WO1994011397A1 - Ghrh agonists - Google Patents

Ghrh agonists Download PDF

Info

Publication number
WO1994011397A1
WO1994011397A1 PCT/US1993/011058 US9311058W WO9411397A1 WO 1994011397 A1 WO1994011397 A1 WO 1994011397A1 US 9311058 W US9311058 W US 9311058W WO 9411397 A1 WO9411397 A1 WO 9411397A1
Authority
WO
WIPO (PCT)
Prior art keywords
leu
ala
ser
asp
abu
Prior art date
Application number
PCT/US1993/011058
Other languages
French (fr)
Inventor
Jozsef Zsigo
Original Assignee
The Administrators Of The Tulane Educational Fund
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by The Administrators Of The Tulane Educational Fund filed Critical The Administrators Of The Tulane Educational Fund
Priority to AU57271/94A priority Critical patent/AU5727194A/en
Publication of WO1994011397A1 publication Critical patent/WO1994011397A1/en

Links

Classifications

    • 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
    • C07K14/60Growth hormone-releasing factor [GH-RF], i.e. somatoliberin
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides

Definitions

  • the present invention relates to peptides having influence on the function of the pituitary gland in humans and other animals.
  • the present invention is directed to a synthetic peptide which promotes the release of growth hormone by the pituitary gland.
  • hypothalamus controls the secretory functions of the adenohypophysis with the hypothalamus producing special substances which stimulate or inhibit the secretion of each pituitary hormone.
  • Hypothaiamic releasing factors have been characterized for the pituitary hormone thyrotropin (the tripeptide TRF), for the pituitary gonadotropins luteinizing hormone and follicle stimulating hormone (the decapeptide LRF, LH-RH or GnRH) and for the pituitary hormone adrenocorticotropin (the 41-amino acid poly peptide CRF).
  • GHRHs or GRFs growth hormone releasing hormones or GH-releasing factor
  • Analogs of the native structures have also been synthesized in order to elucidate structure-activity relationships and, eventually, to provide synthetic congeners with improved properties, such as increased growth hormone release and/or increased metabolic stability.
  • Studies with the synthetic human growth hormone releasing hormone (hGHRH or hGRF) and its analogs have revealed that: a) deletion of the NH 2 -terminal tyrosine residue of HGRF causes its activity to drop to 0.1 %; N-acetylation of this residue or change of replacement of L by D isomers lowers the in vitro bioactivity of hGRF (1-40)-0H to 2-3% and causes a 10-12 fold increase in the in vivo potency of hGRF (1 -29)-NH 2 ; these findings indicate that the presence of said residue is essential for imparting the hGRF molecule with high bioactivity; b) fragments containing the first 29 residues at least and being terminated with an amide group, e.g., hGRF (1-29)-NH
  • novel synthetic peptides of this invention are extremely potent in stimulating the release of pituitary GH in animals, including humans. These synthetic peptides retain their physiological activity in solution for an extended period of time and are resistant to enzymatic degradation in the body. Without in any way limiting the invention or its scope, Applicants wish to express their understanding that this retention of activity in vitro and resistance to in vivo degradation are due to the omega-guanidino lower alkyl group at the terminal 29- position of the peptide and the presence non-coded amino acids in the enzymic cleavage site(s) of the synthetic peptides.
  • the synthetic peptides (abbreviated [PeP]) have the sequence: Q 1 -CO-R 2 -R 3 -Ala 4 -lle 6 -Phe ⁇ -Thr 7 -R 8 -Ser 9 -R 10 -Arg 11 -R 12 -R 13 -R 1 -R 1 B -Gln 1 ⁇ -R 17 -R 18 - Ala 19 -Arg 20 -R 21 -R 22 -R 23 -R 24 -R 25 -lle 2 ⁇ -R 27 -R 28 -NH-Q 2
  • Q 1 is 3-(5-hydroxyindolyl)-methyl or an omega or alpha-omega substituted alkyl of the structure:
  • [ ⁇ ] is phenyl
  • Y is H, -NH 2 , CH 3 CONH- or CH 3 NH-;
  • Z is H or CH 3 ; m is 1 or 2; and n is 0, 1 , or 2; R 2 is Ala, D-Ala, D-N-Methyl-Ala, Abu or Aib
  • R 3 is Asp, D-Asp, Glu or D-Glu
  • R 8 is Asn, D-Asn, Ser, D-Ser,or Abu
  • R 10 is Tyr, D-Tyr,or 5-HTP
  • R 12 is Lys, D-Lys, Arg or Orn R 13 is Val, lie, or Tbg
  • the synthetic peptides are synthesized by a suitable method such as by exclusively solid phase techniques, by partial solid-phase techniques, by fragment condensation or by classical solution phase synthesis.
  • the C-terminal residue (here, Q 2 ) is appropriately linked (anchored) to an inert solid support (resin). Then, an amino acid bearing protecting groups for its alpha amino group (and, where appropriate, for its amino acid side chain) is coupled in the C- > N direction. After completion of this coupling step, the alpha amino protecting group is removed from this newly added amino acid residue and the next amino acid (suitably protected) is added, and so forth.
  • the N-terminai protecting groups are removed after each residue is added, but the side chain protecting groups, e.g., X 2 , X 3 etc. in formula [PR][PeP] below are not yet removed.
  • the peptide is cleaved from the support and then freed from any side chain protecting group(s) under conditions that are minimally destructive towards residues in the sequence. This must be followed by a careful purification and scrupulous characterization of the synthetic product, so as to ensure that the desired structure is indeed the one obtained.
  • alpha amino function of the amino acids during the coupling step with an acid or base sensitive protecting group.
  • protecting groups should have the properties of being stable in the conditions of peptide linkage formation, while being readily removable without destruction of the growing peptide chain or racemization of any of the chiral centers contained herein.
  • Suitable alpha amino protecting group are Boc and Fmoc.
  • the synthetic peptides of Formula I may be formulated in pharmaceutical dosage form and administered to humans or animals for therapeutic or diagnostic purposes. More particularly, the peptides may be used to promote the growth of warm-blooded animals, as, in humans, to treat human growth deficiency by stimulating in vivo synthesis and/or release of endogenous GH; to treat certain nct ' ⁇
  • SUBSTITUTE SHEET (RULE physiological conditions such as severe growth retardation due to chronic renal insufficiency; to offset certain effects of aging, e.g., reducing loss of muscle and bone loss; to accelerate healing and tissue repair; to improve feed utilization, thereby increasing lean/fat ratio favoring muscle gain at the cost of fat; and also to enhance milk production in lactating cattle.
  • the synthetic peptides may be used in a method to ascertain endogenous physiological ability to produce hGH and a diagnostic kit for carrying out this method.
  • FIGURE Figure 1 is a graphical representation of selected data from Table 4 in
  • EXAMPLE XIX herein, wherein "A” represents the peptide of EXAMPLE VIII herein -- i.e., (Dat ⁇ Abu 16 ,Nle 27 ,Asp 28 ,Agm 29 )hGH-RH(1-29) -- and "B" indicates the peptide of EXAMPLE XVI herein -- i.e., (5-Hiaa ⁇ Abu 15 ,Nle 7 ,Asp 28 ,Agm 29 )hGH- RH(1-29).
  • Nle norleucine
  • Nva norvaline
  • Abu alpha amino butyric acid
  • Aib alpha iso-butyric acid
  • Tba alpha-t-butylalanine
  • Tbg alpha-t-butylglycine
  • 5-Hiaa 5-Hydroxy-indolylacetic acid
  • C-MeTyr is meant 1 -methyl-DL-Tyrosine
  • N-MeAla and N-MeTyr are meant N- methyl-alanine and N-methyl-tyrosine respectively.
  • amino acid residue has isomeric forms, it is the L-form of the amino acid that is represented unless otherwise expressly indicated.
  • Other abbreviations used are: AcOH acetic acid
  • amino acid sequences of the synthetic peptides are numbered in correspondence with the amino acid residues in hGH-RH(1-29). That is, the Ala 4 and R 8 of the Formula I peptide occupy the same position in the sequence as the Ala 4 and R 8 residues in hGH-RH(1-29).
  • UBSTITUTE SHEET (RULE 26) lack an N- and a C- terminus respectively, in order to remove any question therefore, it should be understood that the terms N- and C-terminal used with respect to the synthetic peptides of Formula I mean Q 1 and Q 2 .
  • the preferred synthetic peptides of the present invention have the sequence:
  • Q 1 -CO moieties may when taken together form an amino acid residue: thus, when in Q 1 m is 1 , n is 1 and y is NH 2 , Q'-CO forms tyrosyl ("Tyr-"). Even when the Q 1 functional groups do not cause Q 1 to form an amino acid with CO-, the two constituents of the Formula I peptide may together form a readily recognized group. Thus, when in m is 1 , n is 1 and Y and Z are H, Q'-CO together form 3-(4-hydroxyphenyl)propionyl, known as des-amino-Tyr (or "Dat").
  • 3-(5-hydroxyindolyl)methyl as Q 1 with CO forms a 3-(5-hydroxy- indolyDacetyl moiety (or "5-Hiaa”).
  • the Q 1 -CO moieties may be taken as a unitary moiety R 1 and replaced in the Formula I peptides by abbreviations such as Tyr ⁇ Dat 1 , 5-Hiaa 1 , etc. as appropriate.
  • the NH-Q 2 moieties may be taken as a unitary moiety R 29 when together they form a single recognized functional group.
  • p 4
  • This peptide has the structure: Q 1 -CO-Ala 2 -Asp 3 -Ala 4 -lle 6 -Phe ⁇ -Thr 7 -R 8 -Ser 9 -Tyr 10 -Arg 11 -Lys 12 -Val 13 -Leu 14 -R 16 -Gln 16 - Leu 17 -Ser 18 - Ala 19 -Arg 0 -Lys 21 -Leu 22 -Leu 23 -Gln 2 -Asp 2B -lle 2 ⁇ -R 27 -R 28 -NH-O 2 wherein
  • R 8 is Asn, Ser or Abu R 15 is Abu,Ala or Gly R 27 is Met.Tba or NIe and R 28 is Ser or Asp;
  • Especially preferred embodiments include peptides of Formula I in which Q 1 - CO is Dat, Ac-Tyr, N-Me-Tyr, C-Me-Tyr and Hiaa; and NH-Q 2 is Agm. Further preferred embodiments include peptides of Formula I in which Q'-CO is Dat or Hiaa; R 15 is Abu; R 27 is NIe; R 28 is Asp; and NH-Q 2 form Agm.
  • the full formula of this analog is:
  • R 28 is Ser and in Q 2 p is 4, the peptide may be written as: (Dat 1 , Abu 8 , NIe 27 , Agm 29 )hGHRH (1-29) described in Example XIII.
  • the peptides are synthesized by a suitable method such as by exclusively solid phase techniques, by partial solid-phase techniques, by fragment condensation or by classical solution phase synthesis.
  • a suitable method such as by exclusively solid phase techniques, by partial solid-phase techniques, by fragment condensation or by classical solution phase synthesis.
  • the techniques of exclusively solid-phase synthesis are set forth in the textbook "Solid Phase Peptide Synthesis", J.M. Stewart and J.D. Young, Pierce Chem. Company, Rockford, 1 1 1. ,1984 (2nd. ed.), G. Barany and R.B. Merrifield, "The Peptides", Ch. 1 , 1-285, pp. 1979, Academic Press, Inc., and M. Bodanszky, "Principles of Peptide Synthesis", SpringerVerlag, 1984.
  • the synthetic peptides of Formula I are preferably prepared using solid phase synthesis, such as that generally described by Merrifield, J.Am.Chem.Soc, 85, p. 2149 (1963), although other equivalent chemical syntheses known in the art can also be used as previously mentioned.
  • the moiety which forms the C or N-terminal group of the resulting peptide is joined to a polymeric resin support phase via a chemical link.
  • Amino acid residues or oligopeptide fragments are then added sequentially to the alpha amino functional group of the C or N-terminal moiety until the desired peptide sequence is obtained. Because the amino acid residues or oligopeptide fragments are added to the C-terminal Q 2 group here, growth of the synthetic peptides of Formula I begins at the C terminal and progresses toward the N- terminal. When the desired sequence has been obtained, it is removed from the support phase.
  • the peptides of Formula I may be synthesized on a variety of support phases.
  • These support phases may be amino or hydroxy resins such as amino- methyl resins (suitably 1 % cross linked), benzhydrylamine resins (suitably 2% cross linked) p-methylbenzhydrylamine resins (suitably 2% cross linked) and the like.
  • the support phase [SP] is an amino type resin of the formula: H 2 N-CH 2 - ⁇ -[Pm] IX where [Pm] is a polymeric substrate.
  • the initial material joined to the support phase is suitably the C-terminal Q 2 group.
  • the adjacent NH functional group is already affixed to Q 2 .
  • Agm or 4-guanidino butylamine are especially preferred.
  • the NH-Q 2 group is joined to the support phase via a stable but readily cieavable bridging group. It has been found that such a bridge may be readily provided by a sulfonyl phenoxy acetyl moiety.
  • Fmoc-NH-Q 2 -S0 2 -[ ⁇ ]-(M ⁇ )O-CH 2 -CO-[SP] constitute the material joined to the support phase for the synthetic sequence. They are prepared and linked to the support phase as follows.
  • the primary amino group of agmatine i.e., the -NH- group preceding Q 2
  • a tert-butyloxy carbonylating agent suitably ditert-butyl dicarbonate
  • This reaction may take place preferably at ambient temperatures or at 5-10°C in the presence of a base.
  • the protected material is then reacted in a similar solvent system with the arylsulfonyl halide
  • Boc-NH-Q 2 -S0 2 - ⁇ -0-CH 2 -CO-[SP] which represents Q 2 linked to the polymeric substrate support phase via the sulfonyl phenoxy acetyl moiety, more fully expressed as:
  • the coupling is carried out using any of the known dialkyl carbodiimide coupling procedures.
  • diisopropyl-carbodiimide in the presence of 1-hydroxybenzotriazole hydrate in dimethylformamide at ambient temperatures.
  • N,N'dicyclohexyl-carbodiimide there may be employed.
  • the aforesaid Boc- aminoalkyl guanidino-sulfonyl-phenoxyaceticacid is mixed with the carbodiimide in 2 to 1 molar ratio, the formed N,N'dicyclohexyl urea is removed by filtration and the resulting solution is added to the support phase.
  • the protected amino ⁇ alkyl guanidinosulfonyl phenoxyacetic acid is mixed with equimolar BOP and dissolved in DMF containing twice molar NMM in 10% concentration.
  • the activation can be enhanced in the presence of 1-3 molar excess of HOBt yielding an efficient coupling rate to the solid support preferably to an aminomethyl resin at room temperature.
  • N- benzyloxycarbonyl chloride is used in the presence of an aqueous alkali, suitably sodium hydroxide, preferably at about 4N under agitation and cooling to between 1 and 5°C.
  • an aqueous alkali suitably sodium hydroxide, preferably at about 4N under agitation and cooling to between 1 and 5°C.
  • sodium hydrogen carbonate treatment the protected product is precipitated and thereafter is reacted with an aryl-sulfonyl chloride as previously.
  • the Fmoc procedure comprises the sequential steps of reacting N-benzyloxy carbonyl chloride with NH 2 -Q 2 in the presence of a base to form Cbz-NH-Q 2 , reacting said Cbz-NH-Q 2 with a substituted arylsulphonyl halide in the presence of a strong aqueous base and removing the Cbz group by catalytic hydrogenation.
  • the substituted arylsulphonyl halide has the formula:
  • Hal-S0 2 -[ ⁇ ](M.)-O-CH 2 -COOH wherein Hal is chloro or bromo; M, is lower alkyl or lower alkoxy of 1 to 5 carbon atoms located at the positions of the phenyl nucleus other than 1 and 4; and s is 1-3.
  • the reaction yields H 2 N-Q -S0 2 -[ ⁇ ](M,)-O-CH 2 -COOH.
  • the product is reacted with Fmoc-CI in the presence of a base to yield the corresponding Fmoc protected aminoalkyi guanidino-sulfonyl aryloxy acetic acid, i.e.
  • the arylsulfonyl halide should preferably carry between 1 and 3 M substituents which may be alkyl or lower alkoxy, suitably methyl or methoxy.
  • substituents which may be alkyl or lower alkoxy, suitably methyl or methoxy.
  • Boc procedure it is desirable to substitute the phenyl moiety with up to three alkyl or alkoxy groups. These groups weaken the strength of sulfonamide bridge and enable it to be cleaved by trifluoroacetic acid, once all the amino acid residues have been added and one wishes to remove the intermediate from the support phase.
