Abstract:
Poly(ADP-ribose) polymerase-1 (PARP-1) is a central signaling enzyme in a cell nucleus. PARP-1 is a target for the development of radio and chemo sensitizing agents in cancer treatment as well as providing protection from stroke. An SH3 domain and an SH3 ligand domain have now been discovered on the PARP-1 protein. These domains are involved in PARP-1 activation. This discovery makes possible the use of bioinformatics tools for the design of new drugs and strategies for drug target selection, specifically targeting the PARP-1 enzyme.

Description:
CLAIM OF PRIORITY  
       [0001]    This application claims priority from U.S. provisional patent application Ser. No. 60/296,110, filed Jun. 7, 2001. 
     
    
     
       FIELD OF THE INVENTION  
         [0002]    The invention relates generally to cancer treatment, and in particular to overcoming cellular resistance to antitumor agents.  
         BACKGROUND OF THE INVENTION  
         [0003]    DNA repair is a mechanism of resistance to antitumor DNA damaging agents and to radiotherapy. Rosen EM et al.,  Cancer Invest.  17(1): 56-72 (1999). The ability of cancer cells to recognize and repair DNA damage inflicted by cancer therapy is an important mechanism of resistance to treatment. Thus, inhibition of DNA repair is a key strategy in enabling cancer therapy.  
           [0004]    Activation of the poly(ADP-ribose) polymerase-1 (PARP-1) enzyme is an immediate cellular response to genotoxic stress and is part of a genomic surveillance mechanism that responds to DNA damage, triggering signaling events that can lead to cellular recovery. PARP-1 is specifically activated by binding to DNA strand breaks. PARP-1 has been shown to be a target for the development of radio and chemo sensitizing agents in cancer treatment as well as providing protection from stroke. Szabo C &amp; Dawson V L,  Trends Pharmacol Sci.  19(7): 287-98 (1998). Current inhibitors target a conserved catalytic domain of poly(ADP-Ribose) polymerase-1 (PARP-1) present in all of the PARP family members. Ruf A. et al.,  Biochemistry  37(11): 3893-900 (1998); Tentori L et al.,  Pharmacol Res.  45(2): 73-85 (2002); Jacobson M K &amp; Jacobson E L, Trends Biochem Sci. 24(11): 415-7 (1999).  
           [0005]    Knockout experiments have shown that the therapeutic benefits of PARP-1 inhibition are a direct result of the selective inhibition of PARP-1. Shall S &amp; de Murcia G,  Mutat. Res.  4601: 1-15 (2000). Although PARP-1 knockout is not lethal, it leads to genomic instability and enhances the cytotoxicity of DNA damaging agents used in cancer therapy. Several PARP-1 inhibitors are currently in preclinical development for cancer therapy. Each of these inhibitors targets the binding site of the required substrate of the enzyme, nicotinamide adenine dinucleotide (NAD). White A W et al.,  J. Med. Chem.  43: 4084-97 (2000).  
           [0006]    Until recently, PARP-1 was the only known enzyme with ADP-ribose polymerizing activity. PARP-1 has now been found to be one of a family of enzymes with PARP activity. Jacobson M K &amp; Jacobson E L,  Trends Biochem. Sci.  24: 415-7 (1999). Amino acid sequence comparisons of the members of the PARP family indicate that there is similarity in their NAD binding sites (pADPRT domain, see, FIG. 1A). Thus, the current inhibitors lack selectivity, because they target an NAD binding site common to all PARP family members.  
           [0007]    A double knockout of PARP-1 and PARP-2 results in an embryonic lethal. Schreiber V. et al.,  J. Biol. Chem. ( 2002). PARP-1 inhibitors have also inhibit PARP-2, thus it is likely that the current strategy of inhibitor design may lead to toxic effects. Perkins E. et al., Cancer Res. 61(10): 4175-83 (2001).  
           [0008]    Thus, while PARP-1 remains a promising therapeutic target, the discovery of multiple PARPs raises questions of inhibitor selectivity not heretofore considered.  
         SUMMARY OF THE INVENTION  
         [0009]    The invention provides the identification of a Src-homology 3 (SH3) domain (domain C; SEQ ID NO: 1) and an SH3 ligand domain (PXXP motif) (SEQ ID NO: 2) on the poly(ADP-ribose) polymerase-1 (PARP-1) protein (SEQ ID NOS: 4 and 6). The invention also provides that these domains are involved in PARP-1 activation. The mechanism of PARP-1 activation resembles that of src-tyrosine kinase activation. Accordingly, the invention provides new methods for selectively targeting the SH3 domain of PARP-1.  
           [0010]    The overall importance of this invention is a new understanding of the structural mechanisms of enzymes involved in poly ADP-ribosylation and the utilization of this new information in the design of selective inhibitors of the PARP-1 enzyme. Thus, the invention involves a paradigm shift in the design of inhibitors for this anticancer target.  
           [0011]    In one embodiment, the invention provides a method for identifying agents that activate PARP-1, including the steps of:  
           [0012]    (a) contacting a test compound with PARP-1 or a functional fragment thereof, wherein the functional fragment contains the PARP-1 SH-3 domain, the PARP-1 SH3-ligand domain, or both domains;  
           [0013]    (b) assaying whether contacting the compound results in activation of PARP-1; and  
           [0014]    (c) identifying the test compound as a compound that activates PARP-1.  
           [0015]    In another embodiment, the invention provides a method for identifying agents that inactivate PARP-1, including the steps of:  
           [0016]    (a) contacting a test compound with PARP-1 or a functional fragment thereof, wherein the functional fragment contains the PARP-1 SH-3 domain, the PARP-1 SH3-ligand domain, or both domains;  
           [0017]    (b) assaying whether contacting the compound results in inactivation or prevents activation of PARP-1; and  
           [0018]    (c) identifying the test compound as a compound that inactivates or prevents activation of PARP-1.  
           [0019]    In yet another embodiment, the invention provides a method for designing PARP-1 inhibitors, including the steps of  
           [0020]    a) providing the structure of the PARP-1 SH-3 domain or the PARP-1 SH3-ligand domain in a digital format that can be used by a molecular modeling computer program;  
           [0021]    (b) obtaining the structure of a compound suspected of molecularly interacting with the PARP-1 SH-3domain or the PARP-1 SH3-ligand domain;  
           [0022]    (c) providing the structure of the compound suspected of molecularly interacting with the PARP-1 SH-3 domain or the PARP-1 SH3-ligand domain in a digital format that can be used by the molecular modeling computer program;  
           [0023]    (d) operating the molecular modeling computer program to determine  
           [0024]    (i) whether the PARP-1 SH-3 domain molecularly interacts with the compound suspected of molecularly interacting with the PARP-1 SH-3 domain, or  
           [0025]    (ii) whether the PARP-1 SH3-ligand domain molecularly interacts with the compound suspected of molecularly interacting with the PARP-1 SH3-ligand domain; and  
           [0026]    (e) identifying a compound that interacts molecularly as a potential therapeutic agent.  
