CA2137785A1 - Immunoassay and test kit for thrombin-antithrombin iii complex - Google Patents
Immunoassay and test kit for thrombin-antithrombin iii complexInfo
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- CA2137785A1 CA2137785A1 CA 2137785 CA2137785A CA2137785A1 CA 2137785 A1 CA2137785 A1 CA 2137785A1 CA 2137785 CA2137785 CA 2137785 CA 2137785 A CA2137785 A CA 2137785A CA 2137785 A1 CA2137785 A1 CA 2137785A1
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/40—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against enzymes
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N33/00—Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
- G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
- G01N33/50—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
- G01N33/86—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving blood coagulating time or factors, or their receptors
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N2333/00—Assays involving biological materials from specific organisms or of a specific nature
- G01N2333/81—Protease inhibitors
- G01N2333/8107—Endopeptidase (E.C. 3.4.21-99) inhibitors
- G01N2333/811—Serine protease (E.C. 3.4.21) inhibitors
- G01N2333/8121—Serpins
- G01N2333/8128—Antithrombin III
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N2333/00—Assays involving biological materials from specific organisms or of a specific nature
- G01N2333/90—Enzymes; Proenzymes
- G01N2333/914—Hydrolases (3)
- G01N2333/948—Hydrolases (3) acting on peptide bonds (3.4)
- G01N2333/974—Thrombin
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Abstract
The present invention provides an immunoassay for thrombin-antithrombin complex in a human fluid sample. The assay comprises reaction of a human fluid sample with at least two antibodies or immunoreactive fragments thereof, wherein at least one of the antibodies binds to thrombin-antithrombin III complex in the sample, but exhibits essentially no cross-reactivity with antithrombin III and complexes of antithrombin III with other serine proteaste factors.
Description
IMMUNOASSAY AND TEST KIT
FOR THROMBIN-ANTITHROMBIN lll COMPLEX
BACKGROUND OF THE INVENTION
1. Field of the Invention The present invention relates an immunoassay for thrombin-5 anliLhro",bin lll complex which comprises antibodies that specifically bind to the complex in a human fiuid sample.
FOR THROMBIN-ANTITHROMBIN lll COMPLEX
BACKGROUND OF THE INVENTION
1. Field of the Invention The present invention relates an immunoassay for thrombin-5 anliLhro",bin lll complex which comprises antibodies that specifically bind to the complex in a human fiuid sample.
2. Background General agreement exists that blood co~glJI~tion or c!otting includes 10 three essential steps: 1) a complex of subst~nces called prothrombin activator is formed e.~. in ~esl.onse to rupture of a blood vessel or damage to blood itself; 2) the proll,rombin activator catalyzes the conversion of p,oli,ro,nbin to thrombin; and 3) lhloll)bil1 acts as an enzyme to activate elet~ and to convert fibrogen into fibrin threads that enmesh platelets 15 blood cells and plas"~a to form the clot itself.
The enzymatic activity of thrombin can be regulated in various ways including the formation of an inactive complex with alllilhro~bin lll known as the thrombin-antithrombin lll complex or the ~TAT complex~.
20 AnliUIlo"~l~in 111 or UATIII" is a proteinase inhibitor in plasma that complexes with several serine proteinases in addition to thrombin. Thus ATIII is known to form complexes with serine protease factors Xlla Xla Xa and IXa.
It is desi,a~le to measure the amount of TAT complex in a human 25 fluid sample. Determination of levels of the TAT complex will provide an WO 941245~K PCT/US94/03885 .
2 131~ 8~ - 2 -indication of coagulation activity of a patient and aid in the assessment of thrombotic risk and other disorders such as disseminated intrav~scul~r co~gul~tion.
An assay for TAT complex levels in human plasma should provide a selective assessment of TAT complex concentrations, rather than a measurement of the concentration of total complexes of ATIII in a plasma sample, e.g. complexes of ATIII with factors Xlla, Xla, Xa and IXa in addition to the TAT complex. Such measurement of the "total" complexes of ATIII
provides an indication of the equilibrium of several reactions, some of which may reflect conditions other than those associated with particular TAT
complex levels. For instance, contact activation of factors Xll and Xl may lead predominantly to activation of the complement and kinin systems, therefore Xlla-ATIII and Xla-ATIII complexes may not be indicative of thrombotic risk.
It thus would be desirable to have a means for determining levels of the TAT complex in a human fluid sample. It would be particularly desirable to have an assay for the concentration of TAT complex in a human fluid sample where the assay provided a selective assessment of concenL,alioils of the TAT complex in a test sample, rather than a measurement of the sample's total complexes of ATIII.
SUMMARY OF THE INVENTION
The present invention provides an immunoassay for the detection and measurement of concenl,alion of a human thrombin-anLiLl,rombin lll (TAT) complex in a human fluid sample. The assay comprises contact of a human fluid sample with at least two antibodies or immunoreactive fragments thereof, preferably monoclonal antibodies or reactive fragments wo 94~ 2 1 3 7 7 8 S ~/US94103885 thereof, wherein at least one of the antibodies specifically binds to the TAT
complex in the fluid sample. Preferably each~ of the antibodies of the assay specifically binds to the TAT complex. As use~ herein, "specifically binds to the TAT complex" or other similar phrase indicates that the antibody or 5 antibodies bind to the TAT complex but exhibit substantially or essentially no cross-reactivity with free (i.e., not complexed) antithrombin lll or antithrombin lll complexes of other plasma factors, specifically factor Xa-antithrombin lll complex and factor IXa-antithrombin lll complex. Preferably the mixture of antibodies of the assay bind to different epitopes of the TAT
10 complex, i.e. the antibodies are not competitive. Additionally, the antibodies of the immunoassay of the invention preferably are contacted simultaneously with a human fluid sample so that only a single incubation and wash step is employed. Other aspects of the invention are disclosed infra.
DETAILED DESCRIPTION OF THE INVENTION
The immunoassay of the invention comprises reaction of at least two antiho~ies with a human fluid sample, wherein at least one of the antibodies specifically binds to said TAT complex. rleferably the antibodies are 20 monoclonal antibodies and both of said two antibodies of the assay specifically bind to the TAT complex. The antibody or antibodies of the assay that specifically bind to the TAT complex preferably exhibit less than about 3% cross-reactivity, in an assay such as that described in Example 7 below or similar assay with a human plasma sample, with ATIII, factor Xa-25 a"lilhr~",bin lll complex and factor IXa-antithrombin lll complex. More pre~erably the antibody or antibodies of the invention exhibit less than about 1% cross-reactivity with ATIII and such ATIII complexes. Still more preferably the antibody or antibodies of the invention exhibit less than about 0.2%, or even less than about 0.1% cross-reactivity with antithrombin lll and WO 94/24566 . PCT/USg4/03885 2~3'11~S 4 such ATIII complexes in an assay as described in Example 7 below or similar assay using a human plasma sample. It is also preferred that antibodies of the invention exhibit su~ch~lack of cross-reactivity with free (not complexed) thrombin, i.e. the antibodies of the invention preferably exhibit 5 less than about 3% cross-reactivity with free thrombin in reaction with a human plasma sample, more preferably exhibit less than about 1% cross-reactivity with thrombin, and still more preferably exhibit less than about 0.2%, or even less than about 0.1% cross-reactivity with free thrombin upon contact reaction of the antibody with a human plasma sample. In particular, 10 it was found that specifically preferred monoclonal antibodies of the invention upon contact with a human fluid sample bind to human TAT
complex and exhibited less than about 0.005% cross-reactivity with thrombin, less than about 0.005% cross-reactivity with antithrombin lll, less than about 0.005% cross-reactivity with factor IXa-antithrombin lll complex 15 and less than about 0.02% cross-reactivity with factor Xa-antithrombin lll complex. "Antibody", "antibody of the invention~ or other similar term as used herein includes a whole immunoglobulin as well as antigenic binding fragments or immunoreactive fragments which specifically bind to the TAT
complex, including Fab, Fab', F(ab')2 and F(v).
If only one antibody of the immunoassay specifically binds to the TAT
complex, the other antibody of the assay should bind to the TAT complex but also may exhibit cross-reactivity, e.g. with anLi~hrombin lll or other complexes of a"lill,ro,t,bin lll. Thus references herein to an antibody that 25 "binds" to TAT complex, rather than specifically binds thereto, indicates that the antibody binds to the human TAT complex and also may exhibit cross-reactivity with antithrombin lll, factor Xa-antithrombin lll complex and/or factor IXa-antithrombin lll complex. Antibodies, including monoclonal antibodies, that bind to the TAT complex and also exhibit cross-reactivity wo 94~ 2 1 3 7 7 8 5 pcTlus94lo388s with anlill,ro",bin lll and complexes thereof have been reported. See J.
Dawes, et al., Thrombosis Research, 36:397 (1984); S. Asakura, et al., Bioch. et Bio~hy. Acta, 952:37 (1988); Z. Hrkal, Hybridoma, 10(5):633 (1991); and European Published Patent Application No.0391433A2. In this S embodiment of the invention, preferably the antibody that specifically binds to the TAT complex is used as a carrier antibody and is immobilized on a substrate in a sandwich-type assay, and the cross-reactive antibody is used as the labeled conjugate, although the cross-reactive antibody also can be used as the carrier antibody and the antibody that specifically binds to the 10 TAT complex can be used as the labeled conjugate.
The human fluid sample used in the assay of the invention can be any sample that contains the TAT complex, e.g. blood or urine. Typically a plasma sample is employed.
