WO1986002099A1 - Alpha-amidation enzyme - Google Patents

Alpha-amidation enzyme Download PDF

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Publication number
WO1986002099A1
WO1986002099A1 PCT/US1985/001616 US8501616W WO8602099A1 WO 1986002099 A1 WO1986002099 A1 WO 1986002099A1 US 8501616 W US8501616 W US 8501616W WO 8602099 A1 WO8602099 A1 WO 8602099A1
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Prior art keywords
glycine
peptidyl
enzyme
amidating
amidating monooxygenase
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PCT/US1985/001616
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French (fr)
Inventor
James P. Gilligan
Barry N. Jones
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Unigene Laboratories, Inc.
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Application filed by Unigene Laboratories, Inc. filed Critical Unigene Laboratories, Inc.
Priority to HU853879A priority Critical patent/HU195857B/en
Priority to AT85904514T priority patent/ATE92522T1/en
Publication of WO1986002099A1 publication Critical patent/WO1986002099A1/en
Priority to DK241486A priority patent/DK241486A/en
Priority to FI862216A priority patent/FI100993B1/en
Priority to NO86862100A priority patent/NO862100L/en

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/0004Oxidoreductases (1.)
    • C12N9/0071Oxidoreductases (1.) acting on paired donors with incorporation of molecular oxygen (1.14)
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • 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
    • C07K14/575Hormones
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K16/00Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
    • C07K16/40Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against enzymes
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12YENZYMES
    • C12Y114/00Oxidoreductases acting on paired donors, with incorporation or reduction of molecular oxygen (1.14)
    • C12Y114/17Oxidoreductases acting on paired donors, with incorporation or reduction of molecular oxygen (1.14) with reduced ascorbate as one donor, and incorporation of one atom of oxygen (1.14.17)
    • C12Y114/17003Peptidylglycine monooxygenase (1.14.17.3)

