WOgl/0~875 PCT/JP90/01726 ~? ~ 3 2 and the suspension was seeded in an amount of 100 ~l/well (2,000 cells/well) to a 96-well microtiter plate. The next day, GIT culture solution cont~ining various concentrations of hybridoma culture supernatants, 4 ng/ml rhbFGF and 2.5%
fetal calf serum was added in an amount of 100 ~l/well, and cultivation was conducted at 37C under an atmosphere of 5 C2 and 7% 2 for 3 days. After 3 days, the culture solution was removed, and then GIT culture solution containing 1 mg/ml MTT (4,5-dimethyl-2-thiazolyl-2,5-diphenyl-2H-tetrazolium bromide) and 2.5% fetal calf serum was added in an amount of 100 ~l/well. After cultivation was carried out at 37C under an atmosphere of 5% C2 and 7% 2 for 4 hours, 10% sodium dodecyl sulfate ~SDS) was added in an amount of 100 ~l/ml. After 4 hours, the absorbance at 590 nm was measured with a spectro-photometer for 96 wells ~Titertek) ~MTT method). By this method, the strong neutralizing activity was observed in one well.
(4) Cloning of Hybrid Cells The cells in this well were spread to 0.5 cell per well on a 96-well microtiter plate on which mouse thymocytes had preliminarily been spread as vegetative cells, and cloning was carried out. As a result, hybridoma mouse 3H3 cells ~IFO 50216, FERM BP-2658) were obtained.
The cloned cells were stored in liquid nitrogen, adding dimethyl sulfoxide ~DMSO) to IH medium containing 20% calf serum to a concentration of 10%.
... .. . ...
WOgl/09875 PCT/JP90/01726 2r~ ,7~
Example 3 ~Immunoglobulin Class of Monoclonal Antibody) The culture supernatant of 3H3 cells obtained in Example 2-(3) were reacted with various immunoglobulin samples by a subclass detecting kit (Rio RAD). The results 5 are shown in Table 1.
Table 1 Immunoglobulin sample 3H3 antibody IgGl +
` I G
IgG2b IgG3 IgM
IgA
:~ ....
In Table 1, "+" indicates that the reaction is positive, and "-" indicates that the reaction is negative.
Table 1 shows that the antibody in the culture 2~ supernatant o~ 3H3 cells belonss to IgGl in the i immunoglobulin class.
Example 4 (Purification of Monoclonal Antibody from Culture Supernatant and ~scites) ~1) Purification from Culture Supexnatant The combined solution of the culture supernatant of mouse 3H3 cells and a combining buffer [3 M sodium chloride, 1.5 8 glycine ~pH 8.7)] in a 1:1 ratio was loaded onto a ,;, . :
WO91/0~7~ PCT/JP90/01726 ~ . . i; ~.. , ~ ,.
Protein A column. After washing with a combining buffer, elution was carried out with an elution buffer [0.1 M citric acid (pH 5)]. To the eluate was added 1 M Tris (pH a.0) to neutralize it, followed by dialysis against physiological phosphate buffer.
The IgG amount of the samples was determined according ~`
to the method described in Example 2-t2) in the following manner. Various dilutions of mouse IgG whose concentration was known and the 3H3 antibody were fixed on a 96-well polystyrene microtiter plate with a fixing buffer. After 2 hours, the alkaline phosphatase- labeled anti-mouse IgG goat antibody (Bio RAD) was added thereto. After 2 hours, coloring reaction was conducted by adding a reaction substrate (ELISA method). With respect to mouse IgGl, a determination curve was drawn, and the IgG amount of the samples was determined based on this curve, whereby a 60 ~g/ml solution of the 3H3 antibody was prepared.
Fig. 6 shows the results of the antibody titer to rhbFGF mutein CS23 measured for the monoclonal antibody thus purified, according to the method described in Example 2-(2). One ~g/ml of the rabbit anti-bFGF polyclonal antibody was fixed and rhbFGF mutein CS23 was added thereto. Then, 1 ~ig/ml of the 3H3 antibody was added and 1 ~g/ml of the alkaline phosphatase-labeled anti-mouse IgG goat antibody 25 Wa5 further added thereto. By this method, rhbFGF mutein CS23 could be detected up to 3 ng/ml.
WO91/09X~5 PCT/JP9~/017~6 ~ r~
(2) Purification from Ascites Further, the antibody was purified from ascites. The mouse 3H3 cell strain was injected illtO the mice (Balb/c).
IgG was purified from the ascites according to conventional - 5 methods. Namely, 5 ml of the ascites was subjected to salt precipitation using a 45~ saturated solution of ammonium sulfate, and the precipitate was dissolved in borate buffer (BBS, pH 8.5) containing 0.15 M NaC1, followed by dialysis against BBS at 4C for 20 hours. The dialyzed solution was applied to a DE-50 column (1 cm diameter X 60 cm, Whatman, Great Britain), and the column was eluted with a linear gradient of 0.1 to 0.35 M NaCl in 0.1 M phosphate buffer ~pH
; 8.0), whereby 7 mg of monoclonal antibody 3H3 was obtained from 5 ml of the ascites.
Example 5 (Determination of Antigen Recognition Site) The antigen recognition site of the 3H3 antibody whose antibody titer was measured in Example 4 was examined by competitive binding inhibition experiments. As competitive substances, there were used human aFGF, rhbFGF, rhbFGF
mutein CS23, synthetic peptides pep 1: Pro-Ala-Leu-Pro-Glu-Asp-Gly-Gly-Ser-Tyr [the peptide in which Tyr was added to the C-terminus of N-terminal amino acids 2 to 10 of human bFGF, ~3L~ Y ~ , 10, 309-317 ~1985)] and pep 2:
Leu-Pro-Met-Ser-Ala- Lys-Ser (corresponding to amino acids 141 to 147, refer to European Patent Publication No.
288,687) and heparin sodium.
~O 91/09875 PCr/.lP90/0~726 The synthetic peptides, heparin sodium, human aFGF, rhbFGF and rhbFGF mutein CS23 were diluted with the buffer for dilution used in Example 2-~2) to a concentration of 100 ~g/ml. When the synthetic peptides, heparin sodium, human aFGF, rhbFGF and rhbFGF mutein CS23 were used as the competitive substances, 100 ng/ml of the 3H3 antibody and the competitive substance were suspended, and the suspension was maintained at 37C for 60 minutes.
The amount of antibody not com~ined in this solution was assayed by the EIA shown in Example 2-(2). The results are shown in Table 2.
Table 2 3H3 antibody Human bFGF +
Human aFGF
CS23 +
pepl pep2 Heparin sodium In Table 2, "~" indicates that the competitive inhibition occurred, and "-" indicates that the competitive inhibition did not occur. From these results, the recognition site of the 3H3 antibody is considered to be the peptide of 10th to 141st amino acids of human bFGF molecule ' :. ' - .. ~ . . , .:, . . . . .... . .. .. . .
