WO1998054219A1 - Covalently coupled troponin complexes - Google Patents

Covalently coupled troponin complexes Download PDF

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Publication number
WO1998054219A1
WO1998054219A1 PCT/US1998/010518 US9810518W WO9854219A1 WO 1998054219 A1 WO1998054219 A1 WO 1998054219A1 US 9810518 W US9810518 W US 9810518W WO 9854219 A1 WO9854219 A1 WO 9854219A1
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Prior art keywords
troponin
cardiac troponin
composition
complex
tnl
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PCT/US1998/010518
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French (fr)
Inventor
Nihmat Moriana
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Medical Analysis Systems Inc.
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Priority claimed from US08/865,468 external-priority patent/US6248869B1/en
Application filed by Medical Analysis Systems Inc. filed Critical Medical Analysis Systems Inc.
Priority to JP50078399A priority Critical patent/JP2002508839A/en
Priority to EP98923686A priority patent/EP0983299A1/en
Publication of WO1998054219A1 publication Critical patent/WO1998054219A1/en

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    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/435Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
    • C07K14/46Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans from vertebrates
    • C07K14/47Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans from vertebrates from mammals
    • C07K14/4701Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans from vertebrates from mammals not used
    • C07K14/4716Muscle proteins, e.g. myosin, actin
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N2333/00Assays involving biological materials from specific organisms or of a specific nature
    • G01N2333/435Assays involving biological materials from specific organisms or of a specific nature from animals; from humans
    • G01N2333/46Assays involving biological materials from specific organisms or of a specific nature from animals; from humans from vertebrates
    • G01N2333/47Assays involving proteins of known structure or function as defined in the subgroups
    • G01N2333/4701Details
    • G01N2333/4712Muscle proteins, e.g. myosin, actin, protein

Definitions

  • the present invention relates generally to clinical chemistry.
  • it relates to stabilized troponin complexes useful in the diagnosis of myocardial infarction or other ischemic events.
  • compositions which behave similarly to how constituents present in human bodily fluids (e.g. blood, blood serum, plasma, spinal fluid or urine) behave are used in clinical laboratories. These compositions assist in the determination of whether the clinical instrumentation and procedures used by the laboratory to measure the constituents are accurate. These compositions are also used to calibrate the clinical devices which measure the amount or presence of the constituent in a sample. These compositions will be referred to hereinafter as control compositions or controls . In addition, it is important that the analyte or analyte analog present in the control composition behave similarly to the corresponding analyte to be tested for in a patient's bodily fluid —that is, the control composition should mimic the patient sample.
  • MI myocardial infarction
  • Cardiac troponin I (cTnl) and troponin T have recently become established as the markers of choice in evaluating cardiac distress. See, New England Journal of Medicine Volume 335 No. 18, pages 1342-1349, Antman et al. and pages 1333-1341, Ohman et al.
  • the Troponin complex is present in both skeletal and cardiac muscles and consists of three subunits, Troponin T (“TnT”) the tropomyosin binding subunit, Troponin C (“TnC”), the Ca++ binding subunit and Tnl, which inhibits the actomyosin Mg++-ATPase.
  • TnT Troponin T
  • TnC Troponin C
  • Tnl the Ca++ binding subunit
  • the majority of the research into the troponin complex has centered around the regulatory function and structure of the troponin complex in skeletal muscle.
  • the troponin complex assists in muscle contraction.
  • the TnC molecule has four binding domains to bind divalent metal ions.
  • the Ca++/Mg++ binding sites are in the COOH terminal region and the Ca++ binding sites are in the amino terminal region.
  • the amino terminus of Tnl binds to the COOH terminus region of TnC and to the globular COOH terminus region of TnT .
  • Biochemistry 26, 7042- 7047 reported that the main product of cross-linking between TnC and skeletal muscle Tnl comprises segments derived from the N-terminal regulatory domain of TnC (residues 46 to 78) and the inhibitory region of skeletal Tnl (residues 96-116) .
  • the Troponin complex is also referred to herein as the ternary complex.
  • the presence of Tnl in a complex with other troponin subunits in MI patient serum increases its stability and protects it from further degradation.
  • the troponin complex protects the sites where cardiac- specific antibodies bind.
  • U.S. 08/865,468, filed on May 29, 1997 also discloses methods to isolate the complex from MI patient serum.
  • the cardiac isotype of the myofibrillar contractile protein, Troponin I (“Tnl”) is uniquely located in cardiac muscle.
  • Tnl is the inhibitory subunit of Troponin, a thin filament regulatory protein complex, which confers calcium sensitivity to the cardiac and striated muscle.
  • Cardiac Tnl is found in human serum rapidly (within approximately 4 to 6 hours) following an MI. It reaches a peak level after approximately 18-24 hours and remains at elevated levels in the blood stream for up to 6 to 7 days.
  • immunoassays which can test for human cTnl are valuable to the medical community and to the public.
  • MI patient serum contains Tnl fragment (s) which is the result of the C-terminal processing of cTnl molecule.
  • Tnl fragment s
  • the high sequence homology found in the C-terminal region between cardiac Tnl and skeletal muscle Tnl (Larue et al. 1992 Molec. Immunology 29, 271-278, Vallins et al. 1990 FEBS Lett. 270, 57-61, Leszky et al. 1988 Biochemistry 27, 2821- 2827) produce Tnl antibodies directed against this region having non-cardiac specificity (Larue et al . 1992) .
  • r-Tnl Recombinant cardiac Tnl
  • the primary structure of r-Tnl contains 226 amino acids (SEQ ID NO: 1); 209 of them represent the Tnl sequence (SEQ ID NO: 2) .
  • r-Tnl In addition to the primary sequence of cTnl (SEQ ID NO: 2), r-Tnl, as expressed by Dade International, has a leading sequence of 8 amino acids (MASMTLWM) on the N-terminal, and a tail sequence of 9 amino acids (PMVHHHHHH) on the C-terminal (SEQ ID NO: 1) .
  • the primary structure of the r-Tnl molecule has methionine residues at positions -7, -4, 0, 153, 154, 200 and 211 (SEQ ID NO: 1) . See also Figure 1.
  • Full length cardiac troponin I is known to have the following sequence:
  • the purified CNBr-cTnl isoform has an average of 3-4 times more reactivity than r-Tnl and lower non-specific binding, as measured by radial partition immunoassay.
  • the molecular size of the CNBr- cTnl isoform is comparable in molecular weight to the major degradation product of native cardiac Tnl in MI patient serum.
  • the CNBr-cTnl isoform can be used as calibrators or controls in various cTnl immunoassays.
  • U.S. 08/865,468, filed May 29, 1997 discloses the use of cardiac troponin I fragments of the general sequence X-A-B-Y wherein X comprises any of amino acids 1-27 of full length cardiac troponin I, A comprises residues 28-69 of full length cardiac troponin I, B comprises amino acid residues 70-90 of full length cardiac troponin I, and Y comprises any sequential amino acid sequence of amino acid residues 91-170 of full length cardiac troponin I. These sequences also have increased immunoreactivity and stability over prior art compounds. Troponin T (TnT) with a molecular weight of 39,000
  • Kd is part of the troponin-tropomyosin complex of the thin filament that is part of the muscle contractile apparatus and that contains actin and tropomyosin regulatory elements. Skeletal muscle studies of TnT have found that TnT is structurally asymmetric. Its terminal globular COOH terminal domain (TnT-2) mediates its interaction with Tnl and TnC. TnT-1 at the amino terminus domain interacts with tropomyosin. See, Farah, C. and Reinach, F. (1995) Review: The Troponin complex and regulation of muscle contraction. FASEB Journal 9 755-767.
  • TnT serves as a link between the tropomyosin backbone and the Troponin I/Troponin C complex.
  • TnT has isotypes in cardiac and fast and slow skeletal muscles. It appears in serum about 3 hours after the onset of chest pain and remains elevated for at least 10 days following MI.
  • Troponin T can be obtained as described in J. Biochem . 72: pages 723-735 (1972) or J. Biol . Chem . 249: 4742-4748, or purchased commercially.
  • TnT gene promoter and derivatives thereof are disclosed in U.S. 5,266,488.
  • TnT isoforms of skeletal muscle show variation in a given species in about a 30 amino acid region of the amino terminus and about a 14 amino acid region of the carboxy terminus.
  • the calibrators and controls in Behring' s OPUS® assay are a lyophilized preparation of human cardiac troponin I in processed bovine calf serum with stabilizers.
  • the reconstituted products are stable for seven days when stored at 2 to 8C.
  • the calibrators and controls in Sanofi Pasteur's troponin I assay are a lyophilized preparation in a buffered human serum matrix.
  • the reconstituted calibrators must be used within fifteen minutes after complete reconstitution, but may be aliquoted and stored frozed at -20C for up to about six months.
  • the calibrators and controls in the Dade troponin I assay are provided frozen. When thawed the product is stable for thirty days when stored at 2-8C.
  • compositions of stabilized troponin I and/or troponin T are still necessary because under certain conditions the complex can dissociate (e.g. removal of calcium, presence of detergents such as SDS) . Moreover, the closer the analyte used in the composition is to the actual circulating isoform of the troponin complex, the better the composition will perform as a primary reference material --that is a calibrator on which other calibrators are based.
  • This invention relates to stabilized compositions of: troponin I and troponin C complex (TnlrTnC); troponin T and troponin C complex (TnT:TnC); troponin T and troponin I complexes (Tnl: TnT) and troponin I, troponin T, and troponin C complexes (Tnl : TnC: TnT) for use in immunoassay of cardiac troponins.
  • Troponin I and/or troponin T can be covalently complexed to troponin C to provide a composition that has enhanced stability and/or immunoreactivity over prior art complexes and analytes.
  • Tnl In a Tnl: TnC complex, the Tnl is covalently coupled to TnC.
  • the troponin I may be native or recombinant or may be fragmented or full-length.
  • TnT In a TnT: TnC complex, the TnT is covalently coupled to TnC.
  • the TnT may be native or recombinant or may be fragmented or full-length.
  • TnT Tnl complex the Tnl and TnT are covalently coupled.