Definitions

  • mammalian cells and other eukaryotes can perform certain post- translational processing procedures, while prokaryotes can not.
  • Certain prokaryotes such as E. coli, are widely employed as hosts for the production of mammalian proteins via recombinant DNA (rDNA) technology because they can be readily grown in batch fermentation procedures and because they are genetically well-characterized.
  • rDNA recombinant DNA
  • many mammalian proteins produced by genetic engineering technology require some type of post- translational processing, and this must often be accomplished by using complex, in vitro chemical or enzymatic procedures which are cost-prohibitive for large-scale production applications.
  • One type of processing activity involves the specific amidation (conversion of -COOH group to a -CONH 2 group) of the carboxyl- terminal amino acid of a protein.
  • Many naturally-occurring hormones and peptides contain such a modification, which is often essential if the protein is to be biologically active.
  • An example is calcitonin, where the substitution of a non-amidated proline residue for the amidated proline of the native form results in a 3,000- fold reduction in biological activity.
  • the agent which effects this C- terminal (alpha) amidation recognizes a glycine residue which immediately follows the amino acid to be amidated (R-X-gly, where R is the main body of the protein, X is the residue which is amidated, and "gly" is the glycine residue).
  • R is the main body of the protein
  • X is the residue which is amidated
  • gly is the glycine residue.
  • the glycine is cleaved and actually donates the amino moiety to the penultimate amino acid, thereby amidating it.
  • Enzymatic preparations capable of amidating the carboxyl- terminus of pep tides and proteins have been described from a. variety of sources. For instance, Bradbury, A.F. , et al, Nature 298, 1982, p. 686-688 report an ⁇ -amidating enzyme activity to be present in porcine pituitary.
  • rat hypothalamus also contained an ⁇ -amidating enzyme activity.
  • Glands or organs known to contain amidated peptides may contain an enzyme capable of catalyzing the amidation reaction.
  • lower life forms such as the dog fish (Squalus acanthias) have been reported by O'Donohue T.L., et al, Peptides 3, 1982, p. 353-395, to contain amidated peptides in pituitary extracts.
  • Scheller, R.H. et al, Cell, Vol. 32, 1983, p. 7-22 reported the presence of amidation signal peptides in the marine snail Apylsia.
  • little information has been published on its physicocheraical characteristics. This may be attributed to the very low levels of enzyme present in these neuroendocrine organs.
  • the extracts and partially purified enzyme mixtures contained additional proteolytic enzymes which degrade the potential substrate and products as well as the ⁇ -amidating enzyme.
  • This invention relates to a purified ⁇ -amidating enzyme, its uses, monoclonal antibodies specific for the enzyme, and prokaryotes or other unicellular organisms or host cells isolated from multicellular organisms containing heterologous genetic material which codes for the enzyme. More particularly, the invention is concerned with purified peptidyl-glycine ⁇ - amidating monooxygenase, which is an enzyme extractable from medullary thyroid carcinomas, which has molecular mass of about 60,000 to 65,000 daltons, which has been purified so as to exhibit a single, homogeneous, well-defined band by electrophoretic procedures performed on SDS/ polyacrylamide gels, and which has a specific enzymatic activity of at least 50 mU per mg protein.
  • the invention also provides a method of preparing an ⁇ -amidating peptide from peptide or polypeptide substrates containing a terminal glycine residue by reacting the substrate with oxygen in the presence of the free or immobilized purified enzyme, ascorbate and copper.
  • the invention further provides for the production of monoclonal antibodies to the purified enzyme and for the development of prokaryotes, other unicellular organisms or host cells isolated from multicellular organisms containing a heterologous DNA coding for peptidyl-glycine ⁇ -amidating monooxygenase.
  • homogeneously-purified ⁇ -amidating enzyme can be obtained through a multistep procedure employing a combination of size exclusion and ion exchange chromatography from solid tumor tissue extracts, tumor cell- lines, and the tissue culture medium from such cell lines.
  • the enzyme has been extracted from rat medullary thyroid carcinomas developed in WAG/Rij Wistar rats as described by Roos, B.A., et al, Endocrinology, 1979, Vol. 150, #1, p. 27-32. This tissue has been deposited as IVI-10028.
  • the enzyme has also been extracted from other sources, notably human and rat medullary thyroid carcinoma cell lines.
  • the rat cell line 77(74) was derived from rat medullary thyroid carcinoma tumors by serial passages as described by Muszynski, M. et al, JBC 1983, Vol. 258, pp. 11678-83. This cell line has been deposited as IVI-10029.