           [0027]    In a specific embodiment, small peptides with the sequence RIAPEAPV (SEQ ID NO: 7) compete with the natural ligand of PARP-1 protein to affect PARP-1 activity. 
       
    
    
     BRIEF DESCRIPTION OF THE DRAWINGS  
       [0028]    [0028]FIG. 1 is a set of graphic representations of enzymes in the PARP family. FIG. 1A shows the overall domain organization of PARP family members, PARP-1 (SEQ ID NOS: 4 and 6); PARP-2 (SEQ ID NOS: 9 and 11); PARP-3 (SEQ ID NO: 13); tankyrase (SEQ ID NO: 15) and vault-PARP (SEQ ID NO: 17). All PARPs contain a conserved poly ADP-ribosylation domain. Some also contain a DNA binding domain (A, A′, A″) and protein interaction domains (D, G). The conserved ADPRT-fold also found in bacterial toxins (domain F) is shown in the ribbon diagram of the structure of CF-PARP-1. As provided in this invention, PARP-1 contains a SH3 domain (C) and SH3 ligand. FIG. 1B shows the activation mechanism of PARP-1 described in this application, involving the formation of a PARP-1 homodimer through the intermolecular interaction of an SH3 and SH3 ligand domains.  
         [0029]    [0029]FIG. 2 is a pictorial description of the ADP-ribose polymer cycle. Polymer biosynthesis involves the action of PARP-1, which utilizes NAD. ADP-ribose polymers are short lived and degraded by poly(ADP-ribose) glycohydrolase (PARG).  
         [0030]    [0030]FIG. 3 is a ribbon drawing of the catalytic fragment of PARP-1 (CF-PARP-1). The N-terminal all alpha domain is on the left side of the figure and the ADP-ribosyltransferase domain or ADPRT on the right. The all alpha domain forms a pocket for the binding of the adenine portion the NAD substrate (also known as the donor site). The ADPRT fold binds the acceptor site or elongating poly(ADP-ribose) polymer. The PXXP SH3 ligand (SEQ ID NO: 2) lies in a loop at the interface between the all alpha domain and the ADPRT fold. The gain of function mutation L613F (SEQ ID NO: 18) maps to the all alpha helical domain right at the interface where the PXXP motif is localized.  
         [0031]    [0031]FIG. 4 shows the structure of CF-PARP-1 and its inhibitor complexes. The NAD substrate binding site (donor site) with the adenine moiety binding is in a deep pocket, while the nicotinamide portion is localized in a shallow pocket next to the terminal ADP-ribose unit of the polymer (acceptor site).  
         [0032]    [0032]FIG. 5 is a diagram of the tertiary structure of a typical SH3 module, showing the surface responsible for recognition of the PXXP ligand. Two clusters of aromatic residues in the sequence form the peptide-binding surface. The conserved YDF motif (SEQ ID NO: 19) is found at the N-terminal end of the SH3 sequence at the beginning of the first loop (also known as RT-loop). The WXXPXXY motif (SEQ ID NO: 20) is found at the C-terminal end just before the very last strand. The two loops surrounding the peptide-binding surface contribute to the specificity of the interaction.  
         [0033]    [0033]FIG. 6 is a sequence alignment of a select group of SH3 domains (top 7 sequences) whose structures have been determined and deposited in the PDB database (first three letters of the sequence identification indicates the PDB code): 1AEY (SEQ ID NO: 21); 1AOJ_A (SEQ ID NO: 22); 1AZE_A (SEQ ID NO: 23); 1AON_B (SEQ ID NO: 24); 1ABO_A (SEQ ID NO: 25); 1ARK (SEQ ID NO: 26); P53BP (SEQ ID NO: 29). The bottom 6 sequences are those from the C domain of PARP-1 from mouse (P_mussh3; SEQ ID NO: 28), rat (P_ratsh3; SEQ ID NO: 29), human (P_humsh3; SEQ ID NO: 30), bovine (P_bovsh3; SEQ ID NO: 31), chicken (P_chksh3; SEQ ID NO: 32) and Xenopus (P_xensh3; SEQ ID NO: 33). 
     
    
     DETAILED DESCRIPTION OF THE INVENTION  
       [0034]    PARP-1 and the unique post-translational modification it catalyzes have previously been considered to function only in the cellular surveillance of genotoxic stress. However, the recent identification of multiple members of a PARP family might force a revision and expansion of this concept.  
         [0035]    PARP-1 is a unique 114 kDa multidomain biosensor that recognizes DNA strand breaks introduced in the genome of eukaryotic cells exposed to radiation or genotoxic agents. The recognition of DNA nicks by two zinc fingers domains of PARP-1 (domain A, FIG. 1), found at its N-terminus, triggers the activity of the catalytic of CF-PARP-1 (domain E+F, FIG. 1) by 500-fold. PARP-1 attaches ADP-ribose (ADPR) to itself (domain D, FIG. 1A) and a growing array of nuclear protein acceptors using nicotinamide adenine dinucleotide (NAD) as a substrate. PARP-1 synthesizes ADP-ribose polymers from NAD +  by attaching NAD +  to glutamic acid of acceptor proteins such as histones, P53 and proteins involved in the formation of DNA repair complexes, such as the Base Excision repair complex (BASC), DNA polβ and XRCC1. The NAD is covalently linked to the terminal ADP-ribose moiety of the elongating ADP-ribose polymer. Ruf A et al.,  Proc. Natl. Acad. Sci. USA  93(15): 7481-5 (1996).  
         [0036]    The active site of all PARPs contain a conserved glutamic acid residue which enables a nucleophilic attack on the glycosidic bond to the nicotinamide portion of NAD by the 2′ hydroxyl of the terminal ADPR unit of the terminal polymer. The adenine portion of NAD binds in a deep pocket of the CF-PARP-1 structure, while the nicotinamide portion of NAD binds in a shallow cavity.  