Antibodies of the invention can be prepared by techniques generally known in the art, and are typically generated to a purified sample of a TAT
complex of human plasma. The antibodies also can be generated from an immunogenic peptide that comprises one or more epitopes of the TAT
20 complex that are not exhibited by free ATIII or thrombin.
More particularly, antibodies can be prepared by immunizing a mamrnal with a purified sample of a TAT complex, or an immunogenic peptide as discussed above, alone or complexed with a carrier. Suitable 25 ma~,n,als include typical laboratory animals such as sheep, goats, rabbits, guinea pigs, rats and mice. Rats and mice, especially mice, are preferred for obtaining monoclonal antibodies. The antigen can be ad",i,-i;,tered to the mammal by any of a number of suitable routes such as subcutaneous, intraperitoneal, intravenous, intramuscular or intracutaneous injection.
wo 94~SC6 PCTnUS94/~ ~5 Preferably immunization is by subcutaneous, intraperitoneal, or intravenous injection. The optimal immunizing interval, immunizing dose, etc. can vary within relatively wide ranges and can be :determined empirically based on this disclosure. Typical procedures involve injection of the antigen several times over a number of weeks. Antibodies are collected from serum of the immunized animal by standard techniques and screened to find antibodies specific for the TAT complex. Monoclonal antibodies can be produced in cells which produce antibodies and those cells used to generate monoclonal antibodies by using standard fusion techniques for forming hybridoma cells. See G. Kohler, et al., Nature, 256:456 (197~). Typically this involves fusing an antibody producing cell with an immortal cell line such as a myeloma cell to produce the hybrid cell. Alternatively, monoclonal antibodies can be produced from cells by the method of Huse, et al., Science. 256:1275 (1989).
One suitable protocol provides for intraperitoneal immunization of a mouse with a composition comprising purified TAT complex conducted over a period of about two to seven months. Spleen ceils then can be removed from the immunized mouse. Sera from the immunized mouse is assayed for titers of antibodies specific for TAT complex prior to excision of spleen cells. The excised mouse spleen cells are then fused to an appropriate homogenic or heterogenic (preferably homogenic) Iymphoid cell line having a marker such as hypoxanthine-guanine phosphoribosyltransferase deficiency (HGPRr) or thymidine kinase deficiency (TK-). Preferably a myeloma cell is employed as the Iymphoid cell line. Myeloma cells and spleen cells are mixed together, e.g. at a ratio of about 1 to 4 myeloma cells to spleen cells. The cells can be fused by the polyethylene glycol (PEG) method. See G. Kohler, et al., Nature, supra. The thus cloned hybridoma is grown in a culture medium, e.g. RPMI-1640. See G. E. More, wo g4~ 2 1 3 7 7 8 S ~/US94103885 et al., Journal of American Medical Association, 199:549 (1967).
Hybridomas, grown after the fusion procedure, are screened such as by radioimmunoassay or enzyme immunoassay for secretion of antibodies that bind specifically to the TAT complex, e.g. antibodies are selected that bind 5 to the TAT complex, but not to ATIII. Preferably an ELISA is employed for the screen. Hybridomas that show positive results upon such screening can be ex~,anded and cloned by limiting dilution method. Further screens are preferably performed to select antibodies that can bind to TAT complex in solution as well as in a human fluid sample.
Antibodies of the invention preferably show an affinity constant with the TAT complex of greater than about 1 x 104 L/M, more preferably greater than about 1 x 105 L/M, still more preferably greater than about 1 x 108 L/M, such constants determined by the method disclosed in Friguet, et al., J. Immunol. Methods, 77:305 (1985).
Preferred antibodies of the invention are highly sensitive for TAT
complex in a human fluid sample. For example, it was found that preferred antibodies detected with precision a concenl,alion of TAT complex of about 20 0.55 ng or greater per ml of plasma sample with recovery of spiked material being essentially 100%.
Immunoassays of the invention generally exhibit good precision. For example, the following results were found for preferred assays of the 25 invention: within assay values for control levels I and ll for n-80 of 3.9% CV
and 6.8% respectively; and between assay precision values for n=80 of 9.3% and 12.2% CV respectively.
WO 94/245CC PC~/US94tQ~885 2~3~7~S
Competitive assays have shown that preferred antibodies of the invention are at least substantially or essentially non-competitive, i.e. two ormore antibodies of the invention show little or no binding interference among themselves when reacted simultàneously with a sample of TAT
5 complex. By use of such antibodies in an immunoassay, a test sample can be incub~ted simultaneously (i.e., single incubation step) with both the bound capture antibody and labeled conjugate antibody of the assay. This is distinct from prior assays that utilize separate incubation and wash steps for each of the capture and conjugate antibodies, e.g. to avoid binding 10 interference between the antibodies.
It has also been found that preferred antibodies of the invention can bind to TAT complex of a human fluid sample, particularly a human plasma sample, that is not diluted, or is diluted only by the solution containing the 15 TAT complex antibody. In particular, it has been found that preferred antibodies of the present invention can bind to TAT complex of a human fluid sample where the fluid sample is diluted only by an equal volume or less of a diluent. This is distinct from at least some prior antibodies that arereported to bind to TAT complex, but will only do so when contacted with a 20 ~JIas",a sample that is diluted to a significant extent, e.g. when a plasma or other test sample is diluted 100 times or more. Such dilution is undesirable as it can add to the complexity of a TAT complex assay that utilizes such antibodies.
Specifically preferred monoclonal antibodies of the invention include D2M, C72, C44-T and SB46, which are mouse monoclonal antibodies that specifically bind to the TAT complex. Hybridomas expressing such monoclonals have been deposited with the American Type Culture Collection (ATCC), 12301 Parklawn Drive, Rockville, Maryland 20852 and wo g4124566 2 1 3 778 5 given Accession No. _ (TAT-4-C44-T-3:ST; expresses C44-T); Accession No. _tTAT-5-B46-4; expresses 5B46); Accession No. _ (TAT-4-C72E;
expresses C72); Accession No. _(TAT-1-D2M; expresses D2M).
Thus antibodies of the invention are particularly suitable for use in an immunoassay for detecting and measuring the concen~lalion of TAT
complex in a human fluid sample. A particularly prefer,ed immunoassay of the invention is a sandwich assay in which the capture antibody is immobilized using known methods such as physical adsorption onto the surface of a support. Suitable supports include, e.g., polymer materials such as polypropylene or polystyrene, glass, metals, cross-linked dextran, agarose, etc. The support may be in a variety of shapes such as a tray, sphere, rods, test tube, etc. A tray having wells such as a miclolilre plate is generally preferred.
The detectably labeled antibody of the assay is formed by coupling the antibody to a reporter, e.g. a radioactive isotopes, an enzyme, a fluorescent or luminescent reagent and the like. Typically used radioactive isotopes '251, Tc99m and 3H. Known isotope labeling methods include iactoperoxidase and Hunter-Bolton methods for t251 and reduction methylation for 3H. See A. Bolton, et al., Biochem. J., 133:529-539 (1972).
Enzyme tags may include peroxidases, alkaline phosphatases, ~-D-galactosidases, glucoseoxidases, and the like. Peroxidases are particularly preferred. The peroxidases can be selected from those derived from various sources, e.g. horseradish, pineapple, fig, sugarcane, java bean, corn. Horseradish peroxidase is a particularly preferred material. Means for covalent labeling of an antibody with such enzymes are known in the art.
Methods suitable for a specific enzyme and antibody can depend on wo s4n4sc6 Pcrluss4lo388s 2~3r~ 5 10-available reactive moieties on the enzyme and antibody and can be readily asce,lained empirically.
``:
The assay of the invention is illustrated by the following protocol 5 using peroxidase as the labei of the conjugate antibody. A test sample, e.g.
a human plasma sample, is added to a TAT complex antibody (i.e., an antibody that binds to the TAT complex) bound on a carrier such a microtiter plate and the antibody-antigen reaction is conducted, followed by addition of the peroxidase labeled TAT complex antibody conjugate 10 obtained as outlined above, and then a further antibody-antigen reaction conducted. The antibody are- typically dissolved in solution prior to contact with a test sample. Suitable diluents include those known in the art for use in immunoassays. A specifically preferred solution for dissolving the antibodies for contact with a test sample contai,)s 20 mmol Tris, 500 mmol 15 sodium chloride, 0.05 mg/ml mouse IgG and 5% BSA.
Preferably both the carrier and conjugate antibodies of the assay of the invention specifically bind to the TAT complex, and the antibody bound to the support, the human fluid sample and labeled antibody are incubated 20 together, followed by a single wash step to remove any unreacted labeled antibody and the human plasma sample other than the reacted TAT
complex. Suitable washing agents include those known in the art for use in immunoassays. A specifically preferred washing buffer solution contains 27.2 9/l imidazole, 17.5 9/l sodium chloride and 4 ml/liter Tween 20. If 25 necessary a substrate for peroxidase is added to the assay and the reaction products are assayed for enzyme activity by measuring the absorbance or fluorescence of the resulting substance. The detected amount of bound labeled antibody is directly proportional to the concentration of TAT complex in the assayed human plasma sample. Thus wo g4~ 2 1 3 7 7 8 5 PCr/uss4lo388s a qua"LiLa~ive determination of the TAT complex concentration in the plasma test sample can be dete",~ined by comparison of the absorbance or fluorescence of the test sample with absorbance values obtained from standardized solutions that contain known amounts of TAT complex. It may 5 be desirable to prepare calibration curves from absorbance values obtained from a number of standardized solutions to facilitate interpretation of values obtained from a test sample.
