US20030036633A1

US20030036633A1 - DNA encoding bradykinin B1 receptor

Info

Publication number: US20030036633A1
Application number: US10/007,343
Authority: US
Inventors: David Linemeyer; John Hess; Joseph Borkowski; Kathleen Bierilo; John Menke
Original assignee: Merck and Co Inc
Current assignee: Merck and Co Inc
Priority date: 1994-04-15
Filing date: 2001-10-22
Publication date: 2003-02-20
Also published as: JP2001506481A; CA2187740C; EP0757716B1; DE69535590T2; EP0757716A1; US5965367A; ATE372375T1; CA2187740A1; US6307027B1; EP0757716A4; US5712111A; DE69535590D1; ES2292168T3; WO1995028474A1

Abstract

DNAs encoding bradykinin B₁receptors from mammalian cells have been cloned and characterized. The recombinant receptor is capable of forming receptors which bind des-Arg¹⁰kallidin and other B₁-specific ligands. The DNA has been expressed in recombinant host cells which produce active recombinant protein. In addition, the recombinant host cells are utilized to establish a method for identifying modulators of the receptor activity, and receptor modulators are identified.

Description

BACKGROUND OF THE INVENTION

Two mammalian bradykinin receptor subtypes, B ₁and B₂, have been defined based on their pharmacological properties (A. Dray, M. Perkins, TINS 16, 99-104 (1993), D. Proud, A. P. Kaplan, Annual Review Immunology 6, 49-83 (1988)). The nonapeptide bradykinin (BK) and the decapeptide Lys-BK (kallidin) are liberated from the large protein precursor kininogen by the proteolytic action of kallikreins. Because of their rapid degradation, these peptide hormones are presumed to mediate local effects. BK and kallidin both activate the B₂receptor. These B₂receptor agonists are then degraded by a carboxypeptidase to produce the B₁receptor agonists des-Arg⁹BK and des-Arg¹⁰kallidin or by the angiotensin converting enzyme (ACE) to yield inactive peptides. The phenomenon of the proteolytic transformation of a compound from B₂to B₁selectivity has been observed not only for the endogenous kinin agonists but also for several synthetic peptide antagonists (K. Wirth, et al., European Journal of Pharmacology 205, 217-218 (1991), D. Regoli, et al., European Journal of Pharmacology 127, 219-224 (1986)). BK and kallidin act as equipotent agonists at the B₂bradykinin receptor subtype. In contrast, BK is totally inactive at the B₁bradykinin receptor subtype. Although traditionally des-Arg⁹BK has been utilized to study the B₁receptor, the most potent agonist for the B₁receptor appears to be des-Arg¹⁰kallidin (D. Regoli, et al., European Journal of Pharmacology 127, 219-224 (1986)).

Bradykinin and kallidin, acting through the B ₂receptor present in smooth muscle and certain neurons, cause pronounced hypotension and are potent mediators of pain and inflammation (A. Dray, supra; D. Proud, supra). In contrast, the B₁receptor is not detected in most normal tissues and appears to act predominantly in pathophysiological conditions (A. Dray, supra). The B₁receptor was originally discovered through a contractile response to des-Arg⁹BK that was observed in rabbit aortic strips only after a prolonged ex vivo incubation (D. Regoli, J. Barabe, W. K. Park, Canadian Journal of Physiology and Pharmacology 55, 855-867 (1977); D. Regoli, F. Marceau, J. Barabe, Canadian Journal of Physiology and Pharmacology 56, 674-677 (1978); D. Regoli, J. Barabe, Pharmacological Reviews 32, 1-46 (1980)). The de novo synthesis of B₁receptors has been reported in vivo following treatment with bacterial lipopolysaccharide (LPS) (D. C. Regoli, R. Marceau, J. Lavigne, European Journal of Pharmacology 71, 105-115 (1981)), and in animal models of antigen arthritis (S. G. Farmer, B. A. McMillan, S. N. Meeker, R. M. Burch, Agents and Action 34, 191-193 (1991)). In vitro studies have implicated a number of cytokines, most notably interleukin-1 (IL-1) and IL-2, as mediators that induce the expression of B₁receptors (D. Regoli, supra; D. Deblois, J. Bouthillier, F. Marceau, British Journal of Pharmacology 93, 969-977 (1988); D. deBlois, J. Bouthillier, F. Marceau, British Journal of Pharmacology 103, 1057-1066 (1991); D. deBlois, J. Bouthillier, R. Marceau, Immunopharmacology 17, 187-198 (1989)). These results, in conjunction with the finding that activation of a B₁bradykinin receptor on mouse macrophages causes the release of cytokines (R. M. Burch, J. R. Connor, C. W. Tiffany, Agents and Action 27, 258-260 (1989); C. W. Tiffany, R. M. Burch, FEBS letters 247, 189-192 (1989)), suggest that the B₁receptor could be an important mediator of chronic inflammation. Significantly, the B₁bradykinin receptor antagonist des-Arg⁹[Leu⁸]BK was recently found to alleviate hyperalgesia in animal models of persistent inflammation (A. Dray, supra; M. N. Perkins, D. Kelly, British Journal of Pharmacology 110, 1441-1444 (1993); M. N. Perkins, E. Campbell, A. Dray, Pain 53, 191-197 (1993)). Thus, a body of evidence implicates the B₁bradykinin receptor in the pathophysiology of inflammation. Relatively little is known about the role for the B₁receptor in healthy tissues, although both B₁and B₂receptors may play a physiological role in renal function (N. -E. Rhaleb, et al., European Journal of Pharmacology 162,419-427 (1989); M. Lortie, D. Regoli, N. -E. Rhaleb, G. E. Plante, American Journal of Physiology 262, R72-R76 (1992)). The apparent inducibility of the B₁receptor under pathological conditions may provide a therapeutic window for the use of B₁receptor antagonists in treating chronic inflammation.

The cloning of the B ₂bradykinin receptor revealed that this receptor is a member of the superfamily of G-protein coupled receptors (A. E. McEachern, et al., Proc. Natl. Acad. Sci. 88, 7724-7728 (1991); S. J. Powell, et al., Genomics 15, 435-438 (1993); J. F. Hess, J. A. Borkowski, G. S. Young, C. D. Strader, R. W. Ransom, Biochem. and Biophys. Res. Comm. 184, 260-268 (1992); D. Eggerickx, E. Raspe, D. Bertrand, G. Vassart, M. Parmentier, Biochem. Biophys. Res. Comm. 187, 1306-1313 (1992)). The rat B₂bradykinin receptor was cloned using a Xenopus oocyte expression system (A. E. McEachern, et al., supra) that exploited the ability of the B₂receptor to act through G-proteins to activate phospholipase C and mobilize Ca²⁺ (R. M. Burch, J. Axelrod, Proc. Natl. Acad. Sci. 84, 6374-6378 (1987); S. R. Slivka, P. A. Insel, J. Biol. Chem 263, 14640-14647 (1988)). Recently, the B₁bradykinin receptor in rabbit aorta and rat mesangial cultured cells has also been shown to activate phospholipase C leading to Ca²⁺ mobilization (K. A. Schneck, supra; M. Issandou, J. -M. Darbon, Journal of Biological Chemistry 259, 9263-9268 (1991); M. M. Tropea, D. Gummelt, M. S. Herzig, L. M. F. Leeb-Lundberg, Journal of Pharmacology and Experimental Therapeutics 264, 930-937 (1993)). Furthermore, both B₁and B₂bradykinin receptor activities were detected when mRNA from the human fibroblast cell line WI-38 was injected into Xenopus laevis oocytes (E. Phillips, M. J. Conder, S. Bevan, P. McIntyre, M. Webb, Journal of Neurochemistry 58, 243-249 (1992). The similarity of ligands for the two bradykinin receptor subtypes suggests a similarity between the B₁and B₂receptor genes. However, the results of genomic Southern analyses indicated that these two receptors are not highly homologous (A. E. McEachern, et al., supra; J. F. Hess, et al., Molecular Pharmacology 45, 1-8 (1994). Therefore, in order to clone the human B₁receptor, we pursued an expression cloning strategy in Xenopus oocytes utilizing the photoprotein aequorin as an indicator of Ca²⁺ mobilization (K. Sandberg, A. J. Markwick, D. P. Trinh, K. J. Catt, FEBS Letters 241, 177-180 (1988); E. Giladi, E. R. Spindel, BioTechniques 10, 744-747 (1991). We isolated a cDNA clone that encodes a G-protein coupled receptor with an amino acid sequence that is 36% identical to that of the B₂bradykinin receptor. The pharmacological properties of this cloned receptor expressed in mammalian cells demonstrate that it is a B₁bradykinin receptor.

SUMMARY OF THE INVENTION

The bradykinin B ₁receptor has been cloned, expressed and characterized. Using a recombinant expression system functional DNA clones encoding the receptor have been isolated. The pharmacological and structural properties of the protein are disclosed, as are the amino acid and nucleotide sequences. The recombinant protein is useful to identify modulators of the receptor. Modulators identified in this process are useful as therapeutic agents. Modulators, as described herein, include but are not limited to agonists, antagonists, suppressors and inducers.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1—The DNA sequence of the human bradykinin receptor B[0005] ₁is shown.
FIG. 2—The amino acid sequence of the human bradykinin receptor B[0006] ₁is shown.
FIG. 3—Relative light units are presented in response to 100 nM bradykinin (open bars) and 20 nM des-Arg[0007] ¹⁰kallidin (closed bars) with increasing fraction number (decreasing in size). Oocytes were injected with an equal volume of sucrose-gradient size fractionated IL-1B induced IMR-90 poly(A)⁺ mRNA and challenged with bradykin agonists. The relative light units obtained with 100 nM bradykinin were divided by 50 to allow plotting both data sets on the same graph. A trace indicating the RNA size markers that were fractionated in a parallel gradient is shown in the upper portion of the figure.
FIG. 4 panels A and B—Luminometer tracings of individual oocytes in response to 20 nM des-Arg[0008] ¹⁰kallidin are shown. Panel A shows the signal obtained using total poly(A)⁺ mRNA isolated from IL-1β induced IMR-90 cells. Panel B shows the signal obtained using clone 33E9 cRNA.
FIG. 5—Displacements of 1 nM [[0009] ³H]des-Arg¹⁰kallidin from COS-7 cells expressing the human B₁bradykinin receptor by increasing concentrations of compounds are shown. Symbols for compounds: des-Arg¹⁰kallidin (q), des-Arg¹⁰[Leu⁹]kallidin (Δ), kallidin (*), HOE 140 (u), des-Arg⁹bradykinin (O), and bradykinin (X).