         [0037]    The use of NAD +  as a substrate by PARP-1 establishes a link between poly ADP-ribosylation and the energy status of the cell. In situations of massive DNA damage, PARP-1 is hyperactivated. NAD +  depletion follows, resulting in cellular necrosis. Thus, regulation of PARP-1 activity is at a crucial intersection in the cellular fate.  
         [0038]    The observation that there is essentially no detectable poly(ADP-ribose) in resting cells suggests that PARPs are generally inactive and, therefore, tightly regulated in vivo. Smith S,  Trends Biochem. Sci.  26: 174-179 (2001).  
         [0039]    Cancer cells are able to evade programmed cell death (apoptosis) by a mechanism that involves PARP-1 inactivation through cleavage by Caspase-3. Smulson M E et al.,  Adv. Enzyme Regul.  40: 183-215 (2000). Consequently, cancer cells retain the ability to signal DNA repair in response to single strand breaks. PARP-1 inhibition in cancer cells mimics its apoptotic inactivation and disables recovery of cancer cells exposed to radiologic or chemotherapeutic agents.  
         [0040]    Current inhibitors of PARP-1 have targeted the catalytic fragment of PARP-1, which contains an NAD binding site. Bousquet J A et al.,  Biochemistry  39: 7722-35 (2000). The current inhibitors of PARP-1 are derivatives of benzamides and fused ring heterocycles that bind to the nicotinamide cavity and inhibit PARP-1 by competing with NAD substrate. U.S. Pat. Nos. 6,201,020, 6,121,278, 5,587,384, 5,215,738; 5,041,653 and 5,032,617. However, because all PARPs contain this conserved binding, the current PARP-1 inhibitors lack selectivity.  
         [0041]    This invention addresses this selectivity issue by providing an understanding of the mechanism of PARP-1 activation, at the molecular level. As described below, the invention puts forward the involvement of an SH3 domain (domain C, FIG. 1; SEQ ID NO: 1) and an SH3-ligand domain (PXXP motif; SEQ ID NO: 2).  
         [0042]    This invention provides a paradigm shift in the design of PARP-1 inhibitors, where the molecular target is a protein interaction interface involved in triggering PARP-1 activity once PARP-1 recognizes damaged DNA, rather than the NAD +  binding site, where all current inhibitor effort has been focused. As described below, PARP-1 activation resulting from DNA strand break recognition results from the action of an SH3 protein interaction module on PARP-1 that potentiates the catalytic dimer. Accordingly, the present invention provides for the development of a new drug discovery paradigm for generation of PARP-1 inhibitors for cancer therapy, by affecting function by allosteric mechanisms. DeDecker B S,  Chem. Biol.  7(5): R103-7 (2000).  
         [0043]    Poly(ADP-ribose) polymerase-1 (PARP-1) is a Key Biosynthetic Target for Drug Discovery. The PARP-1 enzyme has been purified and the gene has been characterized. Cherney B W et al.,  Proc. Natl. Acad. Sci. USA  84(23): 8370-4 (1987); Kurosaki T et al.,  J. Biol. Chem.  262(33): 15990-7 (1987); Uchida K et al.,  Biochem. Biophys. Res. Commun.  148(2): 617-22 (1987); Auer B et al.,  DNA  8(8): 575-80 (1989). The availability of this information led to further developments: (1) structural and site directed mutagenesis studies enabling the definition of several functional domains including two zinc finger domains at the N-terminal (FIG. 1A) that bind to DNA strand breaks, an internal automodification domain similar to that found in the C-terminus of the breast cancer gene (BRCT domain), and a C-terminal catalytic fragment containing a conserved NAD + ; (2) the generation of PARP-1 “knockout” mice that, despite having a normal development and the capability of generating ADPR polymers, are very sensitive to genotoxic stress and have a shorter life span; (3) the detection of the cleavage of PARP-1 by caspases at the DED sequence motif found at the very end of the zinc finger domain (Nicholson, D W et al.,  Nature  376(6535): 37-43 (1995)); (4) the structural determination of the catalytic domain of PARP-1 (CF-PARP-1) (Ruf, A et al.,  Proc. Natl. Acad. Sci. USA  93(15): 7481-5 (1996)), which has structural homology to the ADP-ribosyl transfer (ADPRT) domain of diphtheria, cholera, pertussis and enterotoxins; and (5) the identification of PARP-1 inhibitors, targeting the shallow nicotinamide pocket, and used in cancer therapy as radio and chemosensitizing agents. White A W et al.,  J. Med. Chem.  43(22): 4084-97 (2000); Schlicker A et al.,  Int. J. Radiat. Biol.  75(1): 91-100 (1999)).  
         [0044]    Thus, PARP-1 functions as a cellular biosensor of DNA strands breaks, triggering the poly ADP-ribosylation of chromatin and DNA repair proteins. The recognition of strand breaks results in at least a 200-fold increase in enzyme activity. The catalytic domain serves two functions: (1) automodification of PARP at conserved glutamate residues localized in the BRCT domain, through the formation of dimers. Mendoza-Alvarez H &amp; Alvarez-Gonzalez R,  J. Biol. Chem.  268(30): 22575-80 (1993); and (2) the ADP-ribosylation of other protein acceptors including histones and DNA-repair complexes. The ADP-ribosylation of histones by PARP is thought to be an important step in chromatin decondensation, which may be part of an overall mechanism of freeing the damaged DNA while at the same time recruiting the action of DNA repair complexes.  
         [0045]    PARP-1 is a Member of a New Family of Poly ADP-Ribosylating Proteins. The development of PARP-1 knockout mice revealed that polymer metabolism was not disrupted in PARP-1 knockout mice. Shieh W M et al.,  J. Biol. Chem.  273(46): 30069-72 (1998). This information suggested functional redundancy in the production of poly(ADP-ribose). Two closely related PARPs (PARP-2 (SEQ ID NOS: 9 and 11) and PARP-3 (SEQ ID NO: 13)) were identified in human and Drosophila. Johansson M,  Genomics  57(3): 442-5 (1999); Ame J C et al,  J. Biol. Chem.  274(25): 17860-8 (1999); Kawamura T et al.,  Biochem. Biophys. Res. Commun.  251(1): p. 35-40 (1998).  
         [0046]    The first new PARP member identified was tankyrase (Smith S et al.,  Science  282(5393): 1484-7 (1998)), also a multidomain protein containing the protein interaction modules ankyrin repeats and SAM domains (SEQ ID NO: 15). Tankyrase is responsible for the ADP-ribosylation of TRF1, a protein involved in the assembly and disassembly of the T-loop structure found at the ends of the chromosomes. Tankyrase serves to regulate the function of TRF1 and thus, is a potentially new target for inhibiting the action of telomerase in cancer cells.  