  • This reaction is carried out in the presence of a strong but dilute aqueous base, suitably about 1 N sodium hydroxide.
  • the reaction mixture is acidified and the product extracted, suitably with a water immiscible organic solvent such as ethyl acetate.
  • a water immiscible organic solvent such as ethyl acetate.
  • the extract is then concentrated and hydrogenated, suitably at atmospheric pressure and room temperature in the presence of a catalyst such as palladium on charcoal in a reduction inert solvent. If ethyl acetate is used as the extractant, this may be used as the hydrogenation solvent.
  • the peptide itself may then suitably be built up by solid phase synthesis in the conventional manner.
  • the alpha amino-protecting group of the next amino acid residue is protected by Boc or Fmoc to prevent reaction between the N-terminal of R 28 while this is being reacted with NH 2 -Q 2 .
  • Boc or Fmoc are attached to the NH 2 -Agm or H 2 N-Q 2 -SO 2 -[ ⁇ ](M,)- O-CH 2 -COOH respectively, as described above.
  • the amino acid residues of the synthetic peptides are added sequentially . Because the peptide is constructed from the C-terminal, the residues are added in reverse numerical order, i.e., R 28 , R 27 , and so forth.
  • the protected amino acids are coupled sequentially, with Q 1 finally being added.
  • some may be coupled to one another in a separate vessel and added as an oligo- peptide in the solid phase reaction.
  • the selection of an appropriate coupling reagent is within the skill of the art. Particularly suitable as coupling reagents are N,N'-diisopropyl carbodiimide (DIC) or the BOP carboxyl activating reagent.
  • Each protected amino acid or amino acid sequence is introduced into the solid phase reaction in about a three-fold molar excess, with respect to NH 2 -Q 2 , etc., and the coupling may be carried out in as medium such as DMF: CH 2 CI 2
  • the Q 2 guanidino alkyl end of the Formula I peptide is cleaved from the support phase at the sulfonyl group. If the Boc protocol is utilized, then the cleaving agent is anhydrous hydrofluoric acid; whereas, in the Fmoc protocol the cleaving agent is trifluoroacetic acid.
  • Removal of the intermediate peptide from the resin support is performed by treatment with a reagent such as liquid hydrogen fluoride or trifluoroacetic acid. This also cleaves all remaining side chain protecting groups X 3 , X 7 , X 11 , X 12 and and the anchoring guanidinosulfo bond, if present, and also the alpha amino or alpha-hydroxyl protecting group X 1 . These groups have different values depending on whether Boc or Fmoc protocols are used.
  • side Chain Protecting Groups The protection of reactive side chain functional groups of the various amino acid moieties or peptide fragments is common to solid phase synthesis. These side chain functional groups are protected in order to prevent an undesirable chemical reaction from occurring at said chains. Accordingly, it is common that, as a step in the synthesis, an intermediate compound is produced which includes each of the amino acid residues located in its desired sequence in the peptide chain with side-chain protecting groups (e.g., X 1 , X 7 , etc.) linked to the appropriate residues.
  • side-chain protecting groups e.g., X 1 , X 7 , etc.
  • a side chain amino protecting group is not critical except that generally one is chosen which is not removed during deprotection of the alpha amino groups during the synthesis.
  • the protecting group preferably retains its protecting properties and is not split off under coupling conditions
  • the protecting group should be stable to the reagent, is preferably stable under the coupling reaction conditions selected for removing the alpha amino protecting group at each step of the synthesis and
  • the side chain protecting group must be removable upon the completion of the synthesis of the desired amino acid sequence, under reaction conditions that will not undesirably alter the peptide chain.
  • the side chain protecting groups are attached to the amino acid residues by steps well known in the art.
  • [PR][PeP] has the structure:
  • X 1 is either hydroxyl, or an amino protecting group or nil, depending on the meaning of Y in Formula II (the formula for one of the Q 1 moieties).
  • X 3 is a suitable ester-forming protecting group for the carboxyl group of Asp or Glu.
  • Boc protocol it may form cyclohexyl esters; in the Fmoc protocol tert- butyl esters are preferred.
  • X 7 is a suitable protecting group for the hydroxyl group of Thr or Ser, such as tert-butyl, Bzl.
  • the preferred protecting group in the Boc protocol is Bzl and in the Fmoc protocol it is tert-butyl.
  • X 10 is a suitable protecting group for the phenolic hydroxyl group of Tyr or N- MeTyr, such as tert-butyl, Bzl, 4Br-Cbz and 2,6-dichlorobenzyl (DCB).
  • the preferred protecting group in the Boc protocol is 2,6-dichlorobenzyl and in the Fmoc protocol it is tert-butyl.
  • X 11 is a suitable protecting group for the guanidino group of Arg, such as nitro, Tos, Pmc, Mtr; in the Boc protocol Tos is the preferred group and 2,2,5,7,8- pentamethyl chroman-6-sulfonyl in the Fmoc protocol.
  • X 12 is a suitable protecting group for the side chain amino group of Lys. Illustrative of suitable side chain amino protecting groups are 2-chloro- benzyloxycarbonyl (2-CI-CBz) and tert-butyloxycarbonyl (Boc). In the Boc protocol, 2-chlorobenzyloxycarbonyl is the preferred protecting group and in the Fmoc protocol Boc is thus utilized.
  • X 24 is hydrogen or a protecting group for the imidazole nitrogen of His, such as Tos in the Boc or Trt in the Fmoc protocol.
  • the products of the present invention may be utilized to promote the growth of warm-blooded animals (e.g., humans) and also enhance the milk production of females of milk producing mammals, suitably but not exclusively goats and cows, preferably cows.
  • warm-blooded animals e.g., humans
  • milk production of females of milk producing mammals suitably but not exclusively goats and cows, preferably cows.
  • the peptides of the invention may be administered in the form of pharmaceutically acceptable, nontoxic salts, such as acid addition salts.
  • acid addition salts are hydrochloride, hydrobromide, sulphate, phosphate, fumarate, gluconate, tannate, maleate, acetate, citrate, benzoate, succinate, alginate, pamoate, malate, ascorbate, tartrate, and the like.
  • the compounds of the present invention are suitably administered to the subject humans or animals s.c, i.m., or i.v; intranasally or by pulmonary inhalation; or in a depot form (e.g., microcapsules, microgranules, or cylindrical rod like implants) formulated from a biodegradable suitable polymer (such as D,L- lactide-co-glycolide), the former two depot modes being preferred.
  • a biodegradable suitable polymer such as D,L- lactide-co-glycolide
  • Other equivalent modes of administration are also within the scope of this invention, i.e., continuous drip, depot injections, infusion pump and time release modes such as microcapsules and the like.
  • Administration is in any physiologically acceptable injectable carrier, physiological saline being acceptable, though other carriers known to the art may also be used.
  • the dosage level should be between 0.2 and 2 micrograms/kg body weight per injection except for depot form where the amount injected would be calculated to last from about 15 to about 30 days or longer. These dosage ranges are merely preferred. Administration of non-depot forms may be between 1 and
  • BST1TUTE SHEET (RULE 26) should be much less expensive than that utilizing hGH.
  • development of long-acting delivery systems for these analogs can make this new modality of treatment more practical and convenient.
  • GH growth hormone
  • synthetic hGH is currently approved only for the treatment of growth failure due to a lack of adequate endogenous growth hormone, but hGH has also been used to treat short children who are not classically GH-deficient such as girls with Turner's syndrome; prepubertal children with chronic renal insufficiency and severe growth retardation; and children with non-GH deficient short stature.
  • hGH-RH a 50-100 microgram dose of GH-RH
  • a 50-100 microgram dose of a GH- RH analog of Formula I a 50-100 microgram dose of a GH- RH analog of Formula I
  • means for assaying the GH response evoked by each dose may be any conventional means which will indicate the quantitative amount of hGH present in a blood sample drawn from the patient.
  • the concentration of GH in serum is determined using standard radioimmunoassay ("RIA") procedures, e.g., Miles I.E.M. et al., Lancet n:492-493 (1968) or Odell W. et al. J.Lab.Clin.Med., 70:973-80 (1967).
  • RIA radioimmunoassay
  • the diagnostic test is performed as follows. First, the GH-RH dose is administered. Thirty minutes later, a blood sample is taken for RIA of GH.
  • kits e.g., Nichols Institute of Diagnostics, San Juan Capistrano, CA
  • reference preparations of hGH e.g., NIAMDD-hGH-RP-1
  • hGH e.g., NIAMDD-hGH-RP-1
  • a diagnostic kit for testing endogenous physiological ability to produce GH may incorporate a 50-100 microgram dose of GH-RH; a 50-100 microgram dose of a GH-RH analog peptide of Formula I; and means for assaying the GH response evoked by each dose.
  • the invention further includes a method for ascertaining the endogenous physiological ability to produce hGH and a diagnostic kit for carrying out this method.
  • Glucocorticoids are potent inhibitors of linear growth in man and growth suppression is a well known risk of long term treatment of asthmatic children with steroids. Thus stunted growth is an important consequence of chronic administration of glucocorticoids in childhood.
  • the inhibition of GH secretion is due in some extent to the fact that chronic administration of glucocorticoids suppresses GHRH. This inhibition occurs at the level of the hypothalamus or above and in this situation only the treatment with GHRH agonists will stimulate linear growth.
  • Growth hormone is a potent anabolic hormone that enhances protein synthesis and nitrogen retention and chronic administration of agonistic analogs of GHRH increase the endogenous growth hormone secretion.
  • the therapy with GHRH agonistic analogs has uses in other areas of medicine such as catabolic states causing accelerated weight loss; tissue repair in patients with sever body surface burn, in accelerating healing of nonunion fractures and in some cases of cardiac failure.
  • GH-RH GH-deficient children respond to GH-RH(1-40), GH-RH(1-29) or GH-RH(1-44), with an increase in growth.
  • GH-RH(1-40), GH-RH(1-29) or GH-RH(1-44) respond to GH-RH(1-40), GH-RH(1-29) or GH-RH(1-44), with an increase in growth.
  • Most children who respond to hGH, will respond to GH-RH.
  • GH-RH(1-29)NH 2 given subcutaneously twice a day promoted linear growth in approximately 50% of a group of GH-deficient children (Ross et al, cited above). A small group of severely GH-deficient children will respond to GH-RH after 6(six) months of treatment.
  • Geriatric Patients To reduce the loss of muscle, bone and skin mass and lessen the increase of body fat that normally accompanies the aging process. 2. Catabolic states
  • GHRH agonists could be used during and after space flights to counteract the decrease in GH secretion. Weightlessness of space flight significantly decreases the release of growth hormone. This finding could explain the bone loss and muscle weakness many astronauts experience after prolonged space flights.
  • the following Examples set forth suitable methods of synthesizing by the solid-phase technique, several fragments and novel analogs of hGH-RH which have improved potency.
  • the couplings are preferably carried out as set out in Schedule A for coupling:
  • BOC is used for the alpha amino protection.
  • Benzyl ether is used as the hydroxyl side chain protecting group for Ser and Thr.
  • the phenolic hydroxyl group of Tyr is protected with DCB and the side chain carboxyl group of Asp is protected in the form of the cyclohexyl ester.
  • Tos is used to protect the guanidino group of Arg and 2-CI-Cbz is used as the protecting group for the Lys side-chain. Due to the decreased reaction rate of the 3-(4-hydroxyphenyl)propionic acid N- hydroxy-succinimide ester, a prolonged coupling time 60 minutes was used.
  • X 11 is tosyl
  • X 12 is 2-CI-Cbz.
  • cleave and deprotect the protected peptide-resin In order to cleave and deprotect the protected peptide-resin, it is treated with 1 ml m-cresol and 10 ml hydrogen fluoride (HF) per gram of peptide resin, at 0°C for 45 min. After elimination of the HF under high vacuum and evaporating the traces of the scavenger, the cleaved peptide and resin remainder is washed with dry diethyl ether and ethyl acetate. The peptide is then extracted with 50% aqueous acetic acid, separated from the resin by filtration and lyophilized.
  • HF hydrogen fluoride
  • the crude peptide is purified using either a Beckman Prep-350 preparative HPLC system (with a Beckman Type 163 variable wavelength UV detector) or a Beckman semipreparative HPLC system (with a Beckman 420 Gradient Controller, two 114M Solvent Delivery Modules, a 165 Variable Wavelength Detector and a Kipp and Zonen BD41 Recorder.
  • a Beckman Prep-350 preparative HPLC system with a Beckman Type 163 variable wavelength UV detector
  • a Beckman semipreparative HPLC system with a Beckman 420 Gradient Controller, two 114M Solvent Delivery Modules, a 165 Variable Wavelength Detector and a Kipp and Zonen BD41 Recorder.
  • separations are achieved on a 41.5 x 150 mm.
  • DYNAMAX column packed with spherical C18 silica gel 300 A pore size, 12 um Particle size) (RAININ Inc., Co., Woburn, MA).
  • purification can be performed
  • Solvent A consists of 0.1 % aqueous TFA and solvent B is 0.1 % TFA in 70% aqueous acetonitrile.
  • the column eluate is monitored at 220 nm and 280 nm.
  • the peptide is judged to be substantially (95%) pure by using a Hewlett- Packard HP-1090 liquid chromatograph.
  • the peptides are chromatographed on a 4.6 x 250 mm. W-Porex 5 um C18 column (Phenomenex, Collinso Palos Verdes, CA) at a flow rate of 1.2 ml/min. with a mixture of Solvent A and Solvent B using a gradient (from 40 to 70% B in 30 min).
  • X 1 is t-butyl ether
  • X 3 is t-butyl ester
  • X 11 is 2,2,5, 7,8-pentamethyl-chroman-6- sulphonyl
  • X 12 is Boc.
  • the protected peptide produced as above is utilized as starting material.
  • Dawley rats were anesthetized with pentobarbital (6 mg./100/g., b.w.), injected i.p.; 20 minutes after the injection of pentobarbital, blood samples were taken from the jugular vein (pretreated level) and immediately thereafter hGH-RH (1- 29)NH 2 (as a control) or hGH-RH(1-29)NH 2 analogs were injected i.v. Blood samples were taken from the jugular vein 5 and 15 minutes after the injection. The blood samples were centrifuged, plasma was removed and the GH level was measured by RIA. The result tabulated in Table 2 below are expressed as the mean ⁇ SEM; statistical significance is assessed by Duncan's Multiple Range Test. These results, expressed as potency, appear in Table 3.
  • Example XVIII The proceedings of Example XVIII were repeated except the in vivo effect of hGH-RH analogs on GH release in the rat was tested after i.m. injection. The results are tabulated in Table 6 as mean ⁇ _ SEM and are summarized in terms of potency in Table 7.
  • Example VIII 1 90.52120.5 105.0110.1 70.719.8 3 55.515.0 448.71116.6 126.3116.1
  • Example XVI 1 52.2125 200.0120.2 74.311.7 3 46.7119 640.3158.8 158.7150.6
  • analogs VIII and XVI gave growth hormone levels greater than those from hGHRH alone. The effect was long lasting which indicates that the analogs have not only higher receptor affinity but increased peptidase resistance too.
  • Xaa Ala Asp Ala lie Phe Thr Asn Ser Tyr Arg Lys Val Leu Xaa Gin 1 5 10 15