  • a human cell line HTT 54(34) was developed by B.A. Roos at the VA Medical Center in Cleveland, Ohio using human medullary thyroid carcinoma cells for the primary culture.
  • the human cell line HTT 54(34) has been deposited as IVI-10031. Defined tissue culture media from both the human and rat cell lines have been demonstrated to contain significant levels of ⁇ -amidating enzyme activity, indicating that a portion of the enzyme is secreted from the cells.
  • the enzyme is obtained and purified by first subjecting the crude material to anion exchange chroma tography.
  • the sample for example, can be bulk- loaded on a preparative scale anion exchange column such as a DE-52 resin from Whatman, Limited.
  • the ⁇ -amidating activity-containing product is then subjected to size exclusion chromatography on a resin of appropriate resolving capabilities, for example a Sephacryl S-200 superfine column which is available from Pharmacia Fine Chemicals.
  • the activity-containing eluant fraction is then subjected to ion exchange chromatography using a strong anion exchange matrix.
  • a resin which may be used is the Mono Q HR5/5 strong anion exchange resin from
  • Pharmacia Fine Chemicals and one or more passes on the column may be required for homogeneous purification of the enzyme.
  • Each purification step can be monitored for both protein content and the level of ⁇ -amidation activity. This information is used to calculate the specific activity of the enzyme which serves as an indicator of the relative purity of the enzyme.
  • the resulting enzyme is peptidyl-glycine ⁇ -amidating monooxygenase (rat source, IVI-10032; human source, IVI10033) which has a molecular mass of about 60,000 to 65,000 daltons. It has been purified such that it exhibits a specific enzymatic activity (number of units of ⁇ -amidation activity per milligram of protein) of at least approximately 25 mU and preferably at least approximately 50 mU/mg protein. It has also been purified so as to exhibit a single, homogeneous, well-defined band following electrophoresis on sodium dodecyl sulfate/polyacrylamide gels (SDS-PAGE).
  • SDS-PAGE sodium dodecyl sulfate/polyacrylamide gels
  • the purified peptidyl-glycine ⁇ -amidating monooxygenase is used to amidate the alpha-carboxyl group of a polypeptide having a terminal glycine residue, where the glycine functions as an amino group donator.
  • the substrate peptide or polypeptide can be purified from natural sources, synthesized from its component amino acids, or produced by recombinant DNA techniques.
  • the glycine-terminating polypeptide is combined with oxygen in the presence of an effective amount of the enzyme.
  • the amount of the enzyme required depends on several variables well known to this art including particularly, but not limited to, the following: the specific activity of a given enzyme preparation, the amount and chemical nature of the substrate to be converted, the time within which conversion is to take place and the temperature and pH of the reaction mixture. Those skilled in this art will recognize other variables that may influence the precise amount of enzyme required in a given situation.
  • the oxygen is usually employed in stoichiome trie amount but an excess of the oxygen does not affect the reaction.
  • the presence of copper ions is also required, and can be provided by any copper salt whose anion does not adversely affect the reaction.
  • the peptidyl-glycine ⁇ -amidating monooxygenase has been sufficiently purifed, it is now possible to obtain monoclonal antibodies directed against the enzyme by standard procedures.
  • the monoclonal antibodies allow the enzyme recovery procedures from the medullary thyroid carcinomas to be facilitated or wholly supplanted by immunoabsorption purification procedures.
  • the enzyme has also been sufficiently purified to permit its amino acid sequence to be determined. This information is necessary in order to permit the isolation of the genetic material coding for the enzyme and its subsequent incorporation into an appropriate unicellular organism or host cell isolated from a multicellular organism which does not contain DNA coding for the peptidylglycine ⁇ -amidating enzyme.
  • the ⁇ -amidation activity of the purified enzyme of this invention was demonstrated using a substrate of radioiodinated D-Tyr-Val-Gly, a peptide whose sequence mimics the carboxyl terminus of the melanocyte stimulating hormone precursor. Assays were performed in 100 mM TES (N-tris [hydroxymethyl] me thy 1-2-aminoe thane sulfonic acid) buffer, pH 7.0, at 37°C for three hours. Th product, [ 125 I] Tyr-Val-NH 2 , was separated from the substrate by cation exchange chroma tography. The amidating enzyme activity was also demonstrated using a synthetic substrate which mimicked the sequence of the carboxyl terminus of calcitonin, [Tyr 25 Gly 33 ] calcitonin (26-32).