         [0047]    The second new member of the PARP family identified was vault PARP (SEQ ID NO: 17). Kickhoefer V A et al.,  J. Cell Biol.  146(5): 917-28 (1999). Vault PARP is also a multidomain protein containing the BCRT protein interaction domain, present in PARP-1 and several DNA repair proteins. Vault PARP is a large protein-RNA complex found in the cytoplasm, and currently thought to mediate the transport of mRNA.  
         [0048]    The single conserved domain found in all PARPs is a catalytic fragment of PARP-1 (CF-PARP-1). The structure of CF-PARP-1 was recently determined by Ruf et al.,  Proc. Natl. Acad. Sci. USA  93(15): 7481-5 (1996), and revealed a conserved ADP-ribosyltransferase domain (ADPRT, domain F) core structure also found in bacterial toxins. Like ADPRTs, PARP contains an NAD +  recognition site. A detailed comparison of the structure of PARP with the toxins showed a conserved catalytic glutamic acid at the beginning of the fifth stand (β5) of the ADPRT fold (see, FIG. 4).  
         [0049]    PARP Activation Requires Self-association. The relationship between the oligomeric state of PARP-1 and its activation has been investigated by several techniques, including sedimentation equilibrium, gel permeation, electrophoretic mobility and kinetics measurements. Juarez-Salinas H et al.,  Anal. Biochem.  131(2): 410-8 (1983). PARP-1 in its activated form is a homodimer, but the structural elements required for dimerization remain unknown. The presence of the protein interaction domain, BRCT, suggests that BRCT may potentiate dimerization. BRCT domains are found in several DNA repair proteins leading to the formation of the BRCA-associated genome surveillance complex or BASC and the DNA-base excision complex (BEC). PARP-1 may have a regulatory/assembly function in the formation of these complexes through ADP-ribosylation.  
         [0050]    The structure of Drosophila PARP-1 suggested that PARP-1 protein interactions occurred through a conserved leucine zipper at the N-terminus of the BRCT domain. Uchida K et al.,  Proc. Natl. Acad. Sci. USA  90(8): p. 3481-5 (1993). Evidence in support of this model include: (1) the C-terminal apoptotic cleavage product (lacking only the zinc finger domains) inhibits dimerization and consequently PARP-1 activation (Kim, J W et al.,  J. Biol. Chem.  275(11): 8121-5 (2000)); and (2) deletion mutant analyses of PARP-1 have been used to map the dimerization domain to the vicinity of the BRCT domain containing the putative leucine zipper motif. The recent structural determination of the BRCT domain of XRCC1 (Marintchev A et al.,  Nat. Struct. Biol.  6(9): 884-93 (1999)) and sequence alignment of the BRCT family, including PARP-1-BRCT (Bork P et al.,  FASEB J.  11(1): 68-76 (1997)), maps the putative leucine zipper motif to a surface-exposed N-terminal helix (α1) of this α/β structure. In the crystal structure of XRCC1, the BRCT domain helix α1 was found to be involved in homodimerization and was proposed to mediate protein interactions in vivo.  
         [0051]    SH3 Protein Interaction Modules and Enzyme Activation. Many proteins, including the src family of tyrosine kinases, are regulated by the interaction of SH3 and SH3-ligand domains. Dalgamo DC et al.  Biopolymers  43: 383-400 (1997).  
         [0052]    Cells use protein interaction modules (SH2, SH3, EH, PDZ, WW, PTB) in the recruitment of active molecules into multiprotein signal complexes or in the activation of dormant enzymes. One of these interaction modules is the SH3 domain that binds to proline-rich peptide sequences with the consensus sequence, PXXP (SEQ ID NO: 2), which forms a left-handed polyproline type II helix (PPII). Kuriyan J &amp; Cowbum D,  Annu. Rev. Biophys. Biomol. Struct.  26: 259-88 (1997). The name SH3 stands for the conserved Src-homology domain 3 found in Src-family tyrosine kinases. Along with the SH2 domain, SH3 domains regulate the activation and the localization targeting of Src-kinases. Williams J C et al.,  Trends Biochem. Sci.  23(5): 179-84 (1998). The SH3 domain is a small (˜60 residues) domain with over 250 representative sequences in the SWISSPROT database (SEQ ID NO: 1). All SH3 domains fold into a compact structure made up of two anti-parallel beta sheets of four stands connected by loops of varying sizes (RT-loop and n-src loop, see, FIG. 4). The general peptide-binding surface of the SH3 module is made up of a cluster of aromatic residues, forming three pockets. The two prolines of the core motif PXXP (the SH3-ligand; SEQ ID NO: 2) bind to two hydrophobic pockets containing conserved aromatic residues, while a third pocket is usually lined up with negative charges and usually interacts with a positively charged residue of the ligand. Kardinal C et al.,  Ann. NY Acad. Sci.  886: 289-92 (1999).  
         [0053]    PARP-1 contains an SH3 domain and an SH3-ligand domain. During an analysis of an alignment of several PARP sequences, we found that PARP-1 contains a previously unknown SH3 domain (SEQ ID NO: 30) and a previously unknown SH3-ligand domain (SEQ ID NO: 34). FIG. 1A shows the location of the predicted SH3 and SH3-ligand domains in PARP-1 and shows that these domains are not present in the other members of the PARP family of proteins. From this analysis, the CF-fragment of PARP-1, whose structure had been determined, was found to contain a PXXP sequence localized within a surface accessible loop, which leads to the active site of PARP-1 (FIG. 3 and FIG. 5). The sequence contained a conserved arginine residue (R778, human sequence; SEQ ID NO: 4) found at the N-terminal end of the PXXP, with a three-residue spacing between R778 and the first proline P881 of the PXXP motif (see, TABLE I, below). This is one residue longer than that expected for a standard class I SH3 ligand. The proline-rich binding domain within the human PARP-1 sequence contains the sequence: RIAPPEAPNT (SEQ ID. NO: 35), conforming to the classic PXXP motif.  
         [0054]    TABLE I shows a selected portion of the sequence alignment of PARP family between residues 656-1014 found within a loop connecting beta strand 1 and 2 of the core ADPRT fold (FIG. 2). Only PARP-1 and PARP-2 contain the PXXP SH3 binding core motif, while PARP-3, tankyrase and vault-PARP show little sequence conservation in this loop, which is not only surface accessible, but also lies behind the active site of PARP-1, such that its extension residues form part of the PARP-1 active site.  
