AU2003220708B2 - Nuclear receptor ligands and ligand binding domains - Google Patents

Description

AUSTRALIA

Patents Act COMPLETE SPECIFICATION

(ORIGINAL)

Class Int. Class Application Number: Lodged: Complete Specification Lodged: Accepted: Published: Priority Related Art: Name of Applicant: The Regents of The University of California Actual Inventor(s): THOMAS S SCANLAN, JOHN D BAXTER, ROBERT J FLETTERICK, RICHARD L WAGNER, PETER J KUSHNER, JAMES L APRILETTI, BRIAN L WEST, ANDREW K

SHIAU

Address for Service and Correspondence: PHILLIPS ORMONDE FITZPATRICK Patent and Trade Mark Attorneys 367 Collins Street Melbourne 3000 AUSTRALIA Invention Title: NUCLEAR RECEPTOR LIGANDS AND LIGAND BINDING DOMAINS Our Ref 698625 POF Code: 456002/193871 The following statement is a full description of this invention, including the best method of performing it known to applicant(s): -1- WO 97/21993 PCT/US96/20778 NUCLEAR RECEPTOR LIGANDS AND LIGAND BINDING DOMAINS The present application is a divisional application from the Australian Patent Application Number 34045/00 (which is in turn a divisional application from Australian Patent Application No. 18216/97).

INTRODUCTION

Technical Field This invention relates to computational methods for designing ligands that bind to nuclear receptors, crystals of nuclear receptors, synthetic ligands of nuclear receptors and methods of using synthetic ligands.

Background Nuclear receptors represent a superfamily of proteins that specifically bind a physiologically relevant small molecule, such as hormone or vitamin. As a result of a molecule binding to a nuclear receptor, the nuclear receptor changes the ability of a cell to transcribe DNA, i.e. nuclear receptors modulate the transcription of DNA, although they may have transcription independent actions.

Unlike integral membrane receptors and membrane associated receptors, the nuclear receptors reside in either the cytoplasm or nucleus of eukaryotic cells.

Thus, nuclear receptors comprise a class of intracellular, soluble ligand-regulated transcription factors.

Nuclear receptors include receptors for glucocorticoids (GRs), androgens (ARs), mineralocorticoids (MRs), progestins (PRs). estrogens (ERs), thyroid hormones (TRs), vitamin D (VDRs), retinoids (RARs and RXRs). The so called WO 97/21993 PCT/US96/20778 2.

"orphan receptors" are also part of the nuclear receptor superfamily, as they are structurally homologous to the classic nuclear receptors, such as steroid and thyroid receptors. To date, ligands have not been identified with orphan receptors but it is likely that small molecule ligands will be discovered in the near future for this class of transcription factors. Generally, nuclear receptors specifically bind physiologically relevant small molecules with high affinity and apparent Kd's are commonly in the 0.01 20 nM range, depending on the nuclear receptor/ligand pair.

Development of synthetic ligands that specifically bind to nuclear receptors has been largely guided by the trial and error method of drug design despite the importance of nuclear receptors in a myriad of physiological processes and medical conditions such as hypertension, inflammation, hormone dependent cancers breast and prostate cancer), modulation of reproductive organ modulation, hyperthyroidism, hypercholesterolemia and obesity. Previously, new ligands specific for nuclear receptors were discovered in the absence of information on the three dimensional structure of a nuclear receptor with a bound ligand. Before the present invention, researchers were essentially discovering nuclear receptor ligands by probing in the dark and without the ability to visualize how the amino acids of a nuclear receptor held a ligand in its grasp.

Consequently, it would be advantageous to devise methods and compositions for reducing the time required to discover ligands to nuclear receptors, synthesize such compounds and administer such compounds to organisms to modulate physiological processes regulated by nuclear receptors.

SUMMARY OF THE INVENTION The present invention provides for crystals of nuclear receptor ligand binding domains with a ligand bound to the ligand binding domain (LBD). The crystals of the present invention provide excellent atomic resolution of the amino acids that interact with nuclear receptor ligand, especially thyroid receptor ligands.

The three dimensional model of a nuclear receptor LBD with a ligand bound reveals a previously unknown structure for nuclear receptors and shows that the ligand is bound in a water inaccessible binding cavity of the ligand binding domain of the nuclear receptor.

Throughout the description and claims of the specification the word "comprise" and variations of the word, such as "comprising" and "comprises", is not intended to exclude other additives, components, integers or steps.

WO 97/21993 PCT/US96/20778 3.

The present invention also provides for computational methods using three dimensional models of nuclear receptors that are based on crystals of nuclear receptor LBDs. Generally, the computational method of designing a nuclear receptor ligand determines which amino acid or amino acids of a nuclear receptor LBD interact with a chemical moiety (at least one) of the ligand using a three dimensional model of a crystallized protein comprising a nuclear receptor LBD with a bound ligand, and selecting a chemical modification (at least one) of the chemical moiety to produce a second chemical moiety with a structure that either decreases or increases an interaction between the interacting amino acid and the second chemical moiety compared to the interaction between the interacting amino acid and the corresponding chemical moiety on the natural hormone.

BRIEF DESCRIPTION OF THE DRAWINGS FIG. 1 is a diagram illustrating computational methods for designing ligands that interact with nuclear receptors of the nuclear receptor superfamily.

FIG. 2 is a schematic representation of nuclear receptor structures, indicating regions of homology within family members and functions of the various domains.

FIG. 3 shows the aligned amino acid sequences of the ligand binding domains of several members of the nuclear receptor superfamily.

FIG. 4 is a ribbon drawing of the rat TR-a LBD with secondary structure elements labelled. The ligand (magenta) is depicted as a space-filling model.

Alpha helices and coil conformations are yellow, beta strands are blue.

FIG. 5 shows two cross-sections of a space-filling model of rat TR-a exposing the ligand (magenta) tightly packed within the receptor.

FIG. 6 is a schematic of the ligand binding cavity. Residues which interact with the ligand appear approximately at the site of interaction. Hydrogen bonds are shown as dashed lines between the bonding partners; distances for each bond are listed. Non-bonded contacts are shown as radial spokes which face toward interacting atoms.

FIG. 7 is the distribution of crystallographic temperature factors in the refined rat TR-a LBD. The distribution is represented as a color gradation ranging from less than 15 (dark blue) to greater than 35 (yellow-green).

WO 97/21993 PCT/US96/20778 4.

FIG. 8 is a ribbon drawing of the rat TR-a LBD showing the c-terminal activation domain to ligand. Residues which comprise the c-terminal activation domain (Pro393-Phe405) are depicted as a stick representation. Hydrophobic residues, particularly Phe401 and Phe405 (blue) face inwards toward the ligand.

Glu403 (red) projects outward into the solvent.

FIG. 9 is an electrostatic potential surface of the rat TR-a LBD, calculated using GRAPH. Negative electrostatic potential is red; positive electrostatic potential is blue. The c-terminal activation domain forms a largely hydrophobic (white). The Glu403 is presented as a singular patch of negative charge (red).

FIG. 10 is a diagram comparing agonists and antagonists for several nuclear receptors.

FIG. 11'is the synthetic scheme for preparation of TSI, TS2, TS3, TS4 and FIG. 12 is the synthetic scheme for preparation of TS6 and TS7.

FIG. 13 is the synthetic scheme for preparation of TS8.

FIG. 14 is the synthetic scheme for preparation of TS1O.

FIG. 15 depicts the chemical structures of several TR ligands.

FIG. 16 is a graph illustrating competition assays in which T 3 and triac compete with labeled T 3 for binding to human TR-a or human TR-,3.

FIG. 17 depicts a Scatchard analysis of labelled T 3 binding to TR-ca and TR-,3.

FIG. 18 is a chart showing the effect of TS-10 on the transcriptional regulation of the DR4-ALP reporter gene in the presence or absence of T3 as assayed in TRAFal reporter cells.

FIG. 19 is a chart showing the effect of TS-10 on the transcriptional regulation of the DR4-ALP reporter gene in the presence or absence of T3 as assayed in TRAFP1 reporter cells.

FIG. 20 is a chart showing the effect of TS-10 on the transcriptional regulation of the DR4-ALP reporter gene in the presence or absence of T3 as assayed in HepG2, a liver reporter cell line.

WO 97/21993 PCT/US96/20778 FIG. 21 is a partial ribbon drawing of TR-ac LBD with T3 in the ligand binding cavity. Selected interacting amino acids are labelled, including Ile221, Ile222 and Ser260, Ala263, Ile299 and Leu 276.

FIG. 22 is a partial ribbon drawing of TR-ac LBD with T3 and Dimit superimposed in the ligand binding cavity. Interactions with Ile221, Ile222, Ala260, Ile 299 and Leu276 are labelled.

FIG. 23 is a partial ribbon drawing of TR-oa LBD with T3, illustrating the three Arginine residues (Arg228, Arg262 and Arg 266 (dark stick figures)) of the polar pocket, three water molecules HOH502, HOH503 and HOH504, with hydrogen bonds indicated by dotted lines.

FIG. 24 is a partial ribbon drawing of TR-ca LBD with triac, illustrating the three Arginine residues (dark stick figures) of the polar pocket, water molecules (HOH503, HOH504 and HOH600), with hydrogen bonds indicated by dotted lines.

FIG. 25 is a partial ribbon drawing of the TR-a LBD with T3 and triac superimposed in the ligand binding cavity. The drawing shows several interacting amino acid residues in the polar pocket that remain unchanged whether T3 or triac occupies the ligand binding cavity: Arg262, Asn179, HOH503 and HOH504, and Ser277. Both Arg228 and Arg 266 occupy two different positions, depending on whether T3 or triac is bound.

FIG. 26 is a stereochemical representation of the TRa LBD with Dimit bound.

APPENDIX 1 is an appendix of references.

APPENDIX 2 is a chart of amino acids that interact with a TR ligand, for TR complexed with Dimit, Triac, IpBr2, and T3.

DETAILED DESCRIPTION OF THE INVENTION

INTRODUCTION

The present invention provides new methods, particularly computational methods, and compositions for the generation of nuclear receptor synthetic ligands based on the three dimensional structure of nuclear receptors, particularly the thyroid receptor (herein referred to as Previously, the lack of three WO 97/21993 PCT/US96/20778 6.

dimensional structural information about the ligand binding domain of a nuclear receptor thwarted the field of nuclear receptor drug discovery, especially the absence of three dimensional structural information relating to a nuclear receptor with a ligand bound.

Described herein for the first time are crystals and three dimensional structural information from a nuclear receptor's ligand binding domain (LBD) with a ligand bound. Such crystals offer superior resolution at the atomic level and the ability to visualize the coordination of nuclear receptor ligands by amino acids that comprise the LBD. The present invention also provides computational methods for designing nuclear receptor synthetic ligands using such crystal and three dimensional structural information to generate synthetic ligands that modulate the conformational changes of a nuclear receptor's LED. Such synthetic ligands can be designed using the computational methods described herein and shown, in part, in FIG. 1. These computational methods are particularly useful in designing an antagonist or partial agonist to a nuclear receptor, wherein the antagonist or partial agonist has an extended moiety that prevents any one of a number of ligandinduced molecular events that alter the receptor's influence on the regulation of gene expression, such as preventing the normal coordination of the activation domain observed for a naturally occurring ligand or other ligands that mimic the naturally occurring ligand, such as an agonist. As described herein, synthetic ligands of nuclear receptors will be useful in modulating nuclear receptor activity in a variety of medical conditions.

APPLICABILITY TO NUCLEAR RECEPTORS The present invention, particularly the computational methods, can be used to design drugs for a variety of nuclear receptors, such as receptors for glucocorticoids (GRs), androgens (ARs),.mineralocorticoids (MRs), progestins (PRs), estrogens (ERs), thyroid hormones (TRs), vitamin D (VDRs), retinoid (RARs and RXRs) and peroxisomal proliferators (PPAP). The present invention can also be applied to the "orphan receptors," as they are structurally homologous in terms of modular domains and primary structure to classic nuclear receptors, such as steroid and thyroid receptors. The amino acid homologies of orphan WO 97/21993 PCT/US96/20778 7.

receptors with other nuclear receptors ranges from very low 15%) to in the range of 35% when compared to rat RARa and human TR-O receptors, for example. In addition, as is revealed by the X-ray crystallographic structure of the TR and structural analysis disclosed herein, the overall folding of liganded superfamily members is likely to be similar. Although ligands have not been identified with orphan receptors, once such ligands are identified one skilled in the art will be able to apply the present invention to the design and use of such ligands, as their overall structural modular motif will be similar to other nuclear receptors described herein.

Modular Functional Domains Of Nuclear receptors The present invention will usually be applicable to all nuclear receptors, as discussed herein, in part, to the patterns of nuclear receptor activation, structure and modulation that have emerged as a consequence of determining the three dimensional structures of nuclear receptors with different ligands bound, notably the three dimensional structures or crystallized protein structure of the ligand binding domains for TR-a and TR-f. Proteins of the nuclear receptor superfamily display substantial regions of amino acid homology, as described herein and known in the art see FIG. 2. Members of this family display an overall structural motif of three modular domains (which is similar to the TR three modular domain motif): 1) a variable amino-terminal domain; 2) a highly conserved DNA-binding domain (DBD); and 3) a less conserved carboxyl-terminal ligand-binding domain (LBD).

The modularity of this superfamily permits different domains of each protein to separately accomplish different functions, although the domains can influence each other. The separate function of a domain is usually preserved when a particular domain is isolated from the remainder of the protein. Using conventional protein chemistry techniques a modular domain can sometimes be separated from the parent protein. Using conventional molecular biology techniques each domain can usually be separately expressed with its original function intact or chimerics of two different nuclear receptors can be constructed, wherein the chimerics retain the WO 97/21993 PCT/US96/20778 8.

properties of the individual functional domains of the respective nuclear receptors from which the chimerics were generated.

FIG. 2 provides a schematic representation of family member structures, indicating regions of homology within family members and functions of the various domains.

Amino Terminal Domain The amino terminal domain is the least conserved of the three domains and varies markedly in size among nuclear receptor superfamily members. For example, this domain contains 24 amino acids in the VDR and 603 amino acids in the MR. This domain is involved in transcriptional activation and in some cases its uniqueness may dictate selective receptor-DNA binding and activation of target genes by specific receptor isoforms. This domain can display synergistic and antagonistic interactions with the domains of the LBD. For example, studies with mutated and/or deleted receptors show positive cooperativity of the amino and carboxy terminal domains. In some cases, deletion of either of these domains will abolish the receptor's transcriptional activation functions.

DNA-Binding Domain The DBD is the most conserved structure in the nuclear receptor superfamily. It usually contains about 70 amino acids that fold into two zinc finger motifs, wherein a zinc ion coordinates four cysteines. DBDs contain two perpendicularly oriented a-helixes that extend from the base of the first and second zinc fingers. The two zinc fingers function in concert along with non-zinc finger residues to direct nuclear receptors to specific target sites on DNA and to align receptor homodimer or heterodimer interfaces. Various amino acids in DBD influence spacing between two half-sites (usually comprised of six nucleotides) for receptor dimer binding. For example, GR subfamily and ER homodimers bind to half-sites spaced by three nucleotides and oriented as palindromes. The optimal spacings facilitate cooperative interactions between DBDs, and D box residues are part of the dimerization interface. Other regions of the DBD facilitate DNA- WO 97/21993 PCT/US96/20778 9.

protein and protein-protein interactions required for RXR homodimerization and heterodimerization on direct repeat elements.

The LBD may influence the DNA binding of the DBD, and the influence can also be regulated by ligand binding. For example, TR ligand binding influences the degree to which a TR binds to DNA as a monomer or dimer. Such dimerization also depends on the spacing and orientation of the DNA half sites.

The nuclear receptor superfamily has been subdivided into two subfamilies: 1) GR (GR, AR, MR and PR) and 2) TR (TR, VDR, RAR, RXR, and most orphan receptors) on the basis of DBD structures, interactions with heat shock proteins (hsp), and ability to form heterodimers. GR subgroup members are tightly bound by hsp in the absence of ligand. dimerize following ligand binding and dissociation of hsp, and show homology in the DNA half sites to which they bind. These half sites also tend to be arranged as palindromes. TR subgroup members tend to be bound to DNA or other chromatin molecules when unliganded, can bind to DNA as monomers and dimers, but tend to form heterodimers, and bind DNA elements with a variety of orientations and spacings of the half sites, and also show homology with respect to the nucleotide sequences of the half sites. ER does not belong to either subfamily, since it resembles the GR subfamily in hsp interactions, and the TR subfamily in nuclear localization and DNA-binding properties.

Ligand Binding Domain The LBD is the second most highly conserved domain in these receptors.

Whereas integrity of several different LBD sub-domains is important for ligand binding, truncated molecules containing only the LBD retain normal ligand-binding activity. This domain also participates in other functions, including dimerization, nuclear translocation and transcriptional activation, as described herein.

Importantly, this domain binds the ligand and undergoes ligand-induced conformational changes as detailed herein.

Most members of the superfamily, including orphan receptors, possess at least two transcription activation subdomains, one of which is constitutive and resides in the amino terminal domain and the other of which (AF-2 (also WO 97/21993 PCT/US96/20778 referenced as TAU resides in the ligand-binding domain whose activity is regulated by binding of an agonist ligand. The function of AF-2 requires an activation domain (also called transactivation domain) that is highly conserved among the receptor superfamily (approximately amino acids 1005 to 1022). Most LBDs contain an activation domain. Some mutations in this domain abolish AF-2 function, but leave ligand binding and other functions unaffected. Ligand binding allows the activation domain to serve as an interaction site for essential coactivator proteins that function to stimulate (or in some cases, inhibit) transcription.

The carboxy-terminal activation subdomain, as described herein is in close three dimensional proximity in the LBD to the ligand, so as to allow for ligands bound to the LBD to coordinate (or interact) with amino acid(s) in the activation subdomain. As described herein, the LBD of a nuclear receptor can be expressed, crystallized, its three dimensional structure determined with a ligand bound (either using crystal data from the same receptor or a different receptor or a combination thereof), and computational methods used to design ligands to its LBD, particularly ligands that contain an extension moiety that coordinates the activation domain of the nuclear receptor.