Landscapes

  • Health & Medical Sciences (AREA)
  • Chemical & Material Sciences (AREA)
  • Endocrinology (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Organic Chemistry (AREA)
  • Biophysics (AREA)
  • Gastroenterology & Hepatology (AREA)
  • Biochemistry (AREA)
  • Zoology (AREA)
  • General Health & Medical Sciences (AREA)
  • Genetics & Genomics (AREA)
  • Medicinal Chemistry (AREA)
  • Molecular Biology (AREA)
  • Proteomics, Peptides & Aminoacids (AREA)
  • Toxicology (AREA)
  • Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
  • Peptides Or Proteins (AREA)

Abstract

Synthetic peptides which have the sequence: Q?1-CO-R2-Asp3-Ala4-Ile5-Phe6-Thr7-R8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14-R15-Gln16-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25-Ile26-R27-R28-NH-Q2¿ wherein Q1 is 3-(5-hydroxyindolyl)-methyl or an omega or alpha-omega substituted alkyl of structure (I), where: [ζ] is phenyl; Y is H, -NH¿2?, CH3CONH- or CH3NH-; Z is H or CH3; m is 1 or 2; n is 0, 1 or 2; R?2¿ is Ala, D-Ala, D-N-Methyl-Ala, Abu or Aib; R8 is Asn, D-Asn, Ser, D-Ser, or Abu; R15 is Gly, Ala, Abu or Tbg; R27 is Nle, Ile, Leu, Tga, Tba or Met; R28 is Asp, Asn or Ser; and Q2 is a lower omega-guanidino-alyl group having a formula: -(CH¿2?)p-NH-C(NH2) = NH wherein p is 2-6, and at least one of R?2, R8 and R15¿ is Abu, and the pharmaceutically acceptable addition salts thereof with the pharmaceutically acceptable organic or inorganic bases or acids. Also included in the invention are pharmaceutical dosage form comprising said peptide and an excipient; methods of treating human growth deficiency comprising administering said peptide; a method for ascertaining endogenous physiological ability to produce hGH; and a diagnostic test.