WO9l/0~87s PCT/~P90/01726 - 37 ~ j7~
and binding site of human bFGF to human bFGF receptor or its adjacent site, other than the heparin combining site, or a region adjacent thereto.
Example 6 (Examination of Immuno-Neutralizing Action) As to the 3H3 antibody purified by the method of Example 4(1), the human bFGF-immunoneutralizing activity against rhbFGF was studied by the MTT method of Example 2-(3) (Fig. 7). Namely, the activity was assayed by 3-day proliferation in tbe presence of 2 ng/ml of bFGF of the human umbilical vein endo~helial ~H W E) cell. The proliferation inhibitory effect is shown by the absorbance at OD-590 nm in case of adding the monoclonal antibodies where the value is estimated as 100~ both in the presence of the bFGF and in the absence of the monoclonal antibody.
Referring to Fig. 7, - o - indicates the results of the 3H3 antibody, and - ~ - indicates the results of normal mouse IgG. The line of 44~ indicates the number of cells when the bFGF was not added. When the 3H3 antibody was added, 50 ng/ml thereof hindered the proliferation of the HUVE cells to the number of cells in the absence of the bFGF. The normal mouse IgG did not exhibit the proliferation inhibitory effect.
The assay was further changed to study the proliferation inhibition effect of the HUVE cells. Namely, the HUVE cells were seeded on a 24-well Linbro plate in an amount o~ l X 104 cells/well ~the culture conditions were37he same as with Example 2-t3)). The next day, 2 ng/ml of the bFGF and the 3H3 antibody were added thereto, ~, .. . ., ... . ~ .. . . .
' ' ,. . . ' . . . '. . ., ' ' ' ' ~ . . ., ' '.' , . , ` , , WOgl/09X7~ PCT/JP9~/Ot726 followed by cultivation for 3 days and for 5 days. Then, the number of cells was measured by using a Coulter counter (Coulter Electronics, Inc.) for each case. Referring to Figs. 8(A) and 8(B), Fig. 8(A) shows the results when cultivation was carried out for 3 days, and Fig. 8(B) shows the results when cultivation was carried out for 5 days.
The number of cells when the 3H3 antibody was added was expressed in percentage, taking the number of cells when the bFGF was added and the 3H3 antibody was not added as 100%.
In both of Fig. 8(A) and Fig. 8(B), - o - and - ~ - indicate the effect of the 3H3 antibody in the presence of 2 ng/ml of the bFGF and in the absence of the bFGF, respectively. The IC50 value of the proliferation hindrance (the amount of the antibody which hinders 50~ of cell proliferation when the antibody is not added) shows 13.2 and 7.6 ng/ml in Fig. 8(A) and Fig. 8(B), respéctively. Further, the 3H3 antibody did not affect the number of cells in the absence of the bFGF.
It is clear from the above data that the 3H3 antibody has strong immuno-neutralizing action to the biological activity of the bFGF.
Example 7 (Preparation of Horseradish Peroxidase-Labeled 3H3 Antibody) The purified 3H3 antibody (7 mg/ml) was dialyzed against 0.1 M acetate buffer (pEI 4~5) containing 0.1 M NaCl at 4C for 20 hours, followed by addition of pepsin (0.1 mg) (Sigma, U.S.A.). Then, digestion was carried out at 37C
for 8 hours. The solution was adjusted to pH 8 with l M
i`
., : . ., . , . . ,: : . ~
wo~l/09875 PCT/JP90/01726 ~ ,7`~
Tris to terminate the reaction. The resulting solutlon was placed on a column of Ultrogel AcA44 (IBF, France) and eluted with 0.02 M borate buffer ~pH 8.0) containing 0.15 M
NaCl to obtain F(ab')2. The solution containing F(ab')2 was concentrated to 1 ml. Thenl the concentrated solution was dialyzed against 0.1 M phosphate buffer (pH 6.0) at 4C for 20 hours, and 0.1 ml of a solution ~0.2 M mercaptoethyl-amine, 5 mM EDTA, 0.1 M phosphate buffer (pH 6.0)] was added, followed by reduction at 37C for 90 minutes. The reaction solution was placed on a Sephadex G-25 fine column (1 cm diameter X 60 cm, Pharmacia Fine Chemical, Sweden) and eluted with an eluent ~5 mM EDTA, 0.1 M phosphate buffer (pH
6.0)] to obtain an Fab' fraction.
Additionally, 10 mg of horseradish peroxidase (HRP, Behringer Manheim, West Germany) was dissolved in 1.5 ml of 0.1 M phosphate buffer (pH 7.0), and 3.5 mg of maleimidobutyloxy)succinimide ~GMBS) was dissolved in 100 ~1 of N,N-dimethylformamide ~DMF). The solution of GMBS
in DMF was added to the HRP solution, followed by stirring at 30C for 60 minutes. Then, the resulting solution was placed on the Sephadex G-25 fine column ~1.2 cm diameter X
60 cm) and eluted with 0.1 M phosphate buffer ~pH 7.0) to obtain maleimide group- introduced HRP ~maleimidated HRP).
Fab' and maleimidated HRP were mixed with each other to a mol ratio of 1:1, followed by reaction at 4C for 20 hours.
The reaction solution was applied to an ultrogel AcA44 column and eluted with 0.1 M phosphate buffer ~pH 7.0) to uosl/os~75 PCT/JP~0/01726 ~ q ~ - 40 -obtain an enzyme- labeled antibody (3H3-HRP).
Example 8 (preparation of Antibody-Sensitized Plate) MAbl2 or a 50-50 mixture of MAb52 and MAb98 was diluted with 0.1 M carbonate buf~er (pH 9.6) to a concentration of 10 ~g/ml. The resulting solution was poured in an amount of 100 ~1/well into an immunoplate for EIA ~Maxisoap: Nunc, Denmark), followed by standing at 4C overnight to sensitize or fix the antibody to the plate. After washing the plate with 0.01 M phosphate buffer (pH 7.0) containing 0.15 M
NaCl, 0.01 M phosphate buffer (pH 7.0) containing 0.1~ BSA
was poured into each well. Then, the plate was stored in a chilled place until its use.
Example 9 (Assay of Human bFGF) 1. Preparation of Calibration Curve A. Reaqents ~1) Enzyme-labeled antibody obtained in Example 7, (2) Antibody-sensitized microtiter plate obtained in Example 8, (3) Recombinant human bFGF ~rhbFGF): 0-50 ng/ml, ~4) Buffer AE0.02 M phosphate buffer (pH 7.0) containing 0.15 M NaCl], Bufer B~0.02 M phosphate buffer ~pH 7.Q) containing 25% Blockace ~blocking agent prepared from milk protein) (Dainippon Pharmaceutical), 0.15 M NaCl], ~ 5) Peroxidase substrate solution ~sodium citrate buffer ~pH 5.5) containing 0.02~ hydrogen peroxide and 0.15%
W091/09875 PCT/JPgO/01726 f. ~ r~
o-phenylenediamine], Enzyme reaction-terminating solution(2N sulfuric acid).