Once a computationally designed ligand (CDL) is synthesized as described herein and known in the art, it can be tested using assays to establish its activity as an agonist, partial agonist or antagonist, and affinity, as described herein. After such testing, the CDLs can be further refined by generating LBD crystals with a CDL bound to the LBD. The structure of the CDL can then be further refined using the chemical modification methods described herein for three dimensional models to improve the activity or affinity of the CDL and make second generation CDLs with improved properties, such as that of a super agonist or antagonist described herein.

NUCLEAR RECEPTOR ISOFORMS The present invention also is applicable to generating new synthetic ligands to distinguish nuclear receptor isoforms. As described herein, CDLs can be generated that distinguish between isoforms, thereby allowing the generation of WO 97/21993 PCT/US96/20778 11.

cither tissue specific or function specific synthetic ligands. For instance, GR subfamily members have usually one receptor encoded by a single gene, with the exception that there are two PR isoforms, A and B, translated from the same mRNA by alternate initiation from different AUG codons. This method is especially applicable to the TR subfamily which usually has several receptors that are encoded by two (TR) or three (RAR, RXR, and PPAR) genes or have alternate RNA splicing and such an example for TR is described herein.

NUCLEAR RECEPTOR CRYSTALS The invention provides for crystals made from nuclear receptor ligand binding domains with the ligand bound to the receptor. As exemplified in the Examples, TRs are crystallized with a ligand bound to it. Crystals are made from purified nuclear receptor LBDs that are usually expressed by a cell culture, preferably E. coli. Preferably, different crystals (co-crystals) for the same nuclear receptor are separately made using different ligands, such as a naturally occurring ligand and at least one bromo- or iodo- substituted synthetic ligand that acts as an analog or antagonist of the naturally occurring ligand. Such bromo- and iodosubstitutions act as heavy atom substitutions in nuclear receptor ligands and crystals of nuclear receptor proteins. This method has the advantage for phasing of the crystal in that it bypasses the need for obtaining traditional heavy metal derivatives. After the three dimensional structure is determined for the nuclear receptor LBD with its ligand bound, the three dimensional structure can be used in computational methods to design a synthetic ligand for the nuclear receptor and further activity structure relationships can be determined through routine testing using the assays described herein and known in the art.

Expression and Purification of other. Nuclear Receptor LBD Structures High level expression of nuclear receptor LBDs can be obtained by the techniques described herein as well as others described in the literature. High level expression in E. coli of ligand binding domains of TR and other nuclear receptors, including members of the steroid/thyroid receptor superfamily, such as the estrogen androgen mineralocorticoid progesterone (PR), WO 97/21993 PCTUS96/0778 12.

RAR, RXR and vitamin D (VDR) receptors can also be achieved. Yeast and other eukaryotic expression systems can be used with nuclear receptors that bind heat shock proteins as these nuclear receptors are generally more difficult to express in bacteria, with the exception of ER, which can be expressed in bacteria.

Representative nuclear receptors or their ligand binding domains have been cloned and sequenced: human RAR-a, human RAR-y, human RXR-a, human RXR-f, human PPAR-a, human PPAR-3, human PPAR--r, human VDR, human ER (as described in Seielstad et al., Molecular Endocrinology, vol 9:647-658 (1995), incorporated herein by reference), human GR, human PR, human MR, and human AR. The ligand binding domain of each of these nuclear receptors has been identified and is shown in FIG. 3. Using the information in FIG. 3 in conjunction with the methods described herein and known in the art, one of ordinary skill in the art could express and purify LBDs of any of the nuclear receptors, including those illustrated in FIG. 3, bind it to an appropriate ligand, and crystallize the nuclear receptor's LBD with a bound ligand.

FIG. 3 is an alignment of several members of the steroid/thyroid hormone receptor superfamily that indicates the amino acids to be included in a suitable expression vector.

Extracts of expressing cells are a suitable source of receptor for purification and preparation of crystals of the chosen receptor. To obtain such expression, a vector is constructed in a manner similar to that employed for expression of the rat TR alpha (Apriletti et al. Protein Expression and Purification, 6:368-370 (1995), herein incorporated by reference). The nucleotides encoding the amino acids encompassing the ligand binding domain of the receptor to be expressed, for example the estrogen receptor ligand binding domain (hER-LBD) (corresponding to R at position 725 to L at position 1025 as standardly aligned as shown in the FIG. are inserted into an expression vector such as the one employed by Apriletti et al (1995). For the purposes of obtaining material that will yield good crystals it is preferable to include at least the amino acids corresponding to human TR-1 positions 725 to 1025. Stretches of adjacent amino acid sequences may be included if more structural information is desired. Thus, an expression vector for the,human estrogen receptor can be made by inserting nucleotides encoding amino WO 97/21993 PCTUS96/20778 13.

acids from position 700 to the c-terminus at position 1071. Such a vector gives high yield of receptor in E. coli that can bind hormone (Seielstad et al. Molecular Endocrinology Vol 9:647-658 (1995)). However, the c-terminal region beyond position 1025 is subject to variable proteolysis and can advantageously be excluded from the construct, this technique of avoiding variable proteolysis can also be applied to other nuclear receptors.

TR-at And TR-f As Examples of Nuclear receptor LBD Structure and Function TR Expression, Purification And Crystallization As an example of nuclear receptor structure of the ligand binding domain the a- and 3- isoforms of TR are crystallized from proteins expressed from expression constructs, preferably constructs that can be expressed in E. coli.

Other expression systems, such as yeast or other eukaryotic expression systems can be used. For the TR, the LBD can be expressed without any portion of the DBD or amino-terminal domain. Portions of the DBD or amino-terminus can be included if further structural information with amino acids adjacent the LBD is desired. Generally, for the TR the LBD used for crystals will be less than 300 amino acids in length. Preferably, the TR LBD will be at least 150 amino acids in length, more preferably at least 200 amino acids in length, and most preferably at least 250 amino acids in length. For example the LBD used for crystallization can comprise amino acids spanning from Met 122 to Val 410 of the rat TR-a, Glu 202 to Asp 461 of the human TR-0.

Typically TR LBDs are purified to homogeneity for crystallization. Purity of TR LBDs is measured with SDS-PAGE, mass spectrometry and hydrophobic HPLC. The purified TR for crystallization should be at least 97.5 pure or 97.5%, preferably at least 99.0% pure or 99.0% pure, more preferably at least 99.5% pure or 99.5% pure.

Initially purification of the unliganded receptor can be obtained by conventional techniques, such as hydrophobic interaction chromatography (HPLC), ion exchange chromatography (HPLC), and heparin affinity chromatography.

To achieve higher purification for improved crystals of nuclear receptors, especially the TR subfamily and TR, it will be desirable to ligand shift purify the WO 97/21993 PCTIUS96/20778 14.

nuclear receptor using a column that separates the receptor according to charge.

such as an ion exchange or hydrophobic interaction column, and then bind the eluted receptor with a ligand, especially an agonist. The ligand induces a change in the receptor's surface charge such that when re-chromatographed on the same column, the receptor then elutes at the position of the liganded receptor are removed by the original column run with the unliganded receptor. Usually saturating concentrations of ligand are used in the column and the protein can be preincubated with the ligand prior to passing it over the column. The structural studies detailed herein indicate the general applicability of this technique for obtaining super-pure nuclear receptor LBDs for crystallization.

More recently developed methods involve engineering a "tag" such as with histidine placed on the end of the protein, such as on the amino terminus, and then using a nickle chelation column for purification, Janknecht Proc. Natl. Acad.

Sci. USA Vol 88:8972-8976 (1991) incorporated by reference.

To determine the three dimensional structure of a TR LBD, or a LBD from another member of the nuclear receptor superfamily, it is desirable to co-crystalize the LBD with a corresponding LBD ligand. In the case of TR LBD, it is preferable to separately co-crystalize it with ligands such as T3, IpBr and Dimit that differ in the heavy atoms which they contain. Other TR ligands such as those encompassed by Formula 1 described herein and known in the prior art, can also be used for the generation of co-crystals of TR LBD and TR ligands. Of the compounds encompassed by Formula 1 it is generally desirable to use at least one ligand that has at least one bromo- or iodo- substitution at the R 3 or Rs' position, preferably such compounds will be have at least two such substitutions and more preferably at least 3 such substitutions. As described herein, such substitutions are advantageously used as heavy atoms to help solve the phase problem for the three dimensional structure of the TR LBD and can be used as a generalized method of phasing using a halogen I or Br) substituted ligand, especially for nuclear receptors.

Typically purified LBD, such as TR LBD, is equilibrated at a saturating concentration of ligand at a temperature that preserves the integrity of the protein.

WO 97/21993 PCT/US96/20778 Ligand equilibration can be established between 2 and 370 C, although the receptor tends to be more stable in the 2-20* C range.

Preferably crystals are made with the hanging drop methods detailed herein. Regulated temperature control is desirable to improve crystal stability and quality. Temperatures between 4 and 25 0 C are generally used and it is often preferable to test crystallization over a range of temperatures. In the case of TR it is preferable to use crystallization temperatures from 18 to 25*C, more preferably to 23*C, and most preferably 22 0

C.

Complexes of the TR-ac LBD with a variety of agonists, including 3,5.3'triiodothyronine (T 3 3'-isopropyl-3,5-dibromothyronine (IpBr 2 3'-isopropyl-3.5dimethylthyronine (Dimit), and 3,5,3'-triiodothyroacetic acid (triac), are prepared with by methods described herein. Cocrystals of the rTR-a LBD, with ligand prebound, are prepared by vapor diffusion at ambient temperature from 15% 2methyl-2.4-pentanediol (MPD). The crystals are radiation sensitive, and require freezing to measure complete diffraction data. On a rotating anode X-ray source, the crystals diffract to 3A; synchrotron radiation extends the resolution limit significantly, to as high as 2.0A for T 3 cocrystals. The composition of the thyroid hormone, combined with the ability to prepare and cocrystallize the receptor complexed with a variety of analogs, permitted the unusual phasing strategy. This phasing strategy can be applied to the ligands of the nuclear receptors described therein by generating I and Br substitutions of such ligands. In this strategy, cocrystals of the TR LBD containing four hormone analogs that differ at the and 3' positions IpBr 2 Dimit, and triac) provided isomorphous derivatives.

For this set of analogs, the halogen substiruents (2Br and 31 atoms) function as heavy atoms, while the Dimit cocrystal (3 alkyl groups) acts as the parent. The initial 2.5A multiple isomorphous replacement/anomalous scattering/density modified electron density map allowed the LBD to be traced from skeletons created in the molecular graphics program 05 (Jones, T.A. et al. ACTA Cryst, 47:110-119 (1991), incorporated by reference herein). A model of the LBD was built in four fragments, Argl57-Gly184, Trpl86-Gly197, Serl99-Pro205, and Val210-Phe405, and refined in XPLOR using positional refinement and simulated annealing protocols. Missing residues were built with the aid of difference WO 97/21993 PCT/US96/20778 16.

density. The final model was refined to 21.8% and Rte., 24.4% for data froni45.0 to 2.2A, see Table 3.

This phasing strategy can be applied to the ligands of the nuclear receptors described herein by generating I and Br substitutions of such ligands.

THREE DIMENSIONAL STRUCTURE OF TR LBD Architecture of TR LBD As an example of the three dimensional structure of a nuclear receptor, the folding of the TR-a, LBD is shown in FIG. 4. The TR-a LBD consists of a single structural domain packed in three layers, composed of twelve a-helices, H1-12, and four short P-strands, S1-4, forming a mixed 0-sheet. The buried hormone and three antiparallel a-helices, H5-6, H9, and H10, form the central layer of the domain, as shown in FIG. 4. HI, H2, H3 and S1 form one face of the LBD, with the opposite face formed by H7, H8, H 1, and H12. The first 35 amino acids of the N-terminus (Metl22-Gln156) are not visible in the electron density maps. The three dimensional structure of the heterodimeric RXR:TR DNAbinding domains bound to DNA, amino acids Met 122 Gln151 of the TR DBD make extensive contacts with the minor groove of the DNA8. The five disordered amino acids (Arg152-Gln156), which reside between the last visible residue of the TR DBD and the first visible residue of the LBD likely represent the effective "hinge" linking the LBD and the DBD in the intact receptor.

The predominantly helical composition and the layered arrangement of secondary structure is identical to that of the unliganded hRXRa, confirming the existence of a common nuclear receptor fold between two nuclear receptors.

The TR LBD is visible beginning at Argl57, and continues in an extended coil conformation to the start of HI. A turn of a-helix, H2, covers the hormone binding cavity, immediately followed by short -strand, S1, which forms the edge of the mixed 0-sheet, parallel to S4, the outermost of the three antiparallel strands.

The chain is mostly irregular until H3 begins, antiparallel to HI. H3 bends at Ile221 and Iie222, residues which contact the ligand. The chain turns almost at the end of H3 to form an incomplete a-helix, H4..The first,buried core helix, H5-6, follows, its axis altered by a kink near the ligand at Gly 253. The helix is WO 97/21993 PCT/US96/20778 17.

composed of mostly hydrophobic sidechains interrupted by two striking exceptions: Arg262 is solvent inaccessible and interacts with the ligand carboxylate (1substituent), and Glu256 meets Arg329 from H9 and Arg375 from H11 in a polar invagination. H5-6 terminates in a short 3-strand, S2, of the four strand mixed sheet. S3 and S4 are joined through a left-handed turn, and further linked by a salt bridge between Lys284 and Asp272. Following S4, H7 and H8 form an L, stabilized by a salt bridge between Lys268 and Asp277. The turn between H7 and H8 adopts an unusual conformation, a result of interaction with ligand and its glycine rich sequence. H9 is the second core helix. antiparallel to the neighboring H5-6. Again, two buried polar sidechains are found, Glu315 and Gln320.

Glu315 forms a buried salt bridge with His358 and Arg356. The oxygen of Gln320 forms a hydrogen bond with the buried sidechain of His 175. The chain then switches back again to form H10, also antiparallel to H9. H11 extends diagonally across the full length of the molecule. Immediately after Hll, the chain forms a type 11 turn, at approximately 90' to H11. The chain then turns again to form H 12, which packs loosely against H3 and H11 as part of the hormone or ligand binding cavity. The final five amino acids at the C-terminus, Glu406 Val410, are disordered.

TR LBD's Ligand Binding Cavity As An Example Of A Nuclear Receptor's Buried Ligand Cavity The three dimensional structure of the TR LBD leads to the startling finding that ligand binding cavity of the LBD is solvent inaccessible when a T3 or its isostere is bound to the LBD. This surprising result leads to a new model of nuclear receptor three dimensional structure and function, as further described herein, particularly in the sections elucidating the computational methods of ligand design and the application of such methods to designing nuclear receptor synthetic ligands that contain extended positions that prevent normal activation of the activation domain.

Dimit, the ligand bound to the receptor, is an isostere of T 3 and a thyroid hormone agonist. Therefore the binding of Dimit should reflect that of T3, and the Dimit-bound receptor is expected to be the active conformation of TR. The ligand WO 97/21993 PCT/US96/20778 18.

is buried within the receptor, providing the hydrophobic core for a subdomain of the protein, as shown in FIG. 5 a and b. H5-6 and H9 comprise the hydrophobic core for the rest of the receptor.

An extensive binding cavity is constructed from several structural elements.

The cavity is enclosed from above by H5-6 (Met 256- Arg266), from below by H7 and H8 and the intervening loop (Leu287- Ile299), and along the sides by H2 (185-187), by the turn between S3 and S4 (Leu276-Ser277), by H3 (Phe215- Arg228), by H11 (His381-Mct388) and by H12 (Phe401-Phe405). The volume of the cavity defined by these elements, calculated by GRASP (Columbia University, USA) (600 A3), is essentially the volume of the hormone (530 The remaining volume is occupied by water molecules surrounding the amino-propionic acid substituent. FIG. 6 depicts various contacts (or interactions) between TR's LBD and the ligand.

The planes of the inner and outer (prime ring) rings of the ligand are rotated from planarity about 60* with respect to each other, adopting the 3'-distal conformation (in which the 3' substituent of the outer ring projects down and away from the inner ring). The amino-propionic acid and the outer phenolic ring assume the transoid conformation, each on opposite sides of the inner ring. The torsion angle x, for the amino- propionic acid is 300'.

The amino-propionic acid substituent is packed loosely in a polar pocket formed by side chains from H2, H4 and S3. The carboxylate group forms direct hydrogen bonds with the guanidium group of Arg228 and the amino N of Ser277.

In addition, Arg262, Arg266 and Asn179 interact with the carboxylate through water-mediated hydrogen bonds. The three arginine residues create a significantly positive local electrostatic potential, which may stabilize the negative charge of the carboxylate. No hydrogen bond is formed by the amino nitrogen. The interactions of the amino-propionic acid substituent are consistent with the fact that triac, which lacks the amino nitrogen, has a binding affinity equal to that of T 3 indicating that the amino nitrogen and longer aliphatic chain of T, do not contribute greatly to binding affinity.

The diphenyl ether, in contrast, is found buried within the hydrophobic core. The inner ring packs in a hydrophobic pocket formed by H3, H5-6, and S3.

WO 97/21993 PCT/US96/20778 19.

Pockets for the 3- and 5-methyl substituents are not completely filled, as expected since the van der waals radius of methyl substituent for Dimit is smaller than the iodine substiruent provided by the thyroid hormone T 3 Such pockets are typically to 100 cubic angstroms (although smaller pocket for substitutes are contemplated in the 40 to 80 cubic angstrom range) and could be filled more tightly with better fitting chemical substitutions, as described herein.