  • TnT:TnC:TnI complex either or both of the Tnl or TnT is covalently coupled to TnC.
  • the complexes are useful as calibrators or controls for methods that assay for Tnl, TnC, and/or TnT or for use as primary reference materials.
  • the control composition should contain a buffer or serum base matrix and may contain such metal ions as calcium and/or magnesium ions.
  • the control composition may be lyophilized or liquid.
  • the covalent coupling agents include those coupling agents that provide substantially "native- length" covalent cross-linking between troponin T and/or troponin I with troponin C.
  • the term "native- length" cross-linking as used herein means a covalent bond formed between either troponin I or T with troponin C that provides a covalently coupled complex that has substantially the same immunological activity as non-covalently coupled complex.
  • the length of the covalent bond should approximate the length between troponin I and/or T with troponin C in native complex or between troponin I and troponin T in native complex. But, because protein complexes are rarely rigid in structure, it is to be understood that there is variability in the structure of the complex. The stability and immunological activity of the covalently coupled complex are what is important.
  • Figure 1 shows the amino acid sequence of cardiac troponin as expressed by Dade International (SEQ ID NO.
  • FIG. 2 shows the amino acid sequence of the CNBr cleavage product of recombinant troponin I (human cTnl isoform or TnI-153).
  • Figure 3 shows the stability and immunoreactivity at 45 C of cross-linked rTnI-153:TnC complex at two dilutions of complex.
  • the samples were evaluated using a Stratus II analyzer and Stratus Troponin Fluorometric
  • Figure 4 shows the stability at different temperatures of diluted cross-linked rTnI-153:TnC complex.
  • the samples were evaluated using a Stratus II analyzer and Stratus Troponin Fluorometric Assay Kit both available from Dade International.
  • Figure 5 shows the stability of the cross-linked rTnI-153:TnC complex using three different lots of TnC.
  • Figure 6 shows the stability of cross-linked rTnliTnC complex at 45 C.
  • Figure 7 shows polyacrylamide gels of cross-linked and non-crosslinked complexes of rTnI-153 : TnC.
  • Tnl In a Tnl: TnC complex, the Tnl is covalently coupled to TnC.
  • the cardiac troponin I may be native or recombinant and may be fragmented or full-length. While some uncomplexed troponins can be found in human serum after a myocardial event, most cardiac specific troponin is found as complex. It has been found that the Tnl in the complex is degraded by proteolytic cleavage at the C-terminal end to provide an 18,000 Kd fragment and a 14,000 Kd fragment. Generally the 14,000 Kd fragment is cleaved from the 18,000 Kd fragment.
  • the complexes of the present invention that contain cardiac troponin I contain at least a fragment of troponin I generated from the 14,000 Kd fragment. It is inherent that antibodies for use in immunoassay be generated against that portion of troponin I or troponin complex that includes the 14,000 Kd troponin I sequence. Of course, the antibody must react immunologically (e.g. have an eptitopic site on the fragment) and specifically (e.g. it should not substantially cross react with skeletal muscle troponin I) with the cardiac troponin I or complex used in the calibrator or control.
  • a human cTnl fragment generated from human cardiac r-Tnl by chemical cleavage is a preferred fragment for the Tnl: TnC complex because it is closest to the majority of the native form.
  • the cleavage of r-Tnl by cyanogen bromide (CNBr) results in a major polypeptide of 153 amino acids, hereinafter referred to as the "CNBr-cTnl isoform" (SEQ ID NO: 3) .
  • the CNBr-cTnl isoform represents 73% of the primary structure of human cTnl and is immunologically more reactive than r-Tnl as determined using radial partition immunoassay.
  • the purified CNBr-cTnl isoform has an average of 3-4 times more reactivity than r-Tnl and lower non-specific binding, as measured by radial partition immunoassay, available from Dade International Inc.
  • the molecular size of the CNBr-cTnl isoform is comparable in molecular weight to the major degradation product of native cardiac Tnl in MI patient serum and retained the epitopes for the antibodies used in the Stratus® II Tnl Immunoassay System. (See Vallins et al. (1990) FEBS Let t . 270, 57-61.)
  • the first step in cyanogen bromide cleavage is to carboxymethylate the cysteine residues of r-Tnl (there are two in the Tnl sequence) (SEQ ID NO: 1) at positions 79 and 96 in order to prevent dimerization by inter or intra molecular disulfide bridges.
  • the carboxymethylation of the cysteine residues is not a pre-requisite for the generation of the 153 amino acid isoform.
  • the carboxymethylation facilitates the process by minimizing the complications during or after CNBr digestion.
  • CNBr treatment is carried out on the carboxymethylated r-Tnl . Unlike other possible cleavage reactions (e.g. enzymatic) , the CNBr treatment removes the tail sequence, the leading sequence, and part of the Tnl C-terminal region without affecting the primary sequence of the immunogenic sites.
  • peptides are disclosed in U.S. 08/865,468, filed May 29, 1997 and include cardiac troponin I fragments of the general sequence X-A-B-Y wherein X comprises any of amino acids 1-27 of full length cardiac troponin I, A comprises residues 28-69 of full length cardiac troponin I, B comprises amino acid residues 70-90 of full length cardiac troponin I, and Y comprises any sequential amino acid sequence of amino acid residues 91-170 of full length cardiac troponin I .
  • Preferred residues for X include residues 1-27, 2- 27, 3-27, 4-27, 5-27, 6-27, 7-27, 8-27, 9-27, 10-27, 15-27, 20-27, 21-27, 22-27, 23-27, 24-27, 25-27, 26-27, and 27 of SEQ ID NO: 2. More preferably, X is amino acid 27 of SEQ ID NO: 2.
  • A comprises amino acid residues 28-69 of SEQ ID NO: 2.
  • B comprises amino acid residues 70-90 of SEQ ID NO: 2.
  • Preferred residues of Y include residues 91- 92, 91-93, 91-94, 91-95, 91-96, 91-97, 91-98, 91-99, 91-100, 91-105, 91-110, 91-115, 91-116, 91-117, 91-118, 91-119, 91-120, 91-121, 91-122, 91-123, 91-124, 91-
  • Y can be any of 91-95, 91-100, 91-105, 91-110, 91-115, 91-120, 91-130, 91-140, 91-145, 91-150, 91-153, 91-155, 91-160, 91-165, 91-170 of SEQ ID NO: 2.
  • the lower molecular weight 14,000 Tnl fragment, isolated from a pool of patient serum has been sequenced for N-terminal identification.
  • the N- terminal sequence of the Tnl 14,000 fragment starts at position 27 (Ala) in human cardiac Tnl sequence.
  • the 14,000 fragment is approximately 100 amino acids long, ending in the region from about amino acid 120 to about amino acid 130 in intact cTnl .
  • the N-terminal sequence of the 18,000 fragment starts at or very near the N- terminus of the intact human cTnl .
  • the 18,000 fragment is approximately 140 amino acids long, ending in the region from about amino acid number 135 to about 145 in intact cTnl .
  • one preferred group of fragments has X as 25-27, 26-27 or 27 of SEQ ID NO: 2 and Y as 91 to any of 135-145 of SEQ ID NO: 2.
  • the fragments also may be those cardiac troponin I protein fragments containing the sequence AYATEPHAKKKSKISASRKLQLKTLLLQIAKQEL (SEQ ID NO: 4) or RAYATEPHAKKKSKISASRKLQLKTLLLQIAKQEL (SEQ ID NO: 5) .
  • the fragments may be recombinant sequences such as MADGSSDAAREPRPAPAPIRRRSSNYRAYATEPHAKKKSKISASRKLQLKTLLLQ IAKQELEREAEERRGEKGRALSTRCQPLELAGLGFAELQDLCRQLHARVDKVDEE RYDIEAKVTKNITEIADLTQKIFDLRGKFKRPTLRRVRISADAMMQALLGARAKE SLDLRAHLKQVKKEDTEKENREVGDWRKNIDALSGMEGRKKKKFEES ( SEQ ID NO: 6);
  • ADGSSDAAREPRPAPAPIRRRSSNYRAYATEPHAKKKSKISASRKLQLKTLLLQI AKQELEREAEERRGEKGRALSTRCQ (SEQ ID NO: 7); or similar human or bovine fragments. It should be understood that while human troponin is preferred, other species may be substituted. Generally, these other species lack the appropriate methionine residue in the full length primary structure. However, insertion of methionine into the primary structure at positions that upon cleavage by CNBr would provide an appropriate fragment would allow the use of alternative species.
  • Troponin C is commercially available from a number of sources and the source or species is not critical. Generally, rabbit troponin C is used because of the lower cost, but human and other species can also be used. Recombinant troponin C can also be used.
  • TnC has a Ca++/Mg++ binding domain in the COOH terminal region and a Ca++ binding domain in the amino terminus region and is thought to be "dumb-bell" shaped connected by a long central helix.
  • the covalent coupling agents useful in the present invention include those coupling agents that provide substantially "native-length” covalent cross-linking between troponin T and/or troponin I with troponin C.
  • the preferred coupling agents form covalent bonds between the Tnl or TnT and TnC that approximate the distance between the proteins as they exist in the complex.
  • the cross-linkers may be those "zero-length” crosslinkers such as l-ethyl-3- [ 3- (dimethylamino) propyl] carbodiimide (EDC) and other water soluble carbodiimides providing an amide bond between an activated carboxyl group on one protein and coupling to an amino group on the other protein.
  • the complex is prepared by combining the coupling agent with troponin C and troponin I in a manner specific for the coupling agent.
  • the coupling reaction of the TnC and Tnl should take place in the presence of Ca++ or Mg++ or other divalent metal ions.
  • the conditions will vary depending on the coupling agent utilized, but those conditions can readily be determined by those skilled in the art with reference to known and published methods.
  • the choice of buffer is not critical, although the buffer should have a molarity from about 10 to 200 ⁇ iM.
  • the concentration of calcium and magnesium ion is not critical, but preferably should be from about 20 ⁇ M to about 20 mM. If magnesium ion is used alone it should be in higher concentrations than that used for calcium.