DETAILED DESCRIPTION

The present invention relates to DNA encoding a bradykinin B[0010] ₁receptor (B 1) which is isolated from B₁producing cells. B₁, as used herein, refers to protein which can specifically function as the B₁bradykinin receptor subtype.
The amino acid and DNA sequences of B[0011] ₁were not previously known. Cells capable of producing B₁include, but are not limited to, aortic smooth muscle cells. Cell lines which may produce B₁include, but are not limited to, IMR-90 and WI-38. The preferred cells for the present invention are IMR-90 cells.
Other cells and cell lines may also be suitable for use to isolate B[0012] ₁cDNA. Selection of suitable cells may be done by screening for B₁activity in whole cells or cell extracts. Methods for detecting B₁activity are known in the art and either measure the ability to bind ligands known to interact at the B₁receptor subtype, such as des-Arg¹⁰kallidin, des-Arg⁹bradykinin, des-Arg¹⁰Leu⁹kallidin, and des-Arg⁹Leu⁸bradykinin, or measure phosphatidyl inositol hydrolysis, release of intracellular Ca²⁺ stores, or arachidonic acid release mediated by des-Arg¹⁰kallidin or des-Arg⁹bradykinin. Cells which possess B₁activity in such assays may be suitable for the isolation of B₁DNA.
Because the genetic code is degenerate, more than one codon may be used to encode a particular amino acid, and therefore, the amino acid sequence can be encoded by any of a set of similar DNA oligonucleotides. Only one member of the set will be identical to the B[0013] ₁sequence but will be capable of hybridizing to B₁DNA even in the presence of DNA oligonucleotides with mismatches under appropriate conditions. Under alternate conditions, the mismatched DNA oligonucleotides may still hybridize to the B₁DNA to permit identification and isolation of B₁encoding DNA.
DNA encoding B[0014] ₁from a particular organism may be used to isolate and purify homologues of B₁from other organisms. To accomplish this, the first B₁DNA may be mixed with a sample containing DNA encoding homologues of B₁under appropriate hybridization conditions. The hybridized DNA complex may be isolated and the DNA encoding the homologous DNA may be purified therefrom.
It is known that there is a substantial amount of redundancy in the various codons which code for specific amino acids. Therefore, this invention is also directed to those DNA sequences which contain alternative codons which code for the eventual translation of the identical amino acid. For purposes of this specification, a sequence bearing one or more replaced codons will be defined as a degenerate variation. Also included within the scope of this invention are mutations either in the DNA sequence or the translated protein which do not substantially alter the ultimate physical properties of the expressed protein. For example, substitution of valine for leucine, arginine for lysine, or asparagine for glutamine may not cause a change in functionality of the polypeptide. [0015]
It is known that DNA sequences coding for a peptide may be altered so as to code for a peptide having properties that are different than those of the naturally-occurring peptide. Methods of altering the DNA sequences include, but are not limited to site directed mutagenesis. Examples of altered properties include but are not limited to changes in the affinity of an enzyme for a substrate or a receptor for a ligand. [0016]
As used herein, a “functional derivative” of B[0017] ₁is a compound that possesses a biological activity (either functional or structural) that is substantially similar to the biological activity of B₁. The term “functional derivatives” is intended to include the “fragments,” “variants,” “degenerate variants,” “analogs” and “homologues” or to “chemical derivatives” of B₁. The term “fragment” is meant to refer to any polypeptide subset of B₁. The term “variant” is meant to refer to a molecule substantially similar in structure and function to either the entire B₁molecule or to a fragment thereof. A molecule is “substantially similar” to B₁if both molecules have substantially similar structures or if both molecules possess similar biological activity. Therefore, if the two molecules possess substantially similar activity, they are considered to be variants even if the structure of one of the molecules is not found in the other or even if the two amino acid sequences are not identical.
The term “analog” refers to a molecule substantially similar in function to either the entire B[0018] ₁molecule or to a fragment thereof.
Any of a variety of procedures known in the art may be used to molecularly clone B[0019] ₁DNA. These methods include, but are not limited to, direct functional expression of the B₁genes following the construction of a B₁-containing cDNA or genomic DNA library in an appropriate expression vector system. Another method is to screen B 1-containing cDNA or genomic DNA library constructed in a bacteriophage or plasmid shuttle vector with a labeled oligonucleotide probe designed from the amino acid sequence of the B₁subunits. An additional method consists of screening a B₁-containing cDNA or genomic DNA library constructed in a bacteriophage or plasmid shuttle vector with a partial DNA encoding the B₁receptor. This partial DNA is obtained by the specific PCR amplification of B₁DNA fragments through the design of degenerate oligonucleotide primers from the amino acid sequence of the purified B₁receptor. Another method is to isolate RNA from B₁-producing cells and translate the RNA into protein via an in vitro or an in vivo translation system. The translation of the RNA into a peptide or a protein will result in the production of at least a portion of the B₁protein which can be identified by, for example, by the activity of B₁receptor protein or by immunological reactivity with an anti-B₁antibody. In this method, pools of RNA isolated from B₁-producing cells can be analyzed for the presence of an RNA which encodes at least a portion of the B₁protein. Further fractionation of the RNA pool can be done to purify the B₁RNA from non-B₁RNA. The peptide or protein produced by this method may be analyzed to provide amino acid sequences which in turn are used to provide primers for production of B₁cDNA, or the RNA used for translation can be analyzed to provide nucleotide sequences encoding B₁and produce probes for the production of B₁cDNA. These methods are known in the art and can be found in, for example, Sambrook, J., Fritsch, E. F., Maniatis, T. in Molecular Cloning: A Laboratory Manual, Second Edition, Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y. 1989.
It is readily apparent to those skilled in the art that other types of libraries, as well as libraries constructed from other cells or cell types, may be useful for isolating B[0020] ₁-encoding DNA. Other types of libraries include, but are not limited to, cDNA libraries derived from other cells or cell lines other than IMR-90 cells, and genomic DNA libraries.
It is readily apparent to those skilled in the art that suitable cDNA libraries may be prepared from cells or cell lines which have B[0021] ₁activity. The selection of cells or cell lines for use in preparing a cDNA library to isolate B₁cDNA may be done by first measuring cell associated B₁activity using the ligand binding assay described fully herein.
Preparation of cDNA libraries can be performed by standard techniques well known in the art. Well known cDNA library construction techniques can be found for example, Sambrook, J., Fritsch, E. F., Maniatis, T. in Molecular Cloning: A Laboratory Manual, Second Edition (Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y., 1989). [0022]
It is also readily apparent to those skilled in the art that DNA encoding B[0023] ₁may also be isolated from a suitable genomic DNA library. Construction of genomic DNA libraries can be performed by standard techniques well known in the art. Well known genomic DNA library construction techniques can be found in Sambrook, J., Fritsch, E. F., Maniatis, T. in Molecular Cloning: A Laboratory Manual, Second Edition (Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y., 1989).
In order to clone the B[0024] ₁gene by the above methods, the amino acid sequence of B₁may be necessary. To accomplish this, B₁protein may be purified and partial amino acid sequence determined by manual sequencing or automated sequenators. It is not necessary to determine the entire amino acid sequence, but the linear sequence of two regions of 6 to 8 amino acids from the protein is determined for the production of primers for PCR amplification of a partial B₁DNA fragment.
Once suitable amino acid sequences have been identified, the DNA sequences capable of encoding them are synthesized. Because the genetic code is degenerate, more than one codon may be used to encode a particular amino acid, and therefore, the amino acid sequence can be encoded by any of a set of similar DNA oligonucleotides. Only one member of the set will be identical to the B[0025] ₁sequence but will be capable of hybridizing to B₁DNA even in the presence of DNA oligonucleotides with mismatches under appropriate conditions. Under alternate conditions, the mismatched DNA oligonucleotides may still sufficiently hybridize to the B₁DNA to permit identification and isolation of B₁encoding DNA. Purified biologically active B₁may have several different physical forms. B₁may exist as a full-length nascent or unprocessed polypeptide, or as partially processed polypeptides or combinations of processed polypeptides. The full-length nascent B₁polypeptide may be postranslationally modified by specific proteolytic cleavage events which result in the formation of fragments of the full length nascent polypeptide. A fragment, or physical association of fragments may have the full biological activity associated with B₁(specific binding of des-Arg¹⁰kallidin, and des-Arg⁹bradykinin) however, the degree of B₁activity may vary between individual B₁fragments and physically associated B₁polypeptide fragments.
B[0026] ₁in substantially pure form derived from natural sources or from recombinant host cells according to the purification processes described herein, is found to be a polypeptide encoded by a single mRNA. The B₁polypeptide was found to have an apparent molecular weight of about 40.4 kDa.
The cloned B[0027] ₁DNA obtained through the methods described herein may be recombinantly expressed by molecular cloning into an expression vector containing a suitable promoter and other appropriate transcription regulatory elements, and transferred into prokaryotic or eukaryotic host cells to produce recombinant B₁. Techniques for such manipulations are fully described in Sambrook, J., et al., supra, and are well known in the art.
Expression vectors are defined herein as DNA sequences that are required for the transcription of cloned copies of genes and the translation of their mRNAs in an appropriate host. Such vectors can be used to express eukaryotic genes in a variety of hosts such as bacteria, bluegreen algae, plant cells, insect cells, fungal cells and animal cells. [0028]
Specifically designed vectors allow the shuttling of DNA between hosts such as bacteria-yeast or bacteria-animal cells or bacteria-fungal cells or bacteria-invertebrate cells. An appropriately constructed expression vector should contain: an origin of replication for autonomous replication in host cells, selectable markers, a limited number of useful restriction enzyme sites, a potential for high copy number, and active promoters. A promoter is defined as a DNA sequence that directs RNA polymerase to bind to DNA and initiate RNA synthesis. A strong promoter is one which causes mRNAs to be initiated at high frequency. Expression vectors may include, but are not limited to, cloning vectors, modified cloning vectors, specifically designed plasmids or viruses. [0029]
A variety of mammalian expression vectors may be used to express recombinant B[0030] ₁in mammalian cells. Commercially available mammalian expression vectors which may be suitable for recombinant B₁expression, include but are not limited to, pcDNA3 (Invitrogen), pMC1neo (Stratagene), pXT1 (Stratagene), pSG5 (Stratagene), EBO-pSV2-neo (ATCC 37593) pBPV-1(8-2) (ATCC 37110), pdBPV-MMTneo (342-12) (ATCC 37224), pRSVgpt (ATCC 37199), pRSVneo (ATCC 37198), pSV2-dhfr (ATCC 37146), pUCTag (ATCC 37460), and XZD35 (ATCC 37565).
A variety of bacterial expression vectors may be used to express recombinant B[0031] ₁in bacterial cells. Commercially available bacterial expression vectors which may be suitable for recombinant B₁expression include, but are not limited to pET11a (Novagen), lambda gt11 (Invitrogen), pcDNAII (Invitrogen), pKK223-3 (Pharmacia).
A variety of fungal cell expression vectors may be used to express recombinant B[0032] ₁in fungal cells. Commercially available fungal cell expression vectors which may be suitable for recombinant B₁expression include but are not limited to pYES2 (Invitrogen), Pichia expression vector (Invitrogen).