B. Assay Into each well of the antibody-sensitized plate obtained in Example 8, 100 ~1 of a solution of the bFGF (0.1 to lOOOpg/ml) in buffer B was added, followed by reaction at 4C for 24 hours. After washing each well with buffer A, 100 ~1 of an enzyme- labeled antibody solution diluted 200 times with buffer B was added to each well, followed by further reaction at 25C for 2 hours. Each well was washed with buffer A, and 100 ~1 of the peroxidase substrate solution was added thereto, followed by reaction at 25C for 30 minutes. Then, 100 ~1 of the enzyme reaction-terminating solution was added thereto to terminate reaction. The absorbance at 492 nm was thereafter measured by using an automatic colorimeter for microtiter plates (MTP-32.
Corona). Fig. 9 shows the relationship between the concentration of the hbFGF and the absorbance. Referring to Fig. 9, - o - and - ~ - indicate the relationship between the concentration of the hbFGF and the absorbance when the microtiter plate sensitized with MAbl2 was used and when the microtiter plate sensitized with the 50-50 mixture of MAbS2 and MAb98 was used, respectively. It was revealed that 20 pg/ml of the bFGF protein could be detected, when the plate was sensitized with MAbl2.
2. bFGF Immunoassay Kit and Assay of bFGF
The amount of the bFGF in the test samples was assayed Wo9l/09x7s ~T/JP90/01726 ~ 2 -by using the following bFGF immunoassay kit according to the following procedure:
A. Reagents (1) Enzyme labeled antibody (3H3 antibody-HRP) obtained in Example 7, (2) Antibody-sensitized microtiter plate obtained in Example 8, (3) Recombinant human bFGF (rhbFGF): 0-50 ng/ml, (4) Buffer A C0.02 M phosphate buffer ~pH 7.0) containing 0.15 M NaCl], Buffer B~0.02 M phosphate buffer (pH 7.0) containing 25% Blockace, 0.15 M NaCl], ~S) o-Phenylenediamine, (6) Buffer D used for dissolution of o-phenylenediamine 10.1 M citrate buffer (pH 5.5) containing 0.02 hydrogenperoxide and 0.005% thimerosal], ~7) Enzyme reaction-terminating solution (2N sulfuric : acid), B. Ass~y ~ .
Each well of the antibody-sensitized plate obtained in Example 8 was washed with buffer A, and 100 ~1 of a standard solution of the bFGF in buffer B or a solution of the test sample diluted with bufer B was poured thereinto, ollowed by reaction at 4C for 24 hours. After washing each well 25 with buffer A, 100 ~1 of an enzyme-labeled antibody solution ~:
diluted 200 times with buffer B was added to each well, followed by further reaction at 25C for 2 hours. After :: .
wn ~1/0987~
PCT/JP9OtOt726 washing each well with buffer A, 100 ~1 of a 0.15~ solution of o-phenylenediamine in buffer D was added thereto, followed by reaction at 25C for 30 minutes. Then, 100 ~1 of the enzyme reaction-terminating solution was added thereto to terminate reaction. The absorbance at 492 nm was thereafter measured by using an automatic colorimeter for microtiter plate ~MTP-32. Corona). The calibration curve of the standard bFGF was prepared, and the bFGF concentration was determined from the absorbance obtained for the test 10 samples.
Example 10 (Influence of Heparin in hbFGF Assay System) In Example 9-1, heparin was added to buffer B to a concentration of 0, 1, 10 or 100 ~g/ml, when the standard hbFGF was diluted. Then, the concentration of the hbFGF was assayed in the manner of Example 4-(1). As a result, there were observed no considerable changes in the standard curves with the presence of heparin, as shown in Figs. 10(1) and 10(2).
Referring to Figs. 10(1) and 10(2), Fig. 10~1) indicates the results when MAbl2 was fixed, and Fig. lOt2) indicates the results when the 50-50 mixture of MAb52 and MAb98 was ~ixed. Further in each igure, - -, - o ~
- and - ~ - indicate the results when heparin concentrations are 0, 1, 10 and 100 ~g/ml, respectively.
5 Example 11 ~Reactivity of Acid-Modified hbFGF in hbFGF Assay Systems) A 20 ~1 solution of the hbFGF (in 20 mM Tris-HCl buffer WO9l/09875 PCT/JP90/01726 ~" . ~.'`_J ~);
(pH 7.4) containing hbFGF at a concentration of 200~g/ml and containing 1 M NaC1 was added in an amount of 20 ~1 to laO
~1 of 1 M acetate buffer, followed by incubation at 25C for 0, 1, 3 or 10 minutes. 400 ~1 of 1 M Tris was added thereto to neutralize it, and ~hen the resulting solution was diluted with buffer B used in Example 9-1. Then, calibration curves were prepared for respective incubation times according to the method of Example 9-1, as shown in Figs. 11(1) and 11(2). Referring to Figs. 11(1) and 11(2), Fig. 11(1) indicates the results when MAbl2 was solidified, and Fig. 11(2) indicates the results when the 50-50 mixture of MAb52 and MAb98 was solidified. Further in each figure, - O -, - O -, - a - and - ~ indicate the results when the hbFGF was incubated at pH 4 for 0, 1, 3 and 10 minutes, respectively. Figs. 11(1) and 11~2) show that the hbFGF
modified at pH 4 is reduced in reactivity to about 1~ by incubation for 10 minutes in each assay system. The assay systems of Example 9 are assay systems by which only the native hbFGF can be assayed.
Example 12 (Assay of bFGF in Various Cells) A375 (human melanoma), A431 ~human sguamous cell carcinoma)~ A549 ~human lung cancer), SK-Hepl ~human hepatic cancer) ~all o them were supplied by ATCC, U~S.A.) and human umbilical vein endothelial cells were each scraped in an amount of 2 to 6 X 107 cells by a cell scraper. The cells were washed twice with a phosphate buffered saline ~PBS, pH 7.2) containing 0.15 M NaCl, and then 0.6 ml of PBS
'~.
W~gl/0~75 PC~/JP~0/~1726 .
- 45 - ~r ~ ?
was added thereto, followed by ultrasonication under ice cooling for 25 seconds. After centrifugation at 15,000 rpm, the concentration of the bFGF in the supernatant was determined according to the method of Example 9-2.
The results are shown in Table 3. In Table 3, A shows the results when MAbl2 was fixed, and ~ shows the results when the 50-50 mixture of MAb52 and MAb98 was fixed.
Table 3 Amount of bFGF in Cell ~' .
Amount of bFGF
: A B
~ame of Cell(pg/106 cells)(ng/106 cells) A375 1.4 4.0 A431 1.5 0.5 A549 8.4 8.5 SK-Hepl 4 . 0 11. 7 HUVE 11 . 7 0 . 8 4 From Table 3r it is observed that the difference in measured amount of bFGF between the A assay system and the B
assay system is great. From this fact, the possibility is considered that the N-terminus of the bFGF is cleaved during extraction operation, or that the ~-terminus of the actually produced bFGF is cleaved or masked.