A specifically preferred immunoassay of the invention was conducted 10 as follows. The capture monoclonal antibody and conjugate monoclonal antibody labeled with horseradish peroxidase (HRP) is incubated together with a human plasma sample at 37~C for 30 rninutes. The plate is then washed and incubated for 15 minutes at room temperature with HRP
substrate and the bound conjugate is quantitated.
A preferred immunoassay of the invention was used to measure plasma samples in individuals (n=15) with Disseminated Intravascular Coagulation. Assay results showed TAT complex levels significantly elevated in all but one patient plasma sample. Twelve of the individuals 20 tested had levels of TAT complex greater than 160 ng/ml.
TAT complex can be purified from a human plasma sample by use of carrier complexes coupled with one or more antibodies of the invention and hence the invention includes methods for obtaining purified TAT complex 25 using the antibodies of the invention and related apparatus. A suitable purification procedure provides coupling an antibody of the invention on an appro,c,riate carrier as is known in the art such as a gel or resin then packing the carrier in a column and then eluting a sample solution containing TAT complex through the column to selectively adsorb the TAT
WO g4/245C6 PCT/US94/03885 2~3rt ~l 8,S
complex. The antibody can be suitably coupled onto the carrier by known methods, e.g. the cyanogen bromide method and glutaraldehyde method, aqueous carbodiimide method, active ester method, and the like. The antibody also may be physically adsorbed orl the surface of the carrier.
The antibodies of the invention also can be used to locate and monitor TAT complex in vivo. For example, one or more antibodies of the invention can be labeled with a radionuclide such as 11-indium. The labeled antibody then can be injected intravenously into a human and the 10 human scanned to determine where the labelled antibody accumulates.
The labeled antibody typically will differentially accumulate in areas having high concentrations of TAT complex, e.g. where blood clotting is occurring such as in a hemorrhage site. The amount of labeled antibody can be determined by known scanning methods such as by using a scintigraphic 1 5 camera.
The antibodies of the invention also can be used therapeutically, e.g.
as a carrier for drugs, particularly pharmaceuticals targeted for interaction inthe blood clotting mechanism such as strepo-kinase, TPA and urokinase.
20 The pharmaceutical can be attached to an antibody of the invention by the same means as attachment of a label as specified above, e.g. by a covalent linkage that does not inhibit the specificity of the antibody or the desired pharmacological effect of the drug. The antibody with the attached pl,ar,l,aceutical can be administered to a human in therapeutically effective 25 amounts by any of a number of known means, e.g. parenterally or orally.
For parenteral adminisl,alion the antibody with attached pharmaceutical is typically administered in aqueous and non-aqueous sterile iniection compositions as are known in the art. For oral administration the therapeutic of the invention may be administered to a human in discrete WO g41245C6 PCI IUS94/03885 21~7785 units such as capsules or tablets each containing a predeter",ined amount of the therapeutic, as a solution or a suspension in an aqueous or non-aqueous liquid, as an oil/water liquid emulsion, in powdered carriers such as lactose or sucrose, etc.
All documents mentioned herein are incorporated by reference herein in their entirety.
The following non-limiting examples are illustrative of the invention.
General Comments Purified samples of TAT complex used in the following Examples were generally obtained by procedures described in G. Elgue, et al., Thrombosis and Hemostasis, 63(3):435 (1990). In brief, thrombin and antithrombin lll were reacted and the resultant TAT compiex was isolated by gel filtration. 20% Complete Medium used in the Examples had the following composition per 100 ml:
1 ml 200 mM 1-glutamine, 1 ml 7.5% Na-bicarbonate, 1 ml 5000 u/ml Penicillin & 5000 mcg/ml Streptomycin, 0.05 ml 0.1M 2 ~-mercaptoethanol, 20 ml Fetal Bovine Serum, and to 100 ml with RPMI 1640 (Gibco) without L-glutamine.
HAT media used in the Examples had the following composition: to 100 ml of Complete Medium 1 ml 100X Hypoxanthine Thymidine and 2 ml SOX Aminopterin were added. HATG media used in the Examples had the following composition: to 100 ml of HAT media 1 ml 100X Glycine was added. IL-6 used in the Examples was prepared by adding 500 units 2l37785 Human Recombinant IL-6 (Collaborative Research Inc.) per ml medium.
STM used in the Examples was prepared by adding 5 ~9 salmonella typhimurium mitogen (Ribi Immunochemical Research, Inc.) per ml medium.
5 Example 1 - Immunization The following two groups of BALB/c female mice were immunized with TAT complex to provide spleen donors for the PEG fusions, disclosed below, that generated monoclonal antibodies that specifically bind to the TAT complex.
1. Group 1 BALB/c female mice were sensitized with 7 ~9 each of purified TAT
complex in immunogen emulsion prepared as follows:
0.125 ml TAT complex (325 l~g/ml in 50 mM tris/50 mM NaCI/0.1 M
15 EDTA pH 7.4) 1.500 ml Complete Freund's Adjuvant 1.375 ml Dulbecco's Phosphate Buffered Saline Each mouse was injected with 0.5 ml of this immunogen emulsion i.p. The mice were boosted with doses of 5 to 40 ~9 of purified TAT
20 complex i.p. in an immunization protocol that lasted for approximately seven months.
- 2. Grouo 2 BALB/c female mice were sensitized with 10 ,ug each of purified TAT
25 complex in immunogen emulsion prepared as follows:
0.120 ml TAT complex (321 l~g/ml) 1.000 ml Complete Freund's Adjuvant 0.880 ml Dulbecco's Phosphate Buffered Saline wo ~nA~ PCT~S94/~5 213778~
Each mouse was injected with 0.5 ml of this immunogen emulsion i.p. The mice were boosted with doses of 10 to 11 ,.Lg of TAT complex i.p.
in an immunkalion protocol that lasted approximately nine weeks.
ExamDle2-ELlsA Assay for TAT Antibodies 1. Coatina Microtiter plates with TAT and ATIII
TAT complex and ATIII were each separately diluted in a coating buffer (carbonate buffer pH 9) at a concentration of 1 ~g/ml. 100 ~l of each solution (10 ng TAT complex or ATIII) was placed in each well of the 10 microtiter plates, which were sealed and incubated overnight at 2-8 C. The contents of the wells were then aspirated and the plates were washed once with wash/storage buffer, the wash aspirated, and the plates again resealed. The plates were stored at 2-80C until use.
15 2. Mouse Serum Titration Sera collected from the immunized mice from each of Groups 1 and 2 of Example 1 above were assayed for titers of TAT complex antibodies by ELISA on TAT complex coated microplates. Serially diluted sera (usually tested at dilutions of 1:1000 to as high as 1:3,125,000) were incllh~ted on 20 the microplates and probed with enzyme-labeled sheep or goat anti-mouse conjugates which were subsequently reacted with substrate. Relative titers were determined according to the strength of the color reaction, which was read spectrophotometrically at 405 nm. Pre-immune sera was used as the negative control and a commercially available mouse TAT monoclonal 25 antibody (latron) was used as a positive control in all assays.
Exam~le 3 - Preparation of Hybridomas Hybridomas secreting monoclonal antibodies to TAT were generated by two cell fusions. The P~G fusion technique employed based upon the wo s4n4s66 PcTlus94lo38ss 2~3~ $ 16-technique disclosed by G. Kohler, et al., Nature 256:495 (1975). The myeloma cells used were HRPT-minus P3 - X63-Ag8.653 (P3X) (ATCC CRL
1580). Selection for hybrids was accomplished using HAT media (hypoxanthine, aminopterin and thymidine); unfused P3X myeloma cells will 5 not survive in this medium as they lack the apparatus to use hypoxanthine to produce purines and the aminopterin present in the medium block endogenous synthesis of purines and pyrimidines.
1. Fusion to form Hybridoma TAT-4 10 Splenocyte preparation Spleen cells were obtained from a mouse immunized with TAT
complex as described for Group 1 of Example 1 above. The cells were teased from the spleen using a forceps and needle, then suspended in 12 ml of cold 20% Complete Medium without serum (RPMI 1640 base, Gibco).
The cells were then centrifuged as 200 x 9 for 10 minutes after which the supernatant was removed by aspiration, and the cells resuspended again in the cold medium. This washing process was repeated twice, and the cells resuspended in a final volume of 10 ml. The viable cell count of the splenocytes was 1.7 x 108 at a viability of 98% by trypan blue exclusion 20 technique. Counting methods employed were as disclosed by M. Absher, 'Hemacytometer Counting' in: Kruse, P.F. and Patterson, M.K. eds, Tissue Culture Methods and Ap~lication, Academic Press pp. 395-397: 1973. In brief, a volume of cell suspension is mixed with an equal volume of 0.02%
Trypan Blue and the cells counted in a hemacytometer by standard 25 counting methods.
Myeloma preparation The myeloma cells were harvested mechanically, pooled, and centrifuged at 200 x 9 for 10 minutes after which the supernatant was wo 94~ 2 1 3 7 7 8 5 ~tUS94/03~
removed by as~i,dlio", and the cells resuspended in 50 ml of 20%
Complete Medium. The viable cell count of the myeloma cells was 2.9 x 106viable cells per ml at a viability of 76%.