The outer ring packed tightly in a pocket formed by H3, H5-6, H7, H8, Hll and H12, and the loop between H7 and H8. The ether oxygen is found in a hydrophobic environment defined by Phe218, Leu287, Leu276, and Leu292. The absence of a hydrogen bond to the ether oxygen is consistent with its role in establishing the correct stereochemistry of the phenyl rings, as suggested by potent binding of hormone analogs with structurally similar linkages possessing reduced or negligible hydrogen bonding capability. The 3'-isopropyl substituent contacts Gly290 and 291. The presence of glycine at this position in the pocket can explain the observed relationship between activity and the size of 3'-substituents.

Activity is highest for 3'-isopropyl, and decreases with added bulk. The only hydrogen bond in the hydrophobic cavity is formed between the phenolic hydroxyl and His381 Ne2. The conformation of His381 is stabilized by packing contacts provided by Phe405, and Met256.

The presence of a 5' substituent larger than hydrogen affects the binding affinity for hormone. The more abundant thyroid hormone, 3,5,3',5'-tetraiodo-Lthyronine contains an iodine at this position, and binds the receptor with 2% of the affinity of T3. The structure suggests that discrimination against T4 is accomplished through the combination of steric conflict by Met256 and possibly the constraints imposed by the geometry of the hydrogen bond from His381 to the phenolic hydroxyl. The 5' position is a preferred location for introducing a chemical modification of C-H at the 5' of T3 or and TR agonist, as described herein, that produces an extension from the prime ring and results in the creation of an antagonist or partial agonist.

Deletion and antibody competition studies suggest the involvement of residues Pro162 to Val202 in ligand binding. The region does not directly contact hormone in the bound structure, although H2 packs against residues forming the WO 97/21993 PCT/US96/20778 polar pocket that interacts with the amino-propionic acid group. One role for H2, then, is to stabilize these residues in the bound state, H2, with -strands S3 and S4, might also represent a prevalent entry point for ligand, since the aminopropionic acid of the ligand is oriented toward this region. Studies of receptor binding to T 3 affinity matrices demonstrate that only a linkage to the aminopropionic acid is tolerated, suggesting that steric hindrance present in other linkages prevent binding. Furthermore, the crystallographic temperature factors suggest the coil and 0-strand region is most flexible part of the domain FIG. 7.

Participation of this region, part of the hinge domain between the DBD and LBD, in binding hormone may provide structural means for ligand binding to influence DNA binding, since parts of the Hinge domain contact DNA.

TR LBD Transcriptional Activation Helix As An Example Of A Nuclear Receptor Activation Domain In addition to the startling finding that the ligand binding cavity is solvent inaccessible when loaded with a ligand, the activation helix of TR LED presents a surface to the ligand cavity for interaction between at least one amino acid and the bound ligand. The C-terminal 17 amino acids of the TR, referred to as the activation helix or AF-2 (an example of an LBD activation domain), are implicated in mediating hormone-dependent transcriptional activation. Although, mutations of key residues within the domain decrease ligand-dependent activation it was unclear until the present invention whether such mutations directly affected ligand coordination. Although some mutations of this domain have been noted to reduce or abolish ligand binding, other mutations in more distant sites of the LBD have a similar effect.

Activation domains among nuclear receptors display an analogous three dimensional relationship to the binding cavity, which is a region of the LBD that binds the molecular recognition domain of a ligand, i.e. the activation domain presents a portion of itself to the binding cavity (but necessarily the molecular recognition domain of the ligand). Many nuclear receptors are expected to have such domains, including the retinoid receptors, RAR and RXR, the glucocorticoid receptor GR, and the estrogen receptor ER. Based upon the TR's sequence, the WO 97/21993 PCT/US96/20778 21.

domain is proposed to adopt an amphipathic helical structure. 0-sheer or mixed secondary structures, could be present as activation domains in less related nuclear receptors.

Within the activation domain, the highly conserved motif 4$XEfM, where 4 represents a hydrophobic residue, is proposed to mediate interactions between the receptors and transcriptional coactivators. Several proteins have been identified which bind the TR in a hormone-dependent fashion. One of these, Tripl, is related to a putative yeast coactivator Sugl, and also interacts with both the C-terminal activation domain and a subset of the basal transcriptional machinery, suggesting a role in transactivation by the TR. Other proteins, such as RIP140, SRCI, (Onate, S.A. et. al., Science 270:1354-1357 (1995)) and TF-1 (see also Ledouarim, et. al., EMBO J. 14:2020-2033 (1995)), also interact with other nuclear receptors in a ligand dependent manner through the C-terminal domain. Binding of these proteins can be modulated using the TR ligands described herein especially those TR ligands with extensions that sterically hinder the interaction between the highly conserved motif and other proteins.

The C-terminal activation domain of the TR forms an amphipathic helix, H12, which nestles loosely against the receptor to form part of the hormone binding cavity. The helix packs with the hydrophobic residues facing inward towards the hormone binding cavity, and the charged residues, including the highly-conserved glutamate, extending into the solvent, as shown in FIG. 8. The activation helix of TR LBD presents Phe 401 to the ligand binding cavity and permits direct coordination with the hormone i.e. such amino acids interact with the ligand forming a van der waals contact with the plane of the outer phenyl ring.

Phe 405 also interacts with His 381, perhaps stabilizing its hydrogen bonding conformation, i.e. a favorable hydrogen bond interaction. Participation of Phe 401 and Phe 405 in binding hormone explains how mutation of these residues decreases hormone binding affinity. Furthermore, the impact of these mutations on activation likely derives from a role in stabilizing the domain in the bound structure through increased hydrogen bond interaction of dipole interactions. Glu 403 extends into the solvent, emphasizing its critical role in transactivation. In its observed conformation, presented on the surface as an ordered residue, against a WO 97/21993 PCT/US96/20778 22.

background of predominantly hydrophobic surface, Glu 403 is available to interact with activator proteins described herein, as shown in FIG. 9. The other charged residues, Glu 405 and Asp 406 are disordered, as the helix frays at Phe 405.

Two other sequences in the TR, r2 and r3, activate transcription when expressed as fusion proteins with a DNA-binding domain. The sequences, discovered in the TRB, correspond to TR-a residues Prol58-Ile168 in HI (r2).

and Gly290-Leu3 19 in H8 and H9 Unlike the C-terminal activation domain, r2 and r3 do not appear to represent modular structural units in the rat TR-a LBD, nor present a surface for protein-protein interactions: the critical aspartate/glutamate residues of r3 are located on two separate helices, and do not form a single surface; the charged residues of r2 are engaged in ion pair interactions with residues of the LBD. Thus, r2 and r3 may not function as activation domains in the context of the entire receptor.

Computational Methods For Designing A Nuclear Receptor LBD LIGAND The elucidation of the three dimensional structure of a nuclear receptor ligand binding domain provides an important and useful approach for designing ligands to nuclear receptors using the computational methods described herein. By inspecting the FIGURES it can be determined that the nuclear receptor ligand is bound in a water inaccessible binding cavity in the LBD and that chemical moieties can be added to selected positions on the ligand. Such chemical modifications, usually extensions, can fill up the binding cavity represented in the FIGURES for a tighter fit (or less water) or can be used to disrupt or make contacts with amino acids not in contact with the ligand before the chemical modification was introduced or represented in a figure of the three dimensional model of the LBD. Ligands that interact with nuclear superfamily members can act as agonists, antagonists and partial agonists based on what ligand-induced conformational changes take place.

Agonists induce changes in receptors that place them in an active conformation that allows them to influence transcription, either positively or negatively. There may be several different ligand-induced changes in the receptor's conformation.

WO 97/21993. PCT/US96/20778 23.

Antagonists, bind to receptors, but fail to induce conformational changes that alter the receptor's transcriptional regulatory properties or physiologically relevant conformations. Binding of an antagonist can also block the binding and therefore the actions of an agonist.

Partial agonists bind to receptors and induce only pan of the changes in the receptors that are induced by agonists. The differences can be qualitative or quantitative. Thus, a partial agonist may induce some of the conformation changes induced by agonists, but not others, or it may only induce certain changes to a limited extent.

Ligand-induced Conformational Changes As described herein, the unliganded receptor is in a configuration that is either inactive, has some activity or has repressor activity. Binding of agonist ligands induces conformational changes in the receptor such that the receptor becomes more active, either to stimulate or repress the expression of genes. The receptors may also have non-genomic actions, some of the known types of changes and/or the sequelae of these are listed herein.

WO 97/21993 PCT/US96/20778 24.

Heat Shock Protein Binding For many of the nuclear receptors ligand binding induces a dissociation of heat shock proteins such that the receptors can form dimers in most cases, after which the receptors bind to DNA and regulate transcription.

Nuclear receptors usually have heat shock protein binding domains that present a region for binding to the LBD and can be modulated by the binding of a ligand to the LBD. Consequently, an extended chemical moiety (or more) from the ligand that stabilizes the binding or contact of the heat shock protein binding domain with the LBD can be designed using the computational methods described herein to produce a partial agonist or antagonist. Typically such extended chemical moieties will extend past and away from the molecular recognition domain on the ligand and usually past the buried binding cavity of the ligand.

Dimerization and Heterodimerization With the receptors that are associated with the hsp in the absence of the ligand, dissociation of the hsp results in dimerization of the receptors.

Dimerization is due to receptor domains in both the DBD and the LBD. Although the main stimulus for dimerization is dissociation of the hsp, the ligand-induced conformational changes in the receptors may have an additional facilitative influence. With the receptors that are not associated with hsp in the absence of the ligand, particularly with the TR, ligand binding can affect the pattern of dimerization/heterodimerization. The influence depends on the DNA binding site context, and may also depend on the promoter context with respect to other proteins that may interact with the receptors. A common pattern is to discourage monomer formation, with a resulting preference for heterodimer formation over dimer formation on DNA.

Nuclear receptor LBDs usually have dimerization domains that present a region for binding to another nuclear receptor and can be modulated by the binding of a ligand to the LBD. Consequently, an extended chemical moiety (or more) from the ligand that disrupts the binding or contact of the dimerization domain can be designed using the computational methods described herein to produce a partial agonist or antagonist. Typically such extended chemical moieties WO 97/21993 PCT/US96/20778 will extend past and away from the molecular recognition domain on the ligand and usually past the buried binding cavity of the ligand.

DNA Binding In nuclear receptors that bind to hsp, the ligand-induced dissociation of hsp with consequent dimer formation allows, and therefore, promotes DNA binding.

With receptors that are not associated (as in the absence of ligand), ligand binding tends to stimulate DNA binding of heterodimers and dimers, and to discourage monomer binding to DNA. However, with DNA containing only a single half site, the ligand tends to stimulate the receptor's binding to DNA. The effects are modest and depend on the nature of the DNA site and probably on the presence of other proteins that may interact with the receptors. Nuclear receptors usually have DBD (DNA binding domains) that present a region for binding to DNA and this binding can be modulated by the binding of a ligand to the LBD. Consequently, an extended chemical moiety (or more) from the ligand that disrupts the binding or contact of the DBD can be designed using the computational methods described herein to produce a partial agonist or antagonist. Typically such extended chemical moieties will extend past and away from the molecular recognition domain on the ligand and usually past the buried binding cavity of the ligand.

Repressor Binding Receptors that are not associated with hsp in the absence of ligand frequently act as transcriptional repressors in the absence of the ligand. This appears to be due, in part, to transcriptional repressor proteins that bind to the LBD of the receptors. Agonist binding induces a dissociation of these proteins from the receptors. This relieves the inhibition of transcription and allows the transcriptional transactivation functions of the receptors to become manifest.

Transcriptional Transactivation Functions Ligand binding induces transcriptional activation functions in two basic ways. The first is through dissociation of the hsp from receptors. This dissociation, with consequent dimerization of the receptors and their binding to WO 97/21993 PCTUS96/20778 26.

DNA or other proteins in the nuclear chromatin allows transcriptional regulatory properties of the receptors to be manifest. This may be especially true of such functions on the amino terminus of the receptors.

The second way is to alter the receptor to interact with other proteins involved in transcription. These could be proteins that interact directly or indirectly with elements of the proximal promoter or proteins of the proximal promoter. Alternatively, the interactions could be through other transcription factors that themselves interact directly or indirectly with proteins of the proximal promoter. Several different proteins have been described that bind to the receptors in a ligand-dependent manner. In addition, it is possible that in some cases, the ligand-induced conformational changes do not affect the binding of other proteins to the receptor, but do affect their abilities to regulate transcription.

Nuclear receptors or nuclear receptor LBDs usually have activation domains that present a region for binding to DNA and can be modulated by the binding of a ligand to the LBD. Consequently, an extended chemical moiety (or more) from the ligand that disrupts the binding or contact of the activation domain can be designed using the computational methods described herein to produce a partial agonist or antagonist. Typically such extended chemical moieties will extend past and away from the molecular recognition domain on the ligand and usually past the buried binding cavity of the ligand and in the direction of the activation domain, which is often a helix as seen in the three dimensional model shown in the FIGURES in two dimensions on paper or more conveniently on a computer screen.

Ligand-Induced Conformational Change Plasma proteins bind hormones without undergoing a conformational change through a static binding pocket formed between monomers or domains.

For example, the tetrameric thyroid-binding plasma protein transthyretin forms a solvent-accessible hormone-binding channel at the oligomer interface. The structure of the protein is unchanged upon binding hormone with respect to the appearance of a buried binding cavity with a ligand bound.

WO 97/21993 PCT/US96/20778 27.

However, the structural role for a ligand bound to a nuclear receptor LBD.

like rat TR-a LBD, predicts that the receptor would differ in the bound and unbound states. In the absence of hormone, the receptor would possess a cavity at its core, uncharacteristic of a globular protein. A ligand hormone) completes the hydrophobic core of the active receptor after it binds to the nuclear receptor.

Ligand binding by the receptor is a dynamic process, which regulates receptor function by inducing an altered conformation.

An exact description of the hormone-induced conformational changes requires comparison of the structures of the liganded and the unliganded TR. The structure of the unliganded human RXRao may substitute as a model for the unliganded TR. The rat TR-c LBD and human RXRa LBDs adopt a similar fold, and it is likely that the structural similarity extends to the conformational changes after ligand binding.

There are three major differences between the two structures, which indeed appear to be the result of ligand binding. First, the bound rat TR-a LBD structure is more compact, with the hormone tightly packed within the hydrophobic core of the receptor. By contrast, the unliganded human RXRa LBD contains several internal hydrophobic cavities. The presence of such cavities is unusual in folded proteins, and is likely a reflection of the unliganded state of the receptor. Two of these cavities were proposed as possible binding sites for 9-cis retinoic acid, though these multiple sites only partly overlap with the single buried binding cavity observed in the liganded rat TR-a LBD.

The second difference involves H11 in the rat TR-a LBD, which contributes part of the hormone binding cavity. Hi1, continuous in the rat TR-a LBD, is broken at Cys 432 in the RXR, forming a loop between H10 and H11 in the hRXRa. This residue corresponds to His381 in the TR, which provides a hydrogen bond to the outer ring hydroxyl of the ligand. Furthermore, the hormone binding cavity occupied by ligand in the rat TR-a LBD is interrupted in the hRXRa by the same loop, forming an isolated hydrophobic pocket in the RXR with H6 and H7. In the bound rat TR-a LBD, the corresponding helices H7 and H8 are contiguous with the binding pocket, and enclose the hormone binding cavity from below.

WO 97/21993 PCT/US96/20778 28.

The third difference between the two receptors is the position of the Cterminal activation domain. While the C-terminal activation domain forms ahelices in both receptors, the domain in the rat TR-a LBD follows a proline-rich turn, and lies against the receptor to contribute part of the binding cavity. In contrast, the activation domain in the unliganded hRXRa, is part of a longer helix which projects into the solvent.

These differences lead to a model for an alternate conformation of the TR LBD assumed in the absence of ligand. In the unliganded TR, the subdomain of the receptor surrounding the hormone binding cavity is loosely packed, with the binding cavity occluded by a partly unstructured H 1 providing a partial core for the receptor.

Upon binding hormone, residues which form a coil in the unbound receptor engage the ligand, and continues H11. The ordering of Hll could unblock the hydrophobic cavity, allowing H7 and H8 to interact with hormone. The extended hydrophobic cavity then collapses around the hormone, generating the compact bound structure.

It is possible to predict ligand-induced conformational changes in the Cterminal activation domain that rely, in part, on an extended structure in the unliganded TR that repacks upon ligand binding. The ligand- induced conformation change can be subtle since the amino acid sequence of the rat TR-a in the turn (393-PTELFPP-399) significantly reduces the propensity of the peptide chain of the rat TR-a to form an a-helix and therefore repacking can be accomplished with a minor change in volume.

After the ligand-induced conformational change occurs, it is likely that the conformation of the C-terminal activation domain in the bound structure changes packing compared to the unbound form of the receptor. Binding of the ligand improves the stability of the activation domain. The activation domain packs loosely even in the bound structure, as measured by the distribution of packing interactions for the entire LBD. The packing density for the activation domain, defined as the number of atoms within 4.5A, is 1.5 standard deviations below the mean. For comparison, another surface helix, HI, is 0.5 standard deviations below the mean and the most poorly packed part of the structure, the irregular coil WO 97/21993 PCT/US96/20778 29.

from residues Ile196-Asp206, is 2.0 standard deviations below the mean.

Moreover, the majority of packing contacts for the C-terminal domain in the bound receptor are provided either by residues which interact with ligand, such as His381, or by the ligand itself. The conformation of these residues can be expected to be different in the bound and unbound receptors, and by extension the conformation of C-terminal activation domain which relies upon these interactions.

Without the stabilization provided by a bound ligand, it is likely that the Cterminal activation domain is disordered prior to hormone binding.

The interrelation of ligand-induced conformational changes is evident as described herein. For example, His381 from H 1 and Phe405 from H12 interact in the bound structure to provide a specific hydrogen bond to the phenolic hydroxyl. The ligand-induced changes which affect HI and H12 are reinforcing, and lead to the formation of the compact, bound state.