Example 13 (Antitumor Effect to KlO00 Tumor) The KlO00-Fl cells obtained in Reference Example 2 were ~.
wosl/0987s PCT/JP90/01726 sub ~ a~o~ impLanted in an amount of 3 X lO6 cells/mouse into nude BALB/c mice. Three days after implantation, the 3H3 antibody obtained in Example 4 and nonimmune mouse IgG
were given to the caudal veins in a dose of 200 ~g/mouse/day continuously for 5 days. After implantation, the diameter of the tumors was measured, and the volume thereof ~=0.5 X
(major axis) X (minor axis)2] was calculated. The results are shown in Fig. 12. Referring to Fig. 12, - ~ -, - 4 -and - ~ - indicate the results for an untreated control group, a nonimmune mouse IgG-given group and a 3H3 antibody-given group, respectively. The 3H3 antibody exhibited antitumor effect against the RlO00 tumor (14 days after implantation, the 3H3 antibody-given group is decreased in tumor volume to 34% of that of the untreated control group). The antitumor effect of nonimmune mouse IgG
was not observed. ;
,', ~';'~
,:
., . , ' :
` , ' '~
~
.
.:
~ ' ;~, ~91/0987~ PCT/JP90/017Z6 Incorporated by refere~ce ~ature 249, 123 ~1974) Biophys. Res. Commun. 151, 701 (1988) European Patent Publication No. 281,822 FEBS Letters 213, 189 ~1987) Biophys. Res. Commun. 146, 470 (1987) European Patent Publication No. 237,966 J. Immun. Method 80, 55 tl985) Nature 256, 495 (1975) J. Am. Med. Assoc. 199, 549 (1967) Metabolism, 8, 696 (1971) Hybridoma, 8, 209-221 (1989) European Patent Publication No. 288,687 Biotechnology, 5, 960 (1987) ICUS Short Report, vol. 8, Advances in Gene Technology;
Protein Engineering and Production, Proceedings of the 1988 Miami Bio/Technology Winter Symposium, page 110, IRL
Press J. Mol. Biol., 189, 113-130 (1986) Mol. Cell. Biol. 8, 588-594 ~1988) Methods in Enzymology 101, 20-78 (1983) ~apanese Patent Unexamined Publication tLaid-Open) No.
2-193/1990 ~European Patent Publication No. 281,822) Japanese Patent Unexamined Publication (Laid-Open) No. 62-175182/1987 (EP-225,701) Science, 209, 505-507 (1980) Virology, 8, 396 (1959) Virology, 52, 456 (1973) U.S.P. No. 4,654,304 Regulatory Peptides, 10, 309-317 (1985)
addition of the alkaline phosphatase-labeled anti-mouse IgG
goat antibody ~Bio RAD) as the second antibody. After 2 hours, the second antibody was washed with a rinsing liquid, and then coloring reaction was conducted by ~dding a }5 reaction substrate ~ELISA method). By this method, the rhbFGF mutein CS23 combining activity was observed in 4 wells.
~3) Screening of anti-bFGF Immuno-Neutralizing Antibody-Producing Cells Human umbilical vein-derived vascular endothe}ial cells was suspended in GI~ medium ~commercially available from .`
Wako Pure Chemical Industries, Ltd. Japan; a mammalian serum-derived composition for animal cell cultivation, produced by subjecting mammalian serum to purifying treatment including an inactivation process for cantaminant microorganisms and a salting-out/desalting process; cf. U.S.
Patent No. 4,654,304) containing 2.5~ feta} calf serum, .
WOgl/0~875 PCT/JP90/01726 ~? ~ 3 2 and the suspension was seeded in an amount of 100 ~l/well (2,000 cells/well) to a 96-well microtiter plate. The next day, GIT culture solution cont~ining various concentrations of hybridoma culture supernatants, 4 ng/ml rhbFGF and 2.5%
fetal calf serum was added in an amount of 100 ~l/well, and cultivation was conducted at 37C under an atmosphere of 5 C2 and 7% 2 for 3 days. After 3 days, the culture solution was removed, and then GIT culture solution containing 1 mg/ml MTT (4,5-dimethyl-2-thiazolyl-2,5-diphenyl-2H-tetrazolium bromide) and 2.5% fetal calf serum was added in an amount of 100 ~l/well. After cultivation was carried out at 37C under an atmosphere of 5% C2 and 7% 2 for 4 hours, 10% sodium dodecyl sulfate ~SDS) was added in an amount of 100 ~l/ml. After 4 hours, the absorbance at 590 nm was measured with a spectro-photometer for 96 wells ~Titertek) ~MTT method). By this method, the strong neutralizing activity was observed in one well.
(4) Cloning of Hybrid Cells The cells in this well were spread to 0.5 cell per well on a 96-well microtiter plate on which mouse thymocytes had preliminarily been spread as vegetative cells, and cloning was carried out. As a result, hybridoma mouse 3H3 cells ~IFO 50216, FERM BP-2658) were obtained.
The cloned cells were stored in liquid nitrogen, adding dimethyl sulfoxide ~DMSO) to IH medium containing 20% calf serum to a concentration of 10%.
... .. . ...
WOgl/09875 PCT/JP90/01726 2r~ ,7~
Example 3 ~Immunoglobulin Class of Monoclonal Antibody) The culture supernatant of 3H3 cells obtained in Example 2-(3) were reacted with various immunoglobulin samples by a subclass detecting kit (Rio RAD). The results 5 are shown in Table 1.
Table 1 Immunoglobulin sample 3H3 antibody IgGl +
` I G
IgG2b IgG3 IgM
IgA
:~ ....
In Table 1, "+" indicates that the reaction is positive, and "-" indicates that the reaction is negative.
Table 1 shows that the antibody in the culture 2~ supernatant o~ 3H3 cells belonss to IgGl in the i immunoglobulin class.
Example 4 (Purification of Monoclonal Antibody from Culture Supernatant and ~scites) ~1) Purification from Culture Supexnatant The combined solution of the culture supernatant of mouse 3H3 cells and a combining buffer [3 M sodium chloride, 1.5 8 glycine ~pH 8.7)] in a 1:1 ratio was loaded onto a ,;, . :
WO91/0~7~ PCT/JP90/01726 ~ . . i; ~.. , ~ ,.
Protein A column. After washing with a combining buffer, elution was carried out with an elution buffer [0.1 M citric acid (pH 5)]. To the eluate was added 1 M Tris (pH a.0) to neutralize it, followed by dialysis against physiological phosphate buffer.