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Abstract

Peptidyl-glycine $g(a)-amidating monooxygenase is an enzyme extractable from medullary thyroid carcinoma cell lines and tissue samples, having a molecular mass of about 60,000 to 65,000 daltons. It has been purified so as to exhibit a single, homogeneous, well-defined band using electrophoretic procedures performed on SDS-polyacrylamide gels, and has a specific enzymatic activity of at least 50mU per mg protein. The free or immobilized enzyme, in the presence of Cu?+2 ions, ascorbate, and oxygen, can be used to prepare an $g(a)-amidated protein from a polypeptide substrate possessing a carboxyl-terminal glycine residue. The purified enzyme can be used as an antigen in order to produce enzyme-specific monoclonal antibodies, and can provide the information necessary to design and construct prokaryotes or other appropriate unicellular organisms or host cells isolated from multicellular organisms which possess peptidyl-glycine $g(a)-amidating capability.

Description

ALPHA-AMIDATION ENZYME
BACKGROUND OF THE INVENTION
The intracellular processing (cleavage and/or functional group modification) of precursor forms of native proteins following their translation from nucleic acid coding sequences has been clearly documented.
In general, mammalian cells and other eukaryotes can perform certain post- translational processing procedures, while prokaryotes can not. Certain prokaryotes, such as E. coli, are widely employed as hosts for the production of mammalian proteins via recombinant DNA (rDNA) technology because they can be readily grown in batch fermentation procedures and because they are genetically well-characterized. However, many mammalian proteins produced by genetic engineering technology require some type of post- translational processing, and this must often be accomplished by using complex, in vitro chemical or enzymatic procedures which are cost-prohibitive for large-scale production applications.
One type of processing activity involves the specific amidation (conversion of -COOH group to a -CONH2 group) of the carboxyl- terminal amino acid of a protein. Many naturally-occurring hormones and peptides contain such a modification, which is often essential if the protein is to be biologically active. An example is calcitonin, where the substitution of a non-amidated proline residue for the amidated proline of the native form results in a 3,000- fold reduction in biological activity. The agent which effects this C- terminal (alpha) amidation recognizes a glycine residue which immediately follows the amino acid to be amidated (R-X-gly, where R is the main body of the protein, X is the residue which is amidated, and "gly" is the glycine residue). The glycine is cleaved and actually donates the amino moiety to the penultimate amino acid, thereby amidating it.
Enzymatic preparations capable of amidating the carboxyl- terminus of pep tides and proteins have been described from a. variety of sources. For instance, Bradbury, A.F. , et al, Nature 298, 1982, p. 686-688 report an α -amidating enzyme activity to be present in porcine pituitary.
Husain, I. , and Tate, S.S. , FEBS Letters, Vol. 152, #2, 1983, p. 277-281, described an α -amidating activity present in bovine pituitary neurosecretory granules.
Eipper et al, PNAS Vol. 80, 1983, p. 5144-5148, reported an α-amidating enzyme activity to be present in the anterior, intermediate and posterior lobes of the rat pituitary gland. Gomez et al, FEBS Letters, Vol. 167, #1, 1984, p.
160-164 determined that rat hypothalamus also contained an α-amidating enzyme activity.
Bradbury, A.F. , Smythe, D.G. , in Peptides Structure and Function: Proceedings of the Eighth American Peptide Symposium; p. 249-52 (1983), Editors Hruby, V.J. , and Rich, D.H. , describe the presence of an α -amidating enzyme activity in rat thyroid glands.
Mains R.E. et al, Endocrinology, Vol. 114, 1984, p. 1522-1530, reported that a murine cell line derived from the anterior pituitary lobe (ATT-20) contained an α-amidating enzyme activity that apparently decreased with time in culture.
Glands or organs known to contain amidated peptides may contain an enzyme capable of catalyzing the amidation reaction. For example, lower life forms such as the dog fish (Squalus acanthias) have been reported by O'Donohue T.L., et al, Peptides 3, 1982, p. 353-395, to contain amidated peptides in pituitary extracts. Scheller, R.H. et al, Cell, Vol. 32, 1983, p. 7-22 reported the presence of amidation signal peptides in the marine snail Apylsia. Despite the apparent ubiquitous distribution of this activity in nature, little information has been published on its physicocheraical characteristics. This may be attributed to the very low levels of enzyme present in these neuroendocrine organs.
Heretofore, the purification and characterization of the α-amidating enzyme have not been published. Physicochemical properties of partially purified enzyme preparations, however, have been reported. The first authors to report an approximate molecular weight for the α- amidating enzyme were Bradbury A.F. , et al, Nature, Vol. 298, 1982, p. 686-88. Using Sephadex G100 they suggested a minimum apparent molecular mass of approximately 60,000 daltons. Subsequent studies have suggested the molecular mass of the enzyme to be between 60,000 and 70,000 daltons. These include Husain I., and Tate S. S., FEBS Letters, Vol. 152, #2, 1983, p. 277-281; Eipper B.A., PNAS Vol. B.A., 167, #1, 1984, p. 160-64, and Kizer J.S., et al, PNAS, Vol. 81, 1984, p. 3228-3232.