  • Typical amounts of calcium and/or magnesium are from about 2-5 mM.
  • the buffer may include a salt such as sodium chloride or potassium chloride at from about 50 mM to 500 mM.
  • the amount of troponin C is not critical, but should be in molar amounts equal to or greater than the amount of troponin I that will be utilized. Generally, the amount of troponin C may be from 0.02 mg/mL to 5 mg/mL.
  • the amount of coupling agent may need to be adjusted depending on the amount of troponin C.
  • diluted final coupled product are evaluated immunologically in a troponin I assay (such as those available from Dade International Inc.) and may be compared to native complex or non-covalently coupled complex or commercially available products evaluated in the same manner.
  • a troponin I assay such as those available from Dade International Inc.
  • the clinical range of interest of troponin I or T is about 0.01 ng/mL to less than 1 ⁇ g/mL and typically 0.1 ng/ml to 200 ng/mL.
  • stability may be determined by comparing the immunological activity over time at one or more temperatures in comparison to native complex or non- covalently coupled complex or commercially available products evaluated in the same manner or by running electrophoretic gels of the complexes to evaluate the stability.
  • Native complex may be obtained in serum samples.
  • native complex can be isolated. Methods are known to those skilled in the art. For instance, a preferred method of isolating the Tn complex comprises incubating the sample to be tested with a substrate coated with antibodies to the subunits of the Tn complex. Many antibodies are useful, and can be selected by one of skill in the art. Examples of such antibodies include anti-Tnl, anti-TnC, and anti-TnT antibodies.
  • a preferred substrate is beads, and more preferably the substrate comprises latex beads.
  • the bound complex is eluted under conditions that do not affect association of Tn subunits, e.g. using urea. These conditions can be determined by one of skill in the art.
  • a preferred buffer system comprises urea and lacks SDS.
  • a preferred coupling agent is EDC or other water soluble carbodiimides.
  • EDC EDC or other water soluble carbodiimides.
  • the concentration of EDC is not critical and may be from 1-10 mM.
  • Compounds such as N- hydroxysuccinimide (NHS) or SNHS at about 1-10 mM may be added to enhance the activation of troponin C by water soluble carbodiimides.
  • the NHS is typically added prior to the addition of EDC and incubates with the protein for at least about 5 minutes, although 15 minutes is typical. Then the EDC is added and the mixture is incubated, typically at room temperature, for about 15 minutes, but typically for thirty minutes or more.
  • the reaction proceeds best at mildly acidic pH values (e.g. about 6), but the pH may range from 5- 9.
  • a reducing agent such as mercaptoethanol is added to stop the reaction.
  • reducing agents may be substituted for mercaptoethanol .
  • cardiac troponin I preferably the CNBr-Tnl isoform
  • cardiac troponin I is added to provide a molar ratio of about 1:1 with troponin C, although the amount of Tnl may be less.
  • Tnl is generally in a buffer that contains salt or urea in sufficient amounts to solubilize the Tnl.
  • a typical buffer is 100 mM sodium phosphate, 10 mM Tris and 8 M urea at pH 8 (PTU buffer) .
  • the choice of the buffer is not critical to the invention.
  • the buffer must maintain the solubility of the cTnl .
  • the reactants incubate, generally at room temperature, for about an hour and typically about two hours.
  • the formed complex may be buffer exchanged into another buffer.
  • the activity of the cross-linked complex is measured using a Stratus Troponin immunoassay and compared to native complex.
  • the presence of the covalently cross- linked complex may be confirmed using polyacrylamide gel electrophoresis .
  • the complex will not dissociate under reducing conditions or in the presence of EDTA or other metal complexing agent.
  • the non-specific coupling agents such as EDC
  • calcium or magnesium ion should be present in either the TnC or Tnl solution.
  • the calcium and/or magnesium causes complex formation to occur.
  • the complex forms as it would in native complex so the spatial orientation of the proteins will be comparable to native complex or non-covalently coupled complex.
  • the cross-linking occurs more selectively and the bond formed will "freeze" the complex in the correct conformation.
  • the covalently coupled complex is insensitive to EDTA or other chelating agents (thus, independent of calcium or magnesium) , does not dissociate in the presence of SDS, and is more resistant to higher temperatures than the non-cross- linked complex.
  • TnC rather than the Tnl or TnT, should be subjected to EDC or other water soluble carbodiimide treatments.
  • EDC electrospray
  • the epitopic site would be affected by the non-specific coupling agent — that is the Tnl or fragment would be less immunologically active.
  • TnT: TnC complex and TnT: TnC: Tnl complex are prepared in a similar fashion to the Tnl: TnC.
  • TnT fragments particularly the carboxy fragments such as TnT-2 are preferred.
  • the troponin T should be added in molar amounts equal to or less than the amount of troponin C.
  • Troponin C may be from less than 0.02 mg/mL to 5 mg/mL.
  • the ranges for Tnl and TnT are similar.
  • the TnT : TnC complex is evaluated as described for troponin I complexes, except using an assay for troponin T. Troponin T assays are available from Boehringer Mannheim.
  • a TnT: Tnl complex may also be prepared, however, as with the other complexes of this invention, the immunological (epitopic) sites must be substantially retained. Since both TnT and Tnl are measured immunologically, it is preferred that the epitopic region be retained for both proteins. Thus, less nonspecific coupling agents may be useful than agents such as EDC or oxalic acid derivatives. It has been described that skeletal muscle Tnl complexes with TnT at about amino acids 40-80 of Tnl. See Potter, J.D. et al. (1995) A Direct Regulatory Role of Troponin T and a Dual Role for Troponin C in the Ca++ Regulation of Muscle Control. Journal of Biologi cal Chemistry 210 (6) 2557-2562.
  • the homologous site on cTnl would be useful for coupling.
  • Tnl and TnT are added in approximately equimolar ratios. The amounts may be from 0.02 mg/mL to 5 mg/mL. It is important that the immunological site not be altered. It should be understood that the eptitopic site will vary depending on the antibody used in the assay. The generation of antibodies is described in the art, for example, by Bodor et al., (1992) Development of Monoclonal Antibodies for an Assay of Cardiac Troponin- I and Preliminary Results in Suspected Cases of Myocardial Infarction, Clinical Chemistry 38 (11) 2203-2214.
  • the present invention uses a defined base material useful as a control matrix for containing and maintaining the troponin complexes, the base material comprising an aqueous solution of a buffer to maintain the pH at 5-8, anti-microbial agents and may contain other stabilizers including calcium ions or proteins.
  • the defined base material may be utilized to prepare stock solutions and controls including troponin I or troponin I fragments, troponin T or troponin T fragments complexed with Troponin C or troponin I complexed with troponin T.
  • the resulting solution can be stored as a liquid or frozen or also can be lyophilized if appropriate fillers are included.
  • a stock solution at higher concentrations of troponin I and/or troponin T than those that will be utilized in the final assay control.
  • the stock can be stored frozen or lyophilized and thawed or reconstituted when necessary to prepare the appropriate dilutions of controls or calibration standards.
  • the complexes prepared as described above may be buffer exchanged into an appropriate buffer after covalent coupling.
  • the aqueous solution used to prepare the stock and controls may include a buffer and the buffer may generally be any of the buffers that function in the pH range of 5 to 8. Of these buffers, the buffers that are preferred function are in the pH range of 6-8.
  • the concentration of buffer is between 10 mM to 200 mM. It is preferred to keep the buffer concentration lower - in the range of 20-100 mM.
  • the buffers used for the calibrators or controls contain bovine serum albumin (BSA) .
  • BSA bovine serum albumin
  • the buffer contains, BSA, sugars, salt and an antibacterial agent.
  • buffers examples include HEPS, MES or TRIS buffers.
  • a preferred buffer comprises MES buffer containing 6.5% BSA, at pH 6-7.
  • Other preferred buffers contain a reducing agent, stabilizing protein, chelating agent and a salt as described in the copending application U.S.S.N. 08/400,158, incorporated herein by reference.
  • the fragments are spiked into the serum, e.g., human or bovine, or into diluted serum, e.g., serum diluted 1:1 with MES buffer containing BSA.
  • Anti-microbial and anti-fungal agents may be added to prevent growth and may include those commonly found in the prior art at the concentrations found in the prior art such as gentamycin, clortrimazole, sodium azide, mycostatin, thimerosal, Kathon and/or Proclin 300.
  • stabilizing proteins such as albumin, gelatin, ovalalbumin, or casein may be included.
  • the concentration of stabilizing protein may be from 0 to 15% and preferably from 7 to 12%.
  • the stabilizing protein is albumin and preferably the albumin is substantially protease free.
  • the solution have low protease activity, thus protease inhibitors such as aprotinin and "Protease Inhibitor” (Sigma) are effective.
  • protease inhibitors such as aprotinin and "Protease Inhibitor” (Sigma) are effective.
  • the use of the recombinant fragments as described herein are not as sensitive to protease activity as is the full length protein.
  • the inhibitors may be added and may be used at the manufacturer's recommended concentration.
  • protease inhibitors examples include benzamidine, (2S, 3R) -3-Amino-2-hydroxy-5- methylhexanoyl] -Val-Val-Asp (Amastatin-Sigma) , [2S, 3R] -3-Amino-2-hydroxy-4- [4-nitrophenyl] - butanoyl-L-leucine, Antipain, [2S, 3R] -3-Amino-2- hydroxy-5-methylhexanoyl] -Val-Val-Asp
  • Serum may be included if desired. Again, the use of fragments that are similar to the 14,000 Kd fragments substantially eliminates the concerns of proteases.
  • Controls prepared by this method may be lyophilized by adding those bulking agents that are known in the art, but the controls may also be liquid. In addition, the liquid controls may be frozen to further increase shelf-life.
  • Assays for detecting cTnl and cTnT in MI patient serum utilize a sandwich assay.
  • the complexes of the present invention can also be used to design competitive-type assays for the detection of cTnl or cTnT in serum. In such an assay, a subsaturating amount of antibody to cTnl or cTnT is bound to a solid phase, e.g., a microtiter plate or latex beads.