A variety of insect cell expression vectors may be used to express recombinant B[0033] ₁in insect cells. Commercially available insect cell expression vectors which may be suitable for recombinant expression of B₁include but are not limited to pBlue Bac III (Invitrogen).
An expression vector containing DNA encoding B[0034] ₁may be used for expression of B₁in a recombinant host cell. Recombinant host cells may be prokaryotic or eukaryotic, including but not limited to bacteria such as E. coli, fungal cells such as yeast, mammalian cells including but not limited to cell lines of human, bovine, porcine, monkey and rodent origin, and insect cells including but not limited to Drosophila and silkworm derived cell lines. Cell lines derived from mammalian species which may be suitable and which are commercially available, include but are not limited to, L cells L-M(TK⁻) (ATCC CCL 1.3), L cells L-M (ATCC CCL 1.2), 293 (ATCC CRL 1573), Raji (ATCC CCL 86), CV-1 (ATCC CCL 70), COS-1 (ATCC CRL 1650), COS-7 (ATCC CRL 1651), CHO-K1 (ATCC CCL 61), 3T3 (ATCC CCL 92), NIH/3T3 (ATCC CRL 1658), HeLa (ATCC CCL 2), C1271 (ATCC CRL 1616), BS-C-1 (ATCC CCL 26) and MRC-5 (ATCC CCL 171).
The expression vector may be introduced into host cells via any one of a number of techniques including but not limited to transformation, transfection, lipofection, protoplast fusion, and electroporation. The expression vector-containing cells are clonally propagated and individually analyzed to determine whether they produce B[0035] ₁protein. Identification of B₁expressing host cell clones may be done by several means, including but not limited to immunological reactivity with anti-B₁antibodies, and the presence of host cell-associated B₁activity, such as B₁-specific ligand binding or signal transduction defined as a response mediated by the interaction of B₁-specific ligands at the receptor.
Expression of B[0036] ₁DNA may also be performed using in vitro produced synthetic mRNA or native mRNA. Synthetic mRNA or mRNA isolated from B₁producing cells can be efficiently translated in various cell-free systems, including but not limited to wheat germ extracts and reticulocyte extracts, as well as efficiently translated in cell based systems, including but not limited to microinjection into frog oocytes, with microinjection into frog oocytes being preferred.
To determine the B[0037] ₁DNA sequence(s) that yields optimal levels of B₁activity and/or B₁protein, B₁DNA molecules including, but not limited to, the following can be constructed: the full-length open reading frame of the B₁DNA (encoding a protein of about 40.4 kDa =about base 209 to about base 1267) and several constructs containing portions of the DNA encoding B₁protein. All constructs can be designed to contain none, all or portions of the 5′ or the 3′ untranslated region of B₁DNA. B₁activity and levels of protein expression can be determined following the introduction, both singly and in combination, of these constructs into appropriate host cells. Following determination of the B₁DNA cassette yielding optimal expression in transient assays, this B₁DNA construct is transferred to a variety of expression vectors, for expression in host cells including, but not limited to, mammalian cells, insect cells, E. coli, and yeast cells such as S. cerevisiae.
Host cell transfectants and microinjected oocytes may be assayed for both the levels of B[0038] ₁receptor activity and levels of B₁protein by the following methods. One method for assessing B₁receptor activity involves the direct measurement of binding of specific ligands. In the case of recombinant host cells, this involves the transfection or co-transfection of plasmids containing the B₁DNA. In the case of oocytes, this involves the injection of synthetic or native RNAs for B₁. Following an appropriate period of time to allow for expression, B₁activity is measured. One method for detecting B₁activity involves the direct measurement of B₁activity in whole cells or cellular lysates prepared from host cells transfected with B₁DNA or oocytes injected with B₁RNA. B₁activity is measured by the specific ligand binding characteristics of the B₁receptor or the response to calcium mobilization or phosphatidyl inositol hydrolysis mediated by B₁-specific modulators in host cells expressing B₁DNA or RNA. Modulators, as described herein, include but are not limited to agonists, antagonists, suppressors and inducers.
Following expression of B[0039] ₁in a recombinant host cell, B₁protein may be recovered to provide B₁in purified form. Several B₁purification procedures are available and suitable for use. As described herein, recombinant B₁may be purified from cell lysates and extracts by various combinations of, or individual application of salt fractionation, ion exchange chromatography, size exclusion chromatography, hydroxylapatite adsorption chromatography and hydrophobic interaction chromatography.
In addition, recombinant B[0040] ₁can be separated from other cellular proteins by use of an immunoaffinity column made with monoclonal or polyclonal antibodies specific for full length nascent B₁, or polypeptide fragments of B₁.
Monospecific antibodies to B[0041] ₁are purified from mammalian antisera containing antibodies reactive against B₁or are prepared as monoclonal antibodies reactive with B₁using the technique of Kohler and Milstein, Nature 256, 495-497 (1975). Monospecific antibody as used herein is defined as a single antibody species or multiple antibody species with homogenous binding characteristics for B₁. Homogenous binding as used herein refers to the ability of the antibody species to bind to a specific antigen or epitope, such as those associated with the B₁, as described above. B specific antibodies are raised by immunizing animals such as mice, rats, guinea pigs, rabbits, goats, horses and the like, with rabbits being preferred, with an appropriate concentration of B₁either with or without an immune adjuvant.
Preimmune serum is collected prior to the first immunization. Each animal receives between about 0.1 μg and about 1000 μg of B[0042] ₁associated with an acceptable immune adjuvant. Such acceptable adjuvants include, but are not limited to, Freund's complete, Freund's incomplete, alum-precipitate, water in oil emulsion containing Corynebacterium parvum and tRNA. The initial immunization consists of B₁in, preferably, Freund's complete adjuvant at multiple sites either subcutaneously (SC), intraperitoneally (IP) or both. Each animal is bled at regular intervals, preferably weekly, to determine antibody titer. The animals may or may not receive booster injections following the initial immunization. Those animals receiving booster injections are generally given an equal amount of the antigen in Freund's incomplete adjuvant by the same route. Booster injections are given at about three week intervals until maximal titers are obtained. At about 7 days after each booster immunization or about weekly after a single immunization, the animals are bled, the serum collected, and aliquots are stored at about −20° C.
Monoclonal antibodies (mAb) reactive with B[0043] ₁are prepared by immunizing inbred mice, preferably Balb/c, with B₁. The mice are immunized by the IP or SC route with about 0.1 μg to about 10 μg, preferably about 1 μg, of B₁in about 0.5 ml buffer or saline incorporated in an equal volume of an acceptable adjuvant, as discussed above. Freund's complete adjuvant is preferred. The mice receive an initial immunization on day 0 and are rested for about 3 to about 30 weeks. Immunized mice are given one or more booster immunizations of about 0.1 to about 10 μg of B₁in a buffer solution such as phosphate buffered saline by the intravenous (IV) route. Lymphocytes, from antibody positive mice, preferably splenic lymphocytes, are obtained by removing spleens from immunized mice by standard procedures known in the art. Hybridoma cells are produced by mixing the splenic lymphocytes with an appropriate fusion partner, preferably myeloma cells, under conditions which will allow the formation of stable hybridomas. Fusion partners may include, but are not limited to: mouse myelomas P3/NS1/Ag 4-1; MPC-11; S-194 and Sp 2/0, with Sp 2/0 being preferred. The antibody producing cells and myeloma cells are fused in polyethylene glycol, about 1000 molecular weight, at concentrations from about 30% to about 50%. Fused hybridoma cells are selected by growth in hypoxanthine, thymidine and aminopterin supplemented Dulbecco's Modified Eagles Medium (DMEM) by procedures known in the art. Supernatant fluids are collected from growth positive wells on about days 14, 18, and 21 and are screened for antibody production by an immunoassay such as solid phase immunoradioassay (SPIRA) using B₁as the antigen. The culture fluids are also tested in the Ouchterlony precipitation assay to determine the isotype of the mAb.
Hybridoma cells from antibody positive wells are cloned by a technique such as the soft agar technique of MacPherson, Soft Agar Techniques, in [0044] Tissue Culture Methods and Applications, Kruse and Paterson, Eds., Academic Press, 1973.
Monoclonal antibodies are produced in vivo by injection of pristane primed Balb/c mice, approximately 0.5 ml per mouse, with about 2×10[0045] ⁶to about 6×10⁶hybridoma cells about 4 days after priming. Ascites fluid is collected at approximately 8-12 days after cell transfer and the monoclonal antibodies are purified by techniques known in the art.
In vitro production of anti-B[0046] ₁mAb is carried out by growing the hydridoma in DMEM containing about 2% fetal calf serum to obtain sufficient quantities of the specific mAb. The mAb are purified by techniques known in the art.
Antibody titers of ascites or hybridoma culture fluids are determined by various serological or immunological assays which include, but are not limited to, precipitation, passive agglutination, enzyme-linked immunosorbent antibody (ELISA) technique and radioimmunoassay (RIA) techniques. Similar assays are used to detect the presence of B[0047] ₁in body fluids or tissue and cell extracts.
It is readily apparent to those skilled in the art that the above described methods for producing monospecific antibodies may be utilized to produce antibodies specific for B[0048] ₁polypeptide fragments, or full-length nascent B₁polypeptide. Specifically, it is readily apparent to those skilled in the art that monospecific antibodies may be generated which are specific for the fully functional receptor or fragments thereof.
B[0049] ₁antibody affinity columns are made by adding the antibodies to Affigel-10 (Biorad), a gel support which is activated with N-hydroxysuccinimide esters such that the antibodies form covalent linkages with the agarose gel bead support. The antibodies are then coupled to the gel via amide bonds with the spacer arm. The remaining activated esters are then quenched with 1M ethanolamine HCl (pH 8). The column is washed with water followed by 0.23 M glycine HCl (pH 2.6) to remove any non-conjugated antibody or extraneous protein. The column is then equilibrated in phosphate buffered saline (pH 7.3) and the cell culture supernatants or cell extracts containing B₁are slowly passed through the column. The column is then washed with phosphate buffered saline until the optical density (A₂₈₀) falls to background, then the protein is eluted with 0.23 M glycine-HCl (pH 2.6). The purified B₁protein is then dialyzed against phosphate buffered saline.
The human embryonic fibroblast cell line IMR-90 had been shown previously to express the B[0050] ₁bradykinin receptor subtype (R. H. Goldstein, M. Wall, Journal of Biological Chemistry 259, 9263-9268 (1984). A more detailed pharmacological characterization revealed the presence of approximately 5000 high affinity binding sites for the B₁agonist [³H]des-Arg¹⁰kallidin and approximately 70,000 high affinity binding sites for the B₂agonist [³H]bradykinin per cell. The ability of the B₁receptor expressed in IMR-90 cells to mobilize Ca²⁺ in response to des-Arg¹⁰kallidin was demonstrated using FURA-2 as an indicator. Furthermore, treatment of IMR-90 cells with the cytokine IL-1β was found to stimulate the number of B₁bradykinin receptors approximately 7-fold. Based on these data IL-1β induced IMR-90 cells were used as the source of mRNA for expression cloning.
A cDNA clone encoding a human B[0051] ₁bradykinin receptor was isolated from an IMR-90 fibroblast cDNA library by expression cloning. The photoprotein aequorin was utilized as an indicator of the ability of the B₁receptor agonist des-Arg¹⁰kallidin to mediate Ca²⁺ mobilization in Xenopus laevis oocytes injected with IMR-90 derived RNA. A single clone was isolated with an approximately 1307 bp insert which contains an open reading frame encoding an approximately 353 amino acid protein with the characteristics of a G-protein coupled receptor. The amino acid sequence of the B₁bradykinin receptor is about 36% identical to the amino acid sequence of the B₂bradykinin receptor. The B₁bradykinin receptor expressed in COS-7 cells exhibits high affinity binding for [³H]des-Arg¹⁰kallidin and low affinity for bradykinin. The B₁receptor antagonist des-Arg¹⁰[Leu⁹]kallidin effectively displaces [³H]des-Arg¹⁰kallidin from the cloned receptor, whereas, the B₂receptor antagonist HOE 140 (Hock, F.J. et al. British Journal of Pharmacology 102, 769-773 (1991)) does not. Therefore, the expressed receptor has the pharmacological characteristics of the B₁receptor subtype. The B₁bradykinin receptor has been implicated in chronic inflammation and hyperalgesia, whereas the B₂receptor appears to mediate acute inflammatory and algesic responses. The availability of the cloned human B₁bradykinin receptor allows the identification of modulators useful in B₁-mediated diseases and conditions such as hyperalgesia, as well as acute and chronic inflammatory processes.