                           TABLE I                                   PARP Protein   Peptide Sequence Alignment                           PARP-1 human   GLRIAPPEAPVT-----GYMF:           PARP-1 mouse   GLRIAPPEAPVT-----GYMF:           PARP-1 rat   GLRIAPPEAPVT-----GYMF:           PARP-2 human   GLRIAHPEAPIT-----GYMF:           PARP-2 mouse   GLRVAPPEAPIT-----GYMF:           PARP-3 human   GLRIMPHS---------GGRV:           tankyrase   GFDERHAYI--------GGMF:           vault PARP   APPGYDSVHGVSQTASVTTDF:                      
 
         [0055]    The finding of the PXXP motif prompted an immediate search for regions of the PARP-1 sequence with no known function, but with a high probability of beta sheet prediction using the algorithm of Stultz C M, White J V, &amp; Smith T F,  Protein Sci.  2(3): 305-14 (1993). Since the structure of CF-PARP-1 is known, the search focused on the N-terminal fragment, which contains an assigned domain of no clear function (C domain).  
         [0056]    We performed a secondary structure prediction of PARP-1 N-terminal domain, including predictions for beta sheet, alpha helix and turns and solvent accessibility. The results support the existence of a SH3 domain within the PARP-1 C domain. Since most of the PARP-1 domains have been mapped, the secondary structure prediction focused on the region between the N-terminal zinc fingers and the BRCT domain. This region between residues 240 and 400 (human sequence) showed a 60 reside region with a mostly beta sheet prediction within the PARP-1 C domain (see, FIG. 1A).  
         [0057]    The sequence of PARP-1 between residues 280-350 was compared with sequences of other SH3 domains of known structure obtained from the Protein Data Bank (PDB) database. The Protein Data Bank is operated by Rutgers, The State University of New Jersey; the San Diego Supercomputer Center at the University of California, San Diego; and the National Institute of Standards and Technology—three members of the Research Collaboratory for Structural Bioinformatics (RCSB). FIG. 6 is a sequence alignment of a select group of SH3 domains (top 7 sequences) whose structures have been determined and deposited in the PDB database. The first three letters of the sequence identification indicates the PDB code: 1AEY (SEQ ID NO: 21); 1AOJ_A (SEQ ID NO: 22); 1AZE_A (SEQ ID NO: 23); 1AON_B (SEQ ID NO: 24); 1ABO_A (SEQ ID NO: 25); 1ARK (SEQ ID NO: 26); P53BP (SEQ ID NO: 29). The bottom 6 sequences are those from the C domain of PARP-1 from mouse (P_mussh3; SEQ ID NO: 28), rat (P_ratsh3; SEQ ID NO: 29), human (P_humsh3; SEQ ID NO: 30), bovine (P_bovsh3; SEQ ID NO: 31), chicken (P_chksh3; SEQ ID NO: 32) and Xenopus (P_xensh3; SEQ ID NO: 33).  
         [0058]    [0058]FIG. 6 shows the conserved sequences among the SH3 domains. The determination of which sequences are conserved, as well as guidance for the possible substitution of an equivalent amino acid for any amino acid in a peptide sequence, thereby maintaining the structure and function of the polypeptide, is well-known to those of skill in the molecular biological arts (see, Alberts B et al.,  Molecular Biology of the Cell.  3 rd ed.  (New York: Garland Publishing, 1994); Lewin B,  Genes VI. (New York, Oxford University Press,  1997); Lodish H et al.,  Molecular Cell Biology.  4 th ed.  (New York, W. H. Freeman and Company, 1999); Strachan T &amp; Read A P,  Human Molecular Genetics,  2 nd ed.  (New York: John Wiley &amp; Sons, 1999)). These determinations can be performed using commercially available computer programs, such as DNA Strider and Wisconsin GCG. These determinations can also be performed using more sophisticated molecular modeling software, such as Insight II, described in EXAMPLE 3.  
         [0059]    Based on the conserved sequences of the conserved sequences of the six PARP-1 SH3 domains in FIG. 6, a consensus PARP-1 SH3 domain can be written as DRVXDGMXFGALLPCXECSGQXVFKXDAYYCXGDXXAWTKCXXKTQXPXRKXWVX PKEFXEIXYL (SEQ ID NO: 1))  
         [0060]    The sequence comparison of PARP-1 C domain with that of a select group of SH3 domains with known 3D-structure revealed a set of conserved aromatic residues that map to the peptide-binding surface of SH3 domains. The sequence variability is restricted to three loop regions of the SH3; two of them are the RT and n-src loop, which surround the peptide-binding surface. The sequence comparison below also reveals that PARP-1-SH3 likely belongs to a separate subgroup. The first subgroup represented by the top six sequences represents the classic SH3 domain with recognition favoring class I peptides with an arginine residue at the N-terminal end of the PXXP motif. The second subgroup is represented by P53 binding protein (P53BP), which by far has the largest insertions in the n-src loop and the loop connecting S3 to S4. The PARP-1 vertebrate sequences form the third subgroup, which in terms of size of its loop is closer to subgroup I.  
         [0061]    As shown in FIG. 6, the hydrophobic residues that make up the SH3 core are conserved in PARP-1 SH3. Five strands (S1, S2, S3, S4, S5) form the SH3 domain. A single helical region contains a conserved proline at the beginning. PARP-1 -SH3 differs from other SH3 domain in the lack of conservation of the YDF motif (SEQ ID NO: 19) at the N-terminal end (see FIG. 5). A break in aromatic conservation is also found in P53-binding protein SH3 domain, which does not conserve the C-terminal aromatic motif FXXPXXY (SEQ ID NO: 36). This suggests that at least one set of aromatic motifs must be conserved in the SH3 module.  
         [0062]    Moreover, a published random mutagenesis experiment had been performed in PARP-1, where Trucco et al.,  Mol. Cell Biochem.  193(1-2): 53-60 (1999) were looking for activation deficient mutants of PARP-1 that were still capable of binding to DNA and retaining basal level of activity. The Trucco experiments of revealed a point mutation within domain C, G313E mutation (SEQ ID NO: 37), which generated an “activation deficient mutant”. Trucco suggested that the deficiency of the G313E mutant was a result of either an “induced strong change in the tertiary structure of the enzyme or plays an important role in self-association and/or in heterodimerization with other proteins.” Viewing the Trucco interpretation in light of our SH3 and SH3-ligand domain assignments, domain C may be involved in protein interactions, which is herein proposed to be a novel SH3, SH3-ligand interaction.  