COMPUTATIONAL METHODS USING THREE DIMENSIONAL MODELS AND EXTENSIONS OF LIGANDS The three-dimensional structure of the liganded TR receptor is unprecedented, and will greatly aid in the development of new nuclear receptor synthetic ligands, such as thyroid receptor antagonists. In addition, this receptor superfamily is overall well suited to modem methods including three-dimensional structure elucidation and combinatorial chemistry such as those disclosed in EP 335 628, U.S. patent 5,463,564, which are incorporated herein by reference.

Structure determination using X-ray crystallography is possible because of the solubility properties of the receptors. Computer programs that use crystallography data when practicing the present invention will enable the rational design of ligand to these receptors. Programs such as RASMOL can be used with the atomic coordinates from crystals generated by practicing the invention or used to practice the invention by generating three dimensional models and/or determining the structures involved in ligand binding. Computer programs such as INSIGHT and GRASP allow for further manipulation and the ability to introduce new structures.

In.addition, high throughput binding and bioactivity assays can be devised using WO 97/21993 PCT/US96/20778 purified rccombinant protein and modem reporter gene transcription assays described herein and known in the art in order to refine the activity of a CDL.

Generally the computational method of designing a nuclear receptor synthetic ligand comprises two steps: 1) determining which amino acid or amino acids of a nuclear receptor LBD interacts with a first chemical moiety (at least one) of the ligand using a three dimensional model of a crystallized protein comprising a nuclear receptor LBD with a bound ligand, and 2) selecting a chemical modification (at least one) of the first chemical moiety to produce a second chemical moiety with a structure to either decrease or increase an interaction between the interacting amino acid and the second chemical moiety compared to the interaction between the interacting amino acid and the first chemical moiety.

As shown herein, interacting amino acids form contacts with the ligand and the center of the atoms of the interacting amino acids are usually 2 to 4 angstroms away from the center of the atoms of the ligand. Generally these distances are determined by computer as discussed herein and in McRee 1993, however distances can be determined manually once the three dimensional model is made.

Examples of interacting amino acids are described in Appendix 2. See also Wagner et al., Nature 378(6558):670-697 (1995) for stereochemical figures of three dimensional models. More commonly, the atoms of the ligand and the atoms of interacting amino acids are 3 to 4 angstroms apart. The invention can be practiced by repeating steps 1 and 2 to refine the fit of the ligand to the LBD and to determine a better ligand, such as an agonist. As shown in the FIGURES the three dimensional model of TR can be represented in two dimensions to determine which amino acids contact the ligand and to select a position on the ligand for chemical modification and changing the interaction with a particular amino acid compared to that before chemical modification. The chemical modification may be made using a computer, manually using a two dimensional representation of the three dimensional model or by chemically synthesizing the ligand. The three dimensional model may be made using Appendix 2 and the FIGURES. As an additional step, the three dimensional model may be made using atomic WO 97/21993 PCT/US96/20778 31.

coordinates of nuclear receptor LBDs from crystallized protein as known in the art, see McRee 1993 referenced herein.

The ligand can also interact with distant amino acids after chemical modification of the ligand to create a new ligand. Distant amino acids are generally not in contact with the ligand before chemical modification. A chemical modification can change the structure of the ligand to make as new ligand that interacts with a distant amino acid usually at least 4.5 angstroms away from the ligand. Often distant amino acids will not line the surface of the binding cavity for the ligand, as they are too far away from the ligand to be part of a pocket or surface of the binding cavity.

The interaction between an atom of a LBD amino acid and an atom of an LBD ligand can be made by any force or attraction described in nature. Usually the interaction between the atom of the amino acid and the ligand will be the result of a hydrogen bonding interaction, charge interaction, hydrophobic interaction, van der waals interaction or dipole interaction. In the case of the hydrophobic interaction it is recognized that this is not a per se interaction between the amino acid and ligand, but rather the usual result, in part, of the repulsion of water or other hydrophilic group from a hydrophobic surface. Reducing or enhancing the interaction of the LBD and a ligand can be measured by calculating or testing binding energies, computationally or using thermodynamic or kinetic methods as known in the art.

Chemical modifications will often enhance or reduce interactions of an atom of a LBD amino acid and an atom of an LBD ligand. Steric hinderance will be a common means of changing the interaction of the LBD binding cavity with the activation domain. Chemical modifications are preferably introduced at C-H, C- and C-OH position in ligands, where the carbon is part of the ligand structure which remains the same after modification is complete. In the case of C-H, C could have 1, 2 or 3 hydrogens, but usually only one hydrogen will be replaced.

The H or OH are removed after modification is complete and replaced with the desired chemical moiety.

Because the thyroid receptor is a member of the larger superfamily of hormone-binding nuclear receptors, the rules for agonist and antagonist WO 97/21993 PCT/US96/20778 32.

development will be recognized by one skilled in the art as useful in designing ligands to the entire superfamily. Examining the structures of known agonists and antagonists of the estrogen and androgen receptors supports the generality of antagonist mechanism of action as shown in FIG. The overall folding of the receptor based on a comparison of the reported structure of the unliganded RXR and with amino acid sequences of other superfamily members reveals that the overall folding of receptors of the superfamily is similar. Thus, it is predicted from the structure that there is a general pattern of folding of the nuclear receptor around the agonist or antagonist ligand.

The three dimensional structure of a nuclear receptor with a ligand bound leads to the nonobvious observation that a nuclear receptor folds around agonist ligands, as the binding cavity fits the agonist, especially the agonist's molecular recognition domain, and antagonists commonly have chemical structures that extend beyond the ligand, especially the agonist, and would prohibit folding of the receptor around the ligand to form a buried binding cavity or other groups that have the same effect. The location of the extension could affect the folding in various ways as indicated by the structure. Such extensions on antagonists are shown in FIG. 10 for various receptors and compared to the corresponding agonist.

For example, an extension towards the carboxy-terminal activation helix affects the packing/folding of this helix into the body of the receptor. This in turn can affect the ability of this portion of the nuclear receptor to interact with other proteins or other portions of the receptor, including transcriptional transactivation functions on the opposite end of the linear receptor, or the receptor's amino terminus that may interact directly or indirectly with the carboxy-terminal transactivation domain (including helix 12). Extensions in this direction can also affect the packing of helix 11 of TR (or its analogous helix in nuclear receptors) into the body of the receptor and selectively affect dimerization and heterodimerization of receptors. An extension pointing towards helix 1 can affect the relationship of the DNA binding domain and hinge regions of the receptors with the ligand binding domain and selectively or in addition affect the receptors' WO 97/21993 PCT/US96/20778 33.

binding to DNA and/or interactions of receptors with proteins that interact with this region of the receptor. Other extensions towards helix 11 can be made to affect the packing of this helix and helices 1 and 10 and thereby dimerization.

Such chemical modifications can be assessed using the computational methods described herein. It is also possible that, in some cases, extensions may protrude through the receptor that is otherwise completely or incompletely folded around the ligand. Such protruding extensions could present a steric blockade to interactions with co-activators or other proteins.

The three.dimensional structure with the ligand buried in the binding cavity immediately offers a simple description of a nuclear receptor that has a binding cavity that contains hinges and a lid, composed of one or more structural elements, that move to accommodate and surround the ligand. The ligand to TR can be modified on specific sites with specific classes of chemical groups that will serve to leave the lid and hinge region in open, partially open or closed states to achieve partial agonist or antagonist functions. In these states, the biological response of the TR is different and so the structure can be used to design particular compounds with desired effects.

Knowledge of the three-dimensional structure of the TR-T 3 complex leads.

to a general model for agonist and antagonist design. An important novel feature of the structural data is the fact that the T 3 ligand is completely buried within the central hydrophobic core of the protein. Other ligand-receptor complexes belonging to the nuclear receptor superfamily will have a similarly buried ligand binding site and therefore this model will be useful for agonist/antagonist design for the entire superfamily.

When design of an antagonist is desired, one needs either to preserve the important binding contacts of natural hormone agonist while incorporating an "extension group" that interferes with the normal operation of the ligand-receptor complex or to generate the requisite binding affinity through the interactions of the extensions with receptor domains.

The model applied to antagonist design and described herein is called the "Extension Model." Antagonist compounds for nuclear receptors should contain the same or similar groups that facilitate high-affinity binding to the receptor, and WO 97/21993 PCT/US96/20778 34.

in addition, such compounds should contain a side chain which may be large and/or polar. This side chain could be an actual extension, giving it bulk, or it could be a side group with a charge function that differs from the agonist ligand.

For example, substitution of a CH 3 for CHOH at the 21-position, and alteration at the 1-position from an OH group to a keto group of cortisol generates glucocorticoid antagonist activity (Robsseau, et. al., J. Mol. Biol. 67:99- 115 (1972)). However, in most cases effective antagonists have more bulky extensions. Thus. the antiglucocorticoid (and antiprogestin) RU486 contains a bulky side group at the 11-position (Horwitz, K.B. Endocrine Rev. 13: 146-163 (1992)). The antagonist compound will then bind within the buried ligand binding site of the receptor with reasonably high affinity (100 nM), but the extension function will prevent the receptor-ligand complex from adopting the necessary conformation needed for transcription factor function. The antagonism (which could be in an agonist or antagonist) may manifest itself at the molecular level in a number of ways, including by preventing receptor homo/heterodimer formation at the HRE, by preventing coactivator binding to receptor monomers, homodimers or homo/heterodimers, or by a combination of these effects which otherwise prevent transcription of hormone responsive genes mediated by ligand-induced effects on the HRE. There are several antagonist compounds for nuclear receptors in the prior art (see also Horwitz, Endocrine Rev. 13:146-163 (1992), Raunnaud J.P. et. al., J. Steroid Biochem. 25:811-833 (1986), Keiel et. al., Mol. Cell.

Biol. 14:287-298 (1994) whose antagonist function can be explained by the extension hypothesis. These compounds are shown in FIG. 10 along with their agonist counterparts. Each of these antagonists contains a large extension group attached to an agonist or agonist analogue core structure. Importantly, these antagonist compounds were discovered by chance and not designed with a structure-function hypothesis such as the extension principle.

One method of design of a thyroid antagonist using the extension hypothesis is provided below as a teaching example. The three-dimensional structure of the TR-aDimit complex combined with structure-activity data published in the prior art, especially those reference herein, can be used to establish the following ligand-receptor interactions which are most critical for WO 97/21993 PCT/US96/20778 high-affinity ligand binding. A physical picture of these interactions is shown in FIG. 6. The figure describes the isolated essential contacts for ligand binding.

Because the ligand is buried in the center of the receptor, the structural spacing between these isolated interactions is also important. Thus, our present knowledge of this system dictates that, for this example, a newly designed ligand for the receptor must contain a thyronine structural skeleton, or two substituted aryl groups joined by a one-atom spacer.

The general structure for an antagonist designed by the extension hypothesis is exemplified in the following general description of the substituents of a TR antagonist (referring to Formula RI can have anionic groups such as a carboxylate. phosphonate, phosphate, sulfate or sulfite and is connected to the ring with a 0 to 3 atom linker, comprising one or more C, O, N, S atoms, and preferably a 2 carbon linker. Such R1 can be optionally substituted with an amine -NH2). R3 and R5 are small hydrophobic groups such as -Br, or -CH3.

R3 and R5 can be the same substituents or different. can be a hydrophobic group that may be larger than those of R3 and R5, such as -CH3, -isopropyl, phenyl, -benzyl, 5 and 6 ring heterocycles. is a group that can participate in a hydrogen bond as either a donor or acceptor. Such groups include -OH, -NH,, and -SH. Rs' is an important extension group that makes this compound an antagonist. can be a long chain alkyl I to 9 carbons, straight chain or branched), aryl (benzyl, phenyl and substituted benzyl and phenyl rings (e.g with halogen, alkyl (1 and 5 carbons) and optionally connected to the ring by a -CH2-), heterocycle 5 or 6 atoms, preferably 5 carbons and 1 nitrogen, or five carbons), which can optionally include polar -OH, -NHz, and cationic -NH3, N(CH)3), or anionic (carboxylate, phosphonate, phosphate or sulfate) groups. Rs' can also be a polar -OH, and cationic -NH3, N(CH3)3), and anionic (carboxylate, phosphonate, phosphate or sulfate) groups.

X is the spacer group that appropriately positions the two aromatic rings. This group is usually a one-atom spacer, such as O, S, SO, S02, NH, NZ where Z is an alkyl, CH2, CHOH, CO, C(CH3)OH, and C(CH3)(CH3). R2, R6, R2' and R6' can be and -Cl and are preferably H.

WO 97/21993 PCT/US96/20778 36.

A TR ligand can also be described as a substituted phenylated 3,5 diiodo tyrosine with substituted R5' and R3' groups. R5' can be a long chain alkyl (e.g.

4 to 9 carbons, straight chain or branched), aryl (benzyl. phenyl and substituted benzyl and phenyl rings (e.g with halogen, alkyl (1 and 5 carbons) and optionally connected to the ring by a heterocycle 5 or 6 atoms, preferably carbons and 1 nitrogen, or five carbons), which can optionally include polar (e.g.

-OH, and cationic -NH3, N(CH)3), or anionic (carboxylate, phosphonate, phosphate or sulfate) groups. R5' can also be a polar -OH, and cationic -NH3, N(CH)3), and anionic (carboxylate, phosphonate, phosphate or sulfate) groups. R3' can be -IsoPr, halogen, -CH3, alkyl (1 to 6 carbons) or aryl (benzyl, phenyl and substituted benzyl and phenyl rings (e.g with halogen, alkyl (1 and 5 carbons) and optionally connected to the ring by a heterocycle 5 or 6 atoms, preferably 5 carbons and 1 nitrogen, or five carbons), which can optionally include polar -OH, -NH,, and cationic -NH3, N(CH)3), or anionic (carboxylate, phosphonate, phosphate or sulfate) groups.

A TR antagonist can also be a modified T, agonist (having a diphenyl structure) wherein is alkyl, aryl, 5- or 6-membered heterocyclic aromatic, heteroalkyl, heteroaryl, arylalkyl, heteroaryl alkyl, polyaromatic, polyheteroaromatic, polar or charged groups, wherein said may be substituted with polar or charged groups. The R5' groups are defined, as described herein.

Using these methods the ligands of this example preferably have the following properties: 1. The compounds should bind to the TR with high affinity (for example 100 nM).

2. The compounds should bind the receptor in the same basic orientation as the natural hormone.

3. The extension group RS' should project toward the activation helix (C-terminal helix) of the receptor.

4. The appropriate substituent at RS' should perturb the activation helix from its optimal local structure needed for mediating transcription.

WO 97/21993 PCT/US96/20778 37.

Antagonists may also be designed with multiple extensions in order to block more than one aspect of the folding at any time.

TR ligands super agonists) can be designed (and synthesized) to enhance the interaction of at least one amino acid with at least one chemical moiety on the ligand's molecular recognition domain. One method is to enhance the charge and polar interactions by replacing the carboxylate of T, (R1 position) with phosphonate, phosphate, sulfate or sulfite. This enhances the interaction with Arg 262, Arg 266 and Arg 228. The interaction of at least one amino acid with at least one chemical moicty on the ligand's molecular recognition domain can also be enhanced by increasing the size of RI group to fill the space occupied by water when Dimit is bound (referring to RI). Preferably the group has a complementary charge and hydrophobicity to the binding cavity.

Another way of improving the interaction of at least one amino acid with at least one chemical moiety on the ligand's molecular recognition domain is to restrict the conformation of the dihedral angle between the two phenyl rings of the thyronine ligand in solution. In solution the planes of two phenyl rings are orthogonal where the dihedral angle is 90*. In the TR Dimit structure, the dihedral angle is close to 60*. A TR ligand design that fixes the angle between the two phenyl rings will lead to tighter binding. Such a ligand may be made by connecting the R6' and the R5 positions of a thyronine or a substituted thyroninelike diphenyl. The size of the cyclic connection can fix the angle between the two phenyl rings. Referring specifically to Formula 1, the following cyclic modifications are preferred: 1) R, is connected to 2) R 3 is connected to or 3) R, is connected to R' and R 3 is connected to R2'. The connections can be made by an alkyl or heteroalkyl chain having between 1 to 6 atoms and preferably from 2 to 4 carbon atoms or other atoms. Any position of the heteroalkyl chain can be N, O, P or S. The S and P heteroatoms along said heteroalkyl chain are in any of their possible oxidative states. The N heteroatom or any carbon along the alkyl or heteroalkyl chain may have one or more Z substituents, wherein Z is alkyl, heteroalkyl, aryl, heteroaryl, 5- or 6-membered heterocyclic aromatic.

These compounds can be claimed with the proviso that Formula 1 does not include any prior art compound as of the filing date of this application.

WO 97/21993 PCT/US96/20778 38.

The interaction of at least one amino acid with at least one chemical moicty on the ligand's molecular recognition domain can also be enhanced by selecting a chemical modification that fills the unfilled space between a TR ligand and the LBD in the area of the bridging oxygen (such as in T3, triac or Dimit). Thus, a slighter larger moiety that replaces the ether oxygen can enhance binding. Such a linker may be a mono- or geminal- disubstituted carbon group. A group approximately the same size as oxygen but with greater hydrophobicity is preferred as well as small, hydrophobic groups for the disubstituted carbon.

TR-a AND TR-O SELECTIVITY FOR THE THYROID HORMONE

RECEPTOR

Using the method described herein ligands can be designed that selectively bind to the alpha more than the beta TR. The X-ray crystallographic structure of the rat TR-a LBD provides insight into design of such ligands.

The three dimensional structure reveals that the major difference between the TR-a and TR-f in the ligand binding cavity resides in amino acid Ser 277 (with the side group -CH20H) in the rat TR-a and whose corresponding residue is 331, asparagine (with the side group -CH2CONH2), in the human TR-0. The side chain in human TR-0 is larger, charged and has a different hydrogen bonding potential, which would allow the synthesis of compounds that discriminate between this difference.

For example, in the complex of TRa with triac, Ser277 does not participate in ligand binding. The absence of a role for Ser277 (Asn331 in beta) is consistent with the equal affinity of triac for the alpha and beta isoforms, and indirectly supports the contention that alpha/beta selectivity resides in the amino acid substitution Ser277 to Asn331 and its interaction with Arg228.