The present invention is also directed to methods for screening for compounds which modulate the expression of DNA or RNA encoding B[0052] ₁as well as the function of B₁protein in vivo. Compounds which modulate these activities may be DNA, RNA, peptides, proteins, or non-proteinaceous organic molecules. Compounds may modulate by increasing or attenuating the expression of DNA or RNA encoding B₁, or the function of B₁protein. Compounds that modulate the expression of DNA or RNA encoding B₁or the function of B₁protein may be detected by a variety of assays. The assay may be a simple “yes/no” assay to determine whether there is a change in expression or function. The assay may be made quantitative by comparing the expression or function of a test sample with the levels of expression or function in a standard sample.
Kits containing B[0053] ₁DNA, antibodies to B₁, or B₁protein may be prepared. Such kits are used to detect DNA which hybridizes to B₁DNA or to detect the presence of B₁protein or peptide fragments in a sample. Such characterization is useful for a variety of purposes including but not limited to forensic analyses and epidemiological studies.
The DNA molecules, RNA molecules, recombinant protein and antibodies of the present invention may be used to screen and measure levels of B[0054] ₁DNA, B₁RNA or B₁protein. The recombinant proteins, DNA molecules, RNA molecules and antibodies lend themselves to the formulation of kits suitable for the detection and typing of B₁. Such a kit would comprise a compartmentalized carrier suitable to hold in close confinement at least one container. The carrier would further comprise reagents such as recombinant B₁protein or anti-B₁antibodies suitable for detecting B₁. The carrier may also contain a means for detection such as labeled antigen or enzyme substrates or the like.
Nucleotide sequences that are complementary to the B[0055] ₁encoding DNA sequence can be synthesized for antisense therapy. These antisense molecules may be DNA, stable derivatives of DNA such as phosphorothioates or methylphosphonates, RNA, stable derivatives of RNA such as 2′-O-alkylRNA, or other B₁antisense oligonucleotide mimetics. B₁antisense molecules may be introduced into cells by microinjection, liposome encapsulation or by expression from vectors harboring the antisense sequence. B₁antisense therapy may be particularly useful for the treatment of diseases where it is beneficial to reduce B₁activity.
B[0056] ₁gene therapy may be used to introduce B₁into the cells of target organs. The B₁₄gene can be ligated into viral vectors which mediate transfer of the B₁DNA by infection of recipient host cells. Suitable viral vectors include retrovirus, adenovirus, adeno-associated virus, herpes virus, vaccinia virus, polio virus and the like.
Alternatively, B[0057] ₁DNA can be transferred into cells for gene therapy by non-viral techniques including receptor-mediated targeted DNA transfer using ligand-DNA conjugates or adenovirus-ligand-DNA conjugates, lipofection membrane fusion or direct microinjection. These procedures and variations thereof are suitable for ex vivo as well as in vivo B₁gene therapy. B₁gene therapy may be particularly useful for the treatment of diseases where it is beneficial to elevate B₁activity.
Pharmaceutically useful compositions comprising B[0058] ₁DNA, B₁RNA, or B₁protein, or modulators of B₁receptor activity, may be formulated according to known methods such as by the admixture of a pharmaceutically acceptable carrier. Examples of such carriers and methods of formulation may be found in Remington's Pharmaceutical Sciences. To form a pharmaceutically acceptable composition suitable for effective administration, such compositions will contain an effective amount of the protein, DNA, RNA, or modulator.
Therapeutic or diagnostic compositions of the invention are administered to an individual in amounts sufficient to treat or diagnose B[0059] ₁related disorders. The effective amount may vary according to a variety of factors such as the individual's condition, weight, sex and age. Other factors include the mode of administration.
The pharmaceutical compositions may be provided to the individual by a variety of routes such as subcutaneous, topical, oral and intramuscular. [0060]
The term “chemical derivative” describes a molecule that contains additional chemical moieties which are not normally a part of the base molecule. Such moieties may improve the solubility, half-life, absorption, etc. of the base molecule. Alternatively the moieties may attenuate undesirable side effects of the base molecule or decrease the toxicity of the base molecule. Examples of such moieties are described in a variety of texts, such as Remington's Pharmaceutical Sciences. [0061]
Compounds identified according to the methods disclosed herein may be used alone at appropriate dosages defined by routine testing in order to obtain optimal inhibition of the B[0062] ₁receptor or its activity while minimizing any potential toxicity. In addition, co-administration or sequential administration of other agents may be desirable.
The present invention also has the objective of providing suitable topical, oral, systemic and parenteral pharmaceutical formulations for use in the novel methods of treatment of the present invention. The compositions containing compounds identified according to this invention as the active ingredient for use in the modulation of B[0063] ₁receptors can be administered in a wide variety of therapeutic dosage forms in conventional vehicles for administration. For example, the compounds can be administered in such oral dosage forms as tablets, capsules (each including timed release and sustained release formulations), pills, powders, granules, elixirs, tinctures, solutions, suspensions, syrups and emulsions, or by injection. Likewise, they may also be administered in intravenous (both bolus and infusion), intraperitoneal, subcutaneous, topical with or without occlusion, or intramuscular form, all using forms well known to those of ordinary skill in the pharmaceutical arts. An effective but non-toxic amount of the compound desired can be employed as a B₁modulating agent.
The daily dosage of the products may be varied over a wide range from 0.01 to 1,000 mg per adult human/per day. For oral administration, the compositions are preferably provided in the form of scored or unscored tablets containing 0.01, 0.05, 0.1, 0.5, 1.0, 2.5, 5.0, 10.0, 15.0, 25.0, and 50.0 milligrams of the active ingredient for the symptomatic adjustment of the dosage to the patient to be treated. An effective amount of the drug is ordinarily supplied at a dosage level of from about 0.0001 mg/kg to about 100 mg/kg of body weight per day. The range is more particularly from about 0.001 mg/kg to 10 mg/kg of body weight per day. The dosages of the B[0064] ₁receptor modulators are adjusted when combined to achieve desired effects. On the other hand, dosages of these various agents may be independently optimized and combined to achieve a synergistic result wherein the pathology is reduced more than it would be if either agent were used alone.
Advantageously, compounds of the present invention may be administered in a single daily dose, or the total daily dosage may be administered in divided doses of two, three or four times daily. Furthermore, compounds for the present invention can be administered in intranasal form via topical use of suitable intranasal vehicles, or via transdermal routes, using those forms of transdermal skin patches well known to those of ordinary skill in that art. To be administered in the form of a transdermal delivery system, the dosage administration will, of course, be continuous rather than intermittent throughout the dosage regimen. [0065]
For combination treatment with more than one active agent, where the active agents are in separate dosage formulations, the active agents can be administered concurrently, or they each can be administered at separately staggered times. [0066]
The dosage regimen utilizing the compounds of the present invention is selected in accordance with a variety of factors including type, species, age, weight, sex and medical condition of the patient; the severity of the condition to be treated; the route of administration; the renal and hepatic function of the patient; and the particular compound thereof employed. A physician or veterinarian of ordinary skill can readily determine and prescribe the effective amount of the drug required to prevent, counter or arrest the progress of the condition. Optimal precision in achieving concentrations of drug within the range that yields efficacy without toxicity requires a regimen based on the kinetics of the drug's availability to target sites. This involves a consideration of the distribution, equilibrium, and elimination of a drug. [0067]
In the methods of the present invention, the compounds herein described in detail can form the active ingredient, and are typically administered in admixture with suitable pharmaceutical diluents, excipients or carriers (collectively referred to herein as “carrier” materials) suitably selected with respect to the intended form of administration, that is, oral tablets, capsules, elixirs, syrups and the like, and consistent with conventional pharmaceutical practices. [0068]
For instance, for oral administration in the form of a tablet or capsule, the active drug component can be combined with an oral, non-toxic pharmaceutically acceptable inert carrier such as ethanol, glycerol, water and the like. Moreover, when desired or necessary, suitable binders, lubricants, disintegrating agents and coloring agents can also be incorporated into the mixture. Suitable binders include, without limitation, starch, gelatin, natural sugars such as glucose or beta-lactose, corn sweeteners, natural and synthetic gums such as acacia, tragacanth or sodium alginate, carboxymethylcellulose, polyethylene glycol, waxes and the like. Lubricants used in these dosage forms include, without limitation, sodium oleate, sodium stearate, magnesium stearate, sodium benzoate, sodium acetate, sodium chloride and the like. Disintegrators include, without limitation, starch, methyl cellulose, agar, bentonite, xanthan gum and the like. [0069]
For liquid forms the active drug component can be combined in suitably flavored suspending or dispersing agents such as the synthetic and natural gums, for example, tragacanth, acacia, methyl-cellulose and the like. Other dispersing agents which may be employed include glycerin and the like. For parenteral administration, sterile suspensions and solutions are desired. Isotonic preparations which generally contain suitable preservatives are employed when intravenous administration is desired. [0070]
Topical preparations containing the active drug component can be admixed with a variety of carrier materials well known in the art, such as, e.g., alcohols, aloe vera gel, allantoin, glycerine, vitamin A and E oils, mineral oil, PPG2 myristyl propionate, and the like, to form, e.g., alcoholic solutions, topical cleansers, cleansing creams, skin gels, skin lotions, and shampoos in cream or gel formulations. [0071]
The compounds of the present invention can also be administered in the form of liposome delivery systems, such as small unilamellar vesicles, large unilamellar vesicles and multilamellar vesicles. Liposomes can be formed from a variety of phospholipids, such as cholesterol, stearylamine or phosphatidylcholines. [0072]
Compounds of the present invention may also be delivered by the use of monoclonal antibodies as individual carriers to which the compound molecules are coupled. The compounds of the present invention may also be coupled with soluble polymers as targetable drug carriers. Such polymers can include polyvinyl-pyrrolidone, pyran copolymer, polyhydroxypropylmethacryl-amidephenol, polyhydroxy-ethylaspartamidephenol, or polyethyl-eneoxidepolylysine substituted with palmitoyl residues. Furthermore, the compounds of the present invention may be coupled to a class of biodegradable polymers useful in achieving controlled release of a drug, for example, polylactic acid, polyepsilon caprolactone, polyhydroxy butyric acid, polyorthoesters, polyacetals, polydihydro-pyrans, polycyanoacrylates and cross-linked or amphipathic block copolymers of hydrogels. [0073]
The following examples illustrate the present invention without, however, limiting the same thereto. [0074]