Fusion of the sDlenocytes and myeloma cells The splenocytes and 15 ml of the myeloma cell suspension were combined at spleen cell to myeloma cell ratio of approximately 4:1 with a total viable cell count of 2.13 x 108. The volume was brought up to 50 ml with cold 20% Complete Medium without serum and the cells then centrifuged a,t 200 x 9 for 10 minutes. The cell pellet was then washed twice with this medium at a volume of 50 ml. After the final wash, the supernatant was removed by aspiration and the pellet centrifuged at 200 x g for 3 minutes and the remaining supernatant aspirated. The cells were then fused with 40% PEG (molecular weight 7,000 to 9,000) buffered in RPMI 1640; fusion was performed in a tube held in a warm (370C) water bath. 1 ml of PEG solution warmed to 37 o C was added to the pellet and incubated for 1 minute. The PEG solution was then diluted by addition of 20 ml of warm 20% Complete Medium without serum. The fused cells were incllb~ted at 370C for 10 minutes and then centrifuged at 200 x 9 for 10 minutes.
The fused cell pellet was then resuspended in 50 ml of 20%
Complete Medium and plated at cell densities of 1.09 x 105 to 4.26 x 105 per well. The cells were plated in a final volume of 200 ~11 per well of 20%
Complete Medium, 20% Complete Medium with 2.5 ~Lg/ml STM or 20%
Complete Medium with 250 units/ml IL-6. After overnight incubation at 37OC and 10%CO2, one half of the medium in each well was aspira~ed and the cells feed with 20% HAT, 20% HAT with 5 ~g/ml STM or 20% HAT with 500 units/ml IL-6. The cells were visually scanned and feed periodically wo s4n4s6c Pcr/uss4/0388s 2~3~1185 - ~8-with these media for several weeks while the growth of the hybridomas was ",o"ilored and growing wells screened for the presence of anti-TAT
complex antibodies beginning at day 12 to 14 post-fusion.
2. Fusion of Hybridoma TAT-5 SDlenocyte Dreparation Spleen cells were obtained from a mouse immunized with TAT
complex as described for Group 2 of Example 1 above. The cells were teased from the spleen using forceps and scissors then washed three times in cold RPMI 1640. The cells were resuspended in a final volume of 40 ml of RPiAI 1640; the viable cell count of the splenocytes was 6 x 107 at a viability of 95% by trypan blue exclusion technique.
Myeloma preparation The myeloma cells were harvested mechanically pooled and washed three times in cold RPMI 1640. The cells were resuspended in a final volume of 10 ml; the viable cell count of the myeloma cells was 3.6 x 106 viable cells per ml at a viability of 71%.
Fusion of the splenocytes and myeloma cells The splenocytes and 4.2 ml of the myeloma cell suspension were combined at a spleen cell to myeloma cell ratio of approximately 4:1 with a total viable cell count of 7.5 x 10'. The cell mixture was centrifuged at 200 x g for 8 minutes and the supernatant aspirated. The cells were then fused with 40% PEG (molecular weight 7 000 to 9 000) buffered in RPMI 1640;
fusion was performed in a tube held in a warm (370C) water bath. 1 to 1.5 ml of PEG solution warmed to 37 o C was added to the pellet by dropwise addition over 1 to 1.5 minutes. The PEG solution was then diluted by wo 94~ 21 3 7785 PCT/us94lo388s addition of warm RPMI 1640 to a volume of 50 ml. The fused cells were then centrifuged at 200 x 9 for 10 minutes.
After aspila~ing the supernatant, the fused cell pellet was then resuspended in 50 ml of 20% Complete Medium and plated at 100 ~l per well, or a splenocyte density of 1.2 x 106viable cells per well. After overnight incubation at 37OC and 10% CO2, 100 1.l of 20% HATG (HAT
medium supplemented with glycine) was added to each well. The cells were visually scanned and feed periodically with 20% HATG for several weeks, while the growth of the hybridomas was monitored and growing wells screened for the presence of anti-TAT complex antibodies beginning at day 12 to 14 post-fusion.
Example 4 - Screeninq for Antibodies that Bind S~ecifically to the TAT
1 5 ComPlex Samples of supernatant collected from the growing hybridomas generated in fusions TAT-4 and TAT-5 as described in Example 3 above were screened for activity against TAT complex and ATIII using the antigen 20 coated microplates (1 ~g/ml) described in Example 2 above. Each of the twenty-one antibodies which tested positive for binding to TAT complex and negative for binding to ATIII was selected for the following further screening.
Further screening was carried out by performing sandwich ELISA
25 tests in the presence of ATIII (up to 300 ~g/ml) in solution and by performing sandwich ELlSAs on plasma samples spiked with TAT complex - (up to 50ng/ml). For each ELISA assay performed, 20 ~l of supernatant was added to 80 ~LI of Sample/conjugate Diluent in wells of the coated microplates. The new antibodies were used as the capture (10~Lg/ml) and 30 the conjugate used was a TAT complex monoclonal (D2M). Antibodies WO s4~As66 PCT/US94103885 2,~3~ S - 20 -which showed a low blank, no cross-reactivity with ATIII and which could detect decreasiny TAT levels in linearly diluted plasma were selected.
Incut-~tions: TAT in diluent or plasma/ATIII in diluent 2 hours at room temperature; conjugate 1 hour room temperature; substrate 20 min. room 5 temperature. On the basis of such successive screens, four antibodies were selected for further consideration D2M, C72, C44-T, and 5B46.
Example 5 - Affinity Data The affinity constant for the C44-T capture antibody was determined to be 3 x 10~ L/M. This constant was obtained using the method described in Friguet, et al., Measurements of True Affinity Constant in Solution of Antigen-Antibody complexes by Enzyme-Linked Immunoadsorbent Assay, J.
Immunol. Methods, 77:305 (1985).
The apparent affinity constant for the 5B46 conjugate antibody was determined to be 3.8 x 107. This constant was obtained by performing a competitive assay with HRP-conjugated and unconjugated antibody on antigen coated plates (1~g/ml TAT).
ExamDle 6 - Competition assay Competition assays using different combinations of conjugate and cold antibody were performed on C72 and C44-T plates. Plates were coated with 10~g/ml of C44-T or C72 F (ab')2. Conj~g~tes were diluted to 1.1~g/ml and competing antibodies were added at concenL,alions of 110, 11, and 0.11 ~g!ml. TAT incubation 1 hour at room temperature, Conjugate + IgG incubation 30 minutes at room temperature and slJbsLraLe incub~tion 15 minutes at room temperature. Results showed that a number of different combinations of the four TAT antibodies of the invention of D2M, 2l37785 C72, C44-T and 5B46 did not interfere, or interfered very little with each others binding.
Exam~le 7 - Determination of Antibodv sDecificity Microtiter plates were coated with C44-T F (ab')2 (10,l~g/ml). Other complexes of ATIII (factor XaATIII or factor IXaATIII) were incubated at 50ng/ml for 60 minutes at room temperature. The plates were then washed three times and conjugate (5B46 labeled with HRP) was added at 5.5~g/ml.
After incubation for 30 minutes the plates were washed three times and sub:,lrate was added. The reaction was stopped after 15 minutes for treatment with 1M sulfuric acid. This antibody pair demonstrated no significant cross-reactivity with either complex, specifically with factor Xa-ATIII complex less than 0.004% cross-reactivity was observed; and with factor IXa-ATIII complex less than 0.02% cross-reactivity was observed.
ExamPle 8 - Sandwich Assay Using Monoclonal Antibodies Monoclonal C44-T was immobilized on a solid carrier of ",icroliLer wells. A sample of patient plasma containing TAT complex and a measured amount of monoclonal 5B46, covalently labeled with an enzyme, specifically hor~eradish peroxidase, were then added to the immobilized C44-T for 30 minutes at 37 ~C. The unreacted conjugate (~B46) and any unreacted TAT
are then removed by washing. The amount of bound labeled antibody is directly proportional to the concentration of TAT complex in the test sample.
This invention has been described in detail with reference to preferred embodiments thereof. However, it will be appreciated that those skilled in the art, upon consideration of the disclosure, may make modification and improvements within the spirit and scope of the invention.
The enzymatic activity of thrombin can be regulated in various ways including the formation of an inactive complex with alllilhro~bin lll known as the thrombin-antithrombin lll complex or the ~TAT complex~.
20 AnliUIlo"~l~in 111 or UATIII" is a proteinase inhibitor in plasma that complexes with several serine proteinases in addition to thrombin. Thus ATIII is known to form complexes with serine protease factors Xlla Xla Xa and IXa.
It is desi,a~le to measure the amount of TAT complex in a human 25 fluid sample. Determination of levels of the TAT complex will provide an WO 941245~K PCT/US94/03885 .
2 131~ 8~ - 2 -indication of coagulation activity of a patient and aid in the assessment of thrombotic risk and other disorders such as disseminated intrav~scul~r co~gul~tion.
An assay for TAT complex levels in human plasma should provide a selective assessment of TAT complex concentrations, rather than a measurement of the concentration of total complexes of ATIII in a plasma sample, e.g. complexes of ATIII with factors Xlla, Xla, Xa and IXa in addition to the TAT complex. Such measurement of the "total" complexes of ATIII
provides an indication of the equilibrium of several reactions, some of which may reflect conditions other than those associated with particular TAT
complex levels. For instance, contact activation of factors Xll and Xl may lead predominantly to activation of the complement and kinin systems, therefore Xlla-ATIII and Xla-ATIII complexes may not be indicative of thrombotic risk.
It thus would be desirable to have a means for determining levels of the TAT complex in a human fluid sample. It would be particularly desirable to have an assay for the concentration of TAT complex in a human fluid sample where the assay provided a selective assessment of concenL,alioils of the TAT complex in a test sample, rather than a measurement of the sample's total complexes of ATIII.