In terms of ligand design, these differences mean that for 1-selective ligands, some or all of the following differences should be exploited: 1. The presence of a larger side chain asparagine.

2. The ability of the carbonyl group on the side chain to provide a strong hydrogen bond acceptor.

3. The ability of the amido group on the side chain to provide a two hydrogen bond donors.

WO 97/21993 PCT7US96/20778 39.

4. Adjustment of polarity to reorganize the trapped water in the T3 pocket.

In terms of pharmaceutical design, these differences mean that for a-selective ligands, some or all of the following differences should be exploited: 1. The presence of a smaller side group.

2. The ability of the hydroxyl on the -CH20H side group carbonyl group on the side chain to provide a weak hydrogen donor.

3. Adjustment of polarity to reorganize the trapped water in the T3 pocket.

In both cases these differences can be exploited in a number of ways. For example, they can also be used with a software set for construction of novel organic molecules such as LUDI from Biosym-MSI.

METHODS OF TREATMENT The compounds of Formula 1 can be useful in medical treatments and exhibit biological activity which can be demonstrated in the following tests: the induction of mitochondrial a-glycerophosphate dehydrogenase (GPDH:EC 1.1.99.5). This assay is particularly useful since in certain species e.g. rats it is induced specifically by thyroid hormones and thyromimetics in a close-related manner in responsive tissues e.g. liver, kidney and the heart (Westerfield, Richert, D.A. and Ruegamer, Endocrinology, 1965, 77, 802). The assay allows direct measurement in rates of a thyroid hormone-like effect of compounds and in particular allows measurement of the direct thyroid hormone-like effect on the heart; (ii) the elevation of basal metabolic rate as measured by the increase in whole body oxygen consumption (see Barker et al., Ann. N. Y. Acad. Sci., 86:545-562 (iii) the stimulation of the rate of beating of atria isolated from animals previously dosed with thyromimetrics (see Stephan et al., Biochem.

Pharmacol. (1992) 13:1969-1974; Yokoyama et al., J. Med. Chem. 38:695-707 (1995)); WO 97/21993 PCT/US96/20778 (iv) the change in total plasma cholesterol levels as determined using a cholesterol oxidase kit (for example, the Merck CHOD iodine colorimetric kit.

see also, Stephan et al. (1992)); the measurement of LDL (low density lipoprotein) and HDL (high density lipoprotein) cholesterol in lipoprotein fractions separated by ultracentrifugation; and p (vi) the change in total plasma triglyceride levels as determined using enzymatic color tests, for example the Merck System GPO-PAP method.

The compounds of Formula 1 can be found to exhibit selective thyromimetic activity in these tests, by increasing the metabolic rate of test animals, and raising hepatic GPDH levels at doses which do not significantly modify cardiac GPDH levels.

by lowering plasma cholesterol and triglyceride levels, and the ratio of LDL to HDL cholesterol at doses which do not significantly modify cardiac GPDH levels.

The compounds of Formula 1 may therefore be used in therapy, in the treatment of conditions which can be alleviated by compounds which selectively mimic the effects of thyroid hormones in certain tissues whilst having little or no direct thyromimetic effect on the heart. For example, compounds of Formula 1 which raise hepatic GPDH levels and metabolic rate at doses which do not significantly modify cardiac GPDH levels are indicated in the treatment of obesity.

Agonists of Formula 1 will lower total plasma cholesterol, the ratio of LDL-cholesterol to HDL-cholesterol and triglyceride levels at doses which do not significantly modify cardiac GPDH levels are indicated for use as general antihyperlipidaemic (antihyperlipoproteinaemic) agents i.e. in the treatment of patients having elevated plasma lipid (cholesterol and triglyceride) levels. In addition, in view of this effect on plasma cholesterol and triglyceride, they are also indicated for use as specific anti-hypercholesterolemic and antihypertriglyceridaemic agents.

Patients having elevated plasma lipid levels are considered at risk of developing coronary heart disease or other manifestations of atherosclerosis as a result of their high plasma cholesterol and/or triglyceride concentrations. Further, WO 97/21993 PCT/US96/20778 41.

since LDL-cholesterol is believed to be the lipoprotein which induces atherosclerosis, and HDL-cholesterol believed to transport cholesterol from blood vessel walls to the liver and to prevent the build up of atherosclerotic plaque, antihyperlipidemic agents which lower the ratio of LDL-cholesterol to HDL cholesterol are indicated as anti-atherosclerotic agents, herein incorporated by reference U.S. patents 4,826,876 and 5,466,861.

The present invention also provides a method of producing selective thyromimetic activity in certain tissues except the heart which comprises administering to an animal in need thereof an effective amount to produce said activity of a compound of Formula 1 or a pharmaceutically acceptable salt thereof.

The present invention also relates to a method of lowering plasma lipid levels and a method of lowering the ratio of LDL-cholesterol to HDL-clolesterol levels by suitably administering a compound of this invention or a pharmaceutically acceptable sale thereof.

In addition, compounds of Formula 1 may be indicated in thyroid hormone replacement therapy in patients with compromised cardiac function.

In therapeutic use the compounds of the present invention are usually administered in a standard pharmaceutical composition.

The present invention therefore provides in a further aspect pharmaceutical compositions comprising a compound of Formula 1 or a pharmaceutically acceptable salt thereof and a pharmaceutically acceptable carrier. Such compositions include those suitable for oral, parenteral or rectal administration.

PHARMACEUTICAL COMPOSITIONS Compounds of Formula 1 and their pharmaceutically acceptable salts which are active when given orally can be formulated as liquids for example syrups, suspensions or emulsions, tablets, capsules and lozenges.

A liquid composition will generally consist of a suspension or solution of the compound or pharmaceutically acceptable salt in a suitable liquid carrier(s), for example ethanol, glycerine, sorbitol, non-aqueous solvent such as polyethylene glycol, oils or water, with a suspending agent, preservative, surfactant, wetting WO 97/21993 PCT/US96/20778 42.

agent, flavoring or coloring agent. Alternatively, a liquid formulation can be prepared from a reconstitutable powder.

For example a powder containing active compound, suspending agent, sucrose and a sweetener can be reconstituted with water to form a suspension; and a syrup can be prepared from a powder containing active ingredient, sucrose and a sweetener.

A composition in the form of a tablet can be prepared using any suitable pharmaceutical carrier(s) routinely used for preparing solid compositions.

Examples of such carriers include magnesium stearate, starch, lactose, sucrose, microcrystalline cellulose and binders, for example polyvinylpyrrolidone. The tablet can also be provided with a color film coating, or color included as part of the carrier(s). In addition, active compound can be formulated in a controlled release dosage form as a tablet comprising a hydrophilic or hydrophobic matrix.

A composition in the form of a capsule can be prepared using routine encapsulation procedures, for example by incorporation of active compound and excipients into a hard gelatin capsule. Alternatively, a semi-solid matrix of.active compound and high molecular weight polyethylene glycol can be prepared and filled into a hard gelatin capsule; or a solution of active compound in polyethylene glycol or a suspension in edible oil, for example liquid paraffin or fractionated coconut oil can be prepared and filled into a soft gelatin capsule. Compound of Formula 1 and their pharmaceutically acceptable salts which are active when given parenterally can be formulated for intramuscular or intravenous administration.

A typical composition for intra-muscular administration will consist of a suspension or solution of active ingredient in an oil, for example arachis oil or sesame oil. A typical composition for intravenous administration will consist of a sterile isotonic aqueous solution containing, for example active ingredient, dextrose, sodium chloride, a co-solvent, for example polyethylene glycol and, optionally, a chelating agent, for example ethylenediamine tetracetic acid and an anti-oxidant, for example, sodium metabisulphite. Alternatively, the solution can be freeze dried and then reconstituted with a suitable solvent just prior to administration.

WO 97/21993 PCTIUS96/20778 43.

Compounds of structure and their pharmaceutically acceptable salts which are active on rectal administration can be formulated as suppositories. A typical suppository formulation will generally consist of active ingredient with a binding and/or lubricating agent such as a gelatin or cocoa butter or other low melting vegetable or synthetic wax or fat.

Compounds of Formula 1 and their pharmaceutically acceptable salts which are active on topical administration can be formulated as transdermal compositions.. Such compositions include, for example, a backing, active compound reservoir, a control membrane, liner and contact adhesive.

The typical daily dose of a compound of Formula 1 varies according to individual needs, the condition to be treated and with the route of administration.

Suitable doses are in the general range of from 0.001 to 10 mg/kg bodyweight of the recipient per day.

Within this general dosage range, doses can be chosen at which the compounds of Formula I lower plasma cholesterol levels and raise metabolic rate with little or no direct effect on the heart. In general, but not exclusively, such doses will be in the range of from 0.5 to 10 mg/kg.

In addition, within the general dose range, doses can be chosen at which the compounds of Formula 1 lower plasma cholesterol levels and have little or no effect on the heart without raising metabolic rate. In general, but not exclusively, such doses will be in the range of from 0.001 to 0.5 mg/kg.

It is to be understood that the 2 sub ranges noted above are not mutually exclusive and that the particular activity encountered at a particular dose will depend on the nature of the compound of Formula 1 used.

Preferably, the compound of Formula I is in unit dosage form, for example, a tablet or a capsule so that the patient may self-administer a single dose.

In general, unit doses contain in the range of from 0.05-100 mg of a compound of Formula 1. Preferred unit doses contain from 0.05 to 10 mg of a compound of Formula 1.

The active ingredient may be administered from 1 to 6 times a day. Thus daily doses are in general in the range of from 0.05 to 600 mg per day.

WO 97/21993 PCT/US96/20778 44.

Preferably, daily doses are in the range of from 0.05 to 100 mg per day. Most preferably from 0.05 to 5 mg per day.

EXAMPLES

EXAMPLE I SYNTHESIS OF TR LIGANDS Many TR ligands are known in the art, including T4 (thyroxine), T3, T2 and TS-9. See Jorgensen, Thyroid Hormones and Analogs, in 6 Hormonal Proteins and Peptides, Thyroid Hormones 107-204 (Choh Hao Li ed., 1978), incorporated by reference herein..

The syntheses of several TR ligands are described below.

Synthesis of TS1, TS2, TS3, TS4, TS1, TS2, TS3, TS4 and TS5 and analogs thereof can all be prepared by simple acylation of the nitrogen atom of any thyronine analog, including T3 (3,5,3'-triiodo-L-thyronine), T4 (thyroxine) and 3,5-diiodothyronine. TS1 and TS2 are synthesized by reacting T3 with Ph 2

CHCO

2 NHS (N-hydroxy succinimide- 2,2-diphenylacetate) and C 6

HII

33 CONHS, respectively. TS3 is synthesized by reacting T3 with FMOC-CI (fluorenylmethyloxycarbonylchloride). TS4 is synthesized by reacting T3 with tBOC20 (tBOC anhydride or di-tbutyldicarbonate). TS5, which differs from TS1-4 by having a -H instead of an -I at the R' 3 position, is synthesized by reacting 3,5-diiodothyronine with tBOC 2

O.

The general reaction scheme for TS1, TS2, TS3, TS4 and TS5 is depicted in FIG.

11. It should be noted that in the reaction scheme, both TS5 and its precursor both have a hydrogen rather than an iodine at the R'3 position.

Synthesis of TS6 and TS7 TS6 is synthesized by reacting TS5 with paranitrophenylisocyanate. TS7 is synthesized by reacting TS6 with TFA (trifluoroacetic acid), which cleaves the tBOC group. These reactions are simple organic synthesis reactions that can be performed by anyone of ordinary skill in the art. The synthetic scheme for TS6 and TS7 is diagrammed in FIG. 12.

WO 97/21993 PCT/US96/20778 Synthesis of TS8 TS8 is synthesized by reacting TS5 with Ph,CHNH, (diphenylmethylamine) in the presence of triethylamine and any amide forming condensing reagent, such as TBTU (hydroxybenztriazoleuronium tetrafluoroborate) or HBTU (hydroxybenztriazoleuronium hexafluorophosphate). The synthesis scheme for TS8 is depicted in FIG. 13.

SYNTHESIS OF 3,5-DIIODO-3'ISOPROPYLTHYRONINE DERIVATIVES For designing a class of antagonists, it is important to have a hydrophobic group at the 3' position as well as an extension at the 5' position. Preferred hydrophobic groups at the 3' position include: methyl, benzyl, phenyl, iodo, and heterocyclic structures. The synthesis of a 3,5-diiodo-3'-isopropyl-5'-substituted thyronine is described below. The example provided describes the specific steps for synthesizing the TS10 compound, but this general reaction scheme can be used by one of ordinary skill in the art to synthesize any number of 3,5,-diiodo-3'thyronine derivatives, which are characterized by having an extension at the 5' position. Additional compounds of this class can be synthesized using known organic synthesis techniques.

The synthesis of TS10 is described below and is depicted in FIG. 14.

Numbers used in the reaction scheme for TS10 indicating the reaction product for each step are in parentheses.

2-Formvi-6-isopropvlanisole 2-formyl-6-isopropylanisole (10.0 g, 61 mmol), as made by Casiraghi, et al. JCS Perkin I, 1862 (1980) (incorporated by reference), is added dropwise to a suspension of sodium hydride (3.7 g, 153 mmol) in 50 mL THF and 50 mL of DMF in a round bottom flask. The addition generates an exothermic reaction and formation of a gray solid. Methyl iodide (26.0 g, 183 mmol) is then added dropwise and the reaction mixture is stirred at room temperature for 5 hours. The reaction mixture is quenched with 20 mL of water, then poured into 500 mL of water, and is extracted with ether (2 x 300 mL). The ether layers are combined, washed with water (5 x 1000 mL), dried over magnesium sulfate and concentrated in vacuo to provide 10.2 g of the title compound, with the following 'H NMR (CDCI,) properties: d 10.30 1H), WO 97/21993 PCT/US96/20778 46.

7.63 1H, J=3 Hz), 7.50 1H, J=3 Hz), 7.13 1H, J=3 Hz), 3.81 (s, 3H), 3.31 (heptet, IH, J=7.5 Hz), 1.19 6H, J=7.5 Hz).

2 2 -Hvdroxvnonvl)-6-isopropylanisole (not shown in scheme): Octylmagnesium chloride (8.4 mL, 16.9 mmol, 2.0 M) is added dropwise to a solution of 1 (1.5 g, 8.4 mmol) in 10 mL THF at -78* C. The reaction mixture is stirred for 2 hours with warming to room temperature. The reaction mixture is diluted with 50 mL ether and poured into 50 mL water. The ether layer is washed with brine (1 x 50 mL), dried over sodium sulfate, and concentrated in vacuo.

Flash chromatography (silica gel, 10% ether/hexane 15% ether/hexane) provides 734 mg of the title compound with the following 'H NMR (CDCI,) properties: d 7.33-7.10 3H), 5.00 (br. s. 1H), 3.81 3H), 3.33 (heptet, 1H, J=7 Hz) 1.90-1.19 14H), 0.86 3H, J=6.5 Hz); HRMS found: 292.2404; calc'd: 292.2402.

2 -nonvl-6-isopropylanisole Compound 2 (663 mg, 2.3 mmol) is dissolved in solution of 5 mL ethanol and 5 mL acetic acid, and a spatula tip of palladium on carbon catalyst is added. The reaction mixture is then charged with hydrogen gas (using a simple balloon and needle) and the mixture is stirred at room temperature overnight. The next day, the reaction mixture is poured into ether (100 mL) and the ether layer is extracted with saturated sodium bicarbonate (3 x 100 mL). The ether layer is dried over sodium sulfate and concentrated in vacuo to provide 581 mg of with the following 'H NMR (CDCI,) properties: d 7.14-7.00 3H), 3.75 3H), 3.36 (heptet, 1H, J=6.8 Hz), 2.63 2H, J=7.5 Hz), 1.68-1.15 14H), 0.86 3H, J=5.5 Hz); HRMS (El), mass found: 276.2459; calculated: 276.2453.

Thvronine adduct Fuming nitric acid (0.071 mL) is added to 0.184 mL acetic anhydride chilled to C. Iodine (66 mg) is added to this mixture followed by trifluoroacetic acid (0.124 mL). This mixture is stirred for 1 hour with warming to room temperature, at which point all of the iodine is dissolved.

The reaction mixture was then concentrated in vacuo to provide an oily semi-solid material. The residue was dissolved in 0.7 mL of acetic anhydride and cooled to C. A solution of anisole (581 mg, 2.1 mmol) .in 1.2 mL acetic anhydride WO 97/21993 PCT/US96/20778 47.

and 0.58 mL TFA is added dropwise. The reaction mixture is stirred at -20* for 1 hour, then stirred overnight with warming to room temperature. The reaction mixture is partitioned between water and methylene chloride. The methylene chloride layer is dried over sodium sulfate and concentrated in vacuo to provide the iodonium salt as an oil. This material is not purified or characterized, and is directly introduced into the coupling reaction.

methyl ester (552 mg, 1.0 mmol) prepared according to the procedure of N. Lewis and P. Wallbank, Synthesis 1103 (1987) (incorporated by reference) and all of the crude iodonium salt from above is dissolved in 5 mL of anhydrous methanol. Diazabicyclo[5.4.0]undecane (DBU) (183 mg, 1.2 mmol) and a spatula tip of copper-bronze are added and the resulting mixture is stirred at room temperature overnight. The next day, the reaction mixture is filtered, and the filtrate is concentrated in vacuo. The crude residue is purified by flash chromatography (silica gel, 10% ethyl acetate/hexane) to provide 30 mg of the protected thyronine adduct Deprotected thyronine (TS10): The protected thyronine 4 (30 mg, 0.04 mmol) is dissolved in a mixture of 2.25 mL acetic acid and 2.25 mL 49% hydrobromic acid. The reaction mixture is heated to reflux for 5 hours. The reaction mixture is cooled to room temperature, and the solvents are removed in vacuo. Water is added to triturate the oily residue into a gray solid. This solid material is filtered, washed with water, and dried over PO, in vacuo to provide 24 mg (81%)of the title compound, TS10, with the following 'H NMR (CDCI properties: d 7.57 1H), 6.86 1H), 6.45 1H), 6.34 1H), 4.81 (m, 1H), 3.86 3H), 3.71 3H), 3.33-3.05 3H), 2.58-2.47 2H), 1.62-0.76 23H); MS (LSIMS): M 817.0.