Description

GHRH AGONISTS
This invention was made in part with Government support. The Government has certain rights in this application.
FIELD OF THE INVENTION The present invention relates to peptides having influence on the function of the pituitary gland in humans and other animals. In particular, the present invention is directed to a synthetic peptide which promotes the release of growth hormone by the pituitary gland.
BACKGROUND OF THE INVENTION Physiologists have long recognized that the hypothalamus controls the secretory functions of the adenohypophysis with the hypothalamus producing special substances which stimulate or inhibit the secretion of each pituitary hormone. Hypothaiamic releasing factors have been characterized for the pituitary hormone thyrotropin (the tripeptide TRF), for the pituitary gonadotropins luteinizing hormone and follicle stimulating hormone (the decapeptide LRF, LH-RH or GnRH) and for the pituitary hormone adrenocorticotropin (the 41-amino acid poly peptide CRF). An inhibitory factor, called somatostatin, has also been characterized in the form of a tetradecapeptide which inhibits the secretion of growth hormone (GH). GH releasing hormones or GH-releasing factor (GHRHs or GRFs) have been isolated from human pancreatic tumor as well as rat, porcine, bovine, ovine, caprine and human hypothalami. With the exception of the rat, all characterized GHRHs contain 44 amino acids with an amidated carboxy-terminus.
Each of these hypophysiotropic factors has been reproduced by total synthesis.
Analogs of the native structures have also been synthesized in order to elucidate structure-activity relationships and, eventually, to provide synthetic congeners with improved properties, such as increased growth hormone release and/or increased metabolic stability. Studies with the synthetic human growth hormone releasing hormone (hGHRH or hGRF) and its analogs have revealed that: a) deletion of the NH2-terminal tyrosine residue of HGRF causes its activity to drop to 0.1 %; N-acetylation of this residue or change of replacement of L by D isomers lowers the in vitro bioactivity of hGRF (1-40)-0H to 2-3% and causes a 10-12 fold increase in the in vivo potency of hGRF (1 -29)-NH2; these findings indicate that the presence of said residue is essential for imparting the hGRF molecule with high bioactivity; b) fragments containing the first 29 residues at least and being terminated with an amide group, e.g., hGRF (1-29)-NH2 and hGRF (1-37)-NH2, have at least 50% of the potency of hGRF; removal of the C-terminal amide group or further deletion of amino acids results in a marked decrease in bioactivity even if the C- terminus is amidated, e.g., hGRF (1-29)0H, hGRF (1-27)-NH2 and hGRF (1 -23)NH2 exhibit 12.6%, 1.12% and 0.24% of the potency of hGRF, respectively; these findings indicate the significance of the arginine amide, i.e., -Arg-NH2 residue at position 29 of hGHRH; and c) substituting different amino acids at several sites throughout hGHRH analogs alters the potency of the analogs with respect to hGHRH: U. S. Patent Nos. 4,518,586 (residues 1-3,8,10,15,17,23,25 and 27); 4,528,190 (residues 2,14,27 and 29); and 4,622,312 (residues 1 ,2,12,15 and 27).
With respect to deamidation of the C-terminal carboxamide function, e.g., transformation of hGRF (1-29)NH2 into hGRF (1 -29)0H, which can easily occur by the action of hydrolytic enzymes under physiological conditions or in storage in solution, and which is accompanied with substantial loss of bioactivity. There may be taken into consideration previous observations that the 4-guanidino- butylamino group, the so-called agmatine (Agm) residue, can play the role of the arginine residue in certain tripeptide inhibitors of trypsin-like enzymes (S. Bajusz, et al., in: PEPTIDES, 1982 (K. Blaha and P. Malon, eds.), Walter deGruyter, Berlin- New York, 1983, pp. 643-647 . Only classical (solution) methods have been employed for the preparation of agmatine peptides to date; it is desired to provide methodology for the solid phase synthesis of these peptides using techniques of peptide synthesis which have proven to be suitable for preparing GRFs and their analogs. SUMMARY OF THE INVENTION Synthetic peptides.
The novel synthetic peptides of this invention are extremely potent in stimulating the release of pituitary GH in animals, including humans. These synthetic peptides retain their physiological activity in solution for an extended period of time and are resistant to enzymatic degradation in the body. Without in any way limiting the invention or its scope, Applicants wish to express their understanding that this retention of activity in vitro and resistance to in vivo degradation are due to the omega-guanidino lower alkyl group at the terminal 29- position of the peptide and the presence non-coded amino acids in the enzymic cleavage site(s) of the synthetic peptides.
The synthetic peptides (abbreviated [PeP]) have the sequence: Q1-CO-R2-R3-Ala4-lle6-Pheβ-Thr7-R8-Ser9-R10-Arg11-R12-R13-R1 -R1 B-Gln-R17-R18- Ala19-Arg20-R21-R22-R23-R24-R25-lle-R27-R28-NH-Q2
I. wherein Q1 is 3-(5-hydroxyindolyl)-methyl or an omega or alpha-omega substituted alkyl of the structure: Z
I
(OH) m- [φ] - (CH2) n-C- II
I I
Y where:
[φ] is phenyl;
Y is H, -NH2, CH3CONH- or CH3NH-;
Z is H or CH3; m is 1 or 2; and n is 0, 1 , or 2; R2 is Ala, D-Ala, D-N-Methyl-Ala, Abu or Aib
R3 is Asp, D-Asp, Glu or D-Glu
R8 is Asn, D-Asn, Ser, D-Ser,or Abu
R10 is Tyr, D-Tyr,or 5-HTP
R12 is Lys, D-Lys, Arg or Orn R13 is Val, lie, or Tbg
Figure imgf000006_0001
(CH2)p -NH-C(NH2) = NH III. wherein p is 2 - 6 and the pharmaceutically acceptable addition salts thereof with the pharmaceutically acceptable organic or inorganic bases and organic or inorganic acids. Preferably at least one of R2, R8 or R15 is Abu. (As used herein the symbol -φ- signifies para-substituted phenyl, except when used as -[#]- wherein random, i.e., ortho, meta, para or bis-substitution is signified.)
Synthetic Methods.
The synthetic peptides are synthesized by a suitable method such as by exclusively solid phase techniques, by partial solid-phase techniques, by fragment condensation or by classical solution phase synthesis.
When the analogs of this invention are synthesized by solid-phase method, the C-terminal residue (here, Q2) is appropriately linked (anchored) to an inert solid support (resin). Then, an amino acid bearing protecting groups for its alpha amino group (and, where appropriate, for its amino acid side chain) is coupled in the C- > N direction. After completion of this coupling step, the alpha amino protecting group is removed from this newly added amino acid residue and the next amino acid (suitably protected) is added, and so forth. The N-terminai protecting groups are removed after each residue is added, but the side chain protecting groups, e.g., X2, X3 etc. in formula [PR][PeP] below are not yet removed. After all the desired amino acids have been linked in the proper sequence, the peptide is cleaved from the support and then freed from any side chain protecting group(s) under conditions that are minimally destructive towards residues in the sequence. This must be followed by a careful purification and scrupulous characterization of the synthetic product, so as to ensure that the desired structure is indeed the one obtained.
It is particularly preferred to protect the alpha amino function of the amino acids during the coupling step with an acid or base sensitive protecting group. Such protecting groups should have the properties of being stable in the conditions of peptide linkage formation, while being readily removable without destruction of the growing peptide chain or racemization of any of the chiral centers contained herein. Suitable alpha amino protecting group are Boc and Fmoc.
There are also provided several methods of attaching said omega-guanidino alkyl group to a support phase with improved efficiency and yield , procedures for building up the aforesaid peptide by means of the solid phase syntheses both with BOC and with the very fast Fmoc/BOP strategy and procedures for cleaving said peptide from said support phase with liquid HF and with TF A/scavengers.
Synthetic Intermediates.
Intermediates formed during synthesis of the peptides, attached to the support phase and having protective groups which inhibit reaction by the side chains of certain amino acid residues, also constitute part of the invention.
Medical Applications.
The synthetic peptides of Formula I may be formulated in pharmaceutical dosage form and administered to humans or animals for therapeutic or diagnostic purposes. More particularly, the peptides may be used to promote the growth of warm-blooded animals, as, in humans, to treat human growth deficiency by stimulating in vivo synthesis and/or release of endogenous GH; to treat certain nct'\
SUBSTITUTE SHEET (RULE physiological conditions such as severe growth retardation due to chronic renal insufficiency; to offset certain effects of aging, e.g., reducing loss of muscle and bone loss; to accelerate healing and tissue repair; to improve feed utilization, thereby increasing lean/fat ratio favoring muscle gain at the cost of fat; and also to enhance milk production in lactating cattle. Further, the synthetic peptides may be used in a method to ascertain endogenous physiological ability to produce hGH and a diagnostic kit for carrying out this method.
DESCRIPTION OF THE FIGURE Figure 1 is a graphical representation of selected data from Table 4 in
EXAMPLE XIX herein, wherein "A" represents the peptide of EXAMPLE VIII herein -- i.e., (Dat\Abu16,Nle27,Asp28,Agm29)hGH-RH(1-29) -- and "B" indicates the peptide of EXAMPLE XVI herein -- i.e., (5-Hiaa\Abu15,Nle 7,Asp28,Agm29)hGH- RH(1-29).
DESCRIPTION OF THE PREFERRED EMBODIMENTS A. SYNTHETIC PEPTIDES
1. Nomenclature. The nomenclature used to define the peptides is that specified by the IUPAC-IUB Commissioner on Biochemical Nomenclature (European J. Biochem.. 1984, 138. 9-37). By natural amino acid is meant one of common, naturally occurring amino acids found in proteins comprising Gly, Ala, Val, Leu, lie, Ser, Thr, Lys, Arg, Asp, Asn, Glu, Gin, Cys, Met Phe, Tyr, Pro, Trp and His. Non-native amino acids are abbreviated as follows. By Nle is meant norleucine, by Nva is meant norvaline, by Abu is meant alpha amino butyric acid, by Aib meant alpha iso-butyric acid, by Tba is meant alpha-t-butylalanine, by Tbg is meant alpha-t-butylglycine, by 5-Hiaa is meant 5-Hydroxy-indolylacetic acid, by C-MeTyr is meant 1 -methyl-DL-Tyrosine, by N-MeAla and N-MeTyr are meant N- methyl-alanine and N-methyl-tyrosine respectively. When the amino acid residue has isomeric forms, it is the L-form of the amino acid that is represented unless otherwise expressly indicated. Other abbreviations used are: AcOH acetic acid
AcOEt ethyl acetate
Figure imgf000009_0001
The amino acid sequences of the synthetic peptides are numbered in correspondence with the amino acid residues in hGH-RH(1-29). That is, the Ala4 and R8 of the Formula I peptide occupy the same position in the sequence as the Ala4 and R8 residues in hGH-RH(1-29).
The convention under which the N-terminal of a peptide is placed to the left, and the C-terminal to the right is also followed herein. Strictly speaking however, the synthetic peptides of Formula I have neither an N nor a C terminal since the Q1 or Q2 moieties, at what would otherwise be the N and C termini,
UBSTITUTE SHEET (RULE 26) lack an N- and a C- terminus respectively, in order to remove any question therefore, it should be understood that the terms N- and C-terminal used with respect to the synthetic peptides of Formula I mean Q1 and Q2.
2. Preferred Embodiments.
The preferred synthetic peptides of the present invention have the sequence:
Q'-CO-R^R^AIa^lle^Phe^Thr^R^Ser^Tyr^-Arg^-Lys^-R^-Leu^-R^-Gln^-Leu17- Ser18-Ala19-Arg20-Lys21-Leu 2-Leu23-Gln24-R25-lle-R27-R28-NH-Q2 I. wherein
Figure imgf000010_0001
R2, R3, R8, R15, R27, R28, and Q2 are as defined above and at least one of R2, R8 or R1B is ABu.
Depending on the identity of the functional groups in
Figure imgf000010_0002
the Q1-CO moieties may when taken together form an amino acid residue: thus, when in Q1 m is 1 , n is 1 and y is NH2, Q'-CO forms tyrosyl ("Tyr-"). Even when the Q1 functional groups do not cause Q1 to form an amino acid with CO-, the two constituents of the Formula I peptide may together form a readily recognized group. Thus, when in
Figure imgf000010_0003
m is 1 , n is 1 and Y and Z are H, Q'-CO together form 3-(4-hydroxyphenyl)propionyl, known as des-amino-Tyr (or "Dat"). Alternatively, 3-(5-hydroxyindolyl)methyl as Q1 with CO forms a 3-(5-hydroxy- indolyDacetyl moiety (or "5-Hiaa"). Thus, for convenience's sake, the Q1-CO moieties may be taken as a unitary moiety R1 and replaced in the Formula I peptides by abbreviations such as Tyr\ Dat1, 5-Hiaa1, etc. as appropriate.
Similarly at the N-terminal of the Formula I peptides, the NH-Q2 moieties may be taken as a unitary moiety R29 when together they form a single recognized functional group. Thus, when in Q2, p is 4, the combination of NH and Q2 forms -NH-(CH2)4-NH-C(NH2) =NH, or an agmatine ("Agm") residue.
The use of these abbreviations in Formula I peptides is optional. Thus in an especially preferred peptide, this format is not used. This peptide has the structure: Q1-CO-Ala2-Asp3-Ala4-lle6-Pheβ-Thr7-R8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14-R16-Gln16- Leu17-Ser18- Ala19-Arg 0-Lys21-Leu22-Leu23-Gln2 -Asp2B-lle-R27-R28-NH-O2 wherein
R8 is Asn, Ser or Abu R15 is Abu,Ala or Gly R27 is Met.Tba or NIe and R28 is Ser or Asp;
Especially preferred embodiments include peptides of Formula I in which Q1- CO is Dat, Ac-Tyr, N-Me-Tyr, C-Me-Tyr and Hiaa; and NH-Q2 is Agm. Further preferred embodiments include peptides of Formula I in which Q'-CO is Dat or Hiaa; R15 is Abu; R27 is NIe; R28 is Asp; and NH-Q2 form Agm.
In one very preferred analog, in
Figure imgf000011_0001
m is 1 , n is 1 and Y and Z are H, so that Q1-CO is Dat; R2 is Ala, R8 is Asn, R15 is Abu, R27 is NIe, R28 is Asp; and in Q2, p is 4. The full formula of this analog is:
3-(4-hydroxyphenyl)propionyl1-Ala2-Asp3-Ala -lle6-Pheβ-Thr7-Asn8-Ser9-Tyr10-Arg11- Lys12-Val13-Leu14-Abu16-Gln-Leu17-Ser18-Ala18-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25- lle-Nle27-Asp28-NH-(CH2)4-NH-C(NH2) = NH. This analog may be expressed under a well known convention as follows:
3-(4-hydroxyphenyl)propionyl1-Abu15-Nle27-Asp28-4-guanidino-butylamide hGHRH29(1-29). This is the analog described in Example VIII below; it may be further abbreviated as (Dat1, Abu15, NIe27, Asp28, Agm28)hGHRH (1-29)
Similarly, where Q^CO is Dat, R2 is Ala, R8 is Abu, R1B is Gly, R27 is NIe,
R28 is Ser and in Q2 p is 4, the peptide may be written as: (Dat1, Abu8, NIe27, Agm29)hGHRH (1-29) described in Example XIII.
In another preferred embodiment where Q1 is 3-(5-hydroxyindolyl)-methyl, R2 is Ala, R1B is Abu, R27 is NIe, R28 is Asp and in Q2 p is 4, the peptide may be written: (5-Hiaa1, Abu15, NIe27, Asp28, Agm29)hGHRH (1-29) described in Example XVI. B. SYNTHETIC METHODS
1 . Overview of Synthesis.
The peptides are synthesized by a suitable method such as by exclusively solid phase techniques, by partial solid-phase techniques, by fragment condensation or by classical solution phase synthesis. For example, the techniques of exclusively solid-phase synthesis are set forth in the textbook "Solid Phase Peptide Synthesis", J.M. Stewart and J.D. Young, Pierce Chem. Company, Rockford, 1 1 1. ,1984 (2nd. ed.), G. Barany and R.B. Merrifield, "The Peptides", Ch. 1 , 1-285, pp. 1979, Academic Press, Inc., and M. Bodanszky, "Principles of Peptide Synthesis", SpringerVerlag, 1984. The synthetic peptides of Formula I are preferably prepared using solid phase synthesis, such as that generally described by Merrifield, J.Am.Chem.Soc, 85, p. 2149 (1963), although other equivalent chemical syntheses known in the art can also be used as previously mentioned.
In solid phase synthesis, the moiety which forms the C or N-terminal group of the resulting peptide is joined to a polymeric resin support phase via a chemical link. Amino acid residues or oligopeptide fragments are then added sequentially to the alpha amino functional group of the C or N-terminal moiety until the desired peptide sequence is obtained. Because the amino acid residues or oligopeptide fragments are added to the C-terminal Q2 group here, growth of the synthetic peptides of Formula I begins at the C terminal and progresses toward the N- terminal. When the desired sequence has been obtained, it is removed from the support phase.