Eipper et al, PNAS, Vol. 80, 1983, p. 5144-48, have reported that in addition to molecular oxygen, two cofactors are required for maximal enzyme activity; these are ascorbic acid and copper (II) ion. The chemical reaction resulting in the amidation of the carboxyl- terminus of a peptide requires a source for the amino group. Bradbury, A.F., et al, Nature, Vol. 298,. 1982, p. 686-688, demonstrated that glycine is cleaved and donates the amino moiety to the penultimate amino acid, resulting in the amidation of the latter. The requirement for glycine as the amino group donor has been substantiated by other authors.
Landymore, A.E.N., et al, BBRC Vol. 117, #1, 1983, p. 289-293 demonstrated that D-alanine could also serve as an amino donor in the amidation reaction. Subsequent work by Kizer et al, PNAS, Vol. 81, 1984, p. 3228-3232, showed two distinct enzyme activities in rat brain which were capable of catalyzing the α -amidating reaction. The higher molecular mass species (70,000 daltons) has a specificity restricted for glycine at the carboxyl- terminus of the substrate. The lower molecular mass enzyme accepts a substrate with β-alanine as the carboxyl-terminal amino acid.
The pH optimum for the α -amidating enzyme extracted and partially purified from porcine pituitary was reported by Bradbury A.F., and Smythe D.G., BBRC, Vol. 112, #2, 1983, p. 372-377 to be approximately 7.0. Eipper, B.A., et al, PNAS, Vol. 80, 1983, p. 5144-5148, corroborated these results by reporting a pH optimum of 7 for an α -amidating enzyme which was partially purified from rat pituitaries.
They also noted that enzyme activity declined rapidly at pH levels below 6.5 or above 7.5.
In all of the aforementioned publications, the extracts and partially purified enzyme mixtures contained additional proteolytic enzymes which degrade the potential substrate and products as well as the α-amidating enzyme.
It is therefore the object of the invention to provide a purified α-amidating enzyme which can efficiently be used to produce α -amidated peptides from peptide or polypeptide substrates, to prepare monoclonal antibodies specific for the enzyme, and to construct prokaryotes or other appropriate unicellular organisms or host cells isolated from multicellular organisms containing heterologous DNA coding for the enzyme. This and other objects of the invention will become apparent to those skilled in this art from the following detailed disclosure. SUMMARY OF THE INVENTION
This invention relates to a purified α -amidating enzyme, its uses, monoclonal antibodies specific for the enzyme, and prokaryotes or other unicellular organisms or host cells isolated from multicellular organisms containing heterologous genetic material which codes for the enzyme. More particularly, the invention is concerned with purified peptidyl-glycine α- amidating monooxygenase, which is an enzyme extractable from medullary thyroid carcinomas, which has molecular mass of about 60,000 to 65,000 daltons, which has been purified so as to exhibit a single, homogeneous, well-defined band by electrophoretic procedures performed on SDS/ polyacrylamide gels, and which has a specific enzymatic activity of at least 50 mU per mg protein. [1U = the conversion of 1 millimole of Dansyl-D-Tyr-Val-Gly-COOH to 1 millimole of Dansyl-D-Tyr-Val-CONH2 per minute at 37°C and pH 7.0.] The invention also provides a method of preparing an α -amidating peptide from peptide or polypeptide substrates containing a terminal glycine residue by reacting the substrate with oxygen in the presence of the free or immobilized purified enzyme, ascorbate and copper. The invention further provides for the production of monoclonal antibodies to the purified enzyme and for the development of prokaryotes, other unicellular organisms or host cells isolated from multicellular organisms containing a heterologous DNA coding for peptidyl-glycine α -amidating monooxygenase.
DESCRIPTION OF THE INVENTION
It has now been discovered that homogeneously-purified α -amidating enzyme can be obtained through a multistep procedure employing a combination of size exclusion and ion exchange chromatography from solid tumor tissue extracts, tumor cell- lines, and the tissue culture medium from such cell lines. The enzyme has been extracted from rat medullary thyroid carcinomas developed in WAG/Rij Wistar rats as described by Roos, B.A., et al, Endocrinology, 1979, Vol. 150, #1, p. 27-32. This tissue has been deposited as IVI-10028. The enzyme has also been extracted from other sources, notably human and rat medullary thyroid carcinoma cell lines. The rat cell line 77(74) was derived from rat medullary thyroid carcinoma tumors by serial passages as described by Muszynski, M. et al, JBC 1983, Vol. 258, pp. 11678-83. This cell line has been deposited as IVI-10029. A human cell line HTT 54(34) was developed by B.A. Roos at the VA Medical Center in Cleveland, Ohio using human medullary thyroid carcinoma cells for the primary culture. The human cell line HTT 54(34) has been deposited as IVI-10031. Defined tissue culture media from both the human and rat cell lines have been demonstrated to contain significant levels of α -amidating enzyme activity, indicating that a portion of the enzyme is secreted from the cells.