As mentioned above, this reaction scheme can be modified by one of ordinary skill in the art to synthesize a class of compounds characterized by diiodo-3'isopropylthyronine derivatives, wherein the 3' isopropyl group can be replaced with a hydrophobic group, including methyl, benzyl, phenyl, iodo, and heterocyclic structures, and a wide variety of chemical structures can be incorporated at the 5' position, including alkyl groups, planar aryl, heterocyclic groups, or polar and/or charged groups.

WO 97/21993 PCT/US96/20778 48.

The aldehyde in the above reaction scheme is a versatile synthetic intermediate which allows for the attachment of a variety of chemical moieties to the 5' position of the final thyronine derivative. In addition, a variety of chemical reactions can be used to attach the chemical moieties. These reactions are well known in the art and include organometallic additions to the aldehyde (including Grignard reagents, organolithiums, etc.), reductive amination reactions of the aldehyde with a primary or secondary amine, and Wittig olefination reactions with a phosphorous ylid or stabilized phosphonate anion. Other possibilities include reduction of the aldehyde to a benzyl alcohol allowing for etherification reactions at the 5' position. As mentioned above, these methods allow for a wide variety of chemical structures to be incorporated at the 5' position of the final thyronine derivative, including alkyl groups, planar aryl, heterocyclic groups or polar and/or charged groups.

Synthesis of 3, 5-dibromo-4-(3',5'-diisopropyl-4'-hydroxyphenoxy) benzoic acid (Compound 11).

Br o I OH HO Br A mixture of 2,6-diisopropyl phenol (20 g, 0.11 mol), potassium carbonate (62 g, 0.45 mol), acetone (160 ml) and methyl iodide (28 ml, 0.45 mole) is refluxed for three days. The reaction mixture is filtered through celite, evaporated, dissolved in ether, washed twice with IM sodium hydroxide, dried over magnesium sulphate and concentrated to afford 15.1 g (0.08 mol, 70%) of 2,6-diisopropyl anisole as a slightly yellow oil.

Fuming nitric acid (12.4 ml, 265 mmol) is added dropwise to 31.4 ml of acetic anhydride which is cooled in a dry ice/carbon tetrachloride bath. Iodine WO 97/21993 PCT/US96/20778 49.

11.3 g, 44.4 mmol) is added in one portion followed by dropwise addition of trifluoroacetic acid (20.5 ml, 266 mmole). The reaction mixture is stirred at room temperature until all the iodine is dissolved. Nitrogen oxides are removed by flushing nitrogen into the vessel. The reaction mixture is concentrated, the residue is dissolved in 126 ml of acetic anhydride and is cooled in a dry ice/carbon tetrachloride bath. To the stirred solution 2 6 -diisopropylanisole (51 g, 266 mmol) in 150 ml of acetic anhydride and 22.6 ml of trifluoroacetic acid is added dropwise. The reaction mixture is left to stand at room temperature over night and then is concentrated. The residue is taken up in 150 ml of methanol and treated with 150 ml of 10% aqueous sodium bisulfite solution and 1 liter of 2M sodium borotetrafluoride solution. After the precipitate aggregates, petroleum ether is added and the supernatant is decanted. The precipitate is triturated with petroleum ether, filtered, washed with petroleum ether and dried at room temperature in vacuo. This affords 34 g (57 mmol, 65%) of bis(3,5-diisopropyl-4methoxyphenyl)iodonium tetrafluoroborate as a white solid.

To a stirred solution of 3,5-dibromo-4-hydroxybenzoic acid (12 g, 40.5 mmol) in 250 ml of methanol, thionyl chloride (3 ml) is added dropwise. The reaction mixture is refluxed for five days, water is added and the precipitated product is filtered off. The residue is dissolved in ethyl acetate. From the aqueous phase, methanol is removed by concentration. The aqueous phase is then saturated with sodium chloride, and extracted with ethyl acetate. The combined organic phases are dried over magnesium sulphate, filtered and concentrated. This gives 12.5 g (40.5 mmol, 100%) of 3,5-dibromo-4-hydroxymethyl benzoate as a white crystalline solid.

The products obtained in steps b and c are reacted with each other according to the following protocol. To bis(3,5-diisopropyl-4methoxyphenyl)iodonium tetrafluoroborate (2.86 g, 4.8 mmole) and copper bronze (0.42 g, 6.4 mmole) in 7 ml. of dichloromethane at 0* C is added dropwise a solution of 3,5-dibromo-4-hydroxymethyl benzoate (1.0 g, 3.2 mmole) and triethylamine (0.36 g, 3.5 mmole) in 5 ml of dichloromethane. The reaction mixture is stirred in the dark for eight days and then is filtered through celite.

The filtrate is concentrated and the residue is purified by column chromatography WO 97/21993 PCT/US96/20778 (silica gel, 97:3 petroleum ether/ethyl acetate) to give 0.62 g (1.2 mmole, 39%) of 3,5-dibromo-4-(3',5'-diisopropyl-4'-methoxyphcnoxy)methyl benzoate as a solid.

The product from step d (0.2 g, 0.4 mmole) is dissolved in 2 ml.

dichloromethane, is put under nitrogen and is cooled at -40* C. To the stirred solution is added IM BBr 3 (1.2 ml, 1.2 mmole) dropwise. The reaction mixture is allowed to reach room temperature and then is left over night. It is cooled to 0* C and then hydrolyzed with water. Dichloromethane is removed by concentration and the aqueous phase is extracted with ethyl acetate. The organic phase is washed with IM hydrochloric acid and brine. Then it is dried over magnesium sulphate, filtered and concentrated. The residue is chromatographed (silica, 96:3.6:0.4 dichloromethane/methanol/acetic acid) producing 93 mg (0.2 mmole, 51%) of 3,5-dibromo-4-(3',5'-diisopropyl-4'-hydroxyphenoxy)benzoic acid as a white solid. 'H nmr (CDCI1) 6 1.23 12H, methyl), 3.11 2H, CH), 6.50 2H. 2,6-H) 8.33 2H, TABLE 1 and FIG. 15 depict the structures of several TR ligands.

WO 97/21993 WO 97Z1993PCT/US96I2 0778 51.

FORMULA I

IZ

5 P117 x QOA, 13 2.

TABLE I Cmpd jR, R 4 R, R'l-RRsR TI1 -1 I-OH, -H -CH.CH(NH,)CO.H T. -1 -I -on .01-CHCH(NH,)CO,H TSI -1 -J -1 -OH -H -CHzCH(NHCOCHO 1 jCOH TS2 -1 -I -J -OH -H -CH 2 CHjNHCO(CH), 3 CH, TS3 -1 I-OH -H -CH.CHINH--FMOCJCO,H TS I I-OH4 -H -CHCH!NH-tBOCjCO, H TSS -1 -H -OH -H *CHCHjNH-tBOCJCO, H, TS6 -1 -1 -H -OC(O)NH=0PNOZ -H -CHCHINH-tBOCjCO2

H

T57 -1 -I .1 -OC(O)NH=NHON0. -H *CHICH(NH,)COH TS8 -1 -H -NH-CHOO -H -CHICH(NH-LBOCICO 2

JH

TS9 -1 -1 -IsoPr -OH -H -CHCH4(NH,)COH TSIO 71 T1 -Is -OH

-CHCH(NH,)C,

-0: -0pNO,: Prior Art Compound From SKF phenyl para nitro phenyl WO 97/21993 PCT/US96/20778 52.

EXAMPLE 2 RECEPTOR BINDING ASSAYS OF TR LIGANDS To test the ability of synthesized TR ligands to bind to a thyroid receptor (TR), the binding affinity of a TR ligand for TR is assayed using TR's prepared from rat liver nuclei and 125, T 3 as described in J.D. Apriletti, J.B. Baxter, and T.N. Lavin, J. Biol.

Chem., 263: 9409-9417 (1988). The apparent Kd's are calculated using the method described by Apriletti (1995) and Apriletti (1988). The apparent Kd's are presented in TABLE 2. The apparent Kd's (App.Kd) are determined in the presence of the sample to be assayed, 1 nM 2 1]T 3 and 50g/ml core histones, in buffer E (400 mM KCI, 200 mM potassium phosphate, pH 8.0, 0.5 mM EDTA, 1 mM MgCI 2 10% glycerol, 1 mM DTT) in a volume of 0.21 ml. After incubation overnight at 4°C, 0.2 ml of the incubation mixture is loaded onto a Quick-Sep Sephadex G-25 column (2.7 x 0.9 cm, 1.7 ml bed volume) equilibrated with buffer E. The excluded peak of protein-bound ['"IjT is eluted with 1 ml of buffer E, collected in a test tube, and counted. Specific T 3 binding is calculated by subtracting nonspecific binding from total binding.

WO 97/21993 PCTIUS96/20778 53.

TABLE 2 Coactivation Amsy Compound App.Kd(nM) RIP-140 T30.06 1010 T42 10-9 TSI 4 to-, TS2 1400 nd nd TS3 4 11 'r48 nd 220 106 TS6 10000 mci mc TS7 260 107 TS8 6000 nd nd TS9 I IWO1 15TS1O 400 RIP-140 Binding RIP-140 Binding nd: Not Determined EXAMPLE 3 INCREASED) NUCLEAR PROTE[N COACI-IVATION BY TR LIGANDS To test the ability of TR ligands to activate the binding of TR to the nuclear activation protein RIP-140 (a nuclear protein that can bind to nuclear receptors, such as the estrogen receptor), a TR ligand is liganded to TR and then incubated with RIP-140 as described in V. Cavailles, et al.. EMBO 14(15):3741- 3751 (1995), which is incorporated by reference herein. In this assay, 35s-RIP-140 protein binds to liganded TR but not unliganded TR. Many TR 35s ligands can activate RIP- 140 binding as shown in TABLE 2.

WO 97/21993 PCT/US96/20778 54.

EXAMPLE 4 TR LIGAND BINDING AND TR ACTIVATION IN CULTURED CELLS To test TR activation of transcription in a cellular environment, TR ligands are assayed for their ability to activate a reporter gene, chloramphenicol transferase which has a TR DNA binding sequence operatively linked to it. Either GC or L937 cells (available from the ATCC) can be used, respectively). In such assays, a TR ligand crosses the cell membrane, binds to the TR, and activates the TR, which in turn activates gene transcription of the CAT by binding the TR DNA binding region upstream of the CAT gene. The effective concentration for half maximal gene activation (ECso) is determined by assaying CAT gene activation at various concentrations as described herein and in the literature. The results of CAT gene activation experiments are shown in TABLE 2.

CAT GENE ACTIVATION ASSAYS Functional response to thyroid hormone (3.5,3'-triiodo-L-thyronine,

T

3 and TR ligands is assessed either in a rat pituitary cell line, GC cells, that contain endogenous thyroid hormone receptors (TRs) or U937 cells that contain exogenous TRs expressed as known in the art. GC cells are grown in 10-cm dishes in RPMI 1640 with 10% newborn bovine serum, 2 mM glutamine, 50 units/ml penicillin and 50 Ag/ml streptomycin. For transfections, cells are trypsinized, resuspended in buffer (PBS, 0.1% glucose) and mixed with a TREtkCAT plasmid (10 mg) or phage in 0.5 ml buffer (15 ±5 million cells) and electroporated using a Bio-Rad gene pulser at 0.33 kvolts and 960 mF. The TREtkCAT plasmid contains two copies of a T 3 response element (AGGTCAcaggAGGTCA) cloned in the Hind III site of the pUC19 polylinker immediately upstream of a minimal (-32/+45) thymidine kinase promoter linked to CAT (tkCAT) coding sequences. After electroporation, cells are pooled in growth medium (RPMI with 10% charcoal-treated, hormone stripped, newborn bovine serum), plated in 6-well dishes and treated with either ethanol or hormone. CAT activity is determined 24 hours later as described D. C.

Leitman, R. C. J. Ribeiro, E. R. Mackow, J. D. Baxter, B. L. West, J. Biol. Chem.

266, 9343 (1991), which is incorporated by reference herein.

WO 97/21993 PCTIUS96/2077 EFFECT OF TS-10 ON THE TRANSCRIPTIONAL REGULATION OF THE DR4-ALP REPORTER GENE IN THE PRESENCE OR ABSENCE OF T3.

Characteristics of the TRAF cells: TRAFal are CHO K1 cells stably transformed with an expression vector encoding the human thyroid hormone receptor a 1 and a DR4,ALP reporter vector; TRAFbl are CHO KI cells stably transformed with an expression vector encoding the human thyroid hormone receptor 01 and a DR4-ALP reporter vector.

Interpretation of the effect of compound TS-10 on the transcriptional regulation of the DR4-ALP reporter gene in the presence or absence of T3.

TRAFal reporter cells: TS-10 alone (open circles) induces a partial activation of the expression of the ALP reporter protein amounting to approximately 27% of the maximal effect by the natural thyroid hormone T3. In the presence of T3 (filled circles), has a weak antagonistic effect. The EC50 concentration for the agonistic effect of and the EC50 concentration for its T3 antagonistic effect, respectively, is indicated in FIG. 18.

In FIG. 18, open and filled circles with dotted lines show the dose-dependent effect of TS-10/T3 on the toxicity marker (MTS/PMS), reduction of tetrazolium salt in the mitochondria, displayed on the right y-axis as optical density. There is no obvious toxic effect of TS-10 on the MTS-PMS marker but there is a clear effect on the morphology of the cells, as can be seen under the light microscope, at the highest concentration of (32 mM) both in the absence and presence of T3, respectively (not shown in the figure).

TRAFbl reporter cells: TS-10 alone (open circles) induces a partial activation of the expression of the ALP reporter protein amounting to approximately 35 of the maximal effect by T3. The EC50 concentration for the agonistic effect of TS-10 is indicated in FIG. 19. In the presence of T3 (filled circles), TS-10 shows, if anything, a slight potentiation of the T3 effect on the expression of the ALP reporter protein. The T3 inhibitory effect of TS-10 at its highest concentration used (32 mM) is a toxic effect rather than T3 antagonism.

WO 97/21993 PCT/US96/20778 56.

In FIG. 19, open and filled circles with dotted lines show the dose-dependent effect of TS-10/T3 on the toxicity marker (MTS/PMS), reduction of tetrazolium salt in the mitochondria, displayed on the right y-axis as optical density. There is no obvious toxic effect of TS-10 on the MTS-PMS marker but a clear effect on the morphology of the cells can be observed, under the light microscope, at the highest concentration of TS-10 (32 mM) both in the absence and presence of T3, respectively (not shown in the figure).

HepG2 (HAF18) reporter cells: TS-10 alone (open circles) induces a partial activation of the expression of the ALP reporter protein amounting to slightly more than 50% of the maximal effect by T3. The EC50 concentration for the agonistic effect of TS-10 is indicated in FIG. 20. In the presence of T3 (filled circles), TS-10 shows no effect i.e.

no T3 antagonism nor potentiation/additive effect to T3. Open and filled circles with dotted lines show the dose-dependent effect of TS-10/T3 on the toxicity marker (MTS/PMS), reduction of tetrazolium salt in the mitochondria, displayed on the right yaxis as optical density. There is no obvious toxic effect of TS-10 on the MTS/PMS marker or on the morphology of the cells, as can be observed using a light microscope, at any concentration of TS-10/T3 used.

Example 5 Comparisons of Human TR-a and Human TR-# Competition for ['Izs]T 3 binding to TR LBD by T, and Triac The drug, triac, is a thyroid hormone agonist. Triac is 3,5,3'-triiodothyroacetic acid and is described in Jorgensen, Thyroid Hormones and Analogs in 6 Hormonal Proteins and Peptides, Thyroid Hormones at 150-151 (1978). Another compound that can be used in place of triac is 3 ,5-diiodo-3'-isopropylthyroacetic acid. Competition assays are performed to compare the displacement of [1"I]T 3 from binding with human TR-a LBD or human TR-3 LBD by unlabeled T 3 or triac. The results of such assays are depicted in FIG. 16.

Standard binding reactions are prepared containing 1 nM [('lT 3 30 fmol of human TR-a (empty symbols) or P (solid symbols), and various concentrations of competing unlabeled T3 (circles) or triac (triangles). Assays are performed in duplicate.

WO 97/21993 PCT/US96/20778 57.

Scatchard Analysis of 3 Binding to TR Human TR-a (left panel) or human TR-f (right panel) is assayed for T 3 binding in the presence of increasing concentrations of [Z11]T 3 The apparent equilibrium dissociation constant (20 pM for a and 67 pM for j) is calculated by linear regression analysis and is depicted in FIG. 17.

3, 5-DIBROMO-4-(3',5'-DIISOPROPYL-4'-HYDROXYPHENOXY) BENZOIC ACID IS A TR-A SELECTIVE SYNTHETIC LIGAND.

Br 0 b I

OH

HO Br 3, 5-dibromo-4-(3',5'-diisopropyl-4'-hydroxyphenoxy) benzoic acid (Compound 11), the structure of which is drawn above, is assayed for binding to the two different isoforms of the TR, Tra and TR3. Compound 11 exhibits an IC50 of 1.6 jM for binding to TRa and an IC50 of 0.91 pM for binding to TRO. Assays for determining selective binding to the TRa or TR3 LBD can include reporter assays, as described herein. See also Hollenberg. et al., J. Biol. Chem., 270(24)14274-14280 (1995).