  • the complexes of the present invention are labeled, e.g., with alkaline phosphatase, or horseradish peroxidase.
  • a constant amount of the labeled complex is mixed with the sample of MI patient serum containing an unknown amount of cTnl and/or cTnT .
  • the test sample is then allowed to bind to the subsaturating amount of cTnl and/or cTnT antibody bound to a solid phase.
  • the cTnl and/or cTnT in the sample will compete with the labeled complex for binding with the antibody-coated solid phase. Unbound proteins are removed by washing and the amount of labeled complex bound to the solid phase is measured.
  • the amount of labeled complex bound to the antibody on the solid phase indicates the amount of cTnl or cTnT present in the serum. If the serum contains a high concentration of cTnl or cTnT, it will compete effectively with the labeled complex and little or none of the labeled complex will bind the antibody-coated solid phase.
  • Example 1 Preparation of a defined base material for cardiac markers .
  • Antioxidants such as 200 milligrams of glutathione, 200 milligrams of glucose, 50 gs of ascorbic acid, and 1.1 milliliter of phenol, about 2.7 grams of L-Lactate, about 225 milligrams of calcium chloride or other calcium salt to provide 1-3 mM calcium ion
  • anti-microbial and anti-fungal agents such as about 20 milligrams of chlortrimazole, 35 milligrams of gentamicin, and about 1 milliliter of Proclin 300, about 95 grams of protease free BSA, and about 1 gram of gelatin are combined in an aqueous 50 mM TRIS buffered solution at about pH 7.3 also containing a salt such as sodium chloride (about 30 grams) to provide about one liter of base material.
  • gelatin in solution it is best to add the gelatin in solution by dissolving the gelatin by adding 1 gram of gelatin to 100 milliliters of water and gently heating to dissolve the gelatin. Then the gelatin containing solution is added to the base material.
  • Example 2 The resulting solution is filtered using filters sufficient to remove any bacteria such as a .22 micron filter. A low protein binding filter is preferred.
  • Example 2 A low protein binding filter is preferred.
  • the mixture was incubated for two hours at room temperature.
  • the complex is buffer exchanged.
  • the activity of the crossed linked complex was measured using Stratus Tnl immunoassay.
  • the presence of a covalent cross-linked complex was confirmed on polyacrylamide gel electrophoresis.
  • the resulting complex is less sensitive to environment, including temperature than native complex.
  • the resulting stock solution is sterile filtered using low protein binding filters of 0.22 microns or less.
  • the stock solution may be stored frozen at -20° C for longer than two years.
  • the stock solution may be stored at 2-8° C for more than one week.
  • the stock solution is used to prepare diluted solutions of troponin I in the clinical range of interest (about 0 to 200 ng/mL) by diluting the stock solution in the defined base material prepared in Example 1 or other base material.
  • FIG. 1 shows the stability of two concentrations of diluted stock (25 ng/mL and 45 ng/mL of troponin I) of the complex stored at 45 C. The dilutions are stable for greater than three weeks at 45 C.
  • Figure 4 shows a 28 ng/mL solution was evaluated for stability at 4C, 25C, 37C, and 45 C and was stable for at least six weeks at all temperatures.
  • Figure 5 shows the stability of the complex when prepared with three different lot numbers of commercially available TnC. All lots were stable for over 10 days at 45 C. A full length rTnl-TnC complex was also prepared. The stability of the cross-linked complex at 45 C is shown in Figure 6.
  • Lanes 2-4 show the electrophoretic pattern of covalently linked rTnI-153:TnC complex in the presence of EDTA (a metal chelator) .
  • Lane 5 shows a non covalently linked rTnI-153:TnC complex in the absence of EDTA.
  • Lanes 6-7 show he electrophoretic pattern of non covalently linked rTnI-153:TnC complex in the presence of EDTA. The disappearance of the upper band of complex is evident in Lanes 6-7, but not in Lanes 2-4.
  • Lane 8 is TnC. See, Figure 7.
  • Example 2 is repeated except that troponin T is substituted for the troponin I.
  • Aliquots of stock solution are diluted to the clinical range of interest from 0.01 ng/mL to 10 ng/mL. The aliquots may be analyzed for immunological activity using a troponin T assay such as that assay commercially available from Boehringer Mannheim.
  • Example 2 is repeated except that both troponin I and troponin T are added to the activated troponin C.
  • the ternary complex may be observed using electrophoresis run in the presence of EDTA.
  • the troponin I immunological activity may be evaluated as described in Example 2 and the troponin T immunological activity may be evaluated as described in Example 5.

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Abstract

Stabilized compositions for use in clinical assays for troponin are disclosed. The compositions are covalently coupled complexes of cardiac troponin I, cardiac troponin T, and/or troponin C.

Description

COVALENTLY COUPLED TROPONIN COMPLEXES
Field of Invention
The present invention relates generally to clinical chemistry. In particular, it relates to stabilized troponin complexes useful in the diagnosis of myocardial infarction or other ischemic events.
Cross-References to Related Applications
This application is a continuation-in-part of U.S. Serial No. 08/865,468, filed May 29, 1997 and of U.S. Serial No. 08/874,566, filed on June 13, 1997.
Background of the Invention
The determination of the presence or amount of certain constituents or analytes is useful in the diagnosis of disease and physical well-being. Compositions which behave similarly to how constituents present in human bodily fluids (e.g. blood, blood serum, plasma, spinal fluid or urine) behave are used in clinical laboratories. These compositions assist in the determination of whether the clinical instrumentation and procedures used by the laboratory to measure the constituents are accurate. These compositions are also used to calibrate the clinical devices which measure the amount or presence of the constituent in a sample. These compositions will be referred to hereinafter as control compositions or controls . In addition, it is important that the analyte or analyte analog present in the control composition behave similarly to the corresponding analyte to be tested for in a patient's bodily fluid —that is, the control composition should mimic the patient sample.
Rapid and simple tests that can be used to accurately diagnose the occurrence of myocardial infarction ("MI") or distinguish other ischemic events such as unstable angina are extremely important.
Cardiac troponin I (cTnl) and troponin T have recently become established as the markers of choice in evaluating cardiac distress. See, New England Journal of Medicine Volume 335 No. 18, pages 1342-1349, Antman et al. and pages 1333-1341, Ohman et al.
The Troponin complex is present in both skeletal and cardiac muscles and consists of three subunits, Troponin T ("TnT") the tropomyosin binding subunit, Troponin C ("TnC"), the Ca++ binding subunit and Tnl, which inhibits the actomyosin Mg++-ATPase.
The majority of the research into the troponin complex has centered around the regulatory function and structure of the troponin complex in skeletal muscle. The troponin complex assists in muscle contraction. The TnC molecule has four binding domains to bind divalent metal ions. The Ca++/Mg++ binding sites are in the COOH terminal region and the Ca++ binding sites are in the amino terminal region. In studies of skeletal muscle, in the absence of Ca++, the amino terminus of Tnl binds to the COOH terminus region of TnC and to the globular COOH terminus region of TnT .
Thus, research indicates that Tnl and TnC are anti- parallel and Tnl and TnT are anti-parallel. The presence of calcium ion increases the TnC amino terminus domain' s affinity for the inhibitory and COOH regions of Tnl. In addition, there is a hydrophobic surface in the N-terminal domain of TnC that represents a Ca++ dependent binding site for Tnl and TnT. It has been proposed that the Ca++ dependent reactions relate to the regulatory mechanism and Ca++ independent interactions maintain the structural integrity of the complex. In order to study structure and function of the troponin complex in its regulation of skeletal muscle, cross-linking studies have been accomplished. See, Farah, C. and Reinach, F. Review: The Troponin complex and regula tion of muscle contraction . FASEB Journal 9 pp. 755-767 (1995). Covalent binding between TnC and skeletal muscle Tnl has been formed between the carboxyl groups in the TnC and lysine groups in Tnl using EDC. Kobayoshi et al. (1994), Structure of the troponin complex: implications of photocross-linking of troponin I to troponin C thiol mutants. J. Biol . Chem . 269, 5725-5729. In addition Leszyk et al. (1987) Cross- linking of rabbit skeletal muscle troponin with the photoactive reagent 4-malemidobenzophenone; identification of residues in troponin I that are close to cystein-98 of troponin C. Biochemistry 26, 7042- 7047, reported that the main product of cross-linking between TnC and skeletal muscle Tnl comprises segments derived from the N-terminal regulatory domain of TnC (residues 46 to 78) and the inhibitory region of skeletal Tnl (residues 96-116) . The Troponin complex is also referred to herein as the ternary complex.
U.S. 08/865,468, filed on May 29, 1997 and also owned by applicant, discloses that it had been discovered that the majority of native cTnl in human serum after an MI is associated with TnC and TnT. The presence of Tnl in a complex with other troponin subunits in MI patient serum increases its stability and protects it from further degradation. In addition the troponin complex protects the sites where cardiac- specific antibodies bind. U.S. 08/865,468, filed on May 29, 1997 also discloses methods to isolate the complex from MI patient serum. The cardiac isotype of the myofibrillar contractile protein, Troponin I ("Tnl"), is uniquely located in cardiac muscle. Tnl is the inhibitory subunit of Troponin, a thin filament regulatory protein complex, which confers calcium sensitivity to the cardiac and striated muscle. Troponin I exists in three isoforms: two skeletal Tnl (fast and slow) isoforms (Molecular Weight = 19,800 daltons) and a cardiac Tnl ("cTnl") isoform with an additional 31 residues (human Tnl) on the N-terminus resulting in a molecular weight of 23,000 daltons.
Cardiac Tnl is found in human serum rapidly (within approximately 4 to 6 hours) following an MI. It reaches a peak level after approximately 18-24 hours and remains at elevated levels in the blood stream for up to 6 to 7 days. Thus, immunoassays which can test for human cTnl are valuable to the medical community and to the public.