         [0063]    Thus, the existence of a PARP-1 SH3 domain shows that PARP-1 can be activated by cytoplasmic proteins, independent of DNA damage. Based upon the deduced existence of a PARP-1-SH3 and SH3 ligand domains, a model for PARP-1 activation upon DNA recognition has been formed. The model is summarized in FIG. 1C, which shows that DNA recognition by the zinc fingers, ZI and ZII, triggers PARP-1 activation, through SH3 and SH3-ligand domains. Since PARP-1 activity is known to require dimer formation, dimerization involves the inter-molecular interaction between the SH3 domain of one monomer and the SH3-ligand of a second PARP-1 monomer. Since activation depends on DNA binding, this may trigger dimerization, as shown in FIG. 1B. According to FIG. 1B, dimerization through PARP-1-SH3 puts the automodification/BRCT domain in close proximity to the catalytic domain. FIG. 7 shows two structural possibilities.  
         [0064]    This approach to understanding the PARP-1 mechanism of action is a classic one, where the PARP-1 domains are separated from the full-length protein and the behavior of the separate units identified. Understanding how these domains function individually enables us to address their function in the context of the full length PARP-1 and determine potential coöperativity between domains during PARP-1 activation.  
         [0065]    The discovery of the proline-rich sequence in PARP-1 opens a new area for the design of selective inhibitors of PARP-1 that focuses on the mechanism of PARP-1 activation and not its catalytic activity. This approach includes the generation and use of peptide inhibitors or peptide mimics of proline-rich sequence.  
         [0066]    The importance of this finding is strengthened by the discovery of several PARP-1-like proteins containing a highly conserved catalytic domain. However, these PARP-1 inhibitors have targeted the catalytic domain and as a result, all PARP-1 inhibitors lack selectivity. By contrast, the invention provides methods of selectively targeting PARP-1 for designing therapeutic compounds that are radio- and/or chemosensitizing, for example, or for developing therapeutic agents for stroke or diabetes type 1.  
         [0067]    Jagtap et al.,  Crit. Care Med.  30(5):1071-82 (2002) developed phenanthridinone PARP-1 inhibitors and tested them in vivo and in vivo for the ability to reduce PARP activation and to protect against various cytotoxic events. The compounds were shown to have significant cryoprotective effects in vitro and significant protective effects in shock and reperfusion in vivo. Ha et al.,  Neurobiol.  7(4):225-39 (2000), showed that PARP-1 over-activation caused by cellular insults appears to play a prominent role in stroke and other neurodegenerative processes in which PARP-1 gene deletion and PARP-1 inhibiting drugs provide protection. Mabley, et al., Br.  J. Pharmacol.  133(6):909-19 (2001), investigated the role of PARP in mediating the induction of diabetes and β-cell death in the multiple-low-dose-streptozotocin (MLDS) model of type 1 diabetes. An inhibitor of PARP was found to protect mice from MLDS and prevent β-cell loss, in a dose dependent manner. These publications provide evidence that the activation of PARP contributes to β-cell damage and death in the MLDS model of diabetes, and indicate a use for PARP activation in cytokine-mediated depression of insulin secretion and cell viability in vitro.  
         [0068]    The details of one or more embodiments of the invention are set forth in the accompanying description above. Although any methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present invention, the preferred methods and materials are now described. Other features, objects, and advantages of the invention will be apparent from the description and from the claims. In the specification and the appended claims, the singular forms include plural referents unless the context clearly dictates otherwise. Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. All patents and publications cited in this specification are incorporated by reference.  
         [0069]    The following EXAMPLES are presented in order to more fully illustrate the preferred embodiments of the invention. These EXAMPLES should in no way be construed as limiting the scope of the invention, as defined by the appended claims.  
       EXAMPLE 1  
     PARP-1 Bacterial Expression Vectors  
       [0070]    A fragment containing PARP-1-SH3, residues 280-340 was PCR cloned using primers with BamHI and XhoI restriction sites. The fragment was cloned into two expression vectors, Pet28a (Novagen) and PEGX (Stratagene).  
         [0071]    The two vectors contain a histidine tag and a GST fusion protein respectively. These two tags serve two purposes: (1) for use in a single step purification of PARP-1-SH3 followed by removal of the tag using a thrombin cleavage site (The thrombin used in the cleavage reaction can be removed by using biotinylated thrombin); and (2) the PGEX vector containing the GST fusion protein also serves the purpose of enhancing the solubility of the recombinant protein.  
         [0072]    The fragment can be subcloned into a pTYB(NEB) vector, which attaches a chitin binding/intein self-cleaving domain. Chong S et al.,  Gene  192(2): 271-81 (1997). After induction with IPTG, the fusion protein is purified using a chitin-binding column. Once the fusion protein is attached to the column, DTT is added to induce the self-cleaving activity of intein. The purified native protein is eluted while the intein domain remains attached to the column.  
         [0073]    An SDS PAGE gel has been used to separate the GST purified fusion protein and the thrombin cleaved fragment, releasing the 6 kDa SH3 fragment.  
         [0074]    Both of these constructs can now be used to investigate their ability to bind to full-length PARP-1 using (1) a GST pulldown assay and (2) a surface plasmon resonance assay employing a BIACORE instrument. A PARP-1 activation assay in the presence of different domains can be used to identify interactions necessary for activation.  
       EXAMPLE 2  
     Structure/Function Testing  
       [0075]    The binding of PARP-1 to DNA strand breaks results in its activation by the interaction of SH3 and SH3-ligand domains. This model provides the rationale for the development of a new drug discovery paradigm for generation of PARP-1 inhibitors for cancer therapy.  
         [0076]    Functional Test of the Model Regarding the SH3 and SH3-ligand Domains of PARP-1. Directed mutagenesis is used to generate single amino acid changes to disrupt the peptide recognition surface of the PARP-1 SH3 domain and the SH3-ligand domain. Disruption of either domain results in a PARP-1 that is unable to be activated by DNA strand breaks.  
         [0077]    Human PARP-1 SH3 is mutated at residues that map to a conserved, and predominately aromatic surface (L293A, P294A, C295A, W318A, W333A, P336A and F339A) involved in the recognition of the proline-rich PXXP SH3-ligand (PPII). The site-directed mutants are designed to maintain structural integrity of the SH3 domain, while disrupting its ability to interact with the SH3-ligand found in CF-PARP-1 (TABLE I).  