The enzyme is obtained and purified by first subjecting the crude material to anion exchange chroma tography. The sample, for example, can be bulk- loaded on a preparative scale anion exchange column such as a DE-52 resin from Whatman, Limited. The α -amidating activity-containing product is then subjected to size exclusion chromatography on a resin of appropriate resolving capabilities, for example a Sephacryl S-200 superfine column which is available from Pharmacia Fine Chemicals. The activity-containing eluant fraction is then subjected to ion exchange chromatography using a strong anion exchange matrix. A resin which may be used is the Mono Q HR5/5 strong anion exchange resin from
Pharmacia Fine Chemicals and one or more passes on the column may be required for homogeneous purification of the enzyme. Each purification step can be monitored for both protein content and the level of α -amidation activity. This information is used to calculate the specific activity of the enzyme which serves as an indicator of the relative purity of the enzyme.
The resulting enzyme is peptidyl-glycine α-amidating monooxygenase (rat source, IVI-10032; human source, IVI10033) which has a molecular mass of about 60,000 to 65,000 daltons. It has been purified such that it exhibits a specific enzymatic activity (number of units of α -amidation activity per milligram of protein) of at least approximately 25 mU and preferably at least approximately 50 mU/mg protein. It has also been purified so as to exhibit a single, homogeneous, well-defined band following electrophoresis on sodium dodecyl sulfate/polyacrylamide gels (SDS-PAGE).
The purified peptidyl-glycine α -amidating monooxygenase is used to amidate the alpha-carboxyl group of a polypeptide having a terminal glycine residue, where the glycine functions as an amino group donator. The substrate peptide or polypeptide can be purified from natural sources, synthesized from its component amino acids, or produced by recombinant DNA techniques. The glycine-terminating polypeptide is combined with oxygen in the presence of an effective amount of the enzyme. The amount of the enzyme required depends on several variables well known to this art including particularly, but not limited to, the following: the specific activity of a given enzyme preparation, the amount and chemical nature of the substrate to be converted, the time within which conversion is to take place and the temperature and pH of the reaction mixture. Those skilled in this art will recognize other variables that may influence the precise amount of enzyme required in a given situation. The oxygen is usually employed in stoichiome trie amount but an excess of the oxygen does not affect the reaction. The presence of copper ions is also required, and can be provided by any copper salt whose anion does not adversely affect the reaction. When the enzyme has a specific enzymatic activity of about lmU/mg protein, maximum α -amidation occurs with a concentration of 4.7 uM cupric ions. As the purity of the enzyme is increased, the concentration requirements for the exogenous cupric ion diminishes. The enzymatic activity can also be enhanced by the presence of ascorbate ions which can be provided by any salt, as long as the cation of the salt does not adversely effect the reaction. For purified enzyme having a specific enzymatic activity of approximately 50 mU/mg protein, maximal activity of the α -amidation occurs at about 5.5 mM ascorbate. α - αmidation activity may be increased by the addition of catalase. The α-amidation reaction optimum pH is between 6.5 and 7.5.
Since the peptidyl-glycine α -amidating monooxygenase has been sufficiently purifed, it is now possible to obtain monoclonal antibodies directed against the enzyme by standard procedures. The monoclonal antibodies allow the enzyme recovery procedures from the medullary thyroid carcinomas to be facilitated or wholly supplanted by immunoabsorption purification procedures. The enzyme has also been sufficiently purified to permit its amino acid sequence to be determined. This information is necessary in order to permit the isolation of the genetic material coding for the enzyme and its subsequent incorporation into an appropriate unicellular organism or host cell isolated from a multicellular organism which does not contain DNA coding for the peptidylglycine α -amidating enzyme. This is accomplished by standard recombinant DNA procedures, such as found in Maniatis, E.F. , et al, Molecular Cloning: A Laboratory Manual, Cold Spring Harbor, 1982; or Wu, R. , ed., Methods in Enzymology, Vol. 68, Academic Press, 1979. The resulting cells containing the heterologous DNA coding for peptidyl-glycine α -amidating enzyme allows the production of sufficient quantities of the enzyme in order to perform in vitro post- translational α -amidation and theoretically permits these cells to perform this modification qf a peptide or polypeptide in vivo. The α -amidation activity of the purified enzyme of this invention was demonstrated using a substrate of radioiodinated D-Tyr-Val-Gly, a peptide whose sequence mimics the carboxyl terminus of the melanocyte stimulating hormone precursor. Assays were performed in 100 mM TES (N-tris [hydroxymethyl] me thy 1-2-aminoe thane sulfonic acid) buffer, pH 7.0, at 37°C for three hours. Th product, [ 125I] Tyr-Val-NH2, was separated from the substrate by cation exchange chroma tography. The amidating enzyme activity was also demonstrated using a synthetic substrate which mimicked the sequence of the carboxyl terminus of calcitonin, [Tyr25Gly33] calcitonin (26-32).
Although the present invention has been described in connection with preferred embodiments thereof, many variations and modifications will become apparent to those skilled in the art.