SUMMARY OF THE INVENTION
The present invention provides an immunoassay for the detection and measurement of concenl,alion of a human thrombin-anLiLl,rombin lll (TAT) complex in a human fluid sample. The assay comprises contact of a human fluid sample with at least two antibodies or immunoreactive fragments thereof, preferably monoclonal antibodies or reactive fragments wo 94~ 2 1 3 7 7 8 S ~/US94103885 thereof, wherein at least one of the antibodies specifically binds to the TAT
complex in the fluid sample. Preferably each~ of the antibodies of the assay specifically binds to the TAT complex. As use~ herein, "specifically binds to the TAT complex" or other similar phrase indicates that the antibody or 5 antibodies bind to the TAT complex but exhibit substantially or essentially no cross-reactivity with free (i.e., not complexed) antithrombin lll or antithrombin lll complexes of other plasma factors, specifically factor Xa-antithrombin lll complex and factor IXa-antithrombin lll complex. Preferably the mixture of antibodies of the assay bind to different epitopes of the TAT
10 complex, i.e. the antibodies are not competitive. Additionally, the antibodies of the immunoassay of the invention preferably are contacted simultaneously with a human fluid sample so that only a single incubation and wash step is employed. Other aspects of the invention are disclosed infra.
DETAILED DESCRIPTION OF THE INVENTION
The immunoassay of the invention comprises reaction of at least two antiho~ies with a human fluid sample, wherein at least one of the antibodies specifically binds to said TAT complex. rleferably the antibodies are 20 monoclonal antibodies and both of said two antibodies of the assay specifically bind to the TAT complex. The antibody or antibodies of the assay that specifically bind to the TAT complex preferably exhibit less than about 3% cross-reactivity, in an assay such as that described in Example 7 below or similar assay with a human plasma sample, with ATIII, factor Xa-25 a"lilhr~",bin lll complex and factor IXa-antithrombin lll complex. More pre~erably the antibody or antibodies of the invention exhibit less than about 1% cross-reactivity with ATIII and such ATIII complexes. Still more preferably the antibody or antibodies of the invention exhibit less than about 0.2%, or even less than about 0.1% cross-reactivity with antithrombin lll and WO 94/24566 . PCT/USg4/03885 2~3'11~S 4 such ATIII complexes in an assay as described in Example 7 below or similar assay using a human plasma sample. It is also preferred that antibodies of the invention exhibit su~ch~lack of cross-reactivity with free (not complexed) thrombin, i.e. the antibodies of the invention preferably exhibit 5 less than about 3% cross-reactivity with free thrombin in reaction with a human plasma sample, more preferably exhibit less than about 1% cross-reactivity with thrombin, and still more preferably exhibit less than about 0.2%, or even less than about 0.1% cross-reactivity with free thrombin upon contact reaction of the antibody with a human plasma sample. In particular, 10 it was found that specifically preferred monoclonal antibodies of the invention upon contact with a human fluid sample bind to human TAT
complex and exhibited less than about 0.005% cross-reactivity with thrombin, less than about 0.005% cross-reactivity with antithrombin lll, less than about 0.005% cross-reactivity with factor IXa-antithrombin lll complex 15 and less than about 0.02% cross-reactivity with factor Xa-antithrombin lll complex. "Antibody", "antibody of the invention~ or other similar term as used herein includes a whole immunoglobulin as well as antigenic binding fragments or immunoreactive fragments which specifically bind to the TAT
complex, including Fab, Fab', F(ab')2 and F(v).
If only one antibody of the immunoassay specifically binds to the TAT
complex, the other antibody of the assay should bind to the TAT complex but also may exhibit cross-reactivity, e.g. with anLi~hrombin lll or other complexes of a"lill,ro,t,bin lll. Thus references herein to an antibody that 25 "binds" to TAT complex, rather than specifically binds thereto, indicates that the antibody binds to the human TAT complex and also may exhibit cross-reactivity with antithrombin lll, factor Xa-antithrombin lll complex and/or factor IXa-antithrombin lll complex. Antibodies, including monoclonal antibodies, that bind to the TAT complex and also exhibit cross-reactivity wo 94~ 2 1 3 7 7 8 5 pcTlus94lo388s with anlill,ro",bin lll and complexes thereof have been reported. See J.
Dawes, et al., Thrombosis Research, 36:397 (1984); S. Asakura, et al., Bioch. et Bio~hy. Acta, 952:37 (1988); Z. Hrkal, Hybridoma, 10(5):633 (1991); and European Published Patent Application No.0391433A2. In this S embodiment of the invention, preferably the antibody that specifically binds to the TAT complex is used as a carrier antibody and is immobilized on a substrate in a sandwich-type assay, and the cross-reactive antibody is used as the labeled conjugate, although the cross-reactive antibody also can be used as the carrier antibody and the antibody that specifically binds to the 10 TAT complex can be used as the labeled conjugate.
The human fluid sample used in the assay of the invention can be any sample that contains the TAT complex, e.g. blood or urine. Typically a plasma sample is employed.
Antibodies of the invention can be prepared by techniques generally known in the art, and are typically generated to a purified sample of a TAT
complex of human plasma. The antibodies also can be generated from an immunogenic peptide that comprises one or more epitopes of the TAT
20 complex that are not exhibited by free ATIII or thrombin.
More particularly, antibodies can be prepared by immunizing a mamrnal with a purified sample of a TAT complex, or an immunogenic peptide as discussed above, alone or complexed with a carrier. Suitable 25 ma~,n,als include typical laboratory animals such as sheep, goats, rabbits, guinea pigs, rats and mice. Rats and mice, especially mice, are preferred for obtaining monoclonal antibodies. The antigen can be ad",i,-i;,tered to the mammal by any of a number of suitable routes such as subcutaneous, intraperitoneal, intravenous, intramuscular or intracutaneous injection.
wo 94~SC6 PCTnUS94/~ ~5 Preferably immunization is by subcutaneous, intraperitoneal, or intravenous injection. The optimal immunizing interval, immunizing dose, etc. can vary within relatively wide ranges and can be :determined empirically based on this disclosure. Typical procedures involve injection of the antigen several times over a number of weeks. Antibodies are collected from serum of the immunized animal by standard techniques and screened to find antibodies specific for the TAT complex. Monoclonal antibodies can be produced in cells which produce antibodies and those cells used to generate monoclonal antibodies by using standard fusion techniques for forming hybridoma cells. See G. Kohler, et al., Nature, 256:456 (197~). Typically this involves fusing an antibody producing cell with an immortal cell line such as a myeloma cell to produce the hybrid cell. Alternatively, monoclonal antibodies can be produced from cells by the method of Huse, et al., Science. 256:1275 (1989).
One suitable protocol provides for intraperitoneal immunization of a mouse with a composition comprising purified TAT complex conducted over a period of about two to seven months. Spleen ceils then can be removed from the immunized mouse. Sera from the immunized mouse is assayed for titers of antibodies specific for TAT complex prior to excision of spleen cells. The excised mouse spleen cells are then fused to an appropriate homogenic or heterogenic (preferably homogenic) Iymphoid cell line having a marker such as hypoxanthine-guanine phosphoribosyltransferase deficiency (HGPRr) or thymidine kinase deficiency (TK-). Preferably a myeloma cell is employed as the Iymphoid cell line. Myeloma cells and spleen cells are mixed together, e.g. at a ratio of about 1 to 4 myeloma cells to spleen cells. The cells can be fused by the polyethylene glycol (PEG) method. See G. Kohler, et al., Nature, supra. The thus cloned hybridoma is grown in a culture medium, e.g. RPMI-1640. See G. E. More, wo g4~ 2 1 3 7 7 8 S ~/US94103885 et al., Journal of American Medical Association, 199:549 (1967).
Hybridomas, grown after the fusion procedure, are screened such as by radioimmunoassay or enzyme immunoassay for secretion of antibodies that bind specifically to the TAT complex, e.g. antibodies are selected that bind 5 to the TAT complex, but not to ATIII. Preferably an ELISA is employed for the screen. Hybridomas that show positive results upon such screening can be ex~,anded and cloned by limiting dilution method. Further screens are preferably performed to select antibodies that can bind to TAT complex in solution as well as in a human fluid sample.
Antibodies of the invention preferably show an affinity constant with the TAT complex of greater than about 1 x 104 L/M, more preferably greater than about 1 x 105 L/M, still more preferably greater than about 1 x 108 L/M, such constants determined by the method disclosed in Friguet, et al., J. Immunol. Methods, 77:305 (1985).
Preferred antibodies of the invention are highly sensitive for TAT
complex in a human fluid sample. For example, it was found that preferred antibodies detected with precision a concenl,alion of TAT complex of about 20 0.55 ng or greater per ml of plasma sample with recovery of spiked material being essentially 100%.
Immunoassays of the invention generally exhibit good precision. For example, the following results were found for preferred assays of the 25 invention: within assay values for control levels I and ll for n-80 of 3.9% CV
and 6.8% respectively; and between assay precision values for n=80 of 9.3% and 12.2% CV respectively.
WO 94/245CC PC~/US94tQ~885 2~3~7~S
Competitive assays have shown that preferred antibodies of the invention are at least substantially or essentially non-competitive, i.e. two ormore antibodies of the invention show little or no binding interference among themselves when reacted simultàneously with a sample of TAT
5 complex. By use of such antibodies in an immunoassay, a test sample can be incub~ted simultaneously (i.e., single incubation step) with both the bound capture antibody and labeled conjugate antibody of the assay. This is distinct from prior assays that utilize separate incubation and wash steps for each of the capture and conjugate antibodies, e.g. to avoid binding 10 interference between the antibodies.