         [0078]    In particular, the full length PARP-1 and its mutants are expressed in Sf9 insect cell/baculovirus system and purified using an affinity chromatography on 3-aminobenzamide Afi-Gel 10, which was also used in the crystallization of the CF-PARP-1. Decker P et al.,  Clin. Cancer Res.  5: 1169-72 (1999).  
         [0079]    Site directed mutagenesis is performed using QuickChange® method (Stratagene). All mutations are performed on a subclone of PARP-1 containing either the catalytic fragment of PARP-1 or the domain C of PARP-1 (see, FIG. 1A). Each subclone is engineered with unique restriction sites at both ends allowing us to piece together a point mutated full length PARP-1.  
         [0080]    The PARP-1 activation assay is as described by Rolli V et al.,  Biochemistry  36: 12147-54 (1997). The DNA binding assay is performed as described by Gradwohl G et al,  Proc. Natl. Acad. Sci. USA  87: 2990-4 (1990).  
         [0081]    Also, the PXXP motif is disrupted with the mutations, P881A, P882A and P885A, all of which disable the PPII structure and consequently disable PARP-1 activation. The ability of PARP-1 mutants to bind to DNA and its basal level of activity serves as a control that the mutations are not disabling as to catalytic activity or DNA binding.  
         [0082]    The mutations in PARP-1 SH3 could conceptually generate three potential phenotypes: (1) a constitutively active PARP-1, (2) an activation knockout of PARP-1; or (3) wild type PARP-1 (unlikely). Constitutive active mutants would suggest that the C domain keeps PARP-1 in the OFF state. An activation knockout effect suggests either: (a) that domain C is vital for turning catalytic activity ON, or (b) that the mutation has disrupted PARP-1 structure. The latter possibility is investigated as shown below. The observation of a wild type phenotype for all the seven mutations is unlikely, since there is experimental data maps an activation deficient mutant of PARP-1 to the SH3 domain.  
         [0083]    Structural Analysis by Characterization of the Solution Structure of the Wild Type and Site-Directed Mutants of the SH3 Domain by Circular Dichroism and Screening for Crystallization Conditions. Circular Dichroism (CD) measurements provide a fast, relatively simple and established method for estimating the relative content of protein secondary structure. CD measurements with the purified fragment of PARP-1 SH3 support the deduced beta sheet structure, supporting the fold model and enabling more elaborate methods such as X-ray crystallography and/or NMR. The CD experiments are also performed on site-directed mutants of PARP-1 SH3 (see, above). Since these mutations are designed to alter surface properties and not the predicted SH3, the results provide a control that the mutations have not affected the molecular structure of PARP-1 SH3.  
         [0084]    The structure determination of PARP-1 SH3 using X-ray crystallographic techniques provides the ultimate evidence of an SH3 fold.  
         [0085]    The predicted SH3 domain of PARP-1 and the site directed mutants of PARP-1 SH3 domain are expressed as a GST-fusion protein (PGEX vector, Pharmacia/LKB Technology) and a polyhistidine-tag (HIS-tag) vector (Pet28c, Novagen). The tags are useful for the purification of the predicted SH3 domain and can be cleaved off using a biotinylated thrombin, enabling the capture of the thrombin (Novagen). The CD spectra are measured and program CONTIN (Bousquet J A et al.,  Biochemistry  39, 7722-35 (2000)) used to extract secondary structure content.  
         [0086]    The expressed PARP-1 SH3 peptides are also screened for crystallization, to determine the structure using crystallographic techniques. 3D-structures of the SH3 domains of other proteins are known, thus providing guidance for the analysis of PARP-1 SH3 structure.  
         [0087]    Structure/Function Test of the Physical Interaction of PARP-1 SH3 and SH3-ligand Domains By Direct Binding Experiments. To show that PARP-1 contains a functional SH3 domain involved in its activation, the SH3 domain should be shown to bind directly to the SH3-ligand found in CF-PARP-1.  
         [0088]    Binding of the GST-SH3 fusion construct with the catalytic fragment of PARP-1 (CF-PARP-1) is assayed using glutathione beads to immobilize GST-SH3. Complex detection are done using Western blots with anti-GST and commercial PARP-1 antibodies. CF-PARP-1 mutants that disrupt the putative polyproline helix II (PPH) (SH3-ligand domain) are used as a negative control.  
         [0089]    Binding assays follow procedures used for characterization of SH3 domains. Mosser E A et al.,  Biochemistry  37: 13686-95 (1998). The GST and HIS-tags are used to immobilize the SH3 domain. Then, binding of PARP-1 SH3 to CF-PARP-1 and mutants of CF-PARP-1 with alterations in the SH3-ligand domain (PXXP motif, FIG. 3) is tested as follows: RIAAAEAP, RIAPAEAA and RIAAPEAA. Commercial antibodies against GST, HIS-tag and CF-PARP-1 are used in western blots to identify protein complexes. The ability of PARP-1 SH3 to interfere or compete with the natural SH3 ligand is tested by adding increasing amounts of PARP-1 SH3 to the activation assay of wild type PARP-1.  
       EXAMPLE 3  
     Molecular Modeling in Designing PARP-1 Inhibitors  
       [0090]    Based upon the now determined structure of the SH3 domain and SH3-ligand domain of PARP-1, known and predicted compounds can be tested by molecular simulations for interaction with PARP-1, using InsightII (Molecular Visualization (MolViz) Facility Department of Chemistry Indiana University, Bloomington, Ind. USA) and other modeling software.  
         [0091]    First, the structure of the PARP-1 SH-3domain or the PARP-1 SH3-ligand domain in a digital format that can be used by a molecular modeling computer program. The molecular modeling software generally provides information regarding which digital format is acceptable for that program (for example, for Insight II, see &lt;http://www.accelrys.com/doc/&gt;). Next, the structure of a compound suspected of molecularly interacting with the PARP-1 SH-3 domain or the PARP-1 SH3-ligand domain is obtained. The “molecularly interacting” can be covalent, ionic or other noncovalent binding. Guidance for how the compound may molecularly interact with these domains is provided above. Then, the structure of the compound suspected of molecularly interacting with the PARP-1 SH-3 domain or the PARP-1 SH3-ligand domain in a digital format that can be used by the molecular modeling computer program. The molecular modeling computer program is operated to determine (1) whether the PARP-1 SH-3 domain molecularly interacts with the compound suspected of molecularly interacting with the PARP-1 SH-3 domain, or (2) whether the PARP-1 SH3-ligand domain molecularly interacts with the compound suspected of molecularly interacting with the PARP-1 SH3-ligand domain, using the instructions provided by the molecular modeling software and methods known to those of skill in the bioinformatics art. Based upon this operation, it is possible to identify a compound that interacts molecularly as being a potential therapeutic agent.  