Claims

WHAT IS CLAIMED IS:
1. Peptidyl-glyc ine α-amidating monooxygenase, having a molecular mass of about 60,000 - 65,000 daltons, purified so as to exhibit a single, homogeneous, well-defined band following electrophoresis on SDS/polyacrylamide gels.
2. The peptidyl-glycine α-amidating monooxygenase of Claim 1 having a specific enzymatic activity of at least about 50mUper milligram of protein.
3. The peptidyl-glycine α-amidating monooxygenase of Claim 1 immobilized on a solid support.
4. The peptidyl-glycine α-amidating monooxygenase of Claim 1 extracted from medullary thyroid carcinomas.
5. A recombinant DNA-produced peptidyl-glycine α-amidating monooxygenase.
6. A method of preparing the peptidyl-glycine α-amidating monooxygenase of Claim 1 which comprises subjectins animal tissue extracts to anion exchange chromatography, subjecting the resulting α-amidating activity-containing material to size exclusion chromatography employing chromatographic media capable of separating material having a molecular mass of about 60,000 to 65,000 daltons, and thereafter subjecting the α-amidating activity-containing eluant fraction to strong anion exchange chromatography.
7. The method of Claim 6 wherein the animal tissue extract is from medullary thyroid carcinoma tissue, or medullary thyroid carcinoma cell lines, or from the tissue culture medium from such cell lines, or from any combination thereof.
8. A method of preparing an α-amidated peptide from a peptide or polypeptide substrate ending with an aminodonating residue, comprising the reaction of said substrate with oxygen in the presence of peptidyl-glycine α-amidating monooxygenase.
9. The method of Claim 8 effected in the additional presence of cupric ions.
10. The method of Claim 8 wherein the araino-donating residue is glycine.
11. The method of Claim 8 effected in the additional presence of ascorbate ions and/or catalase.
12. The method of Claim 8 effected at a pH of about 6.5 to 7.5.
13. The method of Claim 11 wherein tife amount of ascorbate constantly exceeds the amount of substrate but is insufficient to inhibit the reaction.
14. The method of Claim 8 wherein the substrate is a recombinant DNA-produced or a naturally occurring or synthetic peptide or polypeptide.
15. A host cell which is a unicellular organism or a host cell isolated from a multicellular organism containing heterologous DNA coding for the peptidyl-glycine α -amidating monooxygenase.
16. A host cell according to Claim 15 which is a unicellular organism.
17. A host cell according to Claim 16 which is a prokaryo te.
18. A prokaryote host cell according to Claim 17 derived from E . coli .
PCT/US1985/001616 1984-09-27 1985-08-26 Alpha-amidation enzyme WO1986002099A1 (en)

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HU853879A HU195857B (en) 1984-09-27 1985-08-26 Process for production of alpha amidated peptides or polipeptides
AT85904514T ATE92522T1 (en) 1984-09-27 1985-08-26 ALPHA AMIDATION ENZYME.
DK241486A DK241486A (en) 1984-09-27 1986-05-23 ALFA-amidating enzyme
FI862216A FI100993B1 (en) 1984-09-27 1986-05-26 Peptidyl glycine amidation monooxygenase
NO86862100A NO862100L (en) 1984-09-27 1986-05-27 ALFA-AMIDERINGSENZYM.