It has also been found that preferred antibodies of the invention can bind to TAT complex of a human fluid sample, particularly a human plasma sample, that is not diluted, or is diluted only by the solution containing the 15 TAT complex antibody. In particular, it has been found that preferred antibodies of the present invention can bind to TAT complex of a human fluid sample where the fluid sample is diluted only by an equal volume or less of a diluent. This is distinct from at least some prior antibodies that arereported to bind to TAT complex, but will only do so when contacted with a 20 ~JIas",a sample that is diluted to a significant extent, e.g. when a plasma or other test sample is diluted 100 times or more. Such dilution is undesirable as it can add to the complexity of a TAT complex assay that utilizes such antibodies.
Specifically preferred monoclonal antibodies of the invention include D2M, C72, C44-T and SB46, which are mouse monoclonal antibodies that specifically bind to the TAT complex. Hybridomas expressing such monoclonals have been deposited with the American Type Culture Collection (ATCC), 12301 Parklawn Drive, Rockville, Maryland 20852 and wo g4124566 2 1 3 778 5 given Accession No. _ (TAT-4-C44-T-3:ST; expresses C44-T); Accession No. _tTAT-5-B46-4; expresses 5B46); Accession No. _ (TAT-4-C72E;
expresses C72); Accession No. _(TAT-1-D2M; expresses D2M).
Thus antibodies of the invention are particularly suitable for use in an immunoassay for detecting and measuring the concen~lalion of TAT
complex in a human fluid sample. A particularly prefer,ed immunoassay of the invention is a sandwich assay in which the capture antibody is immobilized using known methods such as physical adsorption onto the surface of a support. Suitable supports include, e.g., polymer materials such as polypropylene or polystyrene, glass, metals, cross-linked dextran, agarose, etc. The support may be in a variety of shapes such as a tray, sphere, rods, test tube, etc. A tray having wells such as a miclolilre plate is generally preferred.
The detectably labeled antibody of the assay is formed by coupling the antibody to a reporter, e.g. a radioactive isotopes, an enzyme, a fluorescent or luminescent reagent and the like. Typically used radioactive isotopes '251, Tc99m and 3H. Known isotope labeling methods include iactoperoxidase and Hunter-Bolton methods for t251 and reduction methylation for 3H. See A. Bolton, et al., Biochem. J., 133:529-539 (1972).
Enzyme tags may include peroxidases, alkaline phosphatases, ~-D-galactosidases, glucoseoxidases, and the like. Peroxidases are particularly preferred. The peroxidases can be selected from those derived from various sources, e.g. horseradish, pineapple, fig, sugarcane, java bean, corn. Horseradish peroxidase is a particularly preferred material. Means for covalent labeling of an antibody with such enzymes are known in the art.
Methods suitable for a specific enzyme and antibody can depend on wo s4n4sc6 Pcrluss4lo388s 2~3r~ 5 10-available reactive moieties on the enzyme and antibody and can be readily asce,lained empirically.
``:
The assay of the invention is illustrated by the following protocol 5 using peroxidase as the labei of the conjugate antibody. A test sample, e.g.
a human plasma sample, is added to a TAT complex antibody (i.e., an antibody that binds to the TAT complex) bound on a carrier such a microtiter plate and the antibody-antigen reaction is conducted, followed by addition of the peroxidase labeled TAT complex antibody conjugate 10 obtained as outlined above, and then a further antibody-antigen reaction conducted. The antibody are- typically dissolved in solution prior to contact with a test sample. Suitable diluents include those known in the art for use in immunoassays. A specifically preferred solution for dissolving the antibodies for contact with a test sample contai,)s 20 mmol Tris, 500 mmol 15 sodium chloride, 0.05 mg/ml mouse IgG and 5% BSA.
Preferably both the carrier and conjugate antibodies of the assay of the invention specifically bind to the TAT complex, and the antibody bound to the support, the human fluid sample and labeled antibody are incubated 20 together, followed by a single wash step to remove any unreacted labeled antibody and the human plasma sample other than the reacted TAT
complex. Suitable washing agents include those known in the art for use in immunoassays. A specifically preferred washing buffer solution contains 27.2 9/l imidazole, 17.5 9/l sodium chloride and 4 ml/liter Tween 20. If 25 necessary a substrate for peroxidase is added to the assay and the reaction products are assayed for enzyme activity by measuring the absorbance or fluorescence of the resulting substance. The detected amount of bound labeled antibody is directly proportional to the concentration of TAT complex in the assayed human plasma sample. Thus wo g4~ 2 1 3 7 7 8 5 PCr/uss4lo388s a qua"LiLa~ive determination of the TAT complex concentration in the plasma test sample can be dete",~ined by comparison of the absorbance or fluorescence of the test sample with absorbance values obtained from standardized solutions that contain known amounts of TAT complex. It may 5 be desirable to prepare calibration curves from absorbance values obtained from a number of standardized solutions to facilitate interpretation of values obtained from a test sample.
A specifically preferred immunoassay of the invention was conducted 10 as follows. The capture monoclonal antibody and conjugate monoclonal antibody labeled with horseradish peroxidase (HRP) is incubated together with a human plasma sample at 37~C for 30 rninutes. The plate is then washed and incubated for 15 minutes at room temperature with HRP
substrate and the bound conjugate is quantitated.
A preferred immunoassay of the invention was used to measure plasma samples in individuals (n=15) with Disseminated Intravascular Coagulation. Assay results showed TAT complex levels significantly elevated in all but one patient plasma sample. Twelve of the individuals 20 tested had levels of TAT complex greater than 160 ng/ml.
TAT complex can be purified from a human plasma sample by use of carrier complexes coupled with one or more antibodies of the invention and hence the invention includes methods for obtaining purified TAT complex 25 using the antibodies of the invention and related apparatus. A suitable purification procedure provides coupling an antibody of the invention on an appro,c,riate carrier as is known in the art such as a gel or resin then packing the carrier in a column and then eluting a sample solution containing TAT complex through the column to selectively adsorb the TAT
WO g4/245C6 PCT/US94/03885 2~3rt ~l 8,S
complex. The antibody can be suitably coupled onto the carrier by known methods, e.g. the cyanogen bromide method and glutaraldehyde method, aqueous carbodiimide method, active ester method, and the like. The antibody also may be physically adsorbed orl the surface of the carrier.
The antibodies of the invention also can be used to locate and monitor TAT complex in vivo. For example, one or more antibodies of the invention can be labeled with a radionuclide such as 11-indium. The labeled antibody then can be injected intravenously into a human and the 10 human scanned to determine where the labelled antibody accumulates.
The labeled antibody typically will differentially accumulate in areas having high concentrations of TAT complex, e.g. where blood clotting is occurring such as in a hemorrhage site. The amount of labeled antibody can be determined by known scanning methods such as by using a scintigraphic 1 5 camera.
The antibodies of the invention also can be used therapeutically, e.g.
as a carrier for drugs, particularly pharmaceuticals targeted for interaction inthe blood clotting mechanism such as strepo-kinase, TPA and urokinase.
20 The pharmaceutical can be attached to an antibody of the invention by the same means as attachment of a label as specified above, e.g. by a covalent linkage that does not inhibit the specificity of the antibody or the desired pharmacological effect of the drug. The antibody with the attached pl,ar,l,aceutical can be administered to a human in therapeutically effective 25 amounts by any of a number of known means, e.g. parenterally or orally.
For parenteral adminisl,alion the antibody with attached pharmaceutical is typically administered in aqueous and non-aqueous sterile iniection compositions as are known in the art. For oral administration the therapeutic of the invention may be administered to a human in discrete WO g41245C6 PCI IUS94/03885 21~7785 units such as capsules or tablets each containing a predeter",ined amount of the therapeutic, as a solution or a suspension in an aqueous or non-aqueous liquid, as an oil/water liquid emulsion, in powdered carriers such as lactose or sucrose, etc.
All documents mentioned herein are incorporated by reference herein in their entirety.
The following non-limiting examples are illustrative of the invention.
General Comments Purified samples of TAT complex used in the following Examples were generally obtained by procedures described in G. Elgue, et al., Thrombosis and Hemostasis, 63(3):435 (1990). In brief, thrombin and antithrombin lll were reacted and the resultant TAT compiex was isolated by gel filtration. 20% Complete Medium used in the Examples had the following composition per 100 ml:
1 ml 200 mM 1-glutamine, 1 ml 7.5% Na-bicarbonate, 1 ml 5000 u/ml Penicillin & 5000 mcg/ml Streptomycin, 0.05 ml 0.1M 2 ~-mercaptoethanol, 20 ml Fetal Bovine Serum, and to 100 ml with RPMI 1640 (Gibco) without L-glutamine.
HAT media used in the Examples had the following composition: to 100 ml of Complete Medium 1 ml 100X Hypoxanthine Thymidine and 2 ml SOX Aminopterin were added. HATG media used in the Examples had the following composition: to 100 ml of HAT media 1 ml 100X Glycine was added. IL-6 used in the Examples was prepared by adding 500 units 2l37785 Human Recombinant IL-6 (Collaborative Research Inc.) per ml medium.
STM used in the Examples was prepared by adding 5 ~9 salmonella typhimurium mitogen (Ribi Immunochemical Research, Inc.) per ml medium.
5 Example 1 - Immunization The following two groups of BALB/c female mice were immunized with TAT complex to provide spleen donors for the PEG fusions, disclosed below, that generated monoclonal antibodies that specifically bind to the TAT complex.