When reactive side chain functional groups of the various amino acid moieties or peptide fragments that bear them, suitable protecting groups prevent a chemical reaction from occurring at said side chains until the protecting group is ultimately removed. Accordingly, it is common that, as a step in synthesis, an intermediate compound is produced which includes each of the amino acid residues located in its desired sequence in the peptide chain with side-chain protecting groups linked to the appropriate residues. The initial synthetic sequence utilized herein is disclosed in US Patent 4 914 189 which is incorporated by reference herein. Reference is particularly made to Examples I through VII therein.
2. Joining NH7-Q2 to the Support Phase.
The peptides of Formula I may be synthesized on a variety of support phases. These support phases may be amino or hydroxy resins such as amino- methyl resins (suitably 1 % cross linked), benzhydrylamine resins (suitably 2% cross linked) p-methylbenzhydrylamine resins (suitably 2% cross linked) and the like. It is generally preferred that the support phase [SP] is an amino type resin of the formula: H2N-CH2-ø-[Pm] IX where [Pm] is a polymeric substrate.
The initial material joined to the support phase is suitably the C-terminal Q2 group. Preferably, the adjacent NH functional group is already affixed to Q2. Agm or 4-guanidino butylamine are especially preferred.
The NH-Q2 group is joined to the support phase via a stable but readily cieavable bridging group. It has been found that such a bridge may be readily provided by a sulfonyl phenoxy acetyl moiety. Thus, Boc-NH-Q2-S02-ø-(M,)O-CH2-CO-[SP] or
Fmoc-NH-Q2-S02-[ø]-(Mβ)O-CH2-CO-[SP] constitute the material joined to the support phase for the synthetic sequence. They are prepared and linked to the support phase as follows.
2(a). Preparing Boc-NH-Q -SOr,-ά>-(M11)O-CH3-CO-rSP1.
The primary amino group of agmatine (i.e., the -NH- group preceding Q2) is protected with a tert-butyloxy carbonylating agent, suitably ditert-butyl dicarbonate, by reaction. This reaction may take place preferably at ambient temperatures or at 5-10°C in the presence of a base. The protected material is then reacted in a similar solvent system with the arylsulfonyl halide
Hal-S02-ø-O-CH2-COOH wherein Hal is chloro or bromo to form
Boc-NH-Q2-S02-ø-0-CH2-COOH. The protected aminoalkyl guanidino-sulfonyl phenoxyacetic acid is then coupled to the support phase [SP] by the action of a diloweralkyl carbodiimide or BOP on:
H2N-CH2-ø-[Pm] to yield:
Boc-NH-Q2-S02-ø-0-CH2-CO-[SP] which represents Q2 linked to the polymeric substrate support phase via the sulfonyl phenoxy acetyl moiety, more fully expressed as:
Boc-NH-Q2-SO2-ø-O-CH2-CO-NH-CH2-ø-[Pm]
In the preferred procedure, the coupling is carried out using any of the known dialkyl carbodiimide coupling procedures. For example, there may be utilized diisopropyl-carbodiimide in the presence of 1-hydroxybenzotriazole hydrate in dimethylformamide at ambient temperatures. Alternatively, there may be employed N,N'dicyclohexyl-carbodiimide. In this procedure, the aforesaid Boc- aminoalkyl guanidino-sulfonyl-phenoxyaceticacid is mixed with the carbodiimide in 2 to 1 molar ratio, the formed N,N'dicyclohexyl urea is removed by filtration and the resulting solution is added to the support phase.
When BOP is used as the carboxyl activating agent, the protected amino¬ alkyl guanidinosulfonyl phenoxyacetic acid is mixed with equimolar BOP and dissolved in DMF containing twice molar NMM in 10% concentration. The activation can be enhanced in the presence of 1-3 molar excess of HOBt yielding an efficient coupling rate to the solid support preferably to an aminomethyl resin at room temperature.
Where the ultimate synthetic sequence is intended to follow the Boc protocol, the aromatic ring of the arylsulfonyl halide is not substituted since such a situation will permit the use of trifluoroacetic acid as the intermediate deprotecting agent and hydrogen fluoride as the agent for final cleavage from the resin. 2(b). Preparing Fmoc-NH-Q2-SO7-f(&1(Mr)-O-CH,-CO-fSPl.
In place of utilizing Boc to protect the aminoalkyi guanidino moiety, N- benzyloxycarbonyl chloride is used in the presence of an aqueous alkali, suitably sodium hydroxide, preferably at about 4N under agitation and cooling to between 1 and 5°C. Upon sodium hydrogen carbonate treatment, the protected product is precipitated and thereafter is reacted with an aryl-sulfonyl chloride as previously.
More particularly, the Fmoc procedure comprises the sequential steps of reacting N-benzyloxy carbonyl chloride with NH2-Q2 in the presence of a base to form Cbz-NH-Q2, reacting said Cbz-NH-Q2 with a substituted arylsulphonyl halide in the presence of a strong aqueous base and removing the Cbz group by catalytic hydrogenation. The substituted arylsulphonyl halide has the formula:
Hal-S02-[ø](M.)-O-CH2-COOH wherein Hal is chloro or bromo; M, is lower alkyl or lower alkoxy of 1 to 5 carbon atoms located at the positions of the phenyl nucleus other than 1 and 4; and s is 1-3. The reaction yields H2N-Q -S02-[ø](M,)-O-CH2-COOH.
After removal of the Cbz group, the product is reacted with Fmoc-CI in the presence of a base to yield the corresponding Fmoc protected aminoalkyi guanidino-sulfonyl aryloxy acetic acid, i.e.
Fmoc-NH-Q2-S02-[ø](M„)-O-CH2-COOH. This product is then coupled to said support phase [SP] to yield: Fmoc-NH-Q2-SO2-[ø](M,)-O-CH2-CO-[SP], which may be expressed in more detailed fashion:
Fmoc-NH-Q2-SO2-[ø](M,)-O-CH2-CO-CH2-ø-[Pm].
As noted above, the arylsulfonyl halide should preferably carry between 1 and 3 M substituents which may be alkyl or lower alkoxy, suitably methyl or methoxy. This is in contrast to the Boc procedure: here, it is desirable to substitute the phenyl moiety with up to three alkyl or alkoxy groups. These groups weaken the strength of sulfonamide bridge and enable it to be cleaved by trifluoroacetic acid, once all the amino acid residues have been added and one wishes to remove the intermediate from the support phase. This reaction is carried out in the presence of a strong but dilute aqueous base, suitably about 1 N sodium hydroxide. The reaction mixture is acidified and the product extracted, suitably with a water immiscible organic solvent such as ethyl acetate. The extract is then concentrated and hydrogenated, suitably at atmospheric pressure and room temperature in the presence of a catalyst such as palladium on charcoal in a reduction inert solvent. If ethyl acetate is used as the extractant, this may be used as the hydrogenation solvent.
3. Steowise Addition of Amino Acid Residues.
Utilizing the aforementioned Boc- or Fmoc-protected amino-alkyl-guanidino sulfophenoxyacetyl as the anchored C-terminal, the peptide itself may then suitably be built up by solid phase synthesis in the conventional manner. Thus, the alpha amino-protecting group of the next amino acid residue is protected by Boc or Fmoc to prevent reaction between the N-terminal of R28 while this is being reacted with NH2-Q2. These are attached to the NH2-Agm or H2N-Q2-SO2-[ø](M,)- O-CH2-COOH respectively, as described above. The amino acid residues of the synthetic peptides are added sequentially . Because the peptide is constructed from the C-terminal, the residues are added in reverse numerical order, i.e., R28, R27, and so forth.
The protected amino acids are coupled sequentially, with Q1 finally being added. As an alternative to adding each amino acid separately in the synthesis, some may be coupled to one another in a separate vessel and added as an oligo- peptide in the solid phase reaction. The selection of an appropriate coupling reagent is within the skill of the art. Particularly suitable as coupling reagents are N,N'-diisopropyl carbodiimide (DIC) or the BOP carboxyl activating reagent.
Each protected amino acid or amino acid sequence is introduced into the solid phase reaction in about a three-fold molar excess, with respect to NH2-Q2, etc., and the coupling may be carried out in as medium such as DMF: CH2CI2
(1 :1 ) or in DMF or CH2CI2 alone. In cases where incomplete coupling occurs, the coupling procedure is repeated before removal of the alpha amino protecting group prior to the coupling of the next amino acid. The success of the coupling reaction at each stage of the synthesis is preferably monitored by the ninhydrin reaction.
4. Removal of Complete Intermediate from the Support Phase.
When the synthesis is complete, the Q2 guanidino alkyl end of the Formula I peptide is cleaved from the support phase at the sulfonyl group. If the Boc protocol is utilized, then the cleaving agent is anhydrous hydrofluoric acid; whereas, in the Fmoc protocol the cleaving agent is trifluoroacetic acid.
Removal of the intermediate peptide from the resin support is performed by treatment with a reagent such as liquid hydrogen fluoride or trifluoroacetic acid. This also cleaves all remaining side chain protecting groups X3, X7, X11, X12 and and the anchoring guanidinosulfo bond, if present, and also the alpha amino or alpha-hydroxyl protecting group X1. These groups have different values depending on whether Boc or Fmoc protocols are used.
C. SYNTHETIC INTERMEDIATES
1. Side Chain Protecting Groups. The protection of reactive side chain functional groups of the various amino acid moieties or peptide fragments is common to solid phase synthesis. These side chain functional groups are protected in order to prevent an undesirable chemical reaction from occurring at said chains. Accordingly, it is common that, as a step in the synthesis, an intermediate compound is produced which includes each of the amino acid residues located in its desired sequence in the peptide chain with side-chain protecting groups (e.g., X1, X7, etc.) linked to the appropriate residues.
The selection of a side chain amino protecting group is not critical except that generally one is chosen which is not removed during deprotection of the alpha amino groups during the synthesis. In selecting a particular side chain protecting group to be used in the synthesis of the peptides, the following general rules are followed: (a) the protecting group preferably retains its protecting properties and is not split off under coupling conditions, (b) the protecting group should be stable to the reagent, is preferably stable under the coupling reaction conditions selected for removing the alpha amino protecting group at each step of the synthesis and, (c) the side chain protecting group must be removable upon the completion of the synthesis of the desired amino acid sequence, under reaction conditions that will not undesirably alter the peptide chain.
The side chain protecting groups are attached to the amino acid residues by steps well known in the art.
2. Synthetic Intermediates. Also considered to be within the scope of the present invention are intermediates of the formula: [PR] [PeP] attached to a support phase [SP] selected from the group consisting of amino type resins, said combination having the structure:
[PR] [PeP]-SO2-[ø](M.)-O-CH2-CO-SP where M is hydrogen, lower alkyl or lower alkoxy of 1 to 5 carbon atoms, suitably methyl or methoxy, s is 1-3, [SP] is an amino type resin. Suitably [PR][PeP] has the structure:
X1-Q1-CO-R2-Asp3(X3)-Ala -lleB-Pheβ-Thr7(X7)-R8(X7 or Nil)-Ser9(X7)-Tyr10(X10)-
Arg11 (X11)-Lys12(X12)-Val13-Leu14-R1B-Gln-Leu17-Ser18(X7)-Ala19-Arg20(X11)- Lys21(X12)-Leu22-Leu23-Gln24(H or X24 )-Asp2B(X3)-lle-R 7-R28(X3 or X7)-NH-Q2 wherein
X1 is either hydroxyl, or an amino protecting group or nil, depending on the meaning of Y in Formula II (the formula for one of the Q1 moieties).
X3 is a suitable ester-forming protecting group for the carboxyl group of Asp or Glu. In the Boc protocol, it may form cyclohexyl esters; in the Fmoc protocol tert- butyl esters are preferred.
X7 is a suitable protecting group for the hydroxyl group of Thr or Ser, such as tert-butyl, Bzl. The preferred protecting group in the Boc protocol is Bzl and in the Fmoc protocol it is tert-butyl.
X10 is a suitable protecting group for the phenolic hydroxyl group of Tyr or N- MeTyr, such as tert-butyl, Bzl, 4Br-Cbz and 2,6-dichlorobenzyl (DCB). The preferred protecting group in the Boc protocol is 2,6-dichlorobenzyl and in the Fmoc protocol it is tert-butyl.
X11 is a suitable protecting group for the guanidino group of Arg, such as nitro, Tos, Pmc, Mtr; in the Boc protocol Tos is the preferred group and 2,2,5,7,8- pentamethyl chroman-6-sulfonyl in the Fmoc protocol. X12 is a suitable protecting group for the side chain amino group of Lys. Illustrative of suitable side chain amino protecting groups are 2-chloro- benzyloxycarbonyl (2-CI-CBz) and tert-butyloxycarbonyl (Boc). In the Boc protocol, 2-chlorobenzyloxycarbonyl is the preferred protecting group and in the Fmoc protocol Boc is thus utilized. X24 is hydrogen or a protecting group for the imidazole nitrogen of His, such as Tos in the Boc or Trt in the Fmoc protocol.
MEDICAL APPLICATIONS
The products of the present invention may be utilized to promote the growth of warm-blooded animals (e.g., humans) and also enhance the milk production of females of milk producing mammals, suitably but not exclusively goats and cows, preferably cows.
The peptides of the invention may be administered in the form of pharmaceutically acceptable, nontoxic salts, such as acid addition salts. illustrative of such acid addition salts are hydrochloride, hydrobromide, sulphate, phosphate, fumarate, gluconate, tannate, maleate, acetate, citrate, benzoate, succinate, alginate, pamoate, malate, ascorbate, tartrate, and the like.
The compounds of the present invention are suitably administered to the subject humans or animals s.c, i.m., or i.v; intranasally or by pulmonary inhalation; or in a depot form (e.g., microcapsules, microgranules, or cylindrical rod like implants) formulated from a biodegradable suitable polymer (such as D,L- lactide-co-glycolide), the former two depot modes being preferred. Other equivalent modes of administration are also within the scope of this invention, i.e., continuous drip, depot injections, infusion pump and time release modes such as microcapsules and the like. Administration is in any physiologically acceptable injectable carrier, physiological saline being acceptable, though other carriers known to the art may also be used.
The dosage level should be between 0.2 and 2 micrograms/kg body weight per injection except for depot form where the amount injected would be calculated to last from about 15 to about 30 days or longer. These dosage ranges are merely preferred. Administration of non-depot forms may be between 1 and
4 times per day. It is convenient to inject the animal whenever it is milked.
Until the production of growth hormone by recombinant-DNA methods began, the small supply of pituitary-derived human growth hormone limited its use to the treatment of children with growth hormone deficiency. The wide availability of synthetic human growth hormone has made possible long-term studies of other potentially beneficial uses of growth hormone and its more physiologic actions. Although synthetic GH is currently approved in USA only for treatment of growth failure due to lack of endogenous growth hormone, this therapy has also been used to treat short children not classically GH deficient. However the cost of long-term treatment with hGH and the need of daily sc administration are important considerations. Currently, the cost of growth hormone therapy for a child with growth deficiency ranges from $10,000 to 30,000 a year depending on body weight. Treatment of a 70-kg adult with hGH three times a week costs $13,800 a year. Vance, M.L., N.Eng.J.Med. 323: 52-54 (1990). Thus, long- term growth hormone treatment in elderly adults with diminished growth hormone secretion would require a considerable personal and financial investment. In addition there are many children all over the world with growth retardation due to the lack of GH who cannot be treated with hGH because of the cost of this therapy. Consequently there is an urgent need to develop a drug that releases GH and with an affordable price. This alternative method to increase endogenous growth hormone secretion is through the administration of agonistic analogs of growth hormone-releasing hormone. The therapy with GHRH agonistic analogs