         [0092]    Guidance for a comparison of structural and dynamic properties of different simulation methods applied to SH3 can be found in scientific publications, including van Aalten V M F et al.,  Biophys. J.  70: 684-692 (1996), Hansson H et al.,  Biochemistry ( 2001), and Garbay C et al.,  Biochem. Pharmacol.  60(8): 1165-9 (2000), among others.  
       EXAMPLE 4  
     Structural/Functional Model of the L613F PARP-1 Mutant  
       [0093]    To achieve selective targeting of the PARP-1 enzyme, we investigated the structure of the PARP-1 protein and the mechanism of PARP-1 activation upon DNA damage recognition.  
         [0094]    The sequence of PARP-1 has a unique set of domains, including two zinc finger DNA binding domain and a conserved C-terminal domain similar to the breast cancer 1 gene (BRCA1), which is involved in protein-protein interaction also called BRCT. Deng C X &amp; Brodie S G,  BioEssays  22(8): p. 728-37 (2000); Bork P et al.,  Faseb J.  11(1): 68-76 (1997). Also, PARP-1 contains a src homology 3 like domain (SH3) and SH3 ligand domains. Macias M. J et al.,  FEBS Lett.  513(1): 30-7 (2002). Furthermore, the G313E mutation (SEQ ID NO: 37) interferes selectively with the mechanism of activation of PARP-1 and maps to the PARP-1-SH3.  
         [0095]    Based on these lines of evidence we developed a model for PARP-1 activation upon DNA recognition. Since PARP-1 activity requires dimer formation, dimerization should involve the inter-molecular interaction between the SH3 domain of one monomer and the SH3-ligand of a second PARP-1 monomer. This model is a classical approach towards understanding PARP-1 mechanism of action, since we are first separating the domains from the full length PARP-1 and then identifying their behavior as separate units. By first understanding how these domains function individually, we can then address their function in the context of the full length PARP-1 protein and determine potential coöperativity between domains during PARP-1 activation.  
         [0096]    Accordingly, we have now modeled a gain of function mutation L613F that maps to the catalytic fragment of PARP-1, whose structure has been determined. (SEQ ID NO: 18); Ruf A et al.,  Proc. Natl. Acad. Sci. USA.  93(15): 7481-5 (1996). This mutation generates a PARP-1 protein that has a catalytic power (k cat /K M ) one order of magnitude higher than wild type PARP-1, in the absence of DNA. Miranda EA et al.,  Biochem. Biophys. Res. Commun.  212(2): 317-25 (1995). The mutation maps to the catalytic fragment of PARP-1. The structure of the catalytic fragment of PARP-1 contains two domains, an all alpha domain and a conserved ADP-ribosyltransferase domain (ADPRT) (FIG. 3). The two domains interact with each other through a loop that contains a PXXP motif (SEQ ID NO: 2), which should be the ligand for the PARP-1-SH3 domain (see, FIG. 1B). The mutation L613F maps the all alpha domain of CF-PARP-1 right next to the PXXP loop. We produced the structural L613F mutant model utilizing the known structure of the catalytic fragment of PARP-1. The L613F mutation involves an amino acid change to a bulkier hydrophobic residue. This added bulkiness at position 613 affects the structure of the neighboring loop that contains our PXXP proline rich loop. This structural model is consistent with our functional model that suggests that the binding of PARP-1-SH3 to the PXXP loop found in the catalytic fragment of PARP-1 which separate the two domains (all alpha and ADPRT) operates in much the same way that the L613F alteration, which provides a bulkier side chain, affects the activity of CF-PARP-1.  
       EXAMPLE 5  
     Drugs That are Selectively Designed For PARP-1  
       [0097]    In one embodiment, small peptides with the sequence RIAPPEAPV (SEQ ID NO: 7) compete with the natural ligand of PARP-1. This sequence is unique to PARP-1 and should bind poorly to other SH3 domains, such as those that are found in cell signaling molecules such as src-kinases. We generated binding evidence utilizing the software SPOT-SH3, which has been shown to predict the ability of peptide sequences to bind to SH3 domains. Brannetti B et al.,  J. Mol. Biol.  298(2): 313-28 (2000). SPOT-SH3 has been experimentally validated. Politou, A S et al.,  J. Mol. Biol.  316(2): 305-15 (2002).  
         [0098]    Natural ligands of other SH3 domain bind their ligand PXXP sequence with a predicted score in the range 0.7 to 0.9. By contrast, by utilizing the PARP-1 SH3 ligand sequence, we obtain only a score of 0.6. This result shows that the PARP-1 proline-rich sequence RIAPPEAPV should bind poorly to other SH3 sequences, so that peptides with sequence RIAPPEAPV (SEQ ID NO: 7) selectively bind to PARP-1 and inhibit its activity.  
         [0099]    Guidance as to the amount of peptide with sequence RIAPPEAPV (SEQ ID NO: 7) that is sufficient to bind to the PARP-1 SH3 domain and inactivate the PARP-1 or functional fragment thereof is provided by comparison with the amount of inhibitors (derivatives of benzamides and fused ring heterocycles) used to target the conserved NAD binding site (pADPRT domain) of PARP-1, which present in all of the PARP family members. Ruf A. et al.,  Biochemistry  37(11): 3893-900 (1998); Tentori L et al.,  Pharmacol Res.  45(2): 73-85 (2002); Jacobson M K &amp; Jacobson E L,  Trends Biochem Sci.  24(11): 415-7 (1999). See also, U.S. Pat. Nos. 6,201,020, 6,121,278, 5,587,384, 5,215,738; 5,041,653 and 5,032,617, each incorporated herein by reference. Assays to measure an amount of a compound sufficient to affect PARP-1 activity or inhibition are commercially available (Trevigen® PARP Activity Assay Kit and Trevigen® PARP Inhibition Assay Kit; Trevigen, Inc., 8405 Helgerman Court, Gaithersburg, Md. USA 20877).  
         [0100]    The use of peptide mimics is a strategy that has already been successfully used in the design of selective inhibitors for other SH3 domain proteins. Nguyen J T et al.,  Chem. Biol.  7(7): 463-73 (2000). Now, the use of peptide mimics is a useful strategy for increasing the binding potency of peptide ligands to PARP-1-SH3.  
         [0101]    The foregoing description has been presented only for the purposes of illustration and is not intended to limit the invention to the precise form disclosed, but by the claims appended hereto.