It is desirable to use an immunologically reactive human cTnl isoform comparable to that found in MI patient serum. We found that MI patient serum contains Tnl fragment (s) which is the result of the C-terminal processing of cTnl molecule. The high sequence homology found in the C-terminal region between cardiac Tnl and skeletal muscle Tnl (Larue et al. 1992 Molec. Immunology 29, 271-278, Vallins et al. 1990 FEBS Lett. 270, 57-61, Leszky et al. 1988 Biochemistry 27, 2821- 2827) produce Tnl antibodies directed against this region having non-cardiac specificity (Larue et al . 1992) . Our data and Larue et al. 1992 suggest that most of the known cTnl specific antibodies have their epitopes located approximately in the first 75% of the Tnl molecule. Therefore, this portion of the Tnl molecule should function as a MI specific cTnl isoform in most immunoassay systems. Currently cTnl immunoassays are commercially available from Dade International, Behring Diagnostics, and Sanofi Pasteur Diagnostics. The Dade product is the Stratus® Cardiac Troponin-I assay.
Native intact human cTnl is difficult to obtain because of the scarcity of human heart and native intact human cTnl is highly subject to proteolytic degradation during purification. Recombinant cardiac Tnl ("r-Tnl") , unlike the native human cTnl, can be produced and purified in acceptable quantities. As expressed by Dade, the primary structure of r-Tnl contains 226 amino acids (SEQ ID NO: 1); 209 of them represent the Tnl sequence (SEQ ID NO: 2) . In addition to the primary sequence of cTnl (SEQ ID NO: 2), r-Tnl, as expressed by Dade International, has a leading sequence of 8 amino acids (MASMTLWM) on the N-terminal, and a tail sequence of 9 amino acids (PMVHHHHHH) on the C-terminal (SEQ ID NO: 1) . The primary structure of the r-Tnl molecule has methionine residues at positions -7, -4, 0, 153, 154, 200 and 211 (SEQ ID NO: 1) . See also Figure 1.
Full length cardiac troponin I is known to have the following sequence:
ADGSSDAAREPRPAPAPIRRRSSNYRAYATEPHAKKKSKISASRKLQLKT LLLQIAKQELEREAEERRGEKGRALSTRCQPLELTGLGFAELQDLCRQLH ARVDKVDEERYDIEAKVTKNITEIADLTQKIFDLRGKFKRPTLRRVRISA DAMMQALLGARAKESLDLRAHLKVKKEDTEKENREVGDWRKNIDALSGME GRKKKFES (SEQ ID NO: 2) (Armour, K.L. et al., (1993) Cloning and Expression in Escheria Coli of the cDNA Encoding Human Cardiac Troponin I, Gene , 131 (2) :287-292) .
U.S. Serial No .08/564 , 526, also owned by applicants, and incorporated herein by reference, discloses the use of a human cTnl fragment generated from human r-Tnl by chemical cleavage. The cleavage of r-Tnl by cyanogen bromide (CNBr) results in a major polypeptide of 153 amino acids, hereinafter referred to as the "CNBr-cTnl isoform" (SEQ ID NO: 3) . See Figure 2. The CNBr-cTnl isoform represents 73% of the primary structure of human cTnl and is immunologically more reactive than r-Tnl . The purified CNBr-cTnl isoform has an average of 3-4 times more reactivity than r-Tnl and lower non-specific binding, as measured by radial partition immunoassay. The molecular size of the CNBr- cTnl isoform is comparable in molecular weight to the major degradation product of native cardiac Tnl in MI patient serum.
It is desirable to use an immunologically reactive human cTnl isoform comparable to that detected in MI patient serum. The availability of r-Tnl can facilitate the production of cardiac cTnl isoforms. Moreover, since most of the known human cardiac specific Tnl antibodies have their epitopes located approximately in the first 75% of the Tnl molecule, that portion of the Tnl molecule will function as a cTnl isoform in most immunoassays.
The CNBr-cTnl isoform can be used as calibrators or controls in various cTnl immunoassays. U.S. 08/865,468, filed May 29, 1997, discloses the use of cardiac troponin I fragments of the general sequence X-A-B-Y wherein X comprises any of amino acids 1-27 of full length cardiac troponin I, A comprises residues 28-69 of full length cardiac troponin I, B comprises amino acid residues 70-90 of full length cardiac troponin I, and Y comprises any sequential amino acid sequence of amino acid residues 91-170 of full length cardiac troponin I. These sequences also have increased immunoreactivity and stability over prior art compounds. Troponin T (TnT) with a molecular weight of 39,000
Kd is part of the troponin-tropomyosin complex of the thin filament that is part of the muscle contractile apparatus and that contains actin and tropomyosin regulatory elements. Skeletal muscle studies of TnT have found that TnT is structurally asymmetric. Its terminal globular COOH terminal domain (TnT-2) mediates its interaction with Tnl and TnC. TnT-1 at the amino terminus domain interacts with tropomyosin. See, Farah, C. and Reinach, F. (1995) Review: The Troponin complex and regulation of muscle contraction. FASEB Journal 9 755-767. It is reported that skeletal TnT is cleaved into the skeletal TnT-1 and TnT-2TnI-TnC fragments by mild proteolysis. Schaertl, S. et al. (1995) Separation and Characterization of the Two Functional Regions of Troponin Involved in Muscle Thin Filament Regulation. Biochemistry 34 (49) 15890-15894. TnT serves as a link between the tropomyosin backbone and the Troponin I/Troponin C complex. TnT has isotypes in cardiac and fast and slow skeletal muscles. It appears in serum about 3 hours after the onset of chest pain and remains elevated for at least 10 days following MI. Despite its lack of complete cardiac specificity it can be useful because of its rapid appearance into the bloodstream. Troponin T can be obtained as described in J. Biochem . 72: pages 723-735 (1972) or J. Biol . Chem . 249: 4742-4748, or purchased commercially. TnT gene promoter and derivatives thereof are disclosed in U.S. 5,266,488. TnT isoforms of skeletal muscle show variation in a given species in about a 30 amino acid region of the amino terminus and about a 14 amino acid region of the carboxy terminus. Pan, B.S. and Potter, J.D.(1992) Two Genetically Expressed Troponin T fragments Representing α and β Isoforms Exhibit Functional Differences. Journal of Biological Chemistry 267 (82) 23052-23056.
In vi tro stabilized solutions for cardiac markers have been disclosed. U.S. 5,583,200 and Bodor et al., (1992) Development of Monoclonal Antibodies for an Assay of Cardiac Troponin-I and Preliminary Results in Suspected Cases of Myocardial Infarction, Clinical Chemistry 38, (11) 2203-2214 at 2204 disclose stabilized troponin T and/or troponin I using troponin C and calcium ion. U.S. 5,583,200 discloses that serum may be added. U.S. 08/874,566, filed June 13, 1997, discloses improvements in stabilizing the troponin T or troponin I/troponin C complex and discloses solutions useful as calibrators or controls for diagnostic assays measuring troponin. U.S. Serial No .08/564 , 526 and U.S. Serial No. 08/865,468, filed May 29, 1997 also disclose the effect of TnC upon the immunological and biological activity and non-specific binding of the CNBr-cTnl isoform and other fragments. U.S. Serial No .08/564 , 526 discloses the activity of the complex formed by the CNBr - cTnl isoform, TnC and TnT as useful in immunoassays .
The calibrators and controls in Behring' s OPUS® assay are a lyophilized preparation of human cardiac troponin I in processed bovine calf serum with stabilizers. The reconstituted products are stable for seven days when stored at 2 to 8C. The calibrators and controls in Sanofi Pasteur's troponin I assay are a lyophilized preparation in a buffered human serum matrix. The reconstituted calibrators must be used within fifteen minutes after complete reconstitution, but may be aliquoted and stored frozed at -20C for up to about six months. The calibrators and controls in the Dade troponin I assay are provided frozen. When thawed the product is stable for thirty days when stored at 2-8C.
Improved methods and compositions of stabilized troponin I and/or troponin T are still necessary because under certain conditions the complex can dissociate (e.g. removal of calcium, presence of detergents such as SDS) . Moreover, the closer the analyte used in the composition is to the actual circulating isoform of the troponin complex, the better the composition will perform as a primary reference material --that is a calibrator on which other calibrators are based.
Summary of the Invention
This invention relates to stabilized compositions of: troponin I and troponin C complex (TnlrTnC); troponin T and troponin C complex (TnT:TnC); troponin T and troponin I complexes (Tnl: TnT) and troponin I, troponin T, and troponin C complexes (Tnl : TnC: TnT) for use in immunoassay of cardiac troponins.
Troponin I and/or troponin T can be covalently complexed to troponin C to provide a composition that has enhanced stability and/or immunoreactivity over prior art complexes and analytes.
In a Tnl: TnC complex, the Tnl is covalently coupled to TnC. The troponin I may be native or recombinant or may be fragmented or full-length.
In a TnT: TnC complex, the TnT is covalently coupled to TnC. The TnT may be native or recombinant or may be fragmented or full-length.
In a TnT: Tnl complex the Tnl and TnT are covalently coupled.
In a TnT:TnC:TnI complex either or both of the Tnl or TnT is covalently coupled to TnC.
The complexes are useful as calibrators or controls for methods that assay for Tnl, TnC, and/or TnT or for use as primary reference materials.
The control composition should contain a buffer or serum base matrix and may contain such metal ions as calcium and/or magnesium ions. The control composition may be lyophilized or liquid. The covalent coupling agents include those coupling agents that provide substantially "native- length" covalent cross-linking between troponin T and/or troponin I with troponin C. The term "native- length" cross-linking as used herein means a covalent bond formed between either troponin I or T with troponin C that provides a covalently coupled complex that has substantially the same immunological activity as non-covalently coupled complex. Generally the length of the covalent bond should approximate the length between troponin I and/or T with troponin C in native complex or between troponin I and troponin T in native complex. But, because protein complexes are rarely rigid in structure, it is to be understood that there is variability in the structure of the complex. The stability and immunological activity of the covalently coupled complex are what is important.
Brief Description of the Figures
Figure 1 shows the amino acid sequence of cardiac troponin as expressed by Dade International (SEQ ID NO.
1) and of cardiac troponin I (SEQ ID NO. 2) . Figure 2 shows the amino acid sequence of the CNBr cleavage product of recombinant troponin I (human cTnl isoform or TnI-153).