EXAMPLE 1

RNA Isolation [0075]
Oocyte Injections: [0076]
Injection of mRNA or CRNA into Xenopus oocytes was done by a modification of established protocols (A. Coleman, [0077] Transcription and Translation: A Practical Approach. B. D. Hanes, S. J. Higgins, Eds., 1984); Y. Masu, et al., Nature 329, 836-838 (1987)). Oocytes were surgically removed from either albino or pigmented 0. 17% tricaine anesthetized Xenopus laevis (Xenopus One). The excised ovarian lobes were teased apart with jeweler's forceps and then placed into OR-2 (82.5 mM NaCl, 2 mM KCl, 1 mM MgCl₂, 5 mM HEPES pH 7.4) containing 2 mg/ml collagenase B (Boehringer Mannhiem) for 2 hours at room temperature with a change of the buffer at 1 hour. Isolated oocytes were repeatedly washed in OR-2 until the supernatant remained clear. Stage 5 and 6 oocytes were selected and cultured overnight in supplemented OR-2 (OR-2 containing 1.8 mM CaCl₂, 0.5 mg/ml gentamycin and 0.5 mM theophylline). Initially, oocytes were injected with 46 nl of RNA at a concentration of 1 or 2 mg/ml in H₂O, once the pool size became less than 30 clones the cRNA concentration was decreased to 40 ng/ml. RNA was injected using a Nanoject automatic oocyte injector (Drummond Scientific) and injection needles were pulled from 3.5″ Drummond capillaries using a Flaming/Brown Micropipette puller (Sutter Instruments). Two to three days after the RNA injection, oocytes were injected with 92 ng of aequorin (Friday Harbor Photoproteins) resuspended in 46 nl of 1 mM EDTA, as previously described (K. Sandberg, A. J. Markwick, D. P. Trinh, K. J. Catt, FEBS Letters 241, 177-180 (1988); E. Giladi, E. R. Spindel, BioTechniques 10, 744-747 (1991)). The following day, individual oocytes placed in wells of a microtiter dish containing 225 μl OR-2 were challenged with peptide agonists and the aequorin photo response was measured using a ML3000 Microtiter plate luminometer (Dynatech). Oocytes were challenged with several peptides (Peninsula Laboratories) as described in the text and figure legends.
Injection of poly(A)[0078] ⁺ mRNA prepared from IL-1β induced IMR-90 cells into Xenopus laevis oocytes resulted in aequorin mediated luminescence in response to either the B₁agonist des-Arg¹⁰kallidin or the B₂agonist BK (FIG. 3). The poly(A)⁺ mRNA was size-fractionated over a sucrose gradient, fractions were injected into oocytes, and the oocytes were assayed for their ability to respond to either BK or des-Arg¹⁰kallidin. The B₁and B₂receptor transcripts were clearly separated by the size fractionation. The mRNA mediating the response to des-Arg¹⁰kallidin exhibited an apparent size of 1.6-1.8 kb, whereas, the mRNA mediating the response to BK had an apparent size of 4.4-4.6 kb. The apparent size of the mRNA encoding bradykinin response is consistent with the previously determined size of the B₂bradykinin receptor transcript (A. E. McEachern, et al., Proc. Natl. Acad. Sci. 88, 7724-7728 (1991); J. F. Hess, et al., Molecular Pharmacology 45, 1-8 (1994)).

EXAMPLE 2

RNA Fractionation [0079]
IMR-90 cells (ATCC CCL 186) were grown in MEM supplemented with 10% fetal calf serum, glutamine, nonessential amino acids, sodium pyruvate, penicillin and streptomycin (Gibco). Two and a half hours prior to mRNA extraction, IMR-90 cells were exposed to 200 pg/ml IL-1β (R & D Systems). mRNA was purified from these cells using the PolyAtract mRNA isolation system (Promega) and resuspended in H[0080] ₂O at a concentration of 2 mg/ml.
IMR-90 mRNA was size fractionated on a continuous 6 to 20% sucrose gradient in 15 mM PIPES (pH 6.5), 5 mM EDTA and 0.25% N-lauroylsarcosine. 480 μg of mRNA from the IL-1β induced IMR-90 cells was heated to 65° C. for 3 minutes, quickly cooled on ice, and loaded onto the gradient. The RNA was size fractionated by centrifugation at 18° C. for 19 hours at 77,000× g. Fractions (450 μl) from each gradient were collected from the bottom of the tube and their absorbance at OD 260 monitored. Fractions were ethanol precipitated twice and resuspended to a final concentration of 1 μg/μl RNA sizes determination was based on the migration pattern of 80 μg of 9.49-0.24 Kb RNA markers (BRL) loaded on a parallel gradient. [0081]
Library Construction: [0082]
A peak RNA fraction from the sucrose gradient which gave a response to des-Arg[0083] ¹⁰kallidin was utilized to generate a cDNA library. The library was constructed in the mammalian expression vector pcDNA3 using a combination of random hexamers and oligo dT to prime the first strand cDNA synthesis. First strand cDNA synthesis of approximately 3 μg of fraction 14 size-selected mRNA was primed with 50 ng random hexamers and 400 ng of a Not I oligo dT oligonucleotide and synthesized with the BRL Superscript II reverse transcriptase (Gibco-BRL). Following second strand synthesis Bst XI/Eco RI adaptors (Invitrogen) were ligated onto the ends and the cDNA was passed over a BRL cDNA sizing column (Gibco-BRL). The cDNA was cloned into the Bst XI site of pcDNA3 (Invitrogen, San Diego, Calif.) containing a modified polylinker. Plasmid DNA was transformed into XL-1 Blue cells (Stratagene). The library contained greater than 90% inserts with an average insert size of 1.9 kb.
The library was plated in pools of approximately 5000 clones that were used to synthesize cRNA using the T7 RNA polymerase. Colonies were plated on Colony/Plaque screen filters (NEN/Dupont) that were placed on Luria-Bertani (LB) agar plates supplemented with 100 ug/ml ampicillin (Sigma). Replica filters were made, the bacterial colonies were scraped in LB broth, and a frozen glycerol stock was prepared. Plasmid DNA was made using the Wizard DNA purification system (Promega). Plasmid DNA was linearized with Not I and cRNA was synthesized using T7 RNA polymerase with the mCAP RNA capping kit (Stratagene). [0084]
Of the twenty-five pools of cRNA that were injected into Xenopus oocytes, 11 exhibited aequorin-mediated luminescence in response to des-Arg[0085] ¹⁰kallidin. The pool that gave the most robust response was replated and fractionated into 25 pools of approximately 800 clones. Eight pools exhibited a response to des-Arg¹⁰kallidin. The strongest positive pool was further examined using electrophysiology to monitor the Ca²⁺ sensitive Cl⁻ channel. Des-Arg¹⁰kallidin produced a response that was blocked by the B₁receptor antagonist des-Arg¹⁰[Leu]⁹kallidin. This pool was then subdivided into 32 pools of approximately 25 individual clones. Two positive pools, containing 14 and 34 clones, were identified. cRNA was prepared from individual clones and analyzed in Xenopus oocytes. Three individual clones were found to elicit a des-Arg¹⁰kallidin response (FIGS. 4A&B). Restriction analysis, Southern blotting, and preliminary DNA sequence analysis indicated that these individual clones were similar. One clone, 33E9, was chosen for further DNA sequence analysis, expression, and pharmacological characterization. The DNA sequence of both strands was determined by either manual sequencing using Sequenase (USB) or automated sequencing using an ABI 373A sequencing unit (Perkin Elmer).
Primary Structure of the B[0086] ₁Receptor
The DNA sequence of the approximately 1307 bp clone 33E9 contains an open reading frame of about 1059 bp (FIGS. 1 and 2). The proposed initiator methionine at nucleotide about 209 conforms to the Kozak sequence (M. Kozak, [0087] Journal of Cell Biology 108, 229-241 (1989)) at the +4 position but not at the −3 position. The approximately 208 nucleotide putative 5′ untranslated sequence contains a region of relatively high nucleotide identity to a wide variety of human DNA sequences, suggestive of a human repetitive element. The apparent repetitive element appears to be an authentic portion of the mRNA transcript since it was detected in several independently derived cDNA clones. The DNA sequence identity between the open reading frame in clone 33E9 and the DNA encoding the human B₂receptor (S. J. Powell, et al., Genomics 15, 435438 (1993); J. F. Hess, J. A. Borkowski, G. S. Young, C. D. Strader, R. W. Ransom, Biochem. and Biophys. Res. Comm. 184, 260-268 (1992); D. Eggerickx, E. Raspe, D. Bertrand, G. Vassart, M. Parmentier, Biochem. Biophys. Res. Comm. 187, 1306-1313 (1992)) is 54%. This is consistent with the inability of genomic Southern analyses to detect this gene (A. E. McEachem, et al., Proc. Natl. Acad. Sci. 88, 7724-7728 (1991); J. F. Hess, et al., Molecular Pharmacology 45,1-8 (1994)).
The proposed amino acid sequence encoded by the open reading frame is 36% identical to the B[0088] ₂bradykinin receptor. A hydrophobicity plot of the amino acid sequence reveals the seven potential transmembrane spanning domains that are characteristic of G-protein coupled receptors (H. G. Dohlman, J. Thomer, M. G. Caron, R. J. Lefkowitz, Ann. Rev. Biochem. 60, 653-688 (1991); C. D. Strader, I. S. Sigal, R. A. F. Dixon, FASEB 3, 1825-1832 (1989)). Two conserved Cys residues that are proposed to form a disulfide bond between the first and second extracellular loops in nearly all G-protein coupled receptors are also present in the sequence. There are two potential N-linked glycosylation sites in the N-terminal domain of the sequence and one putative site for N-linked glycosylation in the second extracellular loop region. Potential protein kinase C phosphorylation sites are present in intracellular domain 2 and the carboxy-terminal tail. Similar potential phosphorylation sites in other G-protein coupled receptors have been implicated in short-term desensitization of the receptor following agonist stimulation.