The IgG amount of the samples was determined according ~`
to the method described in Example 2-t2) in the following manner. Various dilutions of mouse IgG whose concentration was known and the 3H3 antibody were fixed on a 96-well polystyrene microtiter plate with a fixing buffer. After 2 hours, the alkaline phosphatase- labeled anti-mouse IgG goat antibody (Bio RAD) was added thereto. After 2 hours, coloring reaction was conducted by adding a reaction substrate (ELISA method). With respect to mouse IgGl, a determination curve was drawn, and the IgG amount of the samples was determined based on this curve, whereby a 60 ~g/ml solution of the 3H3 antibody was prepared.
Fig. 6 shows the results of the antibody titer to rhbFGF mutein CS23 measured for the monoclonal antibody thus purified, according to the method described in Example 2-(2). One ~g/ml of the rabbit anti-bFGF polyclonal antibody was fixed and rhbFGF mutein CS23 was added thereto. Then, 1 ~ig/ml of the 3H3 antibody was added and 1 ~g/ml of the alkaline phosphatase-labeled anti-mouse IgG goat antibody 25 Wa5 further added thereto. By this method, rhbFGF mutein CS23 could be detected up to 3 ng/ml.
WO91/09X~5 PCT/JP9~/017~6 ~ r~
(2) Purification from Ascites Further, the antibody was purified from ascites. The mouse 3H3 cell strain was injected illtO the mice (Balb/c).
IgG was purified from the ascites according to conventional - 5 methods. Namely, 5 ml of the ascites was subjected to salt precipitation using a 45~ saturated solution of ammonium sulfate, and the precipitate was dissolved in borate buffer (BBS, pH 8.5) containing 0.15 M NaC1, followed by dialysis against BBS at 4C for 20 hours. The dialyzed solution was applied to a DE-50 column (1 cm diameter X 60 cm, Whatman, Great Britain), and the column was eluted with a linear gradient of 0.1 to 0.35 M NaCl in 0.1 M phosphate buffer ~pH
; 8.0), whereby 7 mg of monoclonal antibody 3H3 was obtained from 5 ml of the ascites.
Example 5 (Determination of Antigen Recognition Site) The antigen recognition site of the 3H3 antibody whose antibody titer was measured in Example 4 was examined by competitive binding inhibition experiments. As competitive substances, there were used human aFGF, rhbFGF, rhbFGF
mutein CS23, synthetic peptides pep 1: Pro-Ala-Leu-Pro-Glu-Asp-Gly-Gly-Ser-Tyr [the peptide in which Tyr was added to the C-terminus of N-terminal amino acids 2 to 10 of human bFGF, ~3L~ Y ~ , 10, 309-317 ~1985)] and pep 2:
Leu-Pro-Met-Ser-Ala- Lys-Ser (corresponding to amino acids 141 to 147, refer to European Patent Publication No.
288,687) and heparin sodium.
~O 91/09875 PCr/.lP90/0~726 The synthetic peptides, heparin sodium, human aFGF, rhbFGF and rhbFGF mutein CS23 were diluted with the buffer for dilution used in Example 2-~2) to a concentration of 100 ~g/ml. When the synthetic peptides, heparin sodium, human aFGF, rhbFGF and rhbFGF mutein CS23 were used as the competitive substances, 100 ng/ml of the 3H3 antibody and the competitive substance were suspended, and the suspension was maintained at 37C for 60 minutes.
The amount of antibody not com~ined in this solution was assayed by the EIA shown in Example 2-(2). The results are shown in Table 2.
Table 2 3H3 antibody Human bFGF +
Human aFGF
CS23 +
pepl pep2 Heparin sodium In Table 2, "~" indicates that the competitive inhibition occurred, and "-" indicates that the competitive inhibition did not occur. From these results, the recognition site of the 3H3 antibody is considered to be the peptide of 10th to 141st amino acids of human bFGF molecule ' :. ' - .. ~ . . , .:, . . . . .... . .. .. . .
WO9l/0~87s PCT/~P90/01726 - 37 ~ j7~
and binding site of human bFGF to human bFGF receptor or its adjacent site, other than the heparin combining site, or a region adjacent thereto.
Example 6 (Examination of Immuno-Neutralizing Action) As to the 3H3 antibody purified by the method of Example 4(1), the human bFGF-immunoneutralizing activity against rhbFGF was studied by the MTT method of Example 2-(3) (Fig. 7). Namely, the activity was assayed by 3-day proliferation in tbe presence of 2 ng/ml of bFGF of the human umbilical vein endo~helial ~H W E) cell. The proliferation inhibitory effect is shown by the absorbance at OD-590 nm in case of adding the monoclonal antibodies where the value is estimated as 100~ both in the presence of the bFGF and in the absence of the monoclonal antibody.
Referring to Fig. 7, - o - indicates the results of the 3H3 antibody, and - ~ - indicates the results of normal mouse IgG. The line of 44~ indicates the number of cells when the bFGF was not added. When the 3H3 antibody was added, 50 ng/ml thereof hindered the proliferation of the HUVE cells to the number of cells in the absence of the bFGF. The normal mouse IgG did not exhibit the proliferation inhibitory effect.
The assay was further changed to study the proliferation inhibition effect of the HUVE cells. Namely, the HUVE cells were seeded on a 24-well Linbro plate in an amount o~ l X 104 cells/well ~the culture conditions were37he same as with Example 2-t3)). The next day, 2 ng/ml of the bFGF and the 3H3 antibody were added thereto, ~, .. . ., ... . ~ .. . . .
' ' ,. . . ' . . . '. . ., ' ' ' ' ~ . . ., ' '.' , . , ` , , WOgl/09X7~ PCT/JP9~/Ot726 followed by cultivation for 3 days and for 5 days. Then, the number of cells was measured by using a Coulter counter (Coulter Electronics, Inc.) for each case. Referring to Figs. 8(A) and 8(B), Fig. 8(A) shows the results when cultivation was carried out for 3 days, and Fig. 8(B) shows the results when cultivation was carried out for 5 days.
The number of cells when the 3H3 antibody was added was expressed in percentage, taking the number of cells when the bFGF was added and the 3H3 antibody was not added as 100%.
In both of Fig. 8(A) and Fig. 8(B), - o - and - ~ - indicate the effect of the 3H3 antibody in the presence of 2 ng/ml of the bFGF and in the absence of the bFGF, respectively. The IC50 value of the proliferation hindrance (the amount of the antibody which hinders 50~ of cell proliferation when the antibody is not added) shows 13.2 and 7.6 ng/ml in Fig. 8(A) and Fig. 8(B), respéctively. Further, the 3H3 antibody did not affect the number of cells in the absence of the bFGF.
It is clear from the above data that the 3H3 antibody has strong immuno-neutralizing action to the biological activity of the bFGF.