Figure 3 shows the stability and immunoreactivity at 45 C of cross-linked rTnI-153:TnC complex at two dilutions of complex. The samples were evaluated using a Stratus II analyzer and Stratus Troponin Fluorometric
Assay Kit both available from Dade International.
Figure 4 shows the stability at different temperatures of diluted cross-linked rTnI-153:TnC complex. The samples were evaluated using a Stratus II analyzer and Stratus Troponin Fluorometric Assay Kit both available from Dade International.
Figure 5 shows the stability of the cross-linked rTnI-153:TnC complex using three different lots of TnC. Figure 6 shows the stability of cross-linked rTnliTnC complex at 45 C.
Figure 7 shows polyacrylamide gels of cross-linked and non-crosslinked complexes of rTnI-153 : TnC.
Detailed Description of the Invention
In a Tnl: TnC complex, the Tnl is covalently coupled to TnC. The cardiac troponin I may be native or recombinant and may be fragmented or full-length. While some uncomplexed troponins can be found in human serum after a myocardial event, most cardiac specific troponin is found as complex. It has been found that the Tnl in the complex is degraded by proteolytic cleavage at the C-terminal end to provide an 18,000 Kd fragment and a 14,000 Kd fragment. Generally the 14,000 Kd fragment is cleaved from the 18,000 Kd fragment. After the cleavage to the 18,000 fragment, an N- terminus proteolytic cleavage occurs at the carboxyl side of Arg 26, thus eliminating the first 26 amino acids of the N-terminus. The 31 amino acid sequence at the N-terminus had been proposed as the best position to direct antibodies against, however, this recent finding suggests that those antibodies would only recognize a fraction of serum Tnl. Thus, it is preferred that the complexes of the present invention that contain cardiac troponin I contain at least a fragment of troponin I generated from the 14,000 Kd fragment. It is inherent that antibodies for use in immunoassay be generated against that portion of troponin I or troponin complex that includes the 14,000 Kd troponin I sequence. Of course, the antibody must react immunologically (e.g. have an eptitopic site on the fragment) and specifically (e.g. it should not substantially cross react with skeletal muscle troponin I) with the cardiac troponin I or complex used in the calibrator or control.
Thus, the use of a human cTnl fragment generated from human cardiac r-Tnl by chemical cleavage is a preferred fragment for the Tnl: TnC complex because it is closest to the majority of the native form. The cleavage of r-Tnl by cyanogen bromide (CNBr) results in a major polypeptide of 153 amino acids, hereinafter referred to as the "CNBr-cTnl isoform" (SEQ ID NO: 3) . The CNBr-cTnl isoform represents 73% of the primary structure of human cTnl and is immunologically more reactive than r-Tnl as determined using radial partition immunoassay. The purified CNBr-cTnl isoform has an average of 3-4 times more reactivity than r-Tnl and lower non-specific binding, as measured by radial partition immunoassay, available from Dade International Inc. As demonstrated in Figure 2 the molecular size of the CNBr-cTnl isoform is comparable in molecular weight to the major degradation product of native cardiac Tnl in MI patient serum and retained the epitopes for the antibodies used in the Stratus® II Tnl Immunoassay System. (See Vallins et al. (1990) FEBS Let t . 270, 57-61.)
Generally described, the first step in cyanogen bromide cleavage is to carboxymethylate the cysteine residues of r-Tnl (there are two in the Tnl sequence) (SEQ ID NO: 1) at positions 79 and 96 in order to prevent dimerization by inter or intra molecular disulfide bridges. The carboxymethylation of the cysteine residues is not a pre-requisite for the generation of the 153 amino acid isoform. (SEQ ID NO:
3.) Rather, the carboxymethylation facilitates the process by minimizing the complications during or after CNBr digestion. CNBr treatment is carried out on the carboxymethylated r-Tnl . Unlike other possible cleavage reactions (e.g. enzymatic) , the CNBr treatment removes the tail sequence, the leading sequence, and part of the Tnl C-terminal region without affecting the primary sequence of the immunogenic sites.
Other preferred peptides are disclosed in U.S. 08/865,468, filed May 29, 1997 and include cardiac troponin I fragments of the general sequence X-A-B-Y wherein X comprises any of amino acids 1-27 of full length cardiac troponin I, A comprises residues 28-69 of full length cardiac troponin I, B comprises amino acid residues 70-90 of full length cardiac troponin I, and Y comprises any sequential amino acid sequence of amino acid residues 91-170 of full length cardiac troponin I .
Preferred residues for X include residues 1-27, 2- 27, 3-27, 4-27, 5-27, 6-27, 7-27, 8-27, 9-27, 10-27, 15-27, 20-27, 21-27, 22-27, 23-27, 24-27, 25-27, 26-27, and 27 of SEQ ID NO: 2. More preferably, X is amino acid 27 of SEQ ID NO: 2.
A comprises amino acid residues 28-69 of SEQ ID NO: 2. B comprises amino acid residues 70-90 of SEQ ID NO: 2. Preferred residues of Y include residues 91- 92, 91-93, 91-94, 91-95, 91-96, 91-97, 91-98, 91-99, 91-100, 91-105, 91-110, 91-115, 91-116, 91-117, 91-118, 91-119, 91-120, 91-121, 91-122, 91-123, 91-124, 91-
125, 91-126, 91-127, 91-128 91-129, 91-130, 91-131, 91- 132, 91-133, 91-134, 91-135, 91-136, 91-137, 91-138, 91-139, 91-140, 91-141, 91-142, 91-143, 91-144, 91- 145, 91-146, 91-147, 91-148, 91-149, 91-150, 91-151,
91-152, 91-153, 91-154, 91-155, 91-160, 91-165, 91-170 of SEQ ID NO: 2. More preferably, Y can be any of 91-95, 91-100, 91-105, 91-110, 91-115, 91-120, 91-130, 91-140, 91-145, 91-150, 91-153, 91-155, 91-160, 91-165, 91-170 of SEQ ID NO: 2.
The lower molecular weight 14,000 Tnl fragment, isolated from a pool of patient serum has been sequenced for N-terminal identification. The N- terminal sequence of the Tnl 14,000 fragment starts at position 27 (Ala) in human cardiac Tnl sequence. The 14,000 fragment is approximately 100 amino acids long, ending in the region from about amino acid 120 to about amino acid 130 in intact cTnl . The N-terminal sequence of the 18,000 fragment starts at or very near the N- terminus of the intact human cTnl . The 18,000 fragment is approximately 140 amino acids long, ending in the region from about amino acid number 135 to about 145 in intact cTnl . Thus, one preferred group of fragments has X as 25-27, 26-27 or 27 of SEQ ID NO: 2 and Y as 91 to any of 135-145 of SEQ ID NO: 2.
The fragments also may be those cardiac troponin I protein fragments containing the sequence AYATEPHAKKKSKISASRKLQLKTLLLQIAKQEL (SEQ ID NO: 4) or RAYATEPHAKKKSKISASRKLQLKTLLLQIAKQEL (SEQ ID NO: 5) . The fragments may be recombinant sequences such as MADGSSDAAREPRPAPAPIRRRSSNYRAYATEPHAKKKSKISASRKLQLKTLLLQ IAKQELEREAEERRGEKGRALSTRCQPLELAGLGFAELQDLCRQLHARVDKVDEE RYDIEAKVTKNITEIADLTQKIFDLRGKFKRPTLRRVRISADAMMQALLGARAKE SLDLRAHLKQVKKEDTEKENREVGDWRKNIDALSGMEGRKKKKFEES ( SEQ ID NO: 6);
ADGSSDAAREPRPAPAPIRRRSSNYRAYATEPHAKKKSKISASRKLQLKTLLLQI AKQELEREAEERRGEKGRALSTRCQ (SEQ ID NO: 7); or similar human or bovine fragments. It should be understood that while human troponin is preferred, other species may be substituted. Generally, these other species lack the appropriate methionine residue in the full length primary structure. However, insertion of methionine into the primary structure at positions that upon cleavage by CNBr would provide an appropriate fragment would allow the use of alternative species.
Troponin C is commercially available from a number of sources and the source or species is not critical. Generally, rabbit troponin C is used because of the lower cost, but human and other species can also be used. Recombinant troponin C can also be used.
The molecular weight of troponin C is about 17,500 Kd. As stated earlier, TnC has a Ca++/Mg++ binding domain in the COOH terminal region and a Ca++ binding domain in the amino terminus region and is thought to be "dumb-bell" shaped connected by a long central helix.
The covalent coupling agents useful in the present invention include those coupling agents that provide substantially "native-length" covalent cross-linking between troponin T and/or troponin I with troponin C. The preferred coupling agents form covalent bonds between the Tnl or TnT and TnC that approximate the distance between the proteins as they exist in the complex. The cross-linkers may be those "zero-length" crosslinkers such as l-ethyl-3- [ 3- (dimethylamino) propyl] carbodiimide (EDC) and other water soluble carbodiimides providing an amide bond between an activated carboxyl group on one protein and coupling to an amino group on the other protein. See, Chemistry of Protein Conjugation and Cross-Linking, CRC Press, Inc. Other coupling agents such as oxalic, malonic and succinic acid derivatives may also be used as may many of those commercially available cross-linkers such as those available from Pierce Chemical Co. The actual coupling agent used is less important than how the covalently coupled complex performs immunologically or with regard to stability when compared to non- covalently coupled complex, native complex or commercially available products.
The complex is prepared by combining the coupling agent with troponin C and troponin I in a manner specific for the coupling agent. The coupling reaction of the TnC and Tnl should take place in the presence of Ca++ or Mg++ or other divalent metal ions. The conditions will vary depending on the coupling agent utilized, but those conditions can readily be determined by those skilled in the art with reference to known and published methods. The choice of buffer is not critical, although the buffer should have a molarity from about 10 to 200 πiM. The concentration of calcium and magnesium ion is not critical, but preferably should be from about 20 μM to about 20 mM. If magnesium ion is used alone it should be in higher concentrations than that used for calcium. Typical amounts of calcium and/or magnesium are from about 2-5 mM. The buffer may include a salt such as sodium chloride or potassium chloride at from about 50 mM to 500 mM. The amount of troponin C is not critical, but should be in molar amounts equal to or greater than the amount of troponin I that will be utilized. Generally, the amount of troponin C may be from 0.02 mg/mL to 5 mg/mL. The amount of coupling agent may need to be adjusted depending on the amount of troponin C.