BST1TUTE SHEET (RULE 26) should be much less expensive than that utilizing hGH. In addition, the development of long-acting delivery systems for these analogs can make this new modality of treatment more practical and convenient.
The ability to produce synthetic growth hormone (GH) by recombinant DNA technology has enabled the manufacture of GH in GH in potentially unlimited quantities. This greatly facilitated the treatment of GH-deficient children. As stated above, synthetic hGH is currently approved only for the treatment of growth failure due to a lack of adequate endogenous growth hormone, but hGH has also been used to treat short children who are not classically GH-deficient such as girls with Turner's syndrome; prepubertal children with chronic renal insufficiency and severe growth retardation; and children with non-GH deficient short stature.
Of the 3 million children born in the USA annually, 90,000 will below the third percentile for height. These children may be labeled as having short stature and may be candidates for GH treatment. Therapy with human growth hormone currently costs about $ 20,000 per year and the average length of treatment is about 10 years. The treatment will usually be stopped when the patient reaches an acceptable adult size (a height of well over five feet) or when the patient matures sexually and the epiphγses close, at which time linear growth ceases, or if the patient fails to respond to the treatment. If all children who are less than the third percentile for height receive a five year course of hGH therapy, hGH for height augmentation therapy will cost at least $8 billion to 10 billion per year. (Lantos J. et al., JAMA 261 :1020:1024, 1989).
It is desirable to ascertain the endogenous physiological ability of children having short stature to produce hGH. This may be done with a diagnostic test based on a 50-100 microgram dose of GH-RH; a 50-100 microgram dose of a GH- RH analog of Formula I; and means for assaying the GH response evoked by each dose. The assay means may be any conventional means which will indicate the quantitative amount of hGH present in a blood sample drawn from the patient.
Usually, the concentration of GH in serum is determined using standard radioimmunoassay ("RIA") procedures, e.g., Miles I.E.M. et al., Lancet n:492-493 (1968) or Odell W. et al. J.Lab.Clin.Med., 70:973-80 (1967).
The diagnostic test is performed as follows. First, the GH-RH dose is administered. Thirty minutes later, a blood sample is taken for RIA of GH.
Various commercially available kits (e.g., Nichols Institute of Diagnostics, San Juan Capistrano, CA) or reference preparations of hGH (e.g., NIAMDD-hGH-RP-1 ) can be used for this RIA.
After waiting 6-24 hours for the effect of GH-RH to wear off, the dose of GH-RH analog is administered. Blood again is drawn again for radioimmunoassay of GH.
The presence of a normal hGH response in the first assay reveals that endogenous hGH producing ability is present. This result also suggests a short, mild course of GH-RH therapy, if any, may be suitable. A low GH response, or no response, to the first dose reveals only that GH-RH must be evaluated in view of the second test result. If a good hGH response follows the second dose, there is clear physiological hGH producing ability which is not evoked by GH-RH. This indicates that a therapy with the GH-RH analog may be desirable. Finally, no or low response to both tests reliably reveals lack of physiological ability to produce hGH, and so suggests therapy with hGH is probably needed.
A diagnostic kit for testing endogenous physiological ability to produce GH may incorporate a 50-100 microgram dose of GH-RH; a 50-100 microgram dose of a GH-RH analog peptide of Formula I; and means for assaying the GH response evoked by each dose.
As indicated above, short stature in children may result from many causes, none of which are immediately apparent. Use of the diagnostic test on all children with this condition would greatly clarify the cause of short stature. Such a widespread screening test would also provide earlier indications for desirable treatment.
Thus, the invention further includes a method for ascertaining the endogenous physiological ability to produce hGH and a diagnostic kit for carrying out this method.
Glucocorticoids are potent inhibitors of linear growth in man and growth suppression is a well known risk of long term treatment of asthmatic children with steroids. Thus stunted growth is an important consequence of chronic administration of glucocorticoids in childhood. The inhibition of GH secretion is due in some extent to the fact that chronic administration of glucocorticoids suppresses GHRH. This inhibition occurs at the level of the hypothalamus or above and in this situation only the treatment with GHRH agonists will stimulate linear growth.
Growth hormone tends to decline with the aging process and may lead to decrease in muscle mass and adiposity. Studies have shown that healthy older men and women with growth hormone deficiency had increases lean body mass and decreases in the mass of adipose tissue after six months of hGH administration. Other effects of long-term administration of hGH on body composition included increase in vertebral-bone density and increase in skin-fold thickness. In addition, it has been reported that daily GHRH injection to menopausal women, for 8 days augments GH responses and IGF-I levels and raises serum osteocalcin levels. Thus the therapy with GHRH agonistic analogs reduces the loss of muscle, bone and skin mass and lessen the increase of body fat that normally accompanies the aging process.
Growth hormone is a potent anabolic hormone that enhances protein synthesis and nitrogen retention and chronic administration of agonistic analogs of GHRH increase the endogenous growth hormone secretion. The therapy with GHRH agonistic analogs has uses in other areas of medicine such as catabolic states causing accelerated weight loss; tissue repair in patients with sever body surface burn, in accelerating healing of nonunion fractures and in some cases of cardiac failure.
Although long term follow-up is necessary before all treatment responses can be ascribed to GH, there has been improvement in cardiac mass and an increase in both cardiac mass and contractility. The therapy with hGH interrupts the cardiac-cachexia cycle. This response is in keeping with other observations that the therapy with GH has a major role in catabolic states in adults. An alternative method to increase endogenous growth hormone secretion in these conditions is the administration of GHRH agonistic analogs.
These agonistic analogs of GH-RH can replace hGH for many applications. GH-deficient children respond to GH-RH(1-40), GH-RH(1-29) or GH-RH(1-44), with an increase in growth. Thorner M.O. et al., N.Engl.J.Med. 312:4-9, 1985; Ross R.J.M. et al., Lancet 1 :5-8, 1987; Takano K, et al., Endocrinol. Japan 35:775-781 , 1988. Most children who respond to hGH, will respond to GH-RH. This is because most GH-deficient children have a hypothalamic defect in GH release, and will show a GH response after the administration of analogues of the hypothalamic hormone GH-RH. Thus repeated administration of GH-RH promotes linear growth. GH-RH(1-29)NH2 given subcutaneously twice a day promoted linear growth in approximately 50% of a group of GH-deficient children (Ross et al, cited above). A small group of severely GH-deficient children will respond to GH-RH after 6(six) months of treatment.
FURTHER CLINICAL APPLICATIONS OF AGONISTIC ANALOGUES OF GHRH IN CHILDREN WITH GROWTH RETARDATION:
1. As a screening test for growth hormone deficiency 2. Treatment of Hypothalamic GHRH deficiency
3. Constitutional growth delay
4. Turner Syndrome
5. Familial short stature 6. Prepubertal children with chronic renal insufficiency and severe growth retardation
7. Infants and children with intrauterine growth retardation
8. Children with GH deficiency following radiotherapy for pituitary or hypothalamic lesions
9. Children on long-term treatment with glucocorticoids and growing at subnormal rate
FURTHER CLINICAL APPLICATIONS OF AGONISTIC ANALOGUES OF GHRH IN ADULTS:
1. Geriatric Patients: To reduce the loss of muscle, bone and skin mass and lessen the increase of body fat that normally accompanies the aging process. 2. Catabolic states
3. Wound healing
4. Delayed healing of fractures
5. Osteoporosis
6. Obesity 7. As an adjunct to total parenteral nutrition in malnourished patients with chronic obstructive pulmonary disease
8. Cardiac failure
9. GHRH agonists could be used during and after space flights to counteract the decrease in GH secretion. Weightlessness of space flight significantly decreases the release of growth hormone. This finding could explain the bone loss and muscle weakness many astronauts experience after prolonged space flights. The following Examples set forth suitable methods of synthesizing by the solid-phase technique, several fragments and novel analogs of hGH-RH which have improved potency. EXAMPLE I
Synthesis of Boc-aqmatine
EXAMPLE II
Synthesis of 4-Chlorosulfonyl Phenoxyacetic Acid (CI-SPA) EXAMPLE III
Boc-aqmatine-fSPAI
EXAMPLE IV
Coupling of Boc-aomatine-fSPAI to Support Phase
EXAMPLE V Synthesis of Cbz-aqmatine
EXAMPLE VI
Synthesis of Aomatine-Sulfonyl- 2.3.5 (and 2.3.6)-Trimethylphenoxy Acetic Acids
EXAMPLE VII Preparing of Fmoc-Agmatine-Sulfonyl-2.3.5 (and 2.3.6)-Trimethylphenoxy
Acetic Acid and coupling to support phase
The initial synthetic sequence utilized herein and indicated by headings above is disclosed in Examples I through VII of US Patent 4 914 189 and are incorporated by reference herein.
EXAMPLE VIII
(Dat1.Abu1B.NIe 7.Asp28.Aom29)hGH-RH(1 -29) The synthesis of an hGHRH analog of the formula: 3-(4-hydroxyphenyl)propionyl1-Ala2-Asp3-Ala4-lleB-Pheβ-Thr7-Asn8-Ser9-Tyr 0-Arg11- Lys12-Val13-Leu14-Abu16-Gln-Leu17-Ser 8-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25- lle-Nle27-Asp28-NH-(CH2)4-NH-C(NH2) = NH was carried out in a stepwise manner on a PS-2755 (Protein Technologies) synthesizer starting with the appropriate Boc-NH-(CH2)4-NH-C(NH2) = N-SO2-ø- OCH2-CO-[SP] in accordance with the procedures set forth below in Schedule A.
Deblocking and neutralization are preferably carried out in accordance with Schedule A as follows: SCHEDULE A Deprotection
Step Reagent Mixing (min)
1. Deprotect: 100% TFA 1 +4
2. DMF wash 1 3. Neutralization: 5% DIEA in DMF 2
4. DMF wash 1
5. Neutralization: 5% DIEA in DMF 2
6. DMF wash (3 X) 1
The couplings are preferably carried out as set out in Schedule A for coupling:
SCHEDULE A Coupling
Step Reagent Mixing (min)
1. Coupling Boc-amino acid (3 eq) in DMF (or preformed HOBt ester of Boc protected 20 ( + 20) amino acid) plus DIC (3eq)
2. DCM wash 1
3. Ac2O(30%) in DMF 10 + 20 4. DMF wash (3 X) 1
Briefly, BOC is used for the alpha amino protection. Benzyl ether is used as the hydroxyl side chain protecting group for Ser and Thr. The phenolic hydroxyl group of Tyr is protected with DCB and the side chain carboxyl group of Asp is protected in the form of the cyclohexyl ester. Tos is used to protect the guanidino group of Arg and 2-CI-Cbz is used as the protecting group for the Lys side-chain. Due to the decreased reaction rate of the 3-(4-hydroxyphenyl)propionic acid N- hydroxy-succinimide ester, a prolonged coupling time 60 minutes was used.
The following compound is obtained:
3-(4-hydroxyphenyl)propionyl1-Ala2-Asp3(X3)-Ala4-lle5-Pheβ-Thr7(X7)-Asn8-Ser9(X7)-- Tyr10-(X10)-Arg11(X11)-Lys12(X12)-Val13-Leu14-Abu1 B-Gln-Leu17-Ser18(X7)-Ala19- Arg20(X11)-Lys21(X12)-Leu2 -Leu23-Gln2 -Asp25(X3)-lle-Nle27-Asp28(X3)-NH-(CH2)4- NH-C(NH2) = N-SO2-ø-OCH2-CO-[SP] wherein X3 is O-cyclohexyl ester, X7 is O-benzyl ether, X10 is O-2,6-DiCI-Bzl ether,
X11 is tosyl, X12 is 2-CI-Cbz.
In order to cleave and deprotect the protected peptide-resin, it is treated with 1 ml m-cresol and 10 ml hydrogen fluoride (HF) per gram of peptide resin, at 0°C for 45 min. After elimination of the HF under high vacuum and evaporating the traces of the scavenger, the cleaved peptide and resin remainder is washed with dry diethyl ether and ethyl acetate. The peptide is then extracted with 50% aqueous acetic acid, separated from the resin by filtration and lyophilized.
Depending on the amount gained, the crude peptide is purified using either a Beckman Prep-350 preparative HPLC system (with a Beckman Type 163 variable wavelength UV detector) or a Beckman semipreparative HPLC system (with a Beckman 420 Gradient Controller, two 114M Solvent Delivery Modules, a 165 Variable Wavelength Detector and a Kipp and Zonen BD41 Recorder. In the preparative system, separations are achieved on a 41.5 x 150 mm. DYNAMAX column packed with spherical C18 silica gel (300 A pore size, 12 um Particle size) (RAININ Inc., Co., Woburn, MA). In the semipreparative system, purification can be performed on a VYDAC C18 reversed phase column (10 x 250 mm., 300 A pore size, 5 um particle size).
Gradient elution is used. Solvent A consists of 0.1 % aqueous TFA and solvent B is 0.1 % TFA in 70% aqueous acetonitrile. The column eluate is monitored at 220 nm and 280 nm.
The peptide is judged to be substantially (95%) pure by using a Hewlett- Packard HP-1090 liquid chromatograph. The peptides are chromatographed on a 4.6 x 250 mm. W-Porex 5 um C18 column (Phenomenex, Rancho Palos Verdes, CA) at a flow rate of 1.2 ml/min. with a mixture of Solvent A and Solvent B using a gradient (from 40 to 70% B in 30 min). EXAMPLE IX
(Ac-Tyr1.Abu8.NIe 7.Aom 9)hGH-RHM-29)
The synthesis of an hGHRH analog of the formula: Ac-Tyr1-Ala2-Asp3-Ala4-lle5-Pheβ-Thr7-Abu8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu 4-Gly15- Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25-lle-Nle 7-Ser 8-NH- (CH2)4-NH-C(NH2) = NH was carried out in a stepwise manner on a PS-2755 (Protein Technologies ) synthesizer starting with the appropriate Fmoc-NH-(CH2)4-C(NH2) = N-SO2- (2,3,5)-trimethyl-[ø]-OCH2-CO-[SP] (i.e., Fmoc-agmatine-sulfonyl-2,3,5,- trimethylphenoxy-acetic acid amino-methyl resin). Deblocking and washing are preferably carried out in accordance with modified Schedule A as follows:
SCHEDULE B FOR FMOC SYNTHESIS DEPROTECTION Step Reaoent Mixing (min)
1. 20%(v/v)piperidin 2x5 in DMF
2. washing with DMF 6x1
SCHEDULE B FOR FMOC SYNTHESIS
COUPLING
1. washing with DMF 3x0.5
2. coupling with 3eq amino acid + 3eq BOP in DMF 20 ( + 10) containing 6 eq NMM +
0-6eq HOBt. repeated coupling: 1 eq
3. washing with DMF 6x1
The following compound is thus obtained:
Ac-Tyr1(X1)-Ala2-Asp3(X3)-Ala -lleB-Pheθ-Thr7(X1 )-Abu8-Ser9(X1 )-Tyr10(X1 )- Arg11(X11)-Lys12(X12)-Val13-Leu 4-Gly15-Gln-Leu17-Ser18(X1)-Ala19-Arg20(X11)- Lys21 (X1 )-Leu22-Leu 3-lle-Nle27-Ser 8(X1 )-NH-(CH2)4-NH-C-(NH2) = N-SO2- TnUTESHEET (RULE 26) 2,3,5,trimethyl[ø]-OCH2-CO-[SP]
X1 is t-butyl ether, X3 is t-butyl ester, X11 is 2,2,5, 7,8-pentamethyl-chroman-6- sulphonyl, X12 is Boc.
The protected peptide produced as above is utilized as starting material.
The cleavage of the peptide from the solid support and the removal of side chain protecting groups was carried out simultaneously by the reaction of the protected peptide resin with a mixture of TFA(90%)-thioanisol(5%)-ethandithiol (2.5%)- water(2.5%) at a temperature 35-40°C for 2-3 hours (10 ml liquid per each gram of resin was used). After completion of the reaction, the reagent was removed on centrifugation in high vacuo at room temperature. The remaining material was washed with ether. The peptide is then extracted with 50% aqueous acetic acid, separated from the resin by filtration and lyophilized. After lyophilization the crude peptide was subjected to purification as described in Example VIII.
EXAMPLE X