EXAMPLE 3

Genomic DNA Cloning of the B[0089] ₁Receptor
A human genomic DNA library is constructed in the cosmid sCOS vector using genomic DNA isolated from human foreskin fibroblast HSF42 cells (Chartrain, N. A., et al. [0090] Journal of Biological Chemistry 269, 6765-6772 (1994)). The recombinant DNA library constructed from genomic DNA of human cells is plated on Colony/Plaque screen hybridization transfer membrane (Dupont/NEN) at a density of approximately 30,000 colonies per plate. Replicas of master plates are lysed and processed for hybridization using standard protocols (Sambrook, J., Fritsch, E. F., Maniatis, T. in Molecular Cloning: A Laboratory Manual, Second Edition, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y., 1989). The DNA is UV crosslinked to the membrane with a Stratalinker (Stratagene). The filters are incubated overnight at 42° C. with radiolabeled probe in 50% formamide hybridization solution, [5× SSC, 5× Denhardt's, 100 μg/ml DNA (Sigma)]. The probe, a DNA fragment containing the coding sequence of the human B₁bradykinin receptor, is generated by random prime labeling (Boehringer Mannheim Biochemicals) in the presence of [α-³²P]dCTP (3000 Ci/mmole). Filters are washed at a final stringency of 0.1× SSC, 0.1% SDS at 42° C. Positives are rescreened to isolate single colonies. DNA is prepared from positive colonies, digested with restriction enzymes, and Southern blot analysis is done to identify restriction fragments for subcloning. A fragment is subcloned into pSP72 (Promega).

EXAMPLE 4

Cloning of B[0091] ₁cDNA into a Mammalian Expression Vector
Mammalian Cell Expression and Characterization [0092]
Transient expression of the cloned B[0093] ₁bradykinin receptor in COS-7 cells was accomplished by electroporation using a Biorad Gene Pulser. Three days post-transfection, cells were processed for a whole cell binding assay as previously published (K. A. Schneck, J. F. Hess, G. Y. Stonesifer, R. W. Ransom, European Journal of Pharmacology—Molecular Pharmacology Section 266, 277-282 (1994)) or membranes were prepared as described previously (Huang, R. -R. C., Dehaven, R. N., Cheung, A. H., Diehl, R. E., Dixon, R. A. F., Strader, C. D., Molecular Pharmacology 37, 304-310 (1990)) and radioligand binding measured as follows. Displacement studies were done with 1 nM [des-Arg¹⁰],[3,4-³H(N)]-kallidin (NEN) in the presence of varying concentrations of competitor compounds. Binding assays were performed at room temperature for 45 minutes. Reactions were terminated by filtration using an Inotech cell harvester onto glass fiber filters (Inotech) that had been briefly soaked in 0.3% polyethyleneimine. The filters were washed five times with 1 ml per well of cold PBS and counted in a liquid scintillation counter. Alternatively, reactions were collected using a Tomtec cell harvester 96 onto 0.3% polyethyleneimine presoaked glass fiber filters (Pharmacia, printed filtermat for use with the 1205 Betaplate). The filter was washed five times with a total of 10 ml per well of cold 1× PBS, dried and sealed in a bag (Pharmacia) containing scintillation fluid. Counting was accomplished using a LKB₁₂₀₅Betaplate liquid scintillation counter.
The B[0094] ₁bradykinin receptor clone 33E9 was transfected into COS-7 cells and the pharmacological properties of the expressed receptor were determined. Scatchard analysis of saturation binding data with [³H]des-Arg¹⁰kallidin indicated a K_dof about 1.0 nM and a B_maxof approximately 120 fmol/mg protein. Mock transfected COS-7 cells do not contain any specific binding for [³H]des-Arg¹⁰kallidin.

The ability of several bradykinin receptor agonists and antagonists to displace 1 nM [ ³H]des-Arg¹⁰kallidin from the cloned receptor was assessed (FIG. 5, Table 1). The IC₅₀for displacement of 1 nM [³H]des-Arg¹⁰kallidin by bradykinin from the cloned receptor is >10 μM. The low affinity of this receptor for bradykinin and high affinity for des-Arg¹⁰kallidin argues strongly that this cloned bradykinin receptor is of the B₁subtype. Competition binding studies yielded a rank order of affinity for kinin agonists of des-Arg¹⁰kallidin>kallidin >des-Arg⁹bradykinin>>bradykinin at the cloned human receptor. This is very similar to the rank order of potency reported for the rabbit B₁bradykinin receptor and identical to that observed for the B₁receptor in IMR-90 cells (Table 1). Both the cloned human receptor and the B₁receptor in IMR-90 cells exhibit a relatively low affinity for the “classical” B₁receptor agonist des-Arg⁹bradykinin which has been reported to a have a high affinity for the B₁receptor in rabbit aorta (K. A. Schneck, J. F. Hess, G. Y. Stonesifer, R. W. Ransom, European Journal of Pharmacology—Molecular Pharmacology Section 266, 277-282 (1994); D. Regoli, J. Barabe, Pharmacological Reviews 32, 1-46 (1980)). The B₁bradykinin receptor present in human aorta also has a relatively low affinity for des-Arg⁹bradykinin (>1000 nM, R.W.R, unpublished data). These results taken together with the lower affinity for des-Arg⁹bradykinin relative to des-Arg¹⁰kallidin in the rabbit (K. A. Schneck, J. F. Hess, G. Y. Stonesifer, R. W. Ransom, European Journal of Pharmacology—Molecular Pharmacology Section 266, 277-282 (1994); D. Regoli, J. Barabe, Pharmacological Reviews 32, 1-46 (1980)) suggest that the most potent natural ligand for the B₁receptor is des-Arg¹⁰kallidin . Therefore, the B₁receptor cloned here appears to be the human homologue of the B₁receptor present in rabbit aorta, and the lower affinity of the human receptor for des-Arg⁹bradykinin appears to be a consequence of species differences.

TABLE 1


Comparison of the peptide binding properties of the cloned human
B₁bradykinin receptor in transiently transfected COS-7 cells (COS
33E9) with the B₁receptor in IMR-90 cells (IMR-90).
The IC₅₀'s were determined by the displacement of 1 nM [³H]des-
Arg¹⁰kallidin in the membrane binding assay described above.

	Competitor	COS 33E9	IMR-90

des-Arg¹⁰kallidin	2.6	nM	2.3	nM
des-Arg¹⁰Leu⁹kallidin	9	nM	7.8	nM
Kallidin	46	nM	44	nM
Hoe 140	>10	μM	>10	μM
Bradykinin	>10	μM	>10	μM
des-Arg⁹bradykinin	1500	nM	660	nM
des-Arg⁹Leu⁸bradykinin	605	nM	266	nM
des-Arg¹⁰HOE 140	94	nM	40	nM
Met-Lys-Bradykinin	71	nM		40	nM
Substance P	>10	μM	>10	μM
Bradykinin_(2-9)	>10	μM	>10	μM
Bradykinin_(1-7)	>10	μM	>10	μM
Neurotensin	>10	μM	>10	μM
Leu-Enkephalin	>10	μM	>10	μM
Angiotensin II	>10	μM	>10	μM
Acetylated Neurotensin_(8-13)	>10	μM	>10	μM
Arg Vasopressin	>10	μM	>10	μM
Oxytocin	>10	μM	>10	μM
Dynorphin_(1-17)	>7	μM	>7	μM
Endothelin I	>1	μM	>1	μM

The ability of several bradykinin receptor antagonists to displace 1 nM [[0096] ³H]des-Arg¹⁰kallidin was also analyzed. The cloned receptor has high affinity binding for the B₁specific antagonist des-Arg¹⁰[Leu⁹]kallidin and des-Arg⁹[Leu⁸]bradykinin (FIG. 5, Table 1). The potent B₂specific antagonist HOE 140 has a very low affinity for the cloned receptor. However, the removal of the C-terminal Arg from HOE 140 results in a significant increase in affinity, as expected for a B₁receptor (K. Wirth, et al., European Journal of Pharmacology 205, 217-218 (1991)). Therefore, the interaction of the cloned receptor with bradykinin receptor antagonists is consistent with the B₁receptor classification.
In summary, we have utilized an expression cloning strategy to isolate a clone encoding a human B[0097] ₁bradykinin receptor. This receptor was isolated by its ability, when expressed in Xenopus oocytes, to functionally respond to the B₁receptor agonist des-Arg¹⁰kallidin. The cloned receptor is a G-protein coupled receptor that is most similar in amino acid sequence to the B₂bradykinin receptor. The pharmacological properties of the cloned receptor expressed in mammalian cells are characteristic of the B₁bradykinin receptor classification.

EXAMPLE 5

Cloning of the B[0098] ₁cDNA into E. coli Expression Vectors
Recombinant B[0099] ₁is produced in E. coli following the transfer of the B₁expression cassette into E. coli expression vectors, including but not limited to, the pET series (Novagen). The pET vectors place B₁expression under control of the tightly regulated bacteriophage T7 promoter. Following transfer of this construct into an E. Coli host which contains a chromosomal copy of the T7 RNA polymerase gene driven by the inducible lac promoter, expression of B₁is induced when an appropriate lac substrate (IPTG) is added to the culture. The levels of expressed B₁are determined by the assays described herein.
The cDNA encoding the entire open reading frame for B[0100] ₁is inserted into the NdeI site of pET 11a. Constructs in the positive orientation are identified by sequence analysis and used to transform the expression host strain BL21. Transformants are then used to inoculate cultures for the production of B₁protein. Cultures may be grown in M9 or ZB media, whose formulation is known to those skilled in the art. After growth to an OD₆₀₀=1.5, expression of B₁is induced with 1 mM IPTG for 3 hours at 37° C.