Clinically significant concentrations of diluted final coupled product are evaluated immunologically in a troponin I assay (such as those available from Dade International Inc.) and may be compared to native complex or non-covalently coupled complex or commercially available products evaluated in the same manner. Generally the clinical range of interest of troponin I or T is about 0.01 ng/mL to less than 1 μg/mL and typically 0.1 ng/ml to 200 ng/mL. In addition, stability may be determined by comparing the immunological activity over time at one or more temperatures in comparison to native complex or non- covalently coupled complex or commercially available products evaluated in the same manner or by running electrophoretic gels of the complexes to evaluate the stability.
Native complex may be obtained in serum samples. In addition, native complex can be isolated. Methods are known to those skilled in the art. For instance, a preferred method of isolating the Tn complex comprises incubating the sample to be tested with a substrate coated with antibodies to the subunits of the Tn complex. Many antibodies are useful, and can be selected by one of skill in the art. Examples of such antibodies include anti-Tnl, anti-TnC, and anti-TnT antibodies. A preferred substrate is beads, and more preferably the substrate comprises latex beads. The bound complex is eluted under conditions that do not affect association of Tn subunits, e.g. using urea. These conditions can be determined by one of skill in the art. A preferred buffer system comprises urea and lacks SDS. A preferred coupling agent is EDC or other water soluble carbodiimides. In a buffered solution containing salt and calcium ions, troponin C is combined with EDC. The concentration of EDC is not critical and may be from 1-10 mM. Compounds such as N- hydroxysuccinimide (NHS) or SNHS at about 1-10 mM may be added to enhance the activation of troponin C by water soluble carbodiimides. The NHS is typically added prior to the addition of EDC and incubates with the protein for at least about 5 minutes, although 15 minutes is typical. Then the EDC is added and the mixture is incubated, typically at room temperature, for about 15 minutes, but typically for thirty minutes or more. The reaction proceeds best at mildly acidic pH values (e.g. about 6), but the pH may range from 5- 9. After a sufficient reaction time, a reducing agent such as mercaptoethanol is added to stop the reaction.
Other reducing agents may be substituted for mercaptoethanol .
Next, cardiac troponin I, preferably the CNBr-Tnl isoform, is added to provide a molar ratio of about 1:1 with troponin C, although the amount of Tnl may be less. Tnl is generally in a buffer that contains salt or urea in sufficient amounts to solubilize the Tnl. A typical buffer is 100 mM sodium phosphate, 10 mM Tris and 8 M urea at pH 8 (PTU buffer) . The choice of the buffer is not critical to the invention. The buffer, however, must maintain the solubility of the cTnl . The reactants incubate, generally at room temperature, for about an hour and typically about two hours. The formed complex may be buffer exchanged into another buffer. The activity of the cross-linked complex is measured using a Stratus Troponin immunoassay and compared to native complex. The presence of the covalently cross- linked complex may be confirmed using polyacrylamide gel electrophoresis . The complex will not dissociate under reducing conditions or in the presence of EDTA or other metal complexing agent.
When using the non-specific coupling agents such as EDC, calcium or magnesium ion should be present in either the TnC or Tnl solution. The calcium and/or magnesium causes complex formation to occur. Thus, the complex forms as it would in native complex so the spatial orientation of the proteins will be comparable to native complex or non-covalently coupled complex. Thus, the cross-linking occurs more selectively and the bond formed will "freeze" the complex in the correct conformation. The covalently coupled complex is insensitive to EDTA or other chelating agents (thus, independent of calcium or magnesium) , does not dissociate in the presence of SDS, and is more resistant to higher temperatures than the non-cross- linked complex.
In addition, generally the TnC, rather than the Tnl or TnT, should be subjected to EDC or other water soluble carbodiimide treatments. For instance, if Tnl is activated by EDC without protection of the epitopic site, there is the possibility that the epitopic site would be affected by the non-specific coupling agent — that is the Tnl or fragment would be less immunologically active.
The TnT: TnC complex and TnT: TnC: Tnl complex are prepared in a similar fashion to the Tnl: TnC. TnT fragments, particularly the carboxy fragments such as TnT-2 are preferred. As described for troponin I, the troponin T should be added in molar amounts equal to or less than the amount of troponin C. Troponin C may be from less than 0.02 mg/mL to 5 mg/mL. The ranges for Tnl and TnT are similar. The TnT : TnC complex is evaluated as described for troponin I complexes, except using an assay for troponin T. Troponin T assays are available from Boehringer Mannheim.
A TnT: Tnl complex may also be prepared, however, as with the other complexes of this invention, the immunological (epitopic) sites must be substantially retained. Since both TnT and Tnl are measured immunologically, it is preferred that the epitopic region be retained for both proteins. Thus, less nonspecific coupling agents may be useful than agents such as EDC or oxalic acid derivatives. It has been described that skeletal muscle Tnl complexes with TnT at about amino acids 40-80 of Tnl. See Potter, J.D. et al. (1995) A Direct Regulatory Role of Troponin T and a Dual Role for Troponin C in the Ca++ Regulation of Muscle Control. Journal of Biologi cal Chemistry 210 (6) 2557-2562. Thus, it is proposed that the homologous site on cTnl would be useful for coupling. Preferably, Tnl and TnT are added in approximately equimolar ratios. The amounts may be from 0.02 mg/mL to 5 mg/mL. It is important that the immunological site not be altered. It should be understood that the eptitopic site will vary depending on the antibody used in the assay. The generation of antibodies is described in the art, for example, by Bodor et al., (1992) Development of Monoclonal Antibodies for an Assay of Cardiac Troponin- I and Preliminary Results in Suspected Cases of Myocardial Infarction, Clinical Chemistry 38 (11) 2203-2214. In addition, several methods that assay for troponin I or T are commercially available. The present invention uses a defined base material useful as a control matrix for containing and maintaining the troponin complexes, the base material comprising an aqueous solution of a buffer to maintain the pH at 5-8, anti-microbial agents and may contain other stabilizers including calcium ions or proteins.
The defined base material may be utilized to prepare stock solutions and controls including troponin I or troponin I fragments, troponin T or troponin T fragments complexed with Troponin C or troponin I complexed with troponin T.
The resulting solution can be stored as a liquid or frozen or also can be lyophilized if appropriate fillers are included.
It is preferred to prepare a stock solution at higher concentrations of troponin I and/or troponin T than those that will be utilized in the final assay control. The stock can be stored frozen or lyophilized and thawed or reconstituted when necessary to prepare the appropriate dilutions of controls or calibration standards. Thus, the complexes prepared as described above may be buffer exchanged into an appropriate buffer after covalent coupling.
The aqueous solution used to prepare the stock and controls may include a buffer and the buffer may generally be any of the buffers that function in the pH range of 5 to 8. Of these buffers, the buffers that are preferred function are in the pH range of 6-8. The concentration of buffer is between 10 mM to 200 mM. It is preferred to keep the buffer concentration lower - in the range of 20-100 mM. Preferably, the buffers used for the calibrators or controls contain bovine serum albumin (BSA) . In certain embodiments the buffer contains, BSA, sugars, salt and an antibacterial agent.
Examples of useful buffers include HEPS, MES or TRIS buffers. A preferred buffer comprises MES buffer containing 6.5% BSA, at pH 6-7. Other preferred buffers contain a reducing agent, stabilizing protein, chelating agent and a salt as described in the copending application U.S.S.N. 08/400,158, incorporated herein by reference.
Alternatively, instead of a buffer, the fragments are spiked into the serum, e.g., human or bovine, or into diluted serum, e.g., serum diluted 1:1 with MES buffer containing BSA.
Anti-microbial and anti-fungal agents may be added to prevent growth and may include those commonly found in the prior art at the concentrations found in the prior art such as gentamycin, clortrimazole, sodium azide, mycostatin, thimerosal, Kathon and/or Proclin 300. In addition, stabilizing proteins such as albumin, gelatin, ovalalbumin, or casein may be included. The concentration of stabilizing protein may be from 0 to 15% and preferably from 7 to 12%. Preferably the stabilizing protein is albumin and preferably the albumin is substantially protease free.
It is preferred that the solution have low protease activity, thus protease inhibitors such as aprotinin and "Protease Inhibitor" (Sigma) are effective. However, the use of the recombinant fragments as described herein are not as sensitive to protease activity as is the full length protein. The inhibitors may be added and may be used at the manufacturer's recommended concentration. Examples of other protease inhibitors include benzamidine, (2S, 3R) -3-Amino-2-hydroxy-5- methylhexanoyl] -Val-Val-Asp (Amastatin-Sigma) , [2S, 3R] -3-Amino-2-hydroxy-4- [4-nitrophenyl] - butanoyl-L-leucine, Antipain, [2S, 3R] -3-Amino-2- hydroxy-5-methylhexanoyl] -Val-Val-Asp
(Epiamastatin-Sigma) , ( [2R, 3R] -3-Amino-2-hydroxy- 4-phenylbutanoyl) -L-leucine (Epibestatin-Sigma) , Foroxymithine, Acetyl-Leu-Leu-Arg-al (Leupeptin- Sigma) , 4-Amino-3-hydroxy-6-methyl-heptanoic acid, 4-Amino-3-hydroxy-6-methylheptanoic acid, N- ( - Rhamnopyranosyloxy-hydroxyphosphinyl) -Leu-Trp and phenyl methane sulfonyl fluoride (PMSF) . It is most preferred that the means to provide a substantially protease free solution is to use substantially protease free proteins such as albumin which is substantially protease free.
Serum may be included if desired. Again, the use of fragments that are similar to the 14,000 Kd fragments substantially eliminates the concerns of proteases.