Dat1. Ser8. Abu15.NIe27.Aom29hGH-RH( 1-29) The synthesis of an hGHRH analog of the formula: 3-(4-hydroxyphenyl)propionyl1-Ala2-Asp3-Ala4-lleB-Pheβ-Thr7-Ser8-Ser9-Tyr10-Arg11- Lys12-Val13-Leu1 -Abu15-Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln -Asp25- lle-Nle27-Ser28-NH-(CH2)4-NH-C-(NH2) = NH was carried out as described in Example VIII, to give another protected peptide- resin having the formula: 3-(4-hydroxyphenyl)propionyf-Ala2-Asp3(OChx)-Ala4-lle5-Pheβ-Thr7(Bzl)-Ser8(Bzl)- Ser8(Bzl)-Tyr10(DCB)-Arg11(Tos)-Lys12(2-CI-Cbz)-Val13-Leu14-Abu1B-Gln1 β-Leu17- Ser18(Bzl)-Ala19-Arg20(Tos)-Lys21(2-CI-Cbz)-Leu22-Leu23-Gln24-Asp25(OChx)-lle- Nle27-Ser28(Bzl)-NH-(CH2)4-NH-C(NH2) = N-[SPA]-[SP], which is then similarly converted to the desired peptide in accordance with the procedure of Example VIII. EXAMPLE XI
(Ac-Tyr1.Ser8.Abu15.NIe27.Aom29)hGH-RH(1-29)
The synthesis of an hGHRH analog of the formula: Ac-Tyr1-Ala2-Asp3-Ala4-lle5-Pheβ-Thr7-Ser8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14- Abu15-Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25-lle-Nle27-Ser28- NH-(CH2)4-NH-C(NH2) = NH was carried out as described in Example VIII to give: Ac-Tyr1 (DCB)-Ala2- Asp3(OChx)-Ala4-lle6-Pheβ-Thr7(Bzl)-Ser8(Bzl)-Ser9(Bzl)-Tyr10(DCB)-Arg11(Tos)- Lys12(2-CI-Cbz)-Val13-Leu14-Abu1B-Gln-Leu17-Ser18(Bzl)-Ala19-Arg20(Tos)-Lys21(2-CI- Cbz)-Leu22-Leu23-Gln2 -Asp2B(OChx)-lle-Nle27-Ser28(Bzl)-NH(CH2)4-NH-C-(NH2)= N-[SPA]-[SP], which is then similarly converted to the desired peptide in accordance with the procedure of Example VIII.
EXAMPLE XII (N-Me-Tv^.Abu^Ata^.Nle^.Aom^lhGH-RHM-∑g)
The synthesis of an hGHRH analog of the formula: N-MeTyr^Ala^Asp^Ala^lle^Phe^Thr^Abu^Sei^-Tyr^-Arg^-Lys^-Val^-Leu14- Ala16-Gln-Leu17-Ser18-Ala19-Arg 0-Lys21-Leu22-Leu23-Gln2 -Asp B-lle-Nle27-Ser28- NH-(CH2)4-NH-C(NH2) = NH is carried out as described in Example VIII to give another protected peptide-resin having the formula:
Boc-N-MeTyr1(DCB)-Ala2-Asp3(COhx)-Ala4-lleB-Pheβ-Thr7(Bzl)-Abu8-Serβ(Bzl)- Tyr 0(DCB)-Arg11(Tos)-Lys12(2-CI-Cbz)-Val13-Leu14-Ala15-Gln-Leu17-Ser18(Bzl)- Ala19-Arg20(Tos)-Lys21(2-CI-Cbz)-Leu22-Leu23-Gln24-Asp25(OCHx)-lle-Nle27- Ser28(Bzl)-NH-(CH2)4-NH-C(NH2) = NH-[SPA]-[SP], which is then similarly converted to the desired peptide in accordance with the procedure of Example VIII.
EXAMPLE XIII (Dat1.Abu8.NIe27.Aom29)hGH-RH(1-29)
The synthesis of an hGHRH analog of the formula: 3-(4-hydroxyphenyl)propionyl1-Ala2-Asp3-Ala4-lle6-Pheβ-Thr7-Abu8-Ser9-Tyr10-Arg11- Lys12-Val13-Leu1 -Gly15-Gln16-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp 25 lle β-Nle27-Ser28-NH-(CH2)4-NH-C-(NH2) = NH is carried out as described in Example IX, with the exception that Dat is incorporated as its HOSu ester in place of Ac-Tyr-OH in position 1 to give another protected peptide-resin having the formula: Dat1-Ala -Asp3(0tBu)-Ala4-lleB-Pheβ-Thr7(tBu)-Abu8-Ser9(tBu)-Tyr10(tBu)-Arg11 (Pcm)- Lys12(Boc)-Val13-Leu14-Gly15-Gln-Leu17-Ser18(tBu)-Ala19-Arg 0(Pmc)-Lys21(Boc)- Leu22-Leu23-Gln2 -Asp 5(OtBu)-lle-Nle27-Ser28(tBu)- NH(CH2)4(NH2) = N- {2,3,5,Trimethyl-[SPA]}-[SP], which is then similarly converted to the desired peptide in accordance with the procedure of Example IX .
EXAMPLE XIV
(C-MeTyr1.Abu15.NIe27.Aom 9)hGH-RH(1-29) The synthesis of an hGHRH analog of the formula: C-MeTyr1-Ala2-Asp3-Ala4-lleB-Pheβ-Thr7-Asn8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14- Abu1B-Gln-Leu17-Ser18-Ala-Arg20-Lys21-Leu22-Leu23-Gln2 -Asp2 -lle-Nle27-Ser28- NH-(CH2)4-NH-C(NH2) = NH was carried out as described in Example VIII, to give another protected peptide- resin having the formula:
Boc-C-MeTyr1-Ala2-Asp3(OChx)-Ala4-lle5-Pheβ-Thr7(Bzl)-Asn8-Ser9(Bzl)-Tyr10(DCB)- Arg11(Tos)-Lys12(2-CI-Cbz)-Val13-Leu14-Ala15-Gln-Leu17-Ser18(Bzl)-Ala19-Arg20(Tos)- Lys21(2-CI-Cbz)-Leu22-Leu23-Gln24-Asp25(OChx)-lle-Nle27-Ser28(Bzl)-NH-(CH2)4-NH- C(NH2) = N-[SPAMSP], which is then similarly converted to the desired peptide in accordance with the procedure of Example VIII.
EXAMPLE XV
(C-MeTyr1.Abu2.AIa1B.NIe27.Asp28.Aom29)hGH-RH(1-29) The synthesis of an hGHRH analog of the formula: C-MeTyr1-Abu2-Asp3-Ala -lle6-Pheβ-Thr7-Asn8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14- Ala1B-Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp2B-lle26-Nle27-Asp28- NH(CH2)4-NH-C(NH2) = NH was carried out as described in Example VIII in position 1 to give another protected peptide-resin having the formula:
HEET RULE 26) Boc-N-MeTyr1-(DCB)-Abu -Asp3(COHx)-Ala4-lle5-Pheθ-Thr7(Bzl)-Asn8-Ser9(Bzl)- Tyr10(DCB)-Arg11(Tos)-Lys12(2-CI-Cbz)-Val13-Leu1 -Ala15-Gln-Leu17-Ser18(Bzl)- Ala19-Arg20(Tos)-Lys21(2-CI-Cbz)-Leu22-Leu23-Gln24-Asp25(OCHx)-lle-Nle27-Asp28 (OChx)-NH-(CH2)4-NH-C(NH2) = N-[SPA]-[SP] which is then similarly converted to the desired peptide in accordance with the procedure of Example VIII.
EXAMPLE XVI
(5-Hiaa1.Abu1B.NIe27.Asp28.Aom29)hGH-RH(1-29) The synthesis of an hGHRH analog of the formula:
5-Hiaa1-Ala2-Asp3-Ala4-lle -Pheβ-Thr7-Asn8-Ser9-Tyr 0-Arg11Lys12-Val13-Leu -Abu15- Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln2 -Asp2B-lle-Nle27-Asp28-NH- (CH2)4-NH-C(NH2) = NH is carried out as described in Example IX, with the exception that Fmoc- Asp(OtBu)-OH was coupled instead of Fmoc-Ser(tBu)-OH in position 28, Fmoc-
Asn-OH was coupled instead of Fmoc-Ser(tBu)-OH in position 8, Fmoc-Ala-OH was coupled instead of Fmoc-Abu-OH in position 2, and 5-Hydroxy indolylacetic acid (5-Hiaa) was coupled in place of Ac-Tyr(tBu)-OH in position 1. The phenolic hydroxyl of the 5-Hiaa was not protected during coupling since with BOP carboxyl activating reagent, amino acids with free hydroxyl group(s) require no further protection during 5-7 coupling cycles. The resulting peptide intermediate is:
5-Hiaa1-Ala2-Asp3(OtBu)-Ala4-lle5-Pheβ-Thr7(tBu)-Asn8-Ser9(tBu)-Tyr10(tBu)-
Arg11(Pmc)-Lys12(Boc)-Val13-Leu14-Abu15-Gln-Leu17-Ser18(tBu)-Ala19-Arg 0(Pmc)-
Lys21-(Boc)-Leu22-Leu23-Gln2 -Asρ2B(OtBu)-lle26-Nle27-Asp28(OtBu)-NH-(CH2)4-NH- C(NH2) = N-[SPA]-[SP], which is then similarly converted to the desired peptide in accordance with the procedure of Example VIII.
Test Procedures
The compounds of the present invention were tested both in vitro and in vivo. Growth hormone releasing activities in vitro are summarized in Table 1. in vivo effect of the compounds on the release of GH in rats after intravenous (i.v.) and subcutaneous (sc.) injections are given in Tables 2 and 3 and Tables 4 and
5, respectively. EXAMPLE XVII
Growth hormone releasing activity in vitro was assayed by using a superfused rat pituitary cell system as described in S. Vigh and A.V. Schally, Peptides 5, Suppl: 241-347,1984, which is incorporated by reference. Each peptide, hGH-RH (1-29)NH2 (as control) and hGHRH analogs of the present invention, was administered for 3 minutes (1 ml. perfusate) at various concentrations as shown below. GH content of the 1 ml. fractions collected was determined by RIA. The potencies of the peptides, based on 4-point assays, were calculated in all the Examples of this specification, by the factorial analyses of Bliss and Marks with 95% confidence limits.
TABLE 1 In vitro effect of hGHRH analogs on the GH Release in a Superfused Rat Pituitary Cell System. Peptide Test conditions(nM) Potency Relative to hGH-RH (1-29ΪNH-, =1
Example VIII 0.03-1.00 4.5
Example IX 0.03-1.00 6
Example X 0.03-1.00 10 Example XI 0.03-1.00 4
Example XIII 0.03-1.00 14
Example XVI 0.03-1.00 2.4
EXAMPLE XVIII For in vivo tests based on intravenous administration, adult male Sprague-
Dawley rats were anesthetized with pentobarbital (6 mg./100/g., b.w.), injected i.p.; 20 minutes after the injection of pentobarbital, blood samples were taken from the jugular vein (pretreated level) and immediately thereafter hGH-RH (1- 29)NH2 (as a control) or hGH-RH(1-29)NH2 analogs were injected i.v. Blood samples were taken from the jugular vein 5 and 15 minutes after the injection. The blood samples were centrifuged, plasma was removed and the GH level was measured by RIA. The result tabulated in Table 2 below are expressed as the mean ± SEM; statistical significance is assessed by Duncan's Multiple Range Test. These results, expressed as potency, appear in Table 3.
TABLE 2
In vivo effect of hGH-RH analogs on the GH release in the rat after i.v. injection Peptide uσ/kα 0 min 5 min 15 min
Saline 68.4110.9 55.5111.5 hGH-RH 497.0 105.7 ( 1-29) NH2 1054.6 287.7 MZ-2-511 457.01126.8 79.2116.0 1018.01175.9 215.5160.5
MZ-3-1492 10511437.7 158.0141.4 1637.81289.5 251.2120.7 Ex VIII 1180.41180.6 157.7119.1 1901.01285.9 517.21196.7
Ex XVI 1596.61395.7 433.6191.3
Figure imgf000035_0001
1757.21139.1 1123.11152.6
TABLE 3
Potency of hGH-RH Analogs of Example VIII and XVI, Relative to hGH-RH(1-29)NH2( = 1 ) as calculated from the data of Table 2 by using the 4-
Point Assay Method hGH-RH Analog After ( min ) Potency Example VIII 5 7.49 15 4 . 02
MZ-2-51 5 2 . 35 15 1.88
MZ-3-149 5 6.22 15 2 . 63
Example XVI 5 24 .89 15 9.83
1 (Dat1, Ala16, NIe27, Agm29)hGH-RH(1-29) 2(Dat1. Ala15, NIe27, Asp28, Agm29)hGH-RH(1-29) 34
EXAMPLE XIX
Subcutaneous evaluation
Adult male rats were used and were anesthetized with pentobarbital (6 mg/100g., b.w.), injected i.p.; 20 minutes after the injection of pentobarbital, blood samples were taken from the jugular vein (pretreated level) and immediately thereafter hGH-RH(1-29)NH2 (as a control) or hGH-RH analogs were injected £_£ Blood samples were taken from the jugular vein 15 and 30 minutes after the injection. The blood samples were centrifuged, plasma was removed and the GH level was measured by RIA. The results are tabulated in Table 4 as mean ± SEM below and are summarized in terms of potency in Table 5.
TABLE 4
Figure imgf000036_0001
In another subcutaneous experiment: Peptide Dose 0 min 15 min 30 min
Figure imgf000037_0001
Saline 41.2111.9 46.012.0 55.0113.0 hGH-RH(1-29)NH2 50 35.2123.6 765.5173.4 112.7111.3
100 45.017.4 101817.0 219.5128.2 Example X 1.0 54.7123.6 486.5162.1 142.6111.3
3.0 55.017.4 913.8198.0 276.0122.3
TABLE 5
Potency of hGHRH analogs of Example VIII, X, and XVI after subcutaneous administration (SO relative to hGHRHd -29)NH2 ( = 1 ) as calculated from the data of table 4 by the 4-point assay method
Figure imgf000037_0002
The proceedings of Example XVIII were repeated except the in vivo effect of hGH-RH analogs on GH release in the rat was tested after i.m. injection. The results are tabulated in Table 6 as mean ±_ SEM and are summarized in terms of potency in Table 7.
UBSTITUTE SHEET (RULE 26) TABLE 6 In vivo effect of hGH-RH analogs on the GH-release in the rat after intramuscular (Im) injection GH Released (ng/mD * _ Peptide Dose 0 min 15 min 30min ug/kg
Saline 71.5115 61.8125.9 72.2114.1 hGH-RH(1-29)NH2 50 78.3131.4 126.7128.4 59.315.3
100 107.3119.7 253.3131.7 103.3117.3 MZ-3-149 1.0 68.015.0 158.0131.4 54.018.5 3.0 76.719.4 189.7115.8 97.0114.1
Example VIII 1 90.52120.5 105.0110.1 70.719.8 3 55.515.0 448.71116.6 126.3116.1
Example XVI 1 52.2125 200.0120.2 74.311.7 3 46.7119 640.3158.8 158.7150.6
TABLE 7 Potency of hGH-RH analogs of example VIII and XVI relative to hGH-RH(1- 29)NH2( = 1 ) as calculated from the date of table 6 using the 4-Point method
Figure imgf000038_0001
Following intravenous administration, the analogs VIII and XVI gave growth hormone levels greater than those from hGHRH alone. The effect was long lasting which indicates that the analogs have not only higher receptor affinity but increased peptidase resistance too.
Following subcutaneous administration, again all three analogs gave greater growth hormone levels than hGHRH. Here also the analogs from Example VIII and XVI produced unusually good results with a prolonged release rate.
SUBSTITUTE SHEET LE 26 The in vitro and in vivo results show different biological activity pattern.
It is believed that in vitro activity depends primarily on binding capacity of the peptide to its receptor, whereas in vivo potency relies also on favorable transport properties, suitable binding to plasma proteins and metabolic stability. The above findings therefore indicate that the analogs tested are resistant to local degradation at the injection site and theγ may also be less susceptible to enzyme degradation in the blood stream and/or have more affinity for GH-RH receptors than hGHRHd -29)NH2.
SEQUENCE LISTING
(1) GENERAL INFORMATION:
(i) APPLICANT: Zsigo, Joszef; Schally, Andrew V. ; Comaru-Schally,
(ii) TITLE OF INVENTION: NOVEL SYNTHETIC AGONISTS OF GROWTH HORMO
RELEASING HORMONE
(iii) NUMBER OF SEQUENCES: 9
(iv) CORRESPONDENCE ADDRESS:
(A) ADDRESSEE: Omri M. Behr, Esq.
(B) STREET: 325 Pierson Avenue
(C) CITY: Edison
(D) STATE: New Jersey
(E) COUNTRY: USA
(F) ZIP: 08837
(v) COMPUTER READABLE FORM:
(A) MEDIUM TYPE: Floppy disk
(B) COMPUTER: IBM PC compatible
(C) OPERATING SYSTEM: PC-DOS/MS-DOS
(D) SOFTWARE: PatentIn Release #1.0, Version #1.25
(vi) CURRENT APPLICATION DATA:
(A) APPLICATION NUMBER: 07/976,345
(B) FILING DATE: 11-13-92
(C) CLASSIFICATION: 1811
(viii) ATTORNEY/AGENT INFORMATION:
(A) NAME: BEHR, OMRI M.
(B) REGISTRATION NUMBER: 22,940
(C) REFERENCE/DOCKET NUMBER: SHAL3.0-015
(ix) TELECOMMUNICATION INFORMATION:
(A) TELEPHONE: (908) 494-5240
(B) TELEFAX: (908) 494-0428
(C) TELEX: 51 1642 BEPATEDIN
(2) INFORMATION FOR SEQ ID NO:l:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide (ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: "Res 1 =
Dat; Res 15 = Abu; Res 27 = NIe;
Res 29 = Agm"
( i) SEQUENCE DESCRIPTION: SEQ ID NO:l:
Xaa Ala Asp Ala lie Phe Thr Asn Ser Tyr Arg Lys Val Leu Xaa Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp lie Xaa Asp Xaa 20 25
(2) INFORMATION FOR SEQ ID NO:2:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
( ii) MOLECULE TYPE : peptide
(ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: "Res 1 =
Ac-Tyr; Res 8 = Abu; Res 27 = NIe;
Res 29 = Agm"
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:
Xaa Ala Asp Ala He Phe Thr Xaa Ser Tyr Arg Lys Val Leu Gly Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Ser Xaa 20 25
(2) INFORMATION FOR SEQ ID NO: 3:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide (ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: /note= "Res 1 =
Dat; Res 15 = Abu; Res 27 = NIe; Res 29 =' Agm"
(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 3:
Xaa Ala Asp Ala He Phe Thr Ser Ser Tyr Arg Lys Val Leu Xaa Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Ser Xaa 20 25
(2) INFORMATION FOR SEQ ID NO:4:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide
(ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: /note= "Res 1 =
Ac-Tyr; Res 15 = Abu; Res 27 = NIe;
Res 29 = Agm"
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:4:
Xaa Ala Asp Ala He Phe Thr Ser Ser Tyr Arg Lys Val Leu Xaa Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Ser Xaa 20 25
(2) INFORMATION FOR SEQ ID NO:5:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide (ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: /note= "Res 1 =
N-Me-Tyr; Res 8 = Abu; Res 27 = NIe;
Res 29 = Agm"
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:5:
Xaa Ala Asp Ala He Phe Thr Xaa Ser Tyr Arg Lys Val Leu Ala Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Ser Xaa 20 25
(2) INFORMATION FOR SEQ ID NO:6:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide
(ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: /note= "Res 1 = Dat; Res 8 = Abu; Res 27 = NIe; Res 29 = Agm"
(Xi) SEQUENCE DESCRIPTION: SEQ ID NO: 6:
Xaa Ala Asp Ala He Phe Thr Xaa Ser Tyr Arg Lys Val Leu Gly Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Ser Xaa 20 25
(2) INFORMATION FOR SEQ ID NO:7:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide (ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: "Res 1 =
C-MeTyr; Res 15 = Abu; Res 27 = NIe; Res 29 = Agm"
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:7:
Xaa Ala Asp Ala He Phe Thr Asn Ser Tyr Arg Lys Val Leu Xaa Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Ser Xaa 20 25
(2) INFORMATION FOR SEQ ID NO:8:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide
(ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: "Res 1 =
C-MeTyr; Res 2 = Abu; Res 27 = NIe;
Res 29 = Agm"
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:8:
Xaa Xaa Asp Ala He Phe Thr Asn Ser Tyr Arg Lys Val Leu Ala Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Asp Xaa 20 25
(2) INFORMATION FOR SEQ ID NO:9:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 29 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: peptide (ix) FEATURE:
(A) NAME/KEY: Peptide
(D) OTHER INFORMATION: /note= "Res 1 = 5-Hiaa; Res 15 = Abu; Res 27 = NIe; Res 29 = Agm"
(Xi) SEQUENCE DESCRIPTION: SEQ ID NO:9:
Xaa Ala Asp Ala He Phe Thr Asn Ser Tyr Arg Lys Val Leu Xaa Gin 1 5 10 15
Leu Ser Ala Arg Lys Leu Leu Gin Asp He Xaa Asp Xaa 20 25