EXAMPLE 6

Cloning of B[0101] ₁cDNA into a Vectors for Expression in Insect Cells
Baculovirus vectors, which are derived from the genome of the AcNPV virus, are designed to provide high level expression of cDNA in the Sf9 line of insect cells (ATCC CRL#1711). Recombinant baculoviruses expressing B[0102] ₁cDNA is produced by the following standard methods (InVitrogen Maxbac Manual): the B₁cDNA constructs are ligated into the polyhedrin gene in a variety of baculovirus transfer vectors, including the pAC360 and the BlueBac vector (InVitrogen). Recombinant baculoviruses are generated by homologous recombination following co-transfection of the baculovirus transfer vector and linearized AcNPV genomic DNA [Kitts, P. A., Nuc. Acid. Res. 18, 5667 (1990)] into Sf9 cells. Recombinant pAC360 viruses are identified by the absence of inclusion bodies in infected cells and recombinant pBlueBac viruses are identified on the basis of B-galactosidase expression (Summers, M. D. and Smith, G. E., Texas Agriculture Exp. Station Bulletin No. 1555). Following plaque purification, B₁expression is measured by the assays described herein.
The cDNA encoding the entire open reading frame for B[0103] ₁is inserted into the BamHI site of pBlueBacII. Constructs in the positive orientation are identified by sequence analysis and used to transfect Sf9 cells in the presence of linear AcNPV wild type DNA.
Authentic, active B[0104] ₁is found in association with the infected cells. Active B₁is extracted from infected cells by hypotonic or detergent lysis.
Alternatively, the human B[0105] ₁receptor is expressed in the Drosophila Schneider 2 cell line by cotransfection of the Schneider 2 cells with a vector containing the B₁receptor DNA downstream and under control of an inducible metallothionin promoter, and a vector encoding the G418 resistant neomycin gene. Following growth in the presence of G418, resistant cells are obtained and induced to express B₁receptor by the addition of CuSO₄. Identification of modulators of the B₁receptor is accomplished by assays using either whole cells or membrane preparations.

EXAMPLE 7

Cloning of B[0106] ₁cDNA into a Yeast Expression Vector
Recombinant B[0107] ₁is produced in the yeast S. cerevisiae following the insertion of the optimal B₁cDNA cistron into expression vectors designed to direct the intracellular or extracellular expression of heterologous proteins. In the case of intracellular expression, vectors such as EmBLyex4 or the like are ligated to the B₁cistron [Rinas, U. et al., Biotechnology 8, 543-545 (1990); Horowitz B. et al., J. Biol. Chem. 265,4189-4192 (1989)]. For extracellular expression, the B₁cistron is ligated into yeast expression vectors which fuse a secretion signal. The levels of expressed B₁are determined by the assays described herein.

EXAMPLE 8

Purification of Recombinant B1 [0108]
Recombinantly produced B[0109] ₁may be purified by antibody affinity chromatography. B₁antibody affinity columns are made by adding the anti-B₁antibodies to Affigel-10 (Biorad), a gel support which is pre-activated with N-hydroxysuccinimide esters such that the antibodies form covalent linkages with the agarose gel bead support. The antibodies are then coupled to the gel via amide bonds with the spacer arm. The remaining activated esters are then quenched with 1M ethanolamine HCl (pH 8). The column is washed with water followed by 0.23 M glycine HCl (pH 2.6) to remove any non-conjugated antibody or extraneous protein. The column is then equilibrated in phosphate buffered saline (pH 7.3) together with appropriate membrane solubilizing agents such as detergents and the cell culture supernatants or cell extracts containing solubilized B₁or B₁subunits are slowly passed through the column. The column is then washed with phosphate-buffered saline together with detergents until the optical density (A280) falls to background, then the protein is eluted with 0.23 M glycine-HCl (pH 2.6) together with detergents. The purified B₁protein is then dialyzed against phosphate buffered saline.
1 2 1 1307 DNA Human 1 cagagaaaac tcctccaaaa gcagctctca ctatcagaaa acccaactac agttgtgaac 60 gccttcattt tctgcctgag gtctcagtcc gtcggcccag actgaagtgc agtggcacaa 120 tcatagctcg ctgcagcctc gaccttccag gcttaaacga ttctcccacc tcagcctctc 180 gagttgctgg gaccacaggt cactgtgcat ggcatcatcc tggccccctc tagagctcca 240 atcctccaac cagagccagc tcttccctca aaatgctacg gcctgtgaca atgctccaga 300 agcctgggac ctgctgcaca gagtgctgcc gacatttatc atctccatct gtttcttcgg 360 cctcctaggg aacctttttg tcctgttggt cttcctcctg ccccggcggc aactgaacgt 420 ggcagaaatc tacctggcca acctggcagc ctctgatctg gtgtttgtct tgggcttgcc 480 cttctgggca gagaatatct ggaaccagtt taactggcct ttcggagccc tcctctgccg 540 tgtcatcaac ggggtcatca aggccaattt gttcatcagc atcttcctgg tggtggccat 600 cagccaggac cgctaccgcg tgctggtgca ccctatggcc agcggaaggc agcagcggcg 660 gaggcaggcc cgggtcacct gcgtgctcat ctgggttgtg gggggcctct tgagcatccc 720 cacattcctg ctgcgatcca tccaagccgt cccagatctg aacatcaccg cctgcatcct 780 gctcctcccc catgaggcct ggcactttgc aaggattgtg gagttaaata ttctgggttt 840 cctcctacca ctggctgcga tcgtcttctt caactaccac atcctggcct ccctgcgaac 900 gcgggaggag gtcagcagga caaggtgcgg gggccgcaag gatagcaaga ccacagcgct 960 gatcctcacg ctcgtggttg ccttcctggt ctgctgggcc ccttaccact tctttgcctt 1020 cctggaattc ttattccagg tgcaagcagt ccgaggctgc ttttgggagg acttcattga 1080 cctgggcctg caattggcca acttctttgc cttcactaac agctccctga atccagtaat 1140 ttatgtcttt gtgggccggc tcttcaggac caaggtctgg gaactttata aacaatgcac 1200 ccctaaaagt cttgctccaa tatcttcatc ccataggaaa gaaatcttcc aacttttctg 1260 gcggaattaa aacagcattg aaccaagaaa aaaaaaaaaa aaaaaaa 1307 2 353 PRT Human 2 Met Ala Ser Ser Trp Pro Pro Leu Glu Leu Gln Ser Ser Asn Gln Ser 1 5 10 15 Gln Leu Phe Pro Gln Asn Ala Thr Ala Cys Asp Asn Ala Pro Glu Ala 20 25 30 Trp Asp Leu Leu His Arg Val Leu Pro Thr Phe Ile Ile Ser Ile Cys 35 40 45 Phe Phe Gly Leu Leu Gly Asn Leu Phe Val Leu Leu Val Phe Leu Leu 50 55 60 Pro Arg Arg Gln Leu Asn Val Ala Glu Ile Tyr Leu Ala Asn Leu Ala 65 70 75 80 Ala Ser Asp Leu Val Phe Val Leu Gly Leu Pro Phe Trp Ala Glu Asn 85 90 95 Ile Trp Asn Gln Phe Asn Trp Pro Phe Gly Ala Leu Leu Cys Arg Val 100 105 110 Ile Asn Gly Val Ile Lys Ala Asn Leu Phe Ile Ser Ile Phe Leu Val 115 120 125 Val Ala Ile Ser Gln Asp Arg Tyr Arg Val Leu Val His Pro Met Ala 130 135 140 Ser Gly Arg Gln Gln Arg Arg Arg Gln Ala Arg Val Thr Cys Val Leu 145 150 155 160 Ile Trp Val Val Gly Gly Leu Leu Ser Ile Pro Thr Phe Leu Leu Arg 165 170 175 Ser Ile Gln Ala Val Pro Asp Leu Asn Ile Thr Ala Cys Ile Leu Leu 180 185 190 Leu Pro His Glu Ala Trp His Phe Ala Arg Ile Val Glu Leu Asn Ile 195 200 205 Leu Gly Phe Leu Leu Pro Leu Ala Ala Ile Val Phe Phe Asn Tyr His 210 215 220 Ile Leu Ala Ser Leu Arg Thr Arg Glu Glu Val Ser Arg Thr Arg Cys 225 230 235 240 Gly Gly Arg Lys Asp Ser Lys Thr Thr Ala Leu Ile Leu Thr Leu Val 245 250 255 Val Ala Phe Leu Val Cys Trp Ala Pro Tyr His Phe Phe Ala Phe Leu 260 265 270 Glu Phe Leu Phe Gln Val Gln Ala Val Arg Gly Cys Phe Trp Glu Asp 275 280 285 Phe Ile Asp Leu Gly Leu Gln Leu Ala Asn Phe Phe Ala Phe Thr Asn 290 295 300 Ser Ser Leu Asn Pro Val Ile Tyr Val Phe Val Gly Arg Leu Phe Arg 305 310 315 320 Thr Lys Val Trp Glu Leu Tyr Lys Gln Cys Thr Pro Lys Ser Leu Ala 325 330 335 Pro Ile Ser Ser Ser His Arg Lys Glu Ile Phe Gln Leu Phe Trp Arg 340 345 350 Asn

Claims

What is claimed is:

1. An isolated and purified DNA molecule which encodes a bradykinin B₁receptor or a functional derivative thereof.

2. The isolated and purified DNA molecule of claim 1, having a nucleotide sequence:

CAGAGAAAACTCCTCCAAAAGCAGCTCTCACTATCAGAAAACCCAACTAC (SEQ. ID. NO.:1) AGTTGTGAACGCCTTCATTTTCTGCCTGAGGTCTCAGTCCGTCGGCCCAG ACTGAAGTGCAGTGGCACAATCATAGCTCGCTGCAGCCTCGACCTTCCAG GCTTAAACGATTCTCCCACCTCAGCCTCTCGAGTTGCTGGGACCACAGGT CACTGTGCATGGCATCATCCTGGCCCCCTCTAGAGCTCCAATCCTCCAAC CAGAGCCAGCTCTTCCCTCAAAATGCTACGGCCTGTGACAATGCTCCAGA AGCCTGGGACCTGCTGCACAGAGTGCTGCCGACATTTATCATCTCCATCT GTTTCTTCGGCCTCCTAGGGAACCTTTTTGTCCTGTTGGTCTTCCTCCTG CCCCGGCGGCAACTGAACGTGGCAGAAATCTACCTGGCCAACCTGGCAGC CTCTGATCTGGTGTTTGTCTTGGGCTTGCCCTTCTGGGCAGAGAATATCT GGAACCAGTTTAACTGGCCTTTCGGAGCCCTCCTCTGCCGTGTCATCAAC GGGGTCATCAAGGCCAATTTGTTCATCAGCATCTTCCTGGTGGTGGCCAT CAGCCAGGACCGCTACCGCGTGCTGGTGCACCCTATGGCCAGCGGAAGGC AGCAGCGGCGGAGGCAGGCCCGGGTCACCTGCGTGCTCATCTGGGTTGTG GGGGGCCTCTTGAGCATCCCCACATTCCTGCTGCGATCCATCCAAGCCGT CCCAGATCTGAACATCACCGCCTGCATCCTGCTCCTCCCCCATGAGGCCT GGCACTTTGCAAGGATTGTGGAGTTAAATATTCTGGGTTTCCTCCTACCA CTGGCTGCGATCGTCTTCTTCAACTACCACATCCTGGCCTCCCTGCGAAC GCGGGAGGAGGTCAGCAGGACAAGGTGCGGGGGCCGCAAGGATAGCAAGA CCACAGCGCTGATCCTCACGCTCGTGGTTGCCTTCCTGGTCTGCTGGGCC CCTTACCACTTCTTTGCCTTCCTGGAATTCTTATTCCAGGTGCAAGCAGT CCGAGGCTGCTTTTGGGAGGACTTCATTGACCTGGGCCTGCAATTGGCCA ACTTCTTTGCCTTCACTAACAGCTCCCTGAATCCAGTAATTTATGTCTTT GTGGGCCGGCTCTTCAGGACCAAGGTCTGGGAACTTTATAAACAATGCAC CCCTAAAAGTCTTGCTCCAATATCTTCATCCCATAGGAAAGAAATCTTCC AACTTTTCTGGCGGAATTAAAACAGCATTGAACCAAGAAAAAAAAAAAAA AAAAAAA

or functional derivatives thereof.