EXAMPLE 6 PREPARATION AND PURIFICATION OF A TR-A LBD Rat TR-a LBD, residues Metl22 Val410, is purified from E. coli ("LBD- 122/410"). The expression vector encoding the rat TR-a LBD is freshly transfected into E. coli strain BL21(DE3) and grown at 22*C in a 50-liter fermenter using 2x LB medium. At an Ao of 2.5-3, IPTG is added to 0.5 mM and growth is continued for 3 h before harvesting. The bacterial pellet is quickly frozen in liquid nitrogen and stored at until processed. Extraction and purification steps are carried out at 4*C. The bacteria are thawed in extraction buffer (20MM Hepes, pH 1 mM EDTA, 0.1% MTG, 0.1 mM PMSF, and 10% glycerol) at a ratio of 10 ml buffer/g bacteria. Bacteria are lysed by incubation for 15 min. with 0.2 mg/ml lysozyme and sonicated at maximum power while simultaneously homogenized with a Brinkmann homogenizer (Model PT WO 97/21993 PCT/US96/20778 58.

10/35 with generator PTA 35/2) until the solution loses its viscosity. After centrifugation for 10 min at 10,000 g, the supernatant is adjusted to 0.4 M KCI, treated with 0.6% PEI to precipitate fragmented DNA, and centrifuged for 10 min at 10,000 g. The rat TR-a LBD in the supernatant is then precipitated with 50% ammonium sulfate and centrifuged for 10 min at 10,000 g. The precipitate is resuspended with buffer B (20 mM IHepes, pH 1 mM EDTA, 1 mM DTT, 0.1 mM PMSF, 0.01% Lubrol, and 10% glycerol) to a final conductivity of 9 mS/cm (approx. 0.7 M ammonium sulfate) and centrifuged 1 h at 100,000g. The supernatant is frozen in liquid nitrogen and stored at The crude extract is thawed, bound with a tracer amount of ['I]T 3 and loaded directly onto a phenyl-Toyopearl hydrophobic interaction column (2.6 x 18 cm, 95 ml bed volume) at 1.5 ml/min. The column is eluted with a 2-h gradient from 0.7 ammonium sulfate. no glycerol to no salt, 20% glycerol in buffer C (20 mM Hepes, pH 8.0, 0.5 mM EDTA, 1 mM DTT, 0.2 mM PMSF). The rat TR-a LBD prebound to tracer 5

I]T,

(less than 0.005% of total rat TR-a LBD) is detected using a flow-through gamma emission detector, whereas unliganded rat TR-a LBD is assayed by postcolumn

['"IJT,

binding assays (described herein).

The phenyl-Toyopearl unliganded rat TR-a LBD peak fractions are pooled, diluted with buffer B to a conductivity of 0.5 mS/cm (equivalent to approx. 20 mM ammonium sulfate), loaded onto a TSK-DEAE anion-exchange column (2 x 15 cm, 47 ml bed volume) at 4 ml/min, and eluted with a 60-min gradient from 50 to 200 mM NaCI in buffer B.

The unliganded rat TR-a LBD peak fractions from TSK-DEAE are pooled, diluted twofold with buffer B, loaded at 0.75 ml/min on a TSK-heparin HPLC column (0.8 x cm, 3 ml bed volume), and eluted with a 50 to 400 mM NaCI gradient in buffer B.

The pool of unliganded rat TR-a LBD peak fractions from the TSK-heparin column is adjusted to 0.7 M ammonium sulfate, loaded at 0.75 ml/min on a TSK-phenyl HPLC column (0.8 x 7.5 cm, 3 ml bed volume), and eluted with a 60-min gradient from 0.7 M ammonium sulfate without glycerol to no salt with 20% glycerol in buffer C. The fractions containing unliganded rat TR-c LBD are pooled and incubated with a five fold excess of hormone for I h, the salt concentration is adjusted to 0.7 M ammonium sulfate, and the sample is reloaded and chromatographed on the same column as described above.

WO 97/21993 PCT/US96/20778 59.

EXAMPLE 7 CRYSTALLIZATION OF LIGANDED TR-a LBD Material from a single LBD-122/410 preparation is divided into batches, and quantitatively bound with one of the following ligands: Dimit, T 3 or triac IpBr, (3,5dibromo-3'isopropylthyronine) for the final purification step.

To maintain full saturation of rat TR-c LBD with a ligand, and to prepare the complex for crystallization, the ligand-bound rat TR-ac LBD is concentrated and desalted in an Amicon Centricon-10 microconcentrator (McGrath et al, Biotechniques, 7:246-247 (1989), incorporated by reference herein), using 10 mM Hepes (pH 3.0 mM DTT, and 1.0 nM to 10 nM ligand.

Factorial crystallization screening trials (Jancarik Kim, J. Appl. Crystallogr.

24:409-411 (1991) incorporated by reference herein) are carried out for rat TR-a LBD bound to selected ligands using hanging-drop vapor diffusion at 17 0 C (with 1 pl protein solution, 1 pl precipitant solution and a 0.5 ml reservoir using silanized coverslip: (McPherson, Preparation and Analysis of Protein Crystals (1982), incorporated by reference herein). Rat TR-ca LBD is not stable at 4 0 C and is stored at -80*C, where it maintains its avidity for hormone and its crystallizability for approximately two to three months. These procedures are carried out as described in McGrath, M.E. et al., J. Mol.

Biol. 237:236-239 (1994) (incorporated by reference).) Crystals are obtained in condition 21 of the screening trials (Jancarik Kim 1991) and conditions are then optimized.

Wedge-shaped crystals are reproducibly obtained with hanging-drop vapor fusion at 22"C with 15% 2-methyl-2,4-pentanediol (MPD), 0.2 M ammonium acetate and 0.1 M sodium cacodylate (pH 3 mM DTT, with 2 pl protein solution, 1 jl. precipitant solution and a 0.6 ml reservoir using silanized coverslip, and with 8.7 mg/ml (Dimit), 5.5 mg/ml (IpBr 2 5 mg/ml (triac), or 2.3 mg/ml (T 3 over a period of three days. Under these conditions, diffraction quality crystals (dimension 0.5 x 0.2 x 0.0075 mm 3 can be grown at ambient temperature (22 The best crystals have a limiting dimension of approximately 100 pin and are obtained at a protein concentration between 2.3 and 8.7 mg/ml in the presence of 3 mM DTT. The crystals are of the monoclinic space group C2, with one monomer in the asymmetric unit.

WO 97/21993 PCT/US96/20778 EXAMPLE 8 CRYSTALLIZATION OF HUMAN TR- LBD COMPLEXED WITH T 3

OR

TRIAC

Human TR-3 LBD complexed with T, and human TR-a LBD complexed with triac are purified according to the same procedures described above for the rat TR-c LBD, with the following modifications.

The expression of human TR-0 LBD differs from the rat TR-ca LBD in that the human TR-0 LBD residues extend from the amino acid at position 716 through the amino acid at position 1022, according to the amino acid numbering scheme for the various nuclear receptor LBDs depicted in FIG. 3. FIG. 3 illustrates a numbering scheme applicable to all of the nuclear receptors listed as well as to any additional homologous nuclear receptors. The vertical lines on FIG. 3 at position 725 and at position 1025 delineate the preferred minimum amino acid sequence necessary to obtain adequate binding of ligand. The amino acid sequence from position 716 to position 1022 according to the numbering scheme of FIG. 3 corresponds to the amino acid positions 202 to 461 according to the conventional numbering of the amino acid sequence of human TR-3 which is publicly available. Also, the human TR-3 LBD is expressed with a histidine tag, as described in Crowe et al., Methods in Molecular Biology 31:371-387 (1994), incorporated by reference herein.

The purification of human TR-0 LBD is the same as that described above for the rat TR-a LBD with the following exceptions. First, before the purification step using the hydrophobic interaction column, a step is added in which the expressed human TR-3 LBD is purified using a nickel NTA column (commercially available from Qiagen, Chatsworth, CA) according to manufacturer's instructions, and eluted with 200 mM imidazole. The second difference is that in the purification of the human TR-3 LBD, the purification step using a heparin column is omitted.

The crystallization of human TR-/ LBD bound to T3 or triac is as follows.

Crystals are obtained in condition 7 of the factorial screen using hanging drops as before at ambient temperature (22 0 C) using the factorial crystallization screening trials of Jancarik Kim (1991) and using the commercially available product from Hampton Research, Riverside). The following are optimum conditions: hexagonal bipyrimidal crystals are grown at 4"C for 2-3 days from hanging drops containing 1.0-1.2 M sodium acetate (pH unadjusted) and 0.1 M sodium cacodylate (pH 3 mM DTT, with either WO 97/21993 CT/US96/20778 61.

a I protein solution, 1 ul precipitant solution or 2 g1 protein solution, 1 sl precipitant solution and a 0.6 ml reservoir using silanized coverslip, at a protein concentration of 7mg/ml. The best crystals have a limiting dimension of 200 Am.

The crystal system for human TR-3 LBD bound to T, or triac is trigonal with the space group p3,21. The unit cell dimensions are cell length a cell length b 68.448 angstroms, cell length c 130.559 angstroms. The angles are a 90*, 0 90° gamma 120°.

EXAMPLE 9 DETERMINATION OF LIGANDED TR-a LBD CRYSTAL STRUCTURE Data from each of three cocrystals (Rat TR-a LBD with Dimit, T3 and IpBr,) is measured on a Mar area detector at Stanford Synchrotron Radiation Laboratory beamline 7-1 (X 1.08 angstroms) using 1.2' oscillations.

Data from the T3 cocrystal is measured with the b* axis approximately parallel with the spindle. The crystals are flash frozen at -178°C in a nitrogen gas stream with the MPD mother liquor serving as the cryosolvent. An orientation matrix for each crystal is determined using REFIX (Kabsch, J. Appl. Crystallogr. 26:795-800 (1993) incorporated by reference). Reflections are integrated with DENZO (commercially available from Molecular Structure Corp., The Woodlands, Texas), and are scaled with SCALEPACK (as described in Otwinowski, Z, Proceedings of the CCP4 Study Weekend.

"Data Collection and Processing." 56-62 (SERC Daresbury Laboratory, Warrington, UK 1993) incorporated by reference).

For the T3 data set, Bijvoet pairs are kept separate, and are locally scaled using MADSYS Hendrickson (Columbia University) and W. Weis (Stanford University)).

Cocrystals prepared from the three isosteric ligands are isomorphous. MIR analysis is performed using programs from the CCP4 suite (Collaborative Computational Project, N.R. Acta Crystallogr. D50:760-763 (1994), incorporated by reference herein).

Difference Pattersons is calculated for both T 3 and IpBr,, taking the Dimit cocrystal as the parent. The positions of the three iodine atoms in the T, difference Patterson are unambiguously determined from the Harker section of the density map as peaks of 11 a above background. The positions for the two bromine atoms in the IpBr, cocrystals, are located independently, as peaks 8a above the noise level. Phases for the LBD-122/410 are calculated from the solution to the IpBr, difference Patterson, and are used to confirm the WO 97/21993 PCT/US96/20778 62.

location of the unique third iodine of the T 3 cocrystal. Halogen positions are refined with MLPHARE, including the anomalous contributions from the iodine atoms (Otwinowski, Z, Proceedings of the CCPR Study Weekend 80-86 (SERC Daresbury Laboratory, Warrington, UK 1991)). The MIRAS phases are improved through solvent flattening/histogram matching using DM (Cowtan, Joint CCP4 and ESF-EACBM Newsletter on Protein Crystallography 31: 34-38 (1994), incorporated by reference herein).

A model of the LBD-122/410 with Dimit bound is built with the program O from the solvent flattened MIRAS 2.5 angstrom electron density map (Jones et al., Acta Crystallogr. A 47:110-119 (1991), incorporated by reference herein). The initial model, without ligand, (Rcryst 40.1 is refined using least-squares protocols with XPLOR.

0 The Dimit ligand is built into unambiguous Fo-Fc difference density during the following round. Subsequent refinement employs both least-squares and simulated annealing protocols with XPLOR (Brunger et al., Science 235:458-460 (1987), incorporated by reference herein). Individual atomic B-factors are refined isotropically. As defined in PROCHECK, all residues are in allowed main-chain torsion angle regions as described in Laskowski et al., J. Appl. Crystallogr. 26:283-291 (1993), incorporated by reference herein. The current model is missing 34 residues (Met 1 2 -Glns 5 at the N-terminus, and residues (Glu 4 6-Val 4 at the C-terminus.

In addition, the following residues are not modeled beyond CO due to poor density: 184, 186, 190, 198, 206, 209, 240, 301, 330, 337, 340, 343, 359, and 395.

The average B-value for protein atoms is 34.5 A 2 The final model consists of the LBD- S 122/410, residues Arg, 5 7 -Ser, 1 3 Trpss-Gly, Ser,,-Asp20 and Asp 2 o0-Phe,,; three cacodylate-modified cysteines: Cys 33 4 Cys 3 ,o and Cys 3 9 and 73 solvent molecules modeled as water (2003 atoms).

*Rs m 100 x E hki E I I, hk i Ii tRer 100 x E hkl FPH-F I h IF The occupancy for the two bromine sites is set to 35 electrons. The occupancies of the iodine sites are relative to this value.

§Phasing power (FH) where (FH) is the mean calculated heavy atom structure factor amplitude and is the mean estimated lack of closure.

I

WO 97/21993 PCT/US96/20778 63.

IlRcullis (iso), where is the mean estimated lack of closure and (iso) is the isomorphous difference.

Rcryst 100 x Eh,, IF.-Fd Ehk IFo where Fo and F, are the observed and calculated structure factor amplitudes (for data F/a The Rfree was calculated using 3% of the data, chosen randomly, and omitted from the refinement.

Correlation coefficient ,hk (1Fjo tF,) x (IFd IF ,hk (Et IF)2x hk (IF FJ) 2 EXAMPLE 10. PHASING OF THE RTRA LBD COMPLEX WITH TRIAC Due to the possible non-isomorphism of the rTRa LBD complex with Triac, a molecular replacement solution is determined using AMORE (Navaza, Acta Crystallographica Section A-Fundamentals of Crystallography 50:157-63 (1994) from a starting model consisting of rTRa LBD complex with T 3 but with the ligand, all water molecules, and the following residues omitted: Asn 179, Arg228, Arg262, Arg266, and Ser 277. Strong peaks are obtained in both the rotation and translation searches, with no significant times the top peak) false solutions observed (Table Strong positive density present in both the anomalous and conventional difference Fourier maps confirm the solution.

Maps are, calculated using sigma-A weighted coefficients output by REFMAC (Murshudov, et al. "Application of Maximum Likelihood Refinements," in the Refinement of Protein Structures, Proceedings of Daresbury Study Weekend (1996)) after cycles of maximum likelihood refinement. Triac, the omitted residues, and water molecules 503, 504, 534 (following the numbering convention for the TR complex with T3) are built into the resulting difference density using O (Jones et. the conformations of these residues are further confirmed in a simulated-annealing omit map (Brunger et. The complete model is then refined using positional least-squares, simulated annealing, and restrained, grouped B factor refinement in XPLOR to an Rcryst of 23.6% and an Rfree of 24.1% EXAMPLE 11. CONNECTING QSAR WITH STRUCTURE IN THE THYROID HORMONE

RECEPTOR

The conclusions of classic thyroid hormone receptor quantitative structure-activity relationships may be summarized as follows: WO 97/21993 PCT/US96/20778 64.

1) the R'-hydroxyl group functions as a hydrogen bond donor; 2) the amino-propionic acid interacts electrostatically through the carboxylate anion with a positively charged residue from the receptor; 3) the preferences of R,/R 5 substituent are I> Br> Me H; 4) the preferences of the R,'-substituent are Ipr> I>Br>Me>

>H.

The structure of the thyroid hormone receptor ligand binding domain complexed with the agonists 3,5,3'-triiodothyronine

(T

3 3,5-dibromo-3'-isopropylthyronine (IpBr,), dimethyl-3'-isopropylthyronine (Dimit), and 3,5,3'-triiodothyroacetic acid (Triac), as provided herein, permits: 1) the identification of receptor determinants of binding at the level of the hydrogen bond; 2) the association of these determinants with the predictions of classic thyroid hormone receptor QSAR; and 3) prediction as to which determinants of binding are rigid, and which are flexible, for both the ligand and the receptor.

This classification for the agonists of the type (RI =amino-propionic, acetic acid;

R

3

,R

5 =I,Br,Me; R 3 '=Ipr,I) is given below (for the representative ligand T 3 F Fiducial (always satisfied) A Adjustable

F

F

F HO o° CH" HCOOH %.f A A WO 97/21993 PCT/US96/20778 Based upon the methods and data described herein, the following is an embodiment of the computational methods of the invention, which permit design of nuclear receptor ligands based upon interactions between the structure of the amino acid residues of the receptor LBD and the four different ligands described herein. The small molecule structures for the ligands can be obtained from Cambridge Structural Database (CSD), and three dimensional models can be constructed using the methods described throughout the specification. The following are factors to consider in designing synthetic ligands: 1) Histidine 381 acts as a hydrogen bond acceptor for the R 4 hydroxyl, with the optimal tautomer maintained by water molecules. See FIG. 23 and FIG 24. Histidine is the only hydrophilic residue in this hydrophobic pocket that surrounds the R 4 substituent.

Histidine can be either a hydrogen bond acceptor or donor, depending on its tautomeric state. It is preferably a hydrogen bond donor, but can tolerate being a hydrogen bond acceptor, as for example, when there is a methoxy at the R 4 position of the ligand; 2) Arginines 228, 262, and 266 interact directly and through water-mediated hydrogen bonds with the Ri-substituent, with the electrostatic interaction provided by Arginine 266 (as in the Triac complex). This polar pocket is illustrated by FIG. 23 FIG. 25. FIG. 23 depicts T 3 in the TRa ligand binding cavity, where T3's aminopropionic R1- substituent interacts with Arg 228, HOH502, H9H503 and HOH504 via hydrogen bonds. FIG. 24 depicts triac in the ligand binding cavity, with its -COOH R, substituent in the polar pocket. In FIG. 24, Arg 228 no longer shares a hydrogen bond with the ligand, but the -COOH R, substituent forms hydrogen bonds with Arg 266.