Example 7 (Preparation of Horseradish Peroxidase-Labeled 3H3 Antibody) The purified 3H3 antibody (7 mg/ml) was dialyzed against 0.1 M acetate buffer (pEI 4~5) containing 0.1 M NaCl at 4C for 20 hours, followed by addition of pepsin (0.1 mg) (Sigma, U.S.A.). Then, digestion was carried out at 37C
for 8 hours. The solution was adjusted to pH 8 with l M
i`
., : . ., . , . . ,: : . ~
wo~l/09875 PCT/JP90/01726 ~ ,7`~
Tris to terminate the reaction. The resulting solutlon was placed on a column of Ultrogel AcA44 (IBF, France) and eluted with 0.02 M borate buffer ~pH 8.0) containing 0.15 M
NaCl to obtain F(ab')2. The solution containing F(ab')2 was concentrated to 1 ml. Thenl the concentrated solution was dialyzed against 0.1 M phosphate buffer (pH 6.0) at 4C for 20 hours, and 0.1 ml of a solution ~0.2 M mercaptoethyl-amine, 5 mM EDTA, 0.1 M phosphate buffer (pH 6.0)] was added, followed by reduction at 37C for 90 minutes. The reaction solution was placed on a Sephadex G-25 fine column (1 cm diameter X 60 cm, Pharmacia Fine Chemical, Sweden) and eluted with an eluent ~5 mM EDTA, 0.1 M phosphate buffer (pH
6.0)] to obtain an Fab' fraction.
Additionally, 10 mg of horseradish peroxidase (HRP, Behringer Manheim, West Germany) was dissolved in 1.5 ml of 0.1 M phosphate buffer (pH 7.0), and 3.5 mg of maleimidobutyloxy)succinimide ~GMBS) was dissolved in 100 ~1 of N,N-dimethylformamide ~DMF). The solution of GMBS
in DMF was added to the HRP solution, followed by stirring at 30C for 60 minutes. Then, the resulting solution was placed on the Sephadex G-25 fine column ~1.2 cm diameter X
60 cm) and eluted with 0.1 M phosphate buffer ~pH 7.0) to obtain maleimide group- introduced HRP ~maleimidated HRP).
Fab' and maleimidated HRP were mixed with each other to a mol ratio of 1:1, followed by reaction at 4C for 20 hours.
The reaction solution was applied to an ultrogel AcA44 column and eluted with 0.1 M phosphate buffer ~pH 7.0) to uosl/os~75 PCT/JP~0/01726 ~ q ~ - 40 -obtain an enzyme- labeled antibody (3H3-HRP).
Example 8 (preparation of Antibody-Sensitized Plate) MAbl2 or a 50-50 mixture of MAb52 and MAb98 was diluted with 0.1 M carbonate buf~er (pH 9.6) to a concentration of 10 ~g/ml. The resulting solution was poured in an amount of 100 ~1/well into an immunoplate for EIA ~Maxisoap: Nunc, Denmark), followed by standing at 4C overnight to sensitize or fix the antibody to the plate. After washing the plate with 0.01 M phosphate buffer (pH 7.0) containing 0.15 M
NaCl, 0.01 M phosphate buffer (pH 7.0) containing 0.1~ BSA
was poured into each well. Then, the plate was stored in a chilled place until its use.
Example 9 (Assay of Human bFGF) 1. Preparation of Calibration Curve A. Reaqents ~1) Enzyme-labeled antibody obtained in Example 7, (2) Antibody-sensitized microtiter plate obtained in Example 8, (3) Recombinant human bFGF ~rhbFGF): 0-50 ng/ml, ~4) Buffer AE0.02 M phosphate buffer (pH 7.0) containing 0.15 M NaCl], Bufer B~0.02 M phosphate buffer ~pH 7.Q) containing 25% Blockace ~blocking agent prepared from milk protein) (Dainippon Pharmaceutical), 0.15 M NaCl], ~ 5) Peroxidase substrate solution ~sodium citrate buffer ~pH 5.5) containing 0.02~ hydrogen peroxide and 0.15%
W091/09875 PCT/JPgO/01726 f. ~ r~
o-phenylenediamine], Enzyme reaction-terminating solution(2N sulfuric acid).
B. Assay Into each well of the antibody-sensitized plate obtained in Example 8, 100 ~1 of a solution of the bFGF (0.1 to lOOOpg/ml) in buffer B was added, followed by reaction at 4C for 24 hours. After washing each well with buffer A, 100 ~1 of an enzyme- labeled antibody solution diluted 200 times with buffer B was added to each well, followed by further reaction at 25C for 2 hours. Each well was washed with buffer A, and 100 ~1 of the peroxidase substrate solution was added thereto, followed by reaction at 25C for 30 minutes. Then, 100 ~1 of the enzyme reaction-terminating solution was added thereto to terminate reaction. The absorbance at 492 nm was thereafter measured by using an automatic colorimeter for microtiter plates (MTP-32.
Corona). Fig. 9 shows the relationship between the concentration of the hbFGF and the absorbance. Referring to Fig. 9, - o - and - ~ - indicate the relationship between the concentration of the hbFGF and the absorbance when the microtiter plate sensitized with MAbl2 was used and when the microtiter plate sensitized with the 50-50 mixture of MAbS2 and MAb98 was used, respectively. It was revealed that 20 pg/ml of the bFGF protein could be detected, when the plate was sensitized with MAbl2.
2. bFGF Immunoassay Kit and Assay of bFGF
The amount of the bFGF in the test samples was assayed Wo9l/09x7s ~T/JP90/01726 ~ 2 -by using the following bFGF immunoassay kit according to the following procedure:
A. Reagents (1) Enzyme labeled antibody (3H3 antibody-HRP) obtained in Example 7, (2) Antibody-sensitized microtiter plate obtained in Example 8, (3) Recombinant human bFGF (rhbFGF): 0-50 ng/ml, (4) Buffer A C0.02 M phosphate buffer ~pH 7.0) containing 0.15 M NaCl], Buffer B~0.02 M phosphate buffer (pH 7.0) containing 25% Blockace, 0.15 M NaCl], ~S) o-Phenylenediamine, (6) Buffer D used for dissolution of o-phenylenediamine 10.1 M citrate buffer (pH 5.5) containing 0.02 hydrogenperoxide and 0.005% thimerosal], ~7) Enzyme reaction-terminating solution (2N sulfuric : acid), B. Ass~y ~ .
Each well of the antibody-sensitized plate obtained in Example 8 was washed with buffer A, and 100 ~1 of a standard solution of the bFGF in buffer B or a solution of the test sample diluted with bufer B was poured thereinto, ollowed by reaction at 4C for 24 hours. After washing each well 25 with buffer A, 100 ~1 of an enzyme-labeled antibody solution ~:
diluted 200 times with buffer B was added to each well, followed by further reaction at 25C for 2 hours. After :: .
wn ~1/0987~
PCT/JP9OtOt726 washing each well with buffer A, 100 ~1 of a 0.15~ solution of o-phenylenediamine in buffer D was added thereto, followed by reaction at 25C for 30 minutes. Then, 100 ~1 of the enzyme reaction-terminating solution was added thereto to terminate reaction. The absorbance at 492 nm was thereafter measured by using an automatic colorimeter for microtiter plate ~MTP-32. Corona). The calibration curve of the standard bFGF was prepared, and the bFGF concentration was determined from the absorbance obtained for the test 10 samples.