Controls prepared by this method may be lyophilized by adding those bulking agents that are known in the art, but the controls may also be liquid. In addition, the liquid controls may be frozen to further increase shelf-life. Currently used assays for detecting cTnl and cTnT in MI patient serum utilize a sandwich assay. However, the complexes of the present invention can also be used to design competitive-type assays for the detection of cTnl or cTnT in serum. In such an assay, a subsaturating amount of antibody to cTnl or cTnT is bound to a solid phase, e.g., a microtiter plate or latex beads. The complexes of the present invention are labeled, e.g., with alkaline phosphatase, or horseradish peroxidase. A constant amount of the labeled complex is mixed with the sample of MI patient serum containing an unknown amount of cTnl and/or cTnT . The test sample is then allowed to bind to the subsaturating amount of cTnl and/or cTnT antibody bound to a solid phase. The cTnl and/or cTnT in the sample will compete with the labeled complex for binding with the antibody-coated solid phase. Unbound proteins are removed by washing and the amount of labeled complex bound to the solid phase is measured. The amount of labeled complex bound to the antibody on the solid phase indicates the amount of cTnl or cTnT present in the serum. If the serum contains a high concentration of cTnl or cTnT, it will compete effectively with the labeled complex and little or none of the labeled complex will bind the antibody-coated solid phase.
Changes in some amino acids of the fragments of Tnl, TnT, and TnC might not affect their performance except those occurring at the epitope(s) where the specific assay antibodies bind and those amino acids of the binding domains for TnC. The affects can readily be determined by gel electrophoresis and immunological analysis of prepared complex.
Example 1 Preparation of a defined base material for cardiac markers .
Antioxidants such as 200 milligrams of glutathione, 200 milligrams of glucose, 50 gs of ascorbic acid, and 1.1 milliliter of phenol, about 2.7 grams of L-Lactate, about 225 milligrams of calcium chloride or other calcium salt to provide 1-3 mM calcium ion, anti-microbial and anti-fungal agents such as about 20 milligrams of chlortrimazole, 35 milligrams of gentamicin, and about 1 milliliter of Proclin 300, about 95 grams of protease free BSA, and about 1 gram of gelatin are combined in an aqueous 50 mM TRIS buffered solution at about pH 7.3 also containing a salt such as sodium chloride (about 30 grams) to provide about one liter of base material.
It is best to add the gelatin in solution by dissolving the gelatin by adding 1 gram of gelatin to 100 milliliters of water and gently heating to dissolve the gelatin. Then the gelatin containing solution is added to the base material.
The resulting solution is filtered using filters sufficient to remove any bacteria such as a .22 micron filter. A low protein binding filter is preferred. Example 2
Cross-Linking of Troponin I and Troponin T Preparation of troponin I stock solution and controls . The cross-linking was accomplished using the
EDC method described by Greaser and Gergely (1971). To 20 mM Mes buffer at pH 6 containing 0.1 M KC1, 0.2 mM CaCl , freshly prepared NHS at 5.7 mM final concentration was added followed by addition of TnC to provide 0.2 mg/mL. The mixture was incubated at room temperature for 15 minutes. The TnC was activated by addition of 5.7 M EDC (final concentration) followed by incubation at room temperature for 30 minutes. The activation step was terminated by addition of β mercaptoethanol (20 mM final concentration) . The CNBr-rTnl isoform (Tnl 153) in PTU buffer was added at a final concentration of 0.175 mg/mL. The mixture was incubated for two hours at room temperature. The complex is buffer exchanged. The activity of the crossed linked complex was measured using Stratus Tnl immunoassay. The presence of a covalent cross-linked complex was confirmed on polyacrylamide gel electrophoresis. The resulting complex is less sensitive to environment, including temperature than native complex. The resulting stock solution is sterile filtered using low protein binding filters of 0.22 microns or less. The stock solution may be stored frozen at -20° C for longer than two years. The stock solution may be stored at 2-8° C for more than one week.
The stock solution is used to prepare diluted solutions of troponin I in the clinical range of interest (about 0 to 200 ng/mL) by diluting the stock solution in the defined base material prepared in Example 1 or other base material.
Example 3 Stability and Immunological Activity of the Covalently Coupled Complex.
Various aliquots representing different concentrations of troponin I complex prepared in Example 2 (of the diluted stock solution) were stored at various temperatures. The aliquots were analyzed on a Stratus II Immunoassay analyzer for troponin I concentration. The change in concentration was evaluated over time. Figure 3 shows the stability of two concentrations of diluted stock (25 ng/mL and 45 ng/mL of troponin I) of the complex stored at 45 C. The dilutions are stable for greater than three weeks at 45 C. Figure 4 shows a 28 ng/mL solution was evaluated for stability at 4C, 25C, 37C, and 45 C and was stable for at least six weeks at all temperatures. Figure 5 shows the stability of the complex when prepared with three different lot numbers of commercially available TnC. All lots were stable for over 10 days at 45 C. A full length rTnl-TnC complex was also prepared. The stability of the cross-linked complex at 45 C is shown in Figure 6.
Example 4 Independence of the complex on calcium ion. Polyacrylamide gels of the complexes were evaluated. Lanes 2-4 show the electrophoretic pattern of covalently linked rTnI-153:TnC complex in the presence of EDTA (a metal chelator) . Lane 5 shows a non covalently linked rTnI-153:TnC complex in the absence of EDTA. Lanes 6-7 show he electrophoretic pattern of non covalently linked rTnI-153:TnC complex in the presence of EDTA. The disappearance of the upper band of complex is evident in Lanes 6-7, but not in Lanes 2-4. Lane 8 is TnC. See, Figure 7.
Example 5
Preparation of Troponin T Controls.
Example 2 is repeated except that troponin T is substituted for the troponin I. Aliquots of stock solution are diluted to the clinical range of interest from 0.01 ng/mL to 10 ng/mL. The aliquots may be analyzed for immunological activity using a troponin T assay such as that assay commercially available from Boehringer Mannheim.
Example 6
Preparation of a ternary complex of Troponin I,
Troponin C and Troponin T. Example 2 is repeated except that both troponin I and troponin T are added to the activated troponin C. The ternary complex may be observed using electrophoresis run in the presence of EDTA. The troponin I immunological activity may be evaluated as described in Example 2 and the troponin T immunological activity may be evaluated as described in Example 5.

Claims

We claim:
1. A composition for use in an assay for the determination of the presence or concentration of cardiac troponin I the composition comprising: a complex of cardiac troponin I or a fragment thereof and troponin C or a fragment thereof wherein the cardiac troponin I is covalently coupled to the troponin C.
2. The composition of claim 1 wherein the composition is used as a diagnostic calibrator, control or reference material for cardiac troponin I.
3. The composition of claim 1 wherein the composition is immobilized on a substrate wherein the substrate is used in a competitive assay for cardiac troponin I .
4. The composition of claim 1 wherein the cardiac troponin I and troponin C are covalently coupled using a water soluble carbodiimide .
5. The composition of claim 1 wherein the cardiac troponin I is recombinant.
6. The composition of claim 5 wherein the cardiac troponin I is a fragment having substantially the amino acid sequence of a CNBr fragment designated rTnI-153.
7. The composition of claim 5 wherein the cardiac troponin I is a fragment of the general sequence
X-A-B-Y wherein X comprises any of amino acids 1- 27 of full length cardiac troponin I, A comprises residues 28-69 of full length cardiac troponin I, B comprises amino acid residues 70-90 of full length cardiac troponin I, and Y comprises any sequential amino acid sequence of amino acid residues 91-170 of full length cardiac troponin I.
8. The composition of claim 7 wherein X is amino acid residue 27 of full length cardiac troponin I, and Y is selected from the group consisting of amino acid residues 91-95, 91-100, 91-105, 91-110, 91-115, 91-120, 91-130, 91-140, 91-150, 91-155, 91-160 and 91-170 of full length cardiac troponin I.
9. A composition for use in an assay for the determination of the presence or concentration of cardiac troponin T the composition comprising: a complex of cardiac troponin T or a fragment thereof and troponin C or a fragment thereof wherein the cardiac troponin T is covalently coupled to the troponin C.
10. The composition of claim 9 wherein the composition is used as a diagnostic calibrator, control or reference material for cardiac troponin T.
11. The composition of claim 9 wherein the composition is immobilized on a substrate wherein the substrate is used in a competitive assay for cardiac troponin T.
12. The composition of claim 9 wherein the cardiac troponin T and troponin C are covalently coupled using a water soluble carbodiimide .
13. The composition of claim 9 wherein the cardiac troponin T is recombinant.
14. A composition for use in an assay for the determination of the presence or concentration of cardiac troponin T or cardiac troponin I the composition comprising: a complex of cardiac troponin T or fragment thereof, cardiac troponin I or a fragment thereof and troponin C or a fragment thereof wherein the cardiac troponin T and cardiac troponin I are covalently coupled to the troponin C.
15. The composition of claim 14 wherein the composition is used as a diagnostic calibrator, control or reference material for cardiac troponin
I or cardiac troponin T.
16. The composition of claim 14 wherein the composition is immobilized on a substrate wherein the substrate is used in a competitive assay for cardiac troponin I or cardiac troponin T.
17. The composition of claim 14 wherein the cardiac troponin I, cardiac troponin T and troponin C are covalently coupled using a water soluble carbodiimide.
18. The composition of claim 14 wherein the cardiac troponin I is a fragment having substantially the amino acid sequence of a CNBr fragment designated rTnI-153.
19. The composition of claim 18 wherein the cardiac troponin I is a fragment of the general sequence X-A-B-Y wherein X comprises any of amino acids 1-27 of full length cardiac troponin I, A comprises residues 28-69 of full length cardiac troponin I, B comprises amino acid residues 70-90 of full length cardiac troponin I, and Y comprises any sequential amino acid sequence of amino acid residues 91-170 of full length cardiac troponin I.
20. A composition for use in an assay for the determination of the presence or concentration of cardiac troponin T or cardiac troponin I the composition comprising: a complex of cardiac troponin T or fragment thereof and cardiac troponin I or a fragment thereof wherein the cardiac troponin T and cardiac troponin I are covalently coupled.
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