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WO1989002460A1 (en) * 1987-09-15 1989-03-23 Genentech, Inc. cDNA ENCODING PEPTIDYL-GLYCINE ALPHA-AMIDATING MONOOXYGENASE (PAM)
WO1990008190A1 (en) * 1989-01-17 1990-07-26 Suntory Limited RECOMBINANT C-TERMINAL α-AMIDATING ENZYME OF HUMAN THYROID ORIGIN
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US6319685B1 (en) 1984-09-27 2001-11-20 Unigene Laboratories, Inc. Alpha-amidating enzyme compositions and processes for their production and use
EP0249412A3 (en) * 1986-06-07 1989-02-22 Hisayuki Matsuo C-terminal alpha-amidating enzyme and process for production and use thereof
EP0249412A2 (en) * 1986-06-07 1987-12-16 Hisayuki Matsuo C-terminal alpha-amidating enzyme and process for production and use thereof
EP0529742A1 (en) * 1987-08-14 1993-03-03 Unigene Laboratories Inc. Alpha-amidating enzyme compositions and processes for their production and use
US5789234A (en) * 1987-08-14 1998-08-04 Unigene Laboratories, Inc. Expression systems for amidating enzyme
WO1989002460A1 (en) * 1987-09-15 1989-03-23 Genentech, Inc. cDNA ENCODING PEPTIDYL-GLYCINE ALPHA-AMIDATING MONOOXYGENASE (PAM)
WO1990008190A1 (en) * 1989-01-17 1990-07-26 Suntory Limited RECOMBINANT C-TERMINAL α-AMIDATING ENZYME OF HUMAN THYROID ORIGIN
EP0382403A3 (en) * 1989-02-06 1991-04-10 Unigene Laboratories Inc. Expression systems for amidating enzyme
EP0382403A2 (en) * 1989-02-06 1990-08-16 Unigene Laboratories Inc. Expression systems for amidating enzyme
EP0448513A3 (en) * 1990-03-21 1991-12-27 Japat Ltd Process for production of peptidylglycine alpha-hydroxylating monooxygenase and use thereof
EP0448513A2 (en) * 1990-03-21 1991-09-25 Japat Ltd Process for production of peptidylglycine alpha-hydroxylating monooxygenase and use thereof
EP1907561A2 (en) * 2005-06-24 2008-04-09 Unigene Laboratories, Inc. Cell lines for expressing enzyme useful in the preparation of amidated products
EP1907561A4 (en) * 2005-06-24 2009-07-15 Unigene Lab Inc Cell lines for expressing enzyme useful in the preparation of amidated products
US8815583B2 (en) 2005-06-24 2014-08-26 Enteris Biopharma, Inc. Cell lines for expressing enzyme useful in the preparation of amidated products

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AU594026B2 (en) 1990-03-01
DE3587506T2 (en) 1994-01-13
DE3587506D1 (en) 1993-09-09
EP0201511A1 (en) 1986-11-20
AU4802785A (en) 1986-04-17
EP0201511A4 (en) 1988-05-31
US4708934A (en) 1987-11-24
DK241486D0 (en) 1986-05-23
HU195857B (en) 1988-07-28
NO862100L (en) 1986-05-27
DK241486A (en) 1986-05-23
HUT41444A (en) 1987-04-28
JP2594037B2 (en) 1997-03-26
FI94361C (en) 1995-08-25
CA1341037C (en) 2000-06-27
FI862216A0 (en) 1986-05-26
LT2661B (en) 1994-04-25
FI100993B1 (en) 1998-03-31
ATE92522T1 (en) 1993-08-15
FI862216A (en) 1986-05-26
FI94361B (en) 1995-05-15
EP0201511B1 (en) 1993-08-04
NO175214C (en) 1994-09-14
JPS62500560A (en) 1987-03-12
RU1802814C (en) 1993-03-15

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