3. The isolated and purified DNA molecule of claim 1, wherein said DNA molecule is genomic DNA.

4. An expression vector for expression of a bradykinin B₁receptor in a recombinant host, wherein said vector contains a recombinant gene encoding a bradykinin B₁receptor or functional derivaative thereof.

5. The expression vector of claim 4, wherein the expression vector contains a cloned gene encoding the bradykinin B₁receptor, having a nucleotide sequence:

CAGAGAAAACTCCTCCAAAAGCAGCTCTCACTATCAGAAAACCCAACTAC (SEQ. ID. NO.:1) AGTTGTGAACGCCTTCATTTTCTGCCTGAGGTCTCAGTCCGTCGGCCCAG ACTGAAGTGCAGTGGCACAATCATAGCTCGCTGCAGCCTCGACCTTCCAG GCTTAAACGATTCTCCCACCTCAGCCTCTCGAGTTGCTGGGACCACAGGT CACTGTGCATGGCATCATCCTGGCCCCCTCTAGAGCTCCAATCCTCCAAC CAGAGCCAGCTCTTCCCTCAAAATGCTACGGCCTGTGACAATGCTCCAGA AGCCTGGGACCTGCTGCACAGAGTGCTGCCGACATTTATCATCTCCATCT GTTTCTTCGGCCTCCTAGGGAACCTTTTTGTCCTGTTGGTCTTCCTCCTG CCCCGGCGGCAACTGAACGTGGCAGAAATCTACCTGGCCAACCTGGCAGC CTCTGATCTGGTGTTTGTCTTGGGCTTGCCCTTCTGGGCAGAGAATATCT GGAACCAGTTTAACTGGCCTTTCGGAGCCCTCCTCTGCCGTGTCATCAAC GGGGTCATCAAGGCCAATTTGTTCATCAGCATCTTCCTGGTGGTGGCCAT CAGCCAGGACCGCTACCGCGTGCTGGTGCACCCTATGGCCAGCGGAAGGC AGCAGCGGCGGAGGCAGGCCCGGGTCACCTGCGTGCTCATCTGGGTTGTG GGGGGCCTCTTGAGCATCCCCACATTCCTGCTGCGATFCATCCAAGCCGT CCCAGATCTGAACATCACCGCCTGCATCCTGCTCCTCCCCCATGAGGCCT GGCACTTTGCAAGGATTGTGGAGTTAAATATTCTGGGTTTCCTCCTACCA CTGGCTGCGATCGTCTTCTTCAACTACCACATCCTGGCCTCCCTGCGAAC GCGGGAGGAGGTCAGCAGGACAAGGTGCGGGGGCCGCAAGGATAGCAAGA CCACAGCGCTGATCCTCACGCTCGTGGTTGCCTTCCTGGTCTGCTGGGCC CCTTACCACTTCTTTGCCTTCCTGGAATTCTTATTCCAGGTGCAAGCAGT CCGAGGCTGCTTTTGGGAGGACTTCATTGACCTGGGCCTGCAATTGGCCA ACTTCTTTGCCTTCACTAACAGCTCCCTGAATCCAGTAATTTATGTCTTT GTGGGCCGGCTCTTCAGGACCAAGGTCTGGGAACTTTATAAACAATGCAC CCCTAAAAGTCTTGCTCCAATATCTTCATCCCATAGGAAAGAAATCTTCC AACTTTTCTGGCGGAATTAAAACAGCATTGAACCAAGAAAAAAAAAAAAA AAAAAAA

or functional derivative thereof.

6. The expression vector of claim 4, wherein the expression vector contains genomic DNA encoding the bradykinin BI receptor.

7. A recombinant host cell containing a recombinantly cloned gene encoding a bradykinin B₁receptor or functional derivative thereof.

8. The recombinant host cell of claim 7, wherein said gene encoding the bradykinin B₁receptor has a nucleotide sequence:

or functional derivative thereof.

9. The recombinant host cell of claim 7, wherein said cloned gene encoding the bradykinin B₁receptor is genomic DNA.

10. A protein, in substantially pure form which functions as a bradykinin B₁receptor.

11. The protein according to claim 10, having an amino acid sequence:

Met Ala Ser Ser Trp Pro Pro Leu Glu Leu Gln Ser Ser Asn (SEQ. ID. NO.:2) Gln Ser Gln Leu Phe Pro Gln Asn Ala Thr Ala Cys Asp Asn Ala Pro Glu Ala Trp Asp Leu Leu His Arg Val Leu Pro Thr Phe Ile Ile Ser Ile Cys Phe Phe Gly Leu Leu Gly Asn Leu Phe Val Leu Leu Val Phe Leu Leu Pro Arg Arg Gln Leu Asn Val Ala Glu Ile Tyr Leu Ala Asn Leu Ala Ala Ser Asp Leu Val Phe Val Leu Gly Leu Pro Phe Trp Ala Glu Asn Ile Trp Asn Gln Phe Asn Trp Pro Phe Gly Ala Leu Leu Cys Arg Val Ile Asn Gly Val Ile Lys Ala Asn Leu Phe Ile Ser Ile Phe Leu Val Val Ala Ile Ser Gln Asp Arg Tyr Arg Val Leu Val His Pro MET Ala Ser Gly Arg Gln Gln Arg Arg Arg Gln Ala Arg Val Thr Cys Val Leu Ile Trp Val Val Gly Gly Leu Leu Ser Ile Pro Thr Phe Leu Leu Arg Ser Ile Gln Ala Val Pro Asp Leu Asn Ile Thr Ala Cys Ile Leu Leu Leu Pro His Glu Ala Trp His Phe Ala Arg Ile Val Glu Leu Asn Ile Leu Gly Phe Leu Leu Pro Leu Ala Ala Ile Val Phe Phe Asn Tyr His Ile Leu Ala Ser Leu Arg Thr Arg Glu Glu Val Ser Arg Thr Arg Cys Gly Gly Arg Lys Asp Ser Lys Thr Thr Ala Leu Ile Leu Thr Leu Val Val Ala Phe Leu Val Cys Trp Ala Pro Tyr His Phe Phe Ala Phe Leu Glu Phe Leu Phe Gln Val Gln Ala Val Arg Gly Cys Phe Trp Glu Asp Phe Ile Asp Leu Gly Leu Gln Leu Ala Asn Phe Phe Ala Phe Thr Asn Ser Ser Leu Asn Pro Val Ile Tyr Val Phe Val Gly Arg Leu Phe Arg Thr Lys Val Trp Glu Leu Tyr Lys Gln Cys Thr Pro Lys Ser Leu Ala Pro Ile Ser Ser Ser His Arg Lys Glu Ile Phe Gln Leu Phe Trp Arg Asn

or functional derivative thereof.

12. A monospecific antibody immunologically reactive with a bradykinin B₁receptor.

13. The antibody of claim 12, wherein the antibody blocks activity of the bradykinin B₁receptor.

14. A process for expression of a bradykinin B₁receptor protein in a recombinant host cell, comprising:

(a) transferring the expression vector of claim 4 into suitable host cells; and

(b) culturing the host cells of step (a) under conditions which allow expression of the bradykinin B₁receptor protein from the expression vector.

15. A method of identifying compounds that modulate bradykinin B₁receptor activity, comprising:

(a) combining a suspected modulator of bradykinin B₁receptor activity with a bradykinin B₁receptor; and

(b) measuring an effect of the modulator on the receptor.

16. The method of claim 15, wherein the effect of the modulator on the receptor is inhibiting or enhancing binding of B₁receptor ligands.

17. The method of claim 15, wherein the effect of the modulator on the receptor is stimulation or inhibition of signal transduction mediated by B₁receptors.

18. The method of claim 17, wherein the effect of the modulator on the receptor is signal transduction mediated by B₁receptors, and said signal transduction is selected from the group consisting of phosphatidyl inositol hydrolysis, release of intracellular Ca²⁺ stores, and arachidonic acid release.

19. A compound active in the method of claim 15, wherein said compound is a modulator of a bradykinin B₁receptor.

20. A compound active in the method of claim 15, wherein said compound is an agonist or antagonist of a bradykinin B₁receptor.

21. A compound active in the method of claim 15, wherein said compound is a modulator of expression of a bradykinin B₁receptor.

22. A pharmaceutical composition comprising a compound active in the method of claim 15, wherein said compound is a modulator of bradykinin B1 receptor activity.

23. A method of treating a patient in need of such treatment for a condition which is mediated by a bradykinin B1 receptor, comprising administration of a bradykinin B1 receptor modulating compound active in the method of claim 15.

24. A method of treating a patient in need of such treatment for a condition which is mediated by a bradykinin B1 receptor and is characterized by hyperalgesia, acute inflammation or chronic inflammation, comprising administration of a bradykinin B1 receptor modulating compound active in the method of claim 15.

25. A method of identifying compounds that modulate bradykinin B₁receptor activity, comprising:

(a) combining a suspected modulator of bradykinin B₁receptor activity with a cell expressing a recombinant bradykinin B₁receptor; and

(b) measuring an effect of the modulator on the receptor.

26. The method of claim 25, wherein the effect of the modulator on the receptor in step (b) is inhibiting or or enhancing binding of B₁receptor ligands.

27. The method of claim 25, wherein the effect of the modulator on the receptor in step (b) is inhibition or enhancement of signal transduction mediated by B₁receptors.

28. The method of claim 27, wherein the signal transduction is selected from a group consisting of phosphatidyl inositol hydrolysis, release of intracellular Ca²⁺ stores, and arachidonic acid release.

29. A compound active in the method of claim 25, wherein said compound is a modulator of a bradykinin B₁receptor.

30. A compound active in the method of claim 25, wherein said compound is an agonist or antagonist of a bradykinin B₁receptor.

31. A compound active in the method of claim 25, wherein said compound is a modulator of expression of a bradykinin B₁receptor.

32. A pharmaceutical composition comprising a compound active in the method of claim 25, wherein said compound is a modulator of bradykinin B1 receptor activity.

33. A method of treating a patient in need of such treatment for a condition which is mediated by a bradykinin B1 receptor, comprising administration of a bradykinin B1 receptor modulating compound active in the method of claim 25.

34. A method of treating a patient in need of such treatment for a condition which is mediated by a bradykinin B1 receptor and is characterized by hyperalgesia, acute inflammation or chronic inflammation, comprising administration of a bradykinin B1 receptor modulating compound active in the method of claim 25.