Claims

Claims
1. A peptide having the formula: Q'-CO-R^Asp^Ala^lle^Phe^Thr'-R^Ser^Tyr^-Arg'^Lys^-Val^-Leu'^R^-GIn16- Leu17-Ser18-Ala 9-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25-lle-R 7-R28-NH-Q2 wherein Q1 is 3-(5-hydroxyindolyl)-methyl or an omega or alpha-omega substituted alkyl of the structure:
Z
I
(OH) m- [φ] - (CH2) n-C-
I I
Y where:
[ø] is phenyl;
Y is H, -NH2, CH3CONH- or CH3NH-; Z is H or CH3; m is 1 or 2; n is 0, 1 or 2;
R2 is Ala, D-Ala, D-N-Methγl-Ala, Abu or Aib;
R8 is Asn, D-Asn, Ser, D-Ser, or Abu; R15 is Gly, Ala, Abu or Tbg;
R27 is NIe, He, Leu, Tga, Tba, or Met
R28 is Asp, Asn or Ser;
Q2 is a lower omega-guanidino-alkγl group having a formula:
-(CH2)P-NH-C(NH2) = NH wherein p is 2 - 6 and at least one of R2, R8 and R15 is Abu, and the pharmaceutically acceptable addition salts thereof with the pharmaceutically acceptable organic or inorganic bases or acids.
2. A peptide according to Claim 1 wherein Q1-CO is Dat, Ac-Tyr, N-Me-Tyr, C-Me-Tyr, and Hiaa, and NH-Q2 is Agm.
3. A peptide according to Claim 2 wherein Q1-CO is Dat or Hiaa
R15 is Abu R27 is NIe, R28 is Asp.
4. A peptide according to Claim 2 wherein Q^CO is Ac-Tyr, Dat, N-Me-Tyr, C-Me-Tyr or Hiaa, R8 is Ser or Abu
R 5 is Abu, or Ala R27 is NIe R28 is Ser
5. A peptide according to Claim 3 wherein Q1-CO is Dat.
6. A peptide according to Claim 3 wherein Q1-CO is Hiaa.
7. A peptide according to Claim 4 wherein Q^CO is Ac-Tyr, N-Me-Tyr or Dat and R8 is Abu.
8. A peptide according to Claim 4 wherein Q1-CO is Dat or Ac-Tyr and R8 is Ser.
9. A peptide according to Claim 5 having the formula: Dat1-Ala2-Asp3-Ala -lleB-Pheβ-Thr7-Asn8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14-Abu15- Gln-Leu17- Ser18-Alal9-Arg20-Lys21-Leu22-Leu23-Gln 4-Asp2B-lle-Nle27-Asp28-Agm29.
10. A peptide according to Claim 4 having the formula: 3-(4-hydroxyphenyl)propionyf-Ala2-Asp3-Ala4-lleB-Pheβ-Thr7-Ser8-Ser9-Tyr10-Arg11- Lys12-Val13-Leuu-Abu-Gln-Leu17-Ser18-Ala19-Arg20-Lys2 -Leu22-Leu23-Gln24-Asp25- lle-Nle27-Ser28-NH-(CH2)4-NH-C-(NH2) = NH
1 1. A peptide according to Claim 2 having the formula: 3-(4-hydroxyphenyl)propionyl1-Ala2-Asp3-Ala4-lle5-Pheβ-Thr7-Abu8-Ser9-Tyr10-Arg11- Lys12-Val13-Leu14-Gly1B-Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu2 -Leu23-Gln 4-Asp25- lle-Nle27-Ser28-NH-(CH2)4-NH-C-(NH2) = NH
12. A peptide according to Claim 2 having the formula: Ac-Tyr -Ala2-Asp3-Ala4-lleB-Pheβ-Thr7-Abu8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14-Gly15- Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25-lle-Nle27-Ser28-NH- (CH2)4-NH-C(NH2) = NH
13. A peptide according to Claim 4 having the formula: Ac-Tyr1-Ala2-Asp3-Ala -lleB-Pheβ-Thr7-Ser8-Ser9-Tyr10-Arg11-Lys12-Val13-Leu14- Abu15-Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu22-Leu23-Gln24-Asp25-lle-Nle27-Ser28- NH-(CH2)4-NH-C(NH2) = NH
14. A peptide according to Claim 6 having the formula: 5-Hiaa1-Ala2-Asp3-Ala4-lleB-Pheβ-Thr7-Asn8-Ser9-Tyr10-Arg11Lys12-Val13-Leu14-Abu15- Gln-Leu17-Ser18-Ala19-Arg20-Lys21-Leu2 -Leu23-Gln 4-Asp2B-lle-Nle27-Asp28-NH- (CH2)4-NH-C(NH2) = NH
15. A pharmaceutical dosage form comprising a peptide according to Claim 1 and an excipient.
16. A method of treating human growth deficiency comprising administering from 0.2 mg to 2 mg of a peptide according to Claim 1 per day per kg body weight.
17. A method for ascertaining the endogenous physiological ability to produce hGH in a subject in need of GH-RH level amplification comprising administration to said subject of an effective amount of a GH-RH peptide according to Claim 1.
18. A method for ascertaining the endogenous physiological ability to produce hGH in patients apparently deficient in hGH, wherein the steps are administering a 50-100 microgram dose of GH-RH to a patient and measuring the hGH response evoked by said GH-RH by radioimmunoassay; and, after the hGH dose has worn off, administering a 50-100 microgram dose of peptide according to Claim 1 and measuring the hGH response evoked by said peptide by
UTE SHEET (RULE 26) -' radioimmunoassay.
19. A diagnostic kit for ascertaining the endogenous physiological ability to produce hGH comprising a 50-100 microgram dose of GH-RH; a 50-100 microgram dose of a peptide of Claim 1 ; and means for assaying the GH response evoked by each dose.
PCT/US1993/011058 1992-11-13 1993-11-10 Ghrh agonists WO1994011397A1 (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
AU57271/94A AU5727194A (en) 1992-11-13 1993-11-10 Ghrh agonists

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
US97634592A 1992-11-13 1992-11-13
US07/976,345 1992-11-13

Publications (1)

Publication Number Publication Date
WO1994011397A1 true WO1994011397A1 (en) 1994-05-26

Family

ID=25524005

Family Applications (1)

Application Number Title Priority Date Filing Date
PCT/US1993/011058 WO1994011397A1 (en) 1992-11-13 1993-11-10 Ghrh agonists

Country Status (2)

Country Link
AU (1) AU5727194A (en)
WO (1) WO1994011397A1 (en)

Cited By (9)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1996022782A1 (en) * 1995-01-24 1996-08-01 The Administrators Of The Tulane Educational Fund Novel highly potent agonists of growth hormone releasing hormone
WO1997017367A1 (en) * 1995-11-03 1997-05-15 Theratechnologies Inc. Method of grf peptides synthesis
US8192719B2 (en) 2006-02-18 2012-06-05 Aeterna Zentaris Gmbh Methods and kits to diagnose growth hormone deficiency by oral administration of EP 1572 or EP 1573 compounds
WO2013095903A1 (en) 2011-12-21 2013-06-27 University Of Miami Novel gh-rh analogs with potent agonistic effects
EP2664343A2 (en) 2008-11-17 2013-11-20 Syntaxin Limited Suppression of cancer
WO2017075535A1 (en) 2015-10-28 2017-05-04 Oxeia Biopharmaceuticals, Inc. Methods of treating neurodegenerative conditions
US10105416B2 (en) 2014-02-05 2018-10-23 The Regents Of The University Of California Methods of treating mild brain injury
EP3473643A1 (en) 2008-06-12 2019-04-24 Ipsen Bioinnovation Limited Fusion proteins for use in the treatemnt of cancer
EP3590956A1 (en) 2008-06-12 2020-01-08 Ipsen Bioinnovation Limited Suppression of neuroendocrine diseases

Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1987006835A1 (en) * 1986-05-12 1987-11-19 Eastman Kodak Company Combinations having synergistic growth hormone releasing activity and methods for use thereof
EP0413839A1 (en) * 1989-08-22 1991-02-27 The Administrators of The Tulane Educational Fund GHRH analogs
WO1991016923A1 (en) * 1990-05-04 1991-11-14 The Administrators Of The Tulane University Educational Fund Novel synthetic grf analogs

Patent Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1987006835A1 (en) * 1986-05-12 1987-11-19 Eastman Kodak Company Combinations having synergistic growth hormone releasing activity and methods for use thereof
EP0413839A1 (en) * 1989-08-22 1991-02-27 The Administrators of The Tulane Educational Fund GHRH analogs
WO1991016923A1 (en) * 1990-05-04 1991-11-14 The Administrators Of The Tulane University Educational Fund Novel synthetic grf analogs

Non-Patent Citations (2)

* Cited by examiner, † Cited by third party
Title
J.BONGERS: "KINETICS OF DIPEPTIDYL PEPTIDASE IV PROTEOLYSIS OF GHRH AND ANALOGS", BICHIMICA ET BIOPHYSICA ACTA, vol. 1122, no. 2, 31 July 1992 (1992-07-31), AMSTERDAM, pages 147 - 153 *
M.ZARANDI ET AL: "POTENT AGONISTS OF ghrh", INTERNATIONAL JOURNAL OF PEPTIDE AND PROTEIN RESEARCH, vol. 39, no. 3, March 1992 (1992-03-01), COPENHAGEN DK, pages 211-217 *

Cited By (14)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5792747A (en) * 1995-01-24 1998-08-11 The Administrators Of The Tulane Educational Fund Highly potent agonists of growth hormone releasing hormone
WO1996022782A1 (en) * 1995-01-24 1996-08-01 The Administrators Of The Tulane Educational Fund Novel highly potent agonists of growth hormone releasing hormone
WO1997017367A1 (en) * 1995-11-03 1997-05-15 Theratechnologies Inc. Method of grf peptides synthesis
US8192719B2 (en) 2006-02-18 2012-06-05 Aeterna Zentaris Gmbh Methods and kits to diagnose growth hormone deficiency by oral administration of EP 1572 or EP 1573 compounds
EP3590956A1 (en) 2008-06-12 2020-01-08 Ipsen Bioinnovation Limited Suppression of neuroendocrine diseases
EP3473643A1 (en) 2008-06-12 2019-04-24 Ipsen Bioinnovation Limited Fusion proteins for use in the treatemnt of cancer
EP3241560A1 (en) 2008-11-17 2017-11-08 Ipsen Bioinnovation Limited Suppression of cancer
EP2664343A2 (en) 2008-11-17 2013-11-20 Syntaxin Limited Suppression of cancer
US9079974B2 (en) * 2011-12-21 2015-07-14 The University Of Miami GH-RH analogs with potent agonistic effects
WO2013095903A1 (en) 2011-12-21 2013-06-27 University Of Miami Novel gh-rh analogs with potent agonistic effects
US10105416B2 (en) 2014-02-05 2018-10-23 The Regents Of The University Of California Methods of treating mild brain injury
US10617740B2 (en) 2014-02-05 2020-04-14 The Regents Of The University Of California Methods of treating mild brain injury
US11241483B2 (en) 2014-02-05 2022-02-08 The Regents Of The University Of California Methods of treating mild brain injury
WO2017075535A1 (en) 2015-10-28 2017-05-04 Oxeia Biopharmaceuticals, Inc. Methods of treating neurodegenerative conditions

Also Published As

Publication number Publication date
AU5727194A (en) 1994-06-08

Similar Documents

Publication Publication Date Title
US5792747A (en) Highly potent agonists of growth hormone releasing hormone
US5846936A (en) Growth hormone releasing factor analogs
US5696089A (en) Histidine substituted growth hormone releasing factor analogs
IE57813B1 (en) Grf analogs iv
AU2012355743B2 (en) Novel GH-RH analogs with potent agonistic effects
US5942489A (en) HGH-RH(1-29)NH2 analogues having antagonistic activity
US6057422A (en) Antagonistic analogs of GH-RH inhibiting IGF-I and -II
WO1994011396A1 (en) Ghrh agonists
EP0734396B1 (en) ANALOGUES OF hGH-RH (1-29)NH2 HAVING ANTAGONISTIC ACTIVITY
WO1997042223A9 (en) hGH-RH(1-29)NH2 ANALOGUES HAVING ANTAGONISTIC ACTIVITY
WO1994011397A1 (en) Ghrh agonists
AU628558B2 (en) Grf analogs viia
EP0413839A1 (en) GHRH analogs
IE892496A1 (en) Ghrh analogs

Legal Events

Date Code Title Description
AK Designated states

Kind code of ref document: A1

Designated state(s): AU BR CA CZ FI HU JP KR NO NZ PL RO SK UA

AL Designated countries for regional patents

Kind code of ref document: A1

Designated state(s): AT BE CH DE DK ES FR GB GR IE IT LU MC NL PT SE

DFPE Request for preliminary examination filed prior to expiration of 19th month from priority date (pct application filed before 20040101)
121 Ep: the epo has been informed by wipo that ep was designated in this application
122 Ep: pct application non-entry in european phase
NENP Non-entry into the national phase

Ref country code: CA