Example 10 (Influence of Heparin in hbFGF Assay System) In Example 9-1, heparin was added to buffer B to a concentration of 0, 1, 10 or 100 ~g/ml, when the standard hbFGF was diluted. Then, the concentration of the hbFGF was assayed in the manner of Example 4-(1). As a result, there were observed no considerable changes in the standard curves with the presence of heparin, as shown in Figs. 10(1) and 10(2).
Referring to Figs. 10(1) and 10(2), Fig. 10~1) indicates the results when MAbl2 was fixed, and Fig. lOt2) indicates the results when the 50-50 mixture of MAb52 and MAb98 was ~ixed. Further in each igure, - -, - o ~
- and - ~ - indicate the results when heparin concentrations are 0, 1, 10 and 100 ~g/ml, respectively.
5 Example 11 ~Reactivity of Acid-Modified hbFGF in hbFGF Assay Systems) A 20 ~1 solution of the hbFGF (in 20 mM Tris-HCl buffer WO9l/09875 PCT/JP90/01726 ~" . ~.'`_J ~);
(pH 7.4) containing hbFGF at a concentration of 200~g/ml and containing 1 M NaC1 was added in an amount of 20 ~1 to laO
~1 of 1 M acetate buffer, followed by incubation at 25C for 0, 1, 3 or 10 minutes. 400 ~1 of 1 M Tris was added thereto to neutralize it, and ~hen the resulting solution was diluted with buffer B used in Example 9-1. Then, calibration curves were prepared for respective incubation times according to the method of Example 9-1, as shown in Figs. 11(1) and 11(2). Referring to Figs. 11(1) and 11(2), Fig. 11(1) indicates the results when MAbl2 was solidified, and Fig. 11(2) indicates the results when the 50-50 mixture of MAb52 and MAb98 was solidified. Further in each figure, - O -, - O -, - a - and - ~ indicate the results when the hbFGF was incubated at pH 4 for 0, 1, 3 and 10 minutes, respectively. Figs. 11(1) and 11~2) show that the hbFGF
modified at pH 4 is reduced in reactivity to about 1~ by incubation for 10 minutes in each assay system. The assay systems of Example 9 are assay systems by which only the native hbFGF can be assayed.
Example 12 (Assay of bFGF in Various Cells) A375 (human melanoma), A431 ~human sguamous cell carcinoma)~ A549 ~human lung cancer), SK-Hepl ~human hepatic cancer) ~all o them were supplied by ATCC, U~S.A.) and human umbilical vein endothelial cells were each scraped in an amount of 2 to 6 X 107 cells by a cell scraper. The cells were washed twice with a phosphate buffered saline ~PBS, pH 7.2) containing 0.15 M NaCl, and then 0.6 ml of PBS
'~.
W~gl/0~75 PC~/JP~0/~1726 .
- 45 - ~r ~ ?
was added thereto, followed by ultrasonication under ice cooling for 25 seconds. After centrifugation at 15,000 rpm, the concentration of the bFGF in the supernatant was determined according to the method of Example 9-2.
The results are shown in Table 3. In Table 3, A shows the results when MAbl2 was fixed, and ~ shows the results when the 50-50 mixture of MAb52 and MAb98 was fixed.
Table 3 Amount of bFGF in Cell ~' .
Amount of bFGF
: A B
~ame of Cell(pg/106 cells)(ng/106 cells) A375 1.4 4.0 A431 1.5 0.5 A549 8.4 8.5 SK-Hepl 4 . 0 11. 7 HUVE 11 . 7 0 . 8 4 From Table 3r it is observed that the difference in measured amount of bFGF between the A assay system and the B
assay system is great. From this fact, the possibility is considered that the N-terminus of the bFGF is cleaved during extraction operation, or that the ~-terminus of the actually produced bFGF is cleaved or masked.
Example 13 (Antitumor Effect to KlO00 Tumor) The KlO00-Fl cells obtained in Reference Example 2 were ~.
wosl/0987s PCT/JP90/01726 sub ~ a~o~ impLanted in an amount of 3 X lO6 cells/mouse into nude BALB/c mice. Three days after implantation, the 3H3 antibody obtained in Example 4 and nonimmune mouse IgG
were given to the caudal veins in a dose of 200 ~g/mouse/day continuously for 5 days. After implantation, the diameter of the tumors was measured, and the volume thereof ~=0.5 X
(major axis) X (minor axis)2] was calculated. The results are shown in Fig. 12. Referring to Fig. 12, - ~ -, - 4 -and - ~ - indicate the results for an untreated control group, a nonimmune mouse IgG-given group and a 3H3 antibody-given group, respectively. The 3H3 antibody exhibited antitumor effect against the RlO00 tumor (14 days after implantation, the 3H3 antibody-given group is decreased in tumor volume to 34% of that of the untreated control group). The antitumor effect of nonimmune mouse IgG
was not observed. ;
,', ~';'~
,:
., . , ' :
` , ' '~
~
.
.:
~ ' ;~, ~91/0987~ PCT/JP90/017Z6 Incorporated by refere~ce ~ature 249, 123 ~1974) Biophys. Res. Commun. 151, 701 (1988) European Patent Publication No. 281,822 FEBS Letters 213, 189 ~1987) Biophys. Res. Commun. 146, 470 (1987) European Patent Publication No. 237,966 J. Immun. Method 80, 55 tl985) Nature 256, 495 (1975) J. Am. Med. Assoc. 199, 549 (1967) Metabolism, 8, 696 (1971) Hybridoma, 8, 209-221 (1989) European Patent Publication No. 288,687 Biotechnology, 5, 960 (1987) ICUS Short Report, vol. 8, Advances in Gene Technology;
Protein Engineering and Production, Proceedings of the 1988 Miami Bio/Technology Winter Symposium, page 110, IRL
Press J. Mol. Biol., 189, 113-130 (1986) Mol. Cell. Biol. 8, 588-594 ~1988) Methods in Enzymology 101, 20-78 (1983) ~apanese Patent Unexamined Publication tLaid-Open) No.
2-193/1990 ~European Patent Publication No. 281,822) Japanese Patent Unexamined Publication (Laid-Open) No. 62-175182/1987 (EP-225,701) Science, 209, 505-507 (1980) Virology, 8, 396 (1959) Virology, 52, 456 (1973) U.S.P. No. 4,654,304 Regulatory Peptides, 10, 309-317 (1985)
Claims (23)
1. A monoclonal antibody which has the following characteristics, immuno-neutralizes the activity of a basic fibroblast growth factor (bFGF) protein and highly sensitively combines with the bFGF protein:
(a) a molecular weight of about 140,000 to 160,000:
(b) does not cross-react with acidic fibroblast growth factor, (c) belongs to immunoglobulin class IgG1, (d) binds with rhbFGF mutein CS23 (a mutein in which the cysteine residues at positions 70 and 88 of hbFGF are substituted for serine residues), (e) it completely inhibits proliferation of a human umbilical vein endothelial (HUVE) cell by addition of 50 ng/ml thereof in the presence of 2 ng/ml of bFGF, and (f) it can determine 20 pg/ml of the bFGF protein by a sandwich enzyme-linked immunosorbent assay (ELISA) using monoclonal antibody MoAb12 (solid phase) and a peroxidase-labeled antibody.