1. Group 1 BALB/c female mice were sensitized with 7 ~9 each of purified TAT
complex in immunogen emulsion prepared as follows:
0.125 ml TAT complex (325 l~g/ml in 50 mM tris/50 mM NaCI/0.1 M
15 EDTA pH 7.4) 1.500 ml Complete Freund's Adjuvant 1.375 ml Dulbecco's Phosphate Buffered Saline Each mouse was injected with 0.5 ml of this immunogen emulsion i.p. The mice were boosted with doses of 5 to 40 ~9 of purified TAT
20 complex i.p. in an immunization protocol that lasted for approximately seven months.
- 2. Grouo 2 BALB/c female mice were sensitized with 10 ,ug each of purified TAT
25 complex in immunogen emulsion prepared as follows:
0.120 ml TAT complex (321 l~g/ml) 1.000 ml Complete Freund's Adjuvant 0.880 ml Dulbecco's Phosphate Buffered Saline wo ~nA~ PCT~S94/~5 213778~
Each mouse was injected with 0.5 ml of this immunogen emulsion i.p. The mice were boosted with doses of 10 to 11 ,.Lg of TAT complex i.p.
in an immunkalion protocol that lasted approximately nine weeks.
ExamDle2-ELlsA Assay for TAT Antibodies 1. Coatina Microtiter plates with TAT and ATIII
TAT complex and ATIII were each separately diluted in a coating buffer (carbonate buffer pH 9) at a concentration of 1 ~g/ml. 100 ~l of each solution (10 ng TAT complex or ATIII) was placed in each well of the 10 microtiter plates, which were sealed and incubated overnight at 2-8 C. The contents of the wells were then aspirated and the plates were washed once with wash/storage buffer, the wash aspirated, and the plates again resealed. The plates were stored at 2-80C until use.
15 2. Mouse Serum Titration Sera collected from the immunized mice from each of Groups 1 and 2 of Example 1 above were assayed for titers of TAT complex antibodies by ELISA on TAT complex coated microplates. Serially diluted sera (usually tested at dilutions of 1:1000 to as high as 1:3,125,000) were incllh~ted on 20 the microplates and probed with enzyme-labeled sheep or goat anti-mouse conjugates which were subsequently reacted with substrate. Relative titers were determined according to the strength of the color reaction, which was read spectrophotometrically at 405 nm. Pre-immune sera was used as the negative control and a commercially available mouse TAT monoclonal 25 antibody (latron) was used as a positive control in all assays.
Exam~le 3 - Preparation of Hybridomas Hybridomas secreting monoclonal antibodies to TAT were generated by two cell fusions. The P~G fusion technique employed based upon the wo s4n4s66 PcTlus94lo38ss 2~3~ $ 16-technique disclosed by G. Kohler, et al., Nature 256:495 (1975). The myeloma cells used were HRPT-minus P3 - X63-Ag8.653 (P3X) (ATCC CRL
1580). Selection for hybrids was accomplished using HAT media (hypoxanthine, aminopterin and thymidine); unfused P3X myeloma cells will 5 not survive in this medium as they lack the apparatus to use hypoxanthine to produce purines and the aminopterin present in the medium block endogenous synthesis of purines and pyrimidines.
1. Fusion to form Hybridoma TAT-4 10 Splenocyte preparation Spleen cells were obtained from a mouse immunized with TAT
complex as described for Group 1 of Example 1 above. The cells were teased from the spleen using a forceps and needle, then suspended in 12 ml of cold 20% Complete Medium without serum (RPMI 1640 base, Gibco).
The cells were then centrifuged as 200 x 9 for 10 minutes after which the supernatant was removed by aspiration, and the cells resuspended again in the cold medium. This washing process was repeated twice, and the cells resuspended in a final volume of 10 ml. The viable cell count of the splenocytes was 1.7 x 108 at a viability of 98% by trypan blue exclusion 20 technique. Counting methods employed were as disclosed by M. Absher, 'Hemacytometer Counting' in: Kruse, P.F. and Patterson, M.K. eds, Tissue Culture Methods and Ap~lication, Academic Press pp. 395-397: 1973. In brief, a volume of cell suspension is mixed with an equal volume of 0.02%
Trypan Blue and the cells counted in a hemacytometer by standard 25 counting methods.
Myeloma preparation The myeloma cells were harvested mechanically, pooled, and centrifuged at 200 x 9 for 10 minutes after which the supernatant was wo 94~ 2 1 3 7 7 8 5 ~tUS94/03~
removed by as~i,dlio", and the cells resuspended in 50 ml of 20%
Complete Medium. The viable cell count of the myeloma cells was 2.9 x 106viable cells per ml at a viability of 76%.
Fusion of the sDlenocytes and myeloma cells The splenocytes and 15 ml of the myeloma cell suspension were combined at spleen cell to myeloma cell ratio of approximately 4:1 with a total viable cell count of 2.13 x 108. The volume was brought up to 50 ml with cold 20% Complete Medium without serum and the cells then centrifuged a,t 200 x 9 for 10 minutes. The cell pellet was then washed twice with this medium at a volume of 50 ml. After the final wash, the supernatant was removed by aspiration and the pellet centrifuged at 200 x g for 3 minutes and the remaining supernatant aspirated. The cells were then fused with 40% PEG (molecular weight 7,000 to 9,000) buffered in RPMI 1640; fusion was performed in a tube held in a warm (370C) water bath. 1 ml of PEG solution warmed to 37 o C was added to the pellet and incubated for 1 minute. The PEG solution was then diluted by addition of 20 ml of warm 20% Complete Medium without serum. The fused cells were incllb~ted at 370C for 10 minutes and then centrifuged at 200 x 9 for 10 minutes.
The fused cell pellet was then resuspended in 50 ml of 20%
Complete Medium and plated at cell densities of 1.09 x 105 to 4.26 x 105 per well. The cells were plated in a final volume of 200 ~11 per well of 20%
Complete Medium, 20% Complete Medium with 2.5 ~Lg/ml STM or 20%
Complete Medium with 250 units/ml IL-6. After overnight incubation at 37OC and 10%CO2, one half of the medium in each well was aspira~ed and the cells feed with 20% HAT, 20% HAT with 5 ~g/ml STM or 20% HAT with 500 units/ml IL-6. The cells were visually scanned and feed periodically wo s4n4s6c Pcr/uss4/0388s 2~3~1185 - ~8-with these media for several weeks while the growth of the hybridomas was ",o"ilored and growing wells screened for the presence of anti-TAT
complex antibodies beginning at day 12 to 14 post-fusion.
2. Fusion of Hybridoma TAT-5 SDlenocyte Dreparation Spleen cells were obtained from a mouse immunized with TAT
complex as described for Group 2 of Example 1 above. The cells were teased from the spleen using forceps and scissors then washed three times in cold RPMI 1640. The cells were resuspended in a final volume of 40 ml of RPiAI 1640; the viable cell count of the splenocytes was 6 x 107 at a viability of 95% by trypan blue exclusion technique.
Myeloma preparation The myeloma cells were harvested mechanically pooled and washed three times in cold RPMI 1640. The cells were resuspended in a final volume of 10 ml; the viable cell count of the myeloma cells was 3.6 x 106 viable cells per ml at a viability of 71%.
Fusion of the splenocytes and myeloma cells The splenocytes and 4.2 ml of the myeloma cell suspension were combined at a spleen cell to myeloma cell ratio of approximately 4:1 with a total viable cell count of 7.5 x 10'. The cell mixture was centrifuged at 200 x g for 8 minutes and the supernatant aspirated. The cells were then fused with 40% PEG (molecular weight 7 000 to 9 000) buffered in RPMI 1640;
fusion was performed in a tube held in a warm (370C) water bath. 1 to 1.5 ml of PEG solution warmed to 37 o C was added to the pellet by dropwise addition over 1 to 1.5 minutes. The PEG solution was then diluted by wo 94~ 21 3 7785 PCT/us94lo388s addition of warm RPMI 1640 to a volume of 50 ml. The fused cells were then centrifuged at 200 x 9 for 10 minutes.
After aspila~ing the supernatant, the fused cell pellet was then resuspended in 50 ml of 20% Complete Medium and plated at 100 ~l per well, or a splenocyte density of 1.2 x 106viable cells per well. After overnight incubation at 37OC and 10% CO2, 100 1.l of 20% HATG (HAT
medium supplemented with glycine) was added to each well. The cells were visually scanned and feed periodically with 20% HATG for several weeks, while the growth of the hybridomas was monitored and growing wells screened for the presence of anti-TAT complex antibodies beginning at day 12 to 14 post-fusion.
Example 4 - Screeninq for Antibodies that Bind S~ecifically to the TAT
1 5 ComPlex Samples of supernatant collected from the growing hybridomas generated in fusions TAT-4 and TAT-5 as described in Example 3 above were screened for activity against TAT complex and ATIII using the antigen 20 coated microplates (1 ~g/ml) described in Example 2 above. Each of the twenty-one antibodies which tested positive for binding to TAT complex and negative for binding to ATIII was selected for the following further screening.
Further screening was carried out by performing sandwich ELISA
25 tests in the presence of ATIII (up to 300 ~g/ml) in solution and by performing sandwich ELlSAs on plasma samples spiked with TAT complex - (up to 50ng/ml). For each ELISA assay performed, 20 ~l of supernatant was added to 80 ~LI of Sample/conjugate Diluent in wells of the coated microplates. The new antibodies were used as the capture (10~Lg/ml) and 30 the conjugate used was a TAT complex monoclonal (D2M). Antibodies WO s4~As66 PCT/US94103885 2,~3~ S - 20 -which showed a low blank, no cross-reactivity with ATIII and which could detect decreasiny TAT levels in linearly diluted plasma were selected.