(a) a molecular weight of about 140,000 to 160,000:
(b) does not cross-react with acidic fibroblast growth factor, (c) belongs to immunoglobulin class IgG1, (d) binds with rhbFGF mutein CS23 (a mutein in which the cysteine residues at positions 70 and 88 of hbFGF are substituted for serine residues), (e) it completely inhibits proliferation of a human umbilical vein endothelial (HUVE) cell by addition of 50 ng/ml thereof in the presence of 2 ng/ml of bFGF, and (f) it can determine 20 pg/ml of the bFGF protein by a sandwich enzyme-linked immunosorbent assay (ELISA) using monoclonal antibody MoAb12 (solid phase) and a peroxidase-labeled antibody.
2. A monoclonal antibody in accordance with claim 1, in which said bFGF protein is a polypeptide containing the following amino acid sequence:
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
3. A cloned hybridoma derived from fusing a spleen cell of a mammal and a homogenic or heterogenic lymphoid cell, said mammal being immunized with a mutein in which at least one cysteine residue of bFGF is substituted for a serine residue.
4. A hybridoma in accordance with claim 3, in which said mammal is a mouse.
5. A hybridoma in accordance with claim 3, in which said lymphoid cell is a myeloma cell.
6. A hybridoma in accordance with claim 3, in which said mutein is a polypeptide containing the following amino acid sequence:
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
7. A hybridoma according to claim 6 which has the characteristics of mouse 3H3 cell.
8. A method for producing a cloned hybridoma comprising a spleen cell from a mammal and a homogenic or heterogenic lymphoid cell, said mammal being immunized with a mutein in which at least one cysteine residue of bFGF is substituted for a serine residue, which comprises subjecting said spleen cell and said lymphoid cell to cell fusion, followed by cloning.
WO 9l/09875 PCT/JP90/01726
WO 9l/09875 PCT/JP90/01726
9. A method in accordance with claim 8, in which said mammal is a mouse.
10. A method in accordance with claim 8, in which said lymphoid cell is a myeloma cell.
11. A method in accordance with claim 8, in which said mutein is a polypeptide containing the following amino acid sequence:
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
12. A method for producing the monoclonal antibody claimed in claim 1, which comprises culturing a cloned hybridoma comprising a spleen cell from a mammal said mammal being immunized with a mutein in which at least one cysteine residue of bFGF is substituted for a serine residue, and a homogenic or heterogenic lymphoid cell in a liquid culture medium or in a peritoneal cavity of the mammal under conditions suitable for antibody production, and recovering the antibody produced.
13. A method in accordance with claim 12, in which said mammal is a mouse.
14. A method in accordance with claim 12, in which said lymphoid cell is a myeloma cell.
15. A method in accordance with claim 12, in which said mutein is a polypeptide containing the following amino acid sequence:
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
16. A method for purifying a bFGF protein, which comprises using the monoclonal antibody claimed in claim 1.
17. A method for detecting or measuring a bFGF
protein, which comprises using the monoclonal antibody claimed in claim 1.
protein, which comprises using the monoclonal antibody claimed in claim 1.
18. A method in accordance with claim 17, in which said bFGF is mutein containing the following amino acid sequence:
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
Phe-Phe-Leu-Arg-Ile-His-Pro-Asp-Gly-Arg-Val-Asp-Gly-Val-Arg-Glu-Lys-Ser-Asp-Pro.
19. A method in accordance with claim l7, in which the bFGF protein is detected or measured by an enzyme immunoassay.
20. A kit of reagents for detecting or measuring a bFGF protein which comprises the monoclonal antibody according to claim 1.
21. The kit of reagents according to claim 20, wherein the monoclonal antibody is produced by the cloned hybridoma according to any of claims 3-5.
22. The kit of reagents according to claim 21, wherein the bFGF protein is a mutein in which at least one cysteine residue of bFGF is substituted for a serine residue.
23. The kit of reagents according to claim 21, which is used in an enzyme-linked immunosorbent assay.
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP33836989 | 1989-12-28 | ||
| JP338369/1989 | 1989-12-28 | ||
| JP169707/1990 | 1990-06-29 | ||
| JP16970790 | 1990-06-29 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2069872A1 true CA2069872A1 (en) | 1991-06-29 |
Family
ID=26492964
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002069872A Abandoned CA2069872A1 (en) | 1989-12-28 | 1990-12-27 | Monoclonal antibody, hybridomas, their production and use |
Country Status (4)
| Country | Link |
|---|---|
| EP (1) | EP0507948A1 (en) |
| JP (1) | JPH05503842A (en) |
| CA (1) | CA2069872A1 (en) |
| WO (1) | WO1991009875A1 (en) |
Families Citing this family (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN104231079A (en) * | 2014-09-12 | 2014-12-24 | 暨南大学 | Antibody targeting high affinity bFGF receptor binding site and application thereof |
Family Cites Families (6)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JPS60145088A (en) | 1984-01-07 | 1985-07-31 | Agency Of Ind Science & Technol | Production of composition for cultivation of animal cell |
| US4935352A (en) | 1985-10-21 | 1990-06-19 | Takeda Chemical Industries, Ltd. | Expression vector for animal cell line and use thereof |
| IL81839A0 (en) | 1986-03-14 | 1987-10-20 | Takeda Chemical Industries Ltd | Polypeptide,dna and its use |
| JP2526965B2 (en) | 1987-02-24 | 1996-08-21 | 武田薬品工業株式会社 | Muteins, DNAs and their uses |
| DE3852561T2 (en) | 1987-03-03 | 1995-07-13 | Takeda Chemical Industries Ltd | Monoclonal antibodies, hybridomas, their production and their use. |
| JP2506944B2 (en) | 1988-06-13 | 1996-06-12 | 松下電器産業株式会社 | Wavelength tunable laser device |
-
1990
- 1990-12-27 EP EP91901637A patent/EP0507948A1/en not_active Withdrawn
- 1990-12-27 CA CA002069872A patent/CA2069872A1/en not_active Abandoned
- 1990-12-27 JP JP3501880A patent/JPH05503842A/en active Pending
- 1990-12-27 WO PCT/JP1990/001726 patent/WO1991009875A1/en not_active Application Discontinuation
Also Published As
| Publication number | Publication date |
|---|---|
| WO1991009875A1 (en) | 1991-07-11 |
| EP0507948A1 (en) | 1992-10-14 |
| JPH05503842A (en) | 1993-06-24 |
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