Incut-~tions: TAT in diluent or plasma/ATIII in diluent 2 hours at room temperature; conjugate 1 hour room temperature; substrate 20 min. room 5 temperature. On the basis of such successive screens, four antibodies were selected for further consideration D2M, C72, C44-T, and 5B46.
Example 5 - Affinity Data The affinity constant for the C44-T capture antibody was determined to be 3 x 10~ L/M. This constant was obtained using the method described in Friguet, et al., Measurements of True Affinity Constant in Solution of Antigen-Antibody complexes by Enzyme-Linked Immunoadsorbent Assay, J.
Immunol. Methods, 77:305 (1985).
The apparent affinity constant for the 5B46 conjugate antibody was determined to be 3.8 x 107. This constant was obtained by performing a competitive assay with HRP-conjugated and unconjugated antibody on antigen coated plates (1~g/ml TAT).
ExamDle 6 - Competition assay Competition assays using different combinations of conjugate and cold antibody were performed on C72 and C44-T plates. Plates were coated with 10~g/ml of C44-T or C72 F (ab')2. Conj~g~tes were diluted to 1.1~g/ml and competing antibodies were added at concenL,alions of 110, 11, and 0.11 ~g!ml. TAT incubation 1 hour at room temperature, Conjugate + IgG incubation 30 minutes at room temperature and slJbsLraLe incub~tion 15 minutes at room temperature. Results showed that a number of different combinations of the four TAT antibodies of the invention of D2M, 2l37785 C72, C44-T and 5B46 did not interfere, or interfered very little with each others binding.
Exam~le 7 - Determination of Antibodv sDecificity Microtiter plates were coated with C44-T F (ab')2 (10,l~g/ml). Other complexes of ATIII (factor XaATIII or factor IXaATIII) were incubated at 50ng/ml for 60 minutes at room temperature. The plates were then washed three times and conjugate (5B46 labeled with HRP) was added at 5.5~g/ml.
After incubation for 30 minutes the plates were washed three times and sub:,lrate was added. The reaction was stopped after 15 minutes for treatment with 1M sulfuric acid. This antibody pair demonstrated no significant cross-reactivity with either complex, specifically with factor Xa-ATIII complex less than 0.004% cross-reactivity was observed; and with factor IXa-ATIII complex less than 0.02% cross-reactivity was observed.
ExamPle 8 - Sandwich Assay Using Monoclonal Antibodies Monoclonal C44-T was immobilized on a solid carrier of ",icroliLer wells. A sample of patient plasma containing TAT complex and a measured amount of monoclonal 5B46, covalently labeled with an enzyme, specifically hor~eradish peroxidase, were then added to the immobilized C44-T for 30 minutes at 37 ~C. The unreacted conjugate (~B46) and any unreacted TAT
are then removed by washing. The amount of bound labeled antibody is directly proportional to the concentration of TAT complex in the test sample.
This invention has been described in detail with reference to preferred embodiments thereof. However, it will be appreciated that those skilled in the art, upon consideration of the disclosure, may make modification and improvements within the spirit and scope of the invention.
Claims (25)
1. An immunoassay for detection of a human thrombin-antithrombin III complex in a human fluid sample, comprising:
contacting a first antibody with the fluid sample, and contacting a second antibody with the fluid sample, wherein at least one of the first and second antibodies specifically bind to the human thrombin-antithrombin III complex.
contacting a first antibody with the fluid sample, and contacting a second antibody with the fluid sample, wherein at least one of the first and second antibodies specifically bind to the human thrombin-antithrombin III complex.
2. The immunoassay of claim 1 wherein both of said antibodies specifically bind to the human thrombin-antithrombin III complex.
3. The immunoassay of claim 1 wherein the first and second antibodies are essentially non-competitive with respect to binding to the complex.
4. The immunoassay of claim 1 wherein the first and second antibodies are contacted substantially simultaneously with the fluid sample.
5. The immunoassay of claim 1 wherein the first antibody is contacted with the fluid sample and then the second antibody is contacted with the fluid sample.
6. The immunoassay of claim 1 wherein the first antibody is adsorbed onto a solid matrix and the second antibody is labeled with a reporter group.
7. The immunoassay of claim 1 wherein the quantity of TAT
complex in the fluid sample is determined.
complex in the fluid sample is determined.
8. The immunoassay of claim 1 wherein the first and second antibodies are monoclonal antibodies.
9. The immunoassay of claim 1 wherein the fluid sample is plasma.
10. The immunoassay of claim 1 wherein the antibody that specifically binds to the thrombin-antithrombin III complex exhibits less than about 1% cross-reactivity with each of thrombin, antithrombin, serine protease factor Xa-antithrombin III complex, and serine protease factor IXa-antithrombin III complex.
11. The immunoassay of claim 1 wherein the antibody that specifically binds to the thrombin-antithrombin III complex exhibits less than about 0.2% cross-reactivity with each of thrombin, antithrombin, serine protease factor Xa-antithrombin III complex, and serine protease factor IXa-antithrombin III complex.
12. The immunoassay of claim 1 wherein the first antibody has the characteristics of D2M C72, C44-T or 5B46.
13. The immunoassay of claim 1 or 12 wherein the second antibody has the characteristics of D2M, C72, C44-T or 5B46.
14. The immunoassay of claim 1 wherein the first antibody is D2M, C72, C44-T or 5B46.
15. The immunoassay of claim 1 or 14 wherein the second antibody is D2M, C72, C44-T or 5B46.
16. The immunoassay of claim 6 where the first antibody has the characteristics of C44-T and the second antibody has the characteristics of 5B46.
17. The immunoassay of claim 6 where the first antibody is C44-T
and the second antibody is 5B46.
and the second antibody is 5B46.
18. A test kit for the detection of a human thrombin-antithrombin III complex in a test sample, comprising a first and second antibody, wherein at least of one said antibodies can specifically bind to the human thrombin-antithrombin III complex.
19. The test kit of claim 18 wherein both of said antibodies specifically bind to the human thrombin-antithrombin III complex.
20. The test kit of claim 18 wherein one of said antibodies specifically binds to the human thrombin-antithrombin III complex, and the other of said antibodies binds to the human thrombin-antithrombin III
complex.
complex.
21. The test kit of claim 18 wherein the first antibody has the characteristics of D2M, C72, C44-T or 5B46.
22. The test kit of claim 16 wherein the second antibody has the characteristics of D2M, C72, C44-T or 5B46.
23. A monoclonal antibody that specifically binds to a human thrombin-antithrombin III complex.
24. The monoclonal antibody of claim 23 that has the characteristics of D2M, C72, C44-T or 5B46.
25. The monoclonal antibody of claim 23 that is D2M, C72, C44-T
or 5B46.
or 5B46.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US4801493A | 1993-04-15 | 1993-04-15 | |
| US08/048,014 | 1993-04-15 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2137785A1 true CA2137785A1 (en) | 1994-10-27 |
Family
ID=21952294
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA 2137785 Abandoned CA2137785A1 (en) | 1993-04-15 | 1994-04-08 | Immunoassay and test kit for thrombin-antithrombin iii complex |
Country Status (5)
| Country | Link |
|---|---|
| EP (1) | EP0646244A1 (en) |
| JP (1) | JPH07508103A (en) |
| AU (1) | AU676907B2 (en) |
| CA (1) | CA2137785A1 (en) |
| WO (1) | WO1994024566A1 (en) |
Families Citing this family (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JPH0759590A (en) * | 1993-08-24 | 1995-03-07 | Oriental Yeast Co Ltd | Antithrombin monoclonal antibody |
| JPH07238099A (en) * | 1994-02-25 | 1995-09-12 | Dai Ichi Pure Chem Co Ltd | Nonoclonal antibody and method for immunoassay using the same |
| ES2407355T3 (en) * | 2001-07-03 | 2013-06-12 | Oklahoma Medical Research Foundation | Test to measure factor VIIa-antithrombin complexes |
| JP7355140B2 (en) * | 2022-02-28 | 2023-10-03 | 住友ベークライト株式会社 | Reagents for detecting or measuring serine proteases |
| CN116284417B (en) * | 2023-02-09 | 2023-10-31 | 山东大学 | Thrombin-antithrombin complex antibody, its preparation method and application |
Family Cites Families (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO1986000910A1 (en) * | 1984-07-30 | 1986-02-13 | Celltech Limited | Immunopurification process |
| WO1990008320A1 (en) * | 1989-01-19 | 1990-07-26 | Teijin Limited | Immunoassay method, reagent and kit |
| AU628960B2 (en) * | 1989-04-07 | 1992-09-24 | Teijin Limited | Method of immunologically assaying human thrombin- antithrombin III complex, assay reagent and kit therefor |
| US5296352A (en) * | 1990-10-02 | 1994-03-22 | Ciba-Geigy Corporation | Monoclonal antibodies directed against complexes formed by thrombin and hirudin |
-
1994
- 1994-04-08 WO PCT/US1994/003885 patent/WO1994024566A1/en not_active Application Discontinuation
- 1994-04-08 EP EP94914090A patent/EP0646244A1/en not_active Withdrawn
- 1994-04-08 CA CA 2137785 patent/CA2137785A1/en not_active Abandoned
- 1994-04-08 JP JP6523334A patent/JPH07508103A/en active Pending
- 1994-04-08 AU AU66293/94A patent/AU676907B2/en not_active Ceased
Also Published As
| Publication number | Publication date |
|---|---|
| JPH07508103A (en) | 1995-09-07 |
| AU6629394A (en) | 1994-11-08 |
| AU676907B2 (en) | 1997-03-27 |
| WO1994024566A1 (en) | 1994-10-27 |
| EP0646244A1 (en) | 1995-04-05 |
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