FIG. 25 superimposes T 3 and triac in the ligand binding cavity and shows several positionally unchanged amino acids and water molecules, and selected changed interacting amino acids and water molecules. The three figures illustrate parts of the polar pocket that can change and those parts that do not move upon binding of different ligands. For example, the Arg 262 at the top of the polar pocket does not move, even when the R, substituent has changed from a -COOH to an aminopropionic acid group. However, the other two Arginines, Arg 228 and Arg 266, demonstrate flexibility in the polar pocket to respond to the change in the size or chemical naure of the R, substituent.; 3) Inner and outer pockets for the R 3

/R

5 substituents are formed by Ser260, Ala263, Ile299; and Phe 218, Ile221, Ile222, respectively. See FIGS. 21 and 22. The WO 97/21993 PcTIUS96/20779 66.

inner pocket is filled by either the R 3 or the R 5 substituent, regardless of the size of the substituent, and may act as a binding determinant by positioning the ligand in the receptor. Optimally, the inner pocket amino acids interact with an R3 or R5 substituent that is no larger than an iodo group. If the inner pocket is filled by the R, substituent, then the outer pocket interacts with the R, substituent and vice versa. The outer pocket can adjust to the size of its substituent through main chain motion centered at the break in helix 3 (Lys220-11e221), suggesting that the bending of H3, and motion of the N-terminal portion of H3, may represent a conformational change induced on ligand binding. The outer pocket has greater flexibility than does the inner pocket in terms of accommodating a larger substituent group.

4) A pocket for the R3'-substituent is formed by Phe 215, Gly290, Met388.

The pocket is incompletely filled by the R,'-iodo substituent, and accommodates the slightly larger 3'-isopropyl substituent by movement of the flexible Met388 side chain and the H7/H8 loop. This pocket can accommodate R 3 substituents that are even larger than isopropyl, for example, a phenyl group.

The above information will facilitate the design of high affinity agonists and antagonists by improving automated QSAR methodologies and informing manual modeling of pharmaceutical lead compounds. For example, the inclusion of discrete water molecules provides a complete description of hydrogen bonding in the polar pocket for use with pharmacophore development: also, the identification of mobile and immobile residues within the receptor suggests physically reasonable constraints for use in molecular mechanics/dynamics calculations.

EXAMPLE 12. DESIGN OF AN INCREASED AFFINITY LIGAND Direct interaction between the receptor and the ligand is limited in the polar pocket, which interacts with the R, substituent. While the lack of complementarity may contain implications for biological regulation, it also provides an opportunity for increasing affinity by optimizing the interaction between the amino acids of the polar pocket and the R, substituent of a synthetic ligand. The structure of the receptor-ligand interactions described herein enables design of an increased affinity synthetic ligand having two complementary modifications: WO 97/21993 PCT/US96/20778 67.

1) Remove the positively charged amine. The strongly positive electrostatic potential predicted for the polar pocket suggests that the positively charged amine of the aminopropionic acid R, substituent may be detrimental to binding. Suitable groups for substitution are suggested by the nature of nearby hydrogen bond partners: for example, Thr 275 O or Ser 277 N. See e.g. Tables in Appendix 2. For example, any any negatively charged substituent would be compatible for interacting with the amino acids of the polar pocket, including carboxylates, carbonyl, phosphonates, and sulfates, comprising 0 to 4 carbons. Another example of an R, substitution is an oxamic acid that replaces the amine of the naturally occurring ligand with one or more carbonyl groups.

2) Incorporate hydrogen bond acceptor and donor groups into the R,substituent to provide broader interactions with the polar pocket scaffold. Such hydrogen bond acceptor and donor groups incorporated into the R1-substituent will allow interactions that would otherwise occur with water molecules in the polar pocket.

Specific waters include HOH 504 (hydrogen bonds with Ala 225 O and Arg 262 NH); and HOH 503 hydrogen bonds with Asn 179 ODI, Ala 180 both of which are present in all four complexes (TR LBD complexed with T3, TR LBC complexed with IpBr 2

TR

LBD complexed with Dimit and TR LBD complexed with Triac). Analysis of the hydrogen bonding network in the polar pocket suggests replacement of HOH 504 with a hydrogen bond acceptor, and HOH 503 with an hydrogen bond donor (although the chemical nature of asparagine probably permits flexibility at this site). Thus, incorporating a hydrogen bond acceptor in an RI substituent that could take the place of the HOH504 or incorporating a hydrogen bond acceptor in an RI substituent that could positionally replace the HOH503, or a combination thereof, are methods of designing novel synthetic TR ligands.

These two design approaches can be used separately or in combination to design synthetic ligands, including those in Table 4 (below).

A corollary to this approach is to design specific interactions to the residues Arg262 and Asn 179. The goal is to build in interactions to these residues by designing ligands that have R, substituents that form hydrogen bonds with water molecules or charged residues in the polar pocket.

WO 97/21993 PCTIUS96120779 68.

Table 4: Synthetic TR Ligands 'R R's R6 R 3 'R Fr2 R 3

RI

RI R2 R3 RS R6 X R'2 R'3 R'4 R'S R'6 C02H H Me Me H 0 H Me OH Me H CH2CO2H I I S Et SH Et CH2CH2CO2H Br Br nPr NH2 O~r CH2CH(NH2)CO2H C1 Cl iPr iPr OCH2CO2H E EtPh nBu.

OCH2CH2CO2H OH off I uiPen NHCH2CO2H NH2 NH2 Br nHex NHCH2CH2CO2H SH SH CI Ph CH2COCOCO2H hetero cycle NHCOCOC02H aryl COC02H CF2C02H COCH2CO2H Any combination of the above substituents in the biphenyl ether scaffold structure shown above may result in a potentially pharmacologically useful ligand for the thyroid hormone receptor. These novel ligands may be antagonists of the thyroid receptor.

WO 97/21993 WO 9721993PCT'/US96120778 A strategy for designing synthetic ligands using the computational methods described herein is summed below:

HO.

For example,

D

0 0 A Hydrogen Bond Acceptor D Hydrogen Bond Donor 0 -OH, -CO RIO can be -OH, -CO can be -CO can be -COOH, -CONH2 See also Table of synthetic TR Ligands WO 97/21993 PCTIIJS9620778 TABLE 3: LBD-122/410 Dimit T3 IpBr, Triac [Data collection Cell dimensions a()117.16 127.39 117.18 118.19 b 80.52 80.20 80.12 831.37 C (Ak) 63.21 6 3.23 63.13 63.73 9 120.58 120.60 [20.69 121.00 Resolution 2.2 2.0 2.1 2.45 Obs. Reflections, 57031 64424 66877 83573 (no.) Unique Reflections, 22327 21023 23966 19453 (no.) Completeness, 87.0 82.4 93.7 96.0 7)3.9 3.5 4.5 Phasing (15.0 2.SA) tR~r(7) 19.6 11.6 No. of sites -3 2 tOccupancy 44.6 (39.8) 35.0 (Anomalous) -50.2 (23.7) 35.0 39.2 (22.3)

FH/E

centric (acentric) 15.0-5.o A 3.67 (4.61) 2.2 (3.09) 5.0-3.0 A -2.23 (2.75) 1.25 (1.85) 3.0.-2.5A 1.64(l.99) 1.15 (1.57) 15.o.5.o A 33 44 5.0-3.o A -45 63 3.0-2.5 A 60 Mean figure of merit 0.62 MR Phasing (30-3 Rotation Search: 309.37 Eyler Angles ()48.96 e, 127.28 I corre1ltion 34.3 coefficient Translation Search: x -0.1571 Fractional coordinates WO 97/21993 PCT/US96/20778 71.

y 0.000 z 0.3421 correlation 65.8 Coefficient 'R factor 31.2 Refinement 15.0-2.2 5.0 2.0 15.0 2.2 25-2.5 Resolution (A) l mI t sl 20.5 22.1 21.4 23.6 Rf 22.7 24.0 22.4 24.1 All publications and patent applications mentioned in this specification are herein incorporated by reference to the same extent as if each individual publication or patent application was specifically and individually indicated to be incorporated by reference.

The nuclear receptor ligands, particularly the TR ligands, of these references are herein incorporated by reference and can be optionally excluded from the claimed compounds with a proviso.

Headings and subheadings are presented only for the convenience of the reader and should not be used to construe the meaning of terms used within such headings and subheadings.

The invention now being fully described, it will be apparent to one of ordinary skill in the art that many changes and modifications can be made thereto without departing from the spirit or scope of the appended claims.

WO 97/21993' Dd-r fff I 72.

UYUUI/

APPENDIX

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Zenke, Munoz, Sap, Vennstrom, B. Beug, H. Cell 61, 1035-1049 WO 97/21993 PCT/US96/20778 Dimit Atom awtzraaicns o( Omrit wiit Thyraid Hor7,.Ore ,ec~plor Amrino Ar~ds Amino Acid Amino Acid Distance In full length a Atom A Cie Gto C19 Cie C19 Cie C19 Ce..

CS

C010: C2 C13 0 4. 04 0. C10.

dio 615 C1 013 04 04 C 17 03 N1 C7 N1

CIS

21 S-PHE 21- PH E 218- PHE 218- PH-E 21a-PHE 218- PHE 21 8-PHE 219-THR 221-ILE 222-ILE 222-iLE 222-ILE: 222-ILE 225-ALA~ 25-A LA" 226-ARG: 228-ARG A 258-ARG 258-MET 259-MET- 259-MET 259-MET 259-MET 259-MET 252-MET -252-ARG 262-ARGc 263-ALA 266-AR G 275-THR- 275-LEU 276-LEU 276-LEU 276-LEU 270-LEU 276-LEU 277-SEb 277-SER Col CE1 0 C a C a C02 CG2

CGI

Col Col.

Ca

CB

C z NH2 NH2

SO,

CE:

C

0 Ca Ce Ca Ce

CA

CA2 -C02 CD2 C02 3.88 3.89 3.89 3.92 4.13 3.77 3.68 4.11 4.18"* 3.72 3 3.95 3.58 2.8 3.70 3.89 3.68 4.03 3 3.42 87 3.85 3.71 344; 3.93 3.51 392-' -4 OS 4.09 3.95 4.17 3.70 WO 97/21993 PCT/US96/20778 77.

Dimit Amino Acid Atom in full length a Atom Distance A f-I1 r N1 03 C17 03 C13 C7 C18 Ci8 C18 C18 C2 C4 C6 C2 C4 02 C4 C6 C8 01.

C8

CIO

01 01 C8

CIO

01 C8 C8 01 C16i 01 C17 03 04 C17 N1 03 C17 04 i /-aSR 277-SER 277-SER 277-SER 277-SER 277-SER 287-LEU 290-GLY 290-GLY 291-GLY 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 299-ILE 381 -HIS 381-HIS 381-HIS 381-HIS 381-HIS 381-HIS 381-HIS 388-MET 401 -PHE 401-PHE 401 -PHE 401-PHE 3-H 2 0 502 3-H,0 2-H,0 2-H,0 2-H 2 0 503 4-H,0 504

N

N

N

CA

CA

OG

C02

C

0

CA

N

CG

CG

CG

CD1 CD1 CD1 CD2 CD2 CD2 CD2 CD2 CD1 CD2 CD2 GO2 CE1 NE2 NE2 NE2

CE

CE1 CEl

CZ

CZ

01 01 01 01 01 01 01 01 01 3.69 3.30 3.19 3.92 3.35 3.92 3.90 4.04 3.54 4.04 4.20 4.18 3.88 4.01 3.88 4.02 4.07 4.05 3.72 3.69 3.98 4.16 3.87 3.90 3.84 3.40 3.72 3.47 3.51 2.64 3.90 4.19 3.37 3.97 3.28 3.77 3.13 3.72 4.04 3.84 3.35 2.56 3.92 2.72 01 L 2.72 Legend to Table XX. The table lists the interactions with Dimit (DMT). The column headings are as follows: #1 The atom of Dimit that interacts with the amino acid of the receptor. These are also numbered in figure X.

#2 The amino acid in the full length rTRo that interacts with the ligand.

#3 The name of the atom in the amino acid (standard nomenclature) where the interaction occurs.

#4 The distance in A between Dimit and the protein atom.

APPENDIX 2 WO 97/21993 WO 97/21993 PCT/US96/20778 78.

Triac Amo Acid Amo Acid Atom in full length a Atom Distance A I1 218-P O 3.2 I1 221-ILE CD1 4.16 I1 222-ILE CA 4.15 I1 222-ILE CB 4.03 1 221-ILE CG1 3.92 C8 222-ILE CD1 4.12 0 c 1 222-ILE CD1 3.7 2 C12 222-ILE CD1 3.79 C13 225-ALA CB 4.17 C3 225-ALA CB 3.86 258-MET SD 3.45 C12 258-MET SD 3.73 258-MET CE 3.66 C12 256-MET CE 3.77 CII 256-MET C 3.68 CII 256-MET O 3.24 C1 259-MET o 3.93 C11 259-MET O 3.24 03 259-MET O 3 2 4 03 259-MET 0 4.09 C1 259-MET CS 3.89 C13 259-MET O 3.74 C14 259-MET 0 3.96 Cl 259-MET CB 3.89 CII 259-MET CB 3.68 C13 259-MET CB 4.01 C14 262-ARG CB 4.07 04 262-ARG CB 3.60 C17 282-ARG

CD

04 262-ARG

CD

03 263-ALA N 3.79 03 263-ALA CA 3.67 03 283-ALA CB 3.49 C11 107-ALA CB 4.00 03 107-ALA CB 3.49 03 266-ARG NH1 3.00 03 275-THR O 3.20 03 278-LEU CA 3.11 N1 276-LEU C 3.52 03 120-LEU N 4.04 C14 120-LEU CA 3.98 03 120-LEU CA 3.11 C14 120-LEU C 3.98 03 120-LEU CB 3.95 02 276-LEU CD1 4.03 11 276-LEU CD1 4.10 C7 276-LEU CD2 3.84 C9 276-LEU CD2 3.73 CII 276-LEU CD2 4.06 02 276-LEU CD2 4.10 APPENDIX 2 WO 97/21993 WO 9721993PC"T/US96ZO778 Triac Amino Acia Amino Acid Atom in full length a Atom Distance A C13 277-SER N 4.06 C14 277-SER N 3.13 04 277-SER N 3.28 03 277-SER N 3.05 C14 277-SER CA 3.76 04 277-SER CA 3.52 C3 277-SER OG 3.87 12 290-GLY 0 3.57 12 292-LEU CG 3.94 C4 292-LEU CG 3.95 C6 292-LEU CG 3.65 C2 292-LEU CD1 4.11 C4 292-LEU CD1 3.85 12 292-LEU CD2 3.98 C4 292-LEU CD2 4.11 C6 292-LEU CD2 3.44 CB 292-LEU CD2 3.28 292-LEU CD2 3.88 01 292-LEU CD2 3.35 13 299-ILE CD1 3.77 CB 381 -HIS CD2 3.87 C11 381-HIS CD2 3.90 01 381-HIS G02 .3.20 01 381 -HIS GE1 3.81 Ce 381-HIS NE? 3.51 Cl0 381-HIS NE? 3.52 01 381 -HIS NE2 2.64 01 388-MET CE 4.03 01 401-PHE CEI 3.86 01 1 401 -PHE CZ 3.70 Legend to Table XX. The table lists the interactions with triac. The column headings are as follows: #1 The atom of triac that interacts with the amino acid of the receptor. These are also numbered in figure X.

#2 The amino acid in the full length rTR& that interacts with the ligand.

#3 The name of the atom in the amino acid (standard nomenclature) where the interaction occurs.

#4 The distance in A between triac and the protein atom.

APPENDIX 2 WO 97/21993 PCTIUS96/20778 lpSR2 Atom Amino Acid Amino Acid Distance in full length a Atom

A

C16 21 S-PHE CD1 C16 215-PHE GEI 3.78 BRi 218-PHE 0 3.24 5BR1 218-PHE C 3.9 ClE 218-PHE CB 3.81 C18 2 18-PHE CB 3.92 BRi 218-PHE CB 4.05 C18 218-PHE CD2 3.92 c18 219-THR CG2 34 BRi 221 -ILE CGI 3.81 BRI 221-ILE CDl 4.07 C6 222-ILE CD1 4.07 C8 222-ILE CD1 3.64 ciO 222-ILE CD1 3.50 C12 222-ILE CD1 3.82 01, 222-ILE CDi 4.08 C13 225-ALA Co 3.76 04 225-ALA GB 4.01 04 228-ARG CZ 3.92 C17 228-ARG NH2 3.26 03' 228-ARG NH2 3.43 04 228-ARG NH2 2.79 CIO 256-MET SD 3.65 C12 256-MET so 3.71 ClO 256-MET CE 3.90 C12 256-MET CE 3.75 BR2 256-MET CE 4.03 Cil 259-MET C 3.98 Cil 259-MET 0 3.52 C16 259-MET 0 3.44 NI 259-MET 0 3.76 Cil 259-MET CB 3.87 262-ARG Ca 4.03 APPENDIX 2 WO 97/21"93 PCTIUS96/20778 APPENDIX 2 WO 97/21993 PCT/US96/20778.

lp8R2 Atom Amino Acid Amino Acid Distance in full length'a Atom

A

C4 292-LEU C D2 4.07 C6 292-LEU CD2 3,75 C8 292-LEU C02 3.67 292-LEU CD2 .92a 8R2 299-ILE CD1 3.68 C8 .361-HIS CID2 3.67 381 -HIS CD2 3.92 01 381-HIS GD2 3.50 01 381-HIS CEl 3.62 Ca 381-HIS NE2 3.36 Cl0 381-HIS NE2 3.34 01 381-HIS NE2 2.62 Ca 401 -PHE CEI 4.02 01 401 -PHE CEl 3.19 C16 401 -PHE CZ 4.03' 01 401 -PHE CZ' 3.06 C17 3-H 2 0 01 03 502H 2 0 01 3.40 04 3-H 2 0 01 C15 2-H 2 0 01 C17 2-H 2 0 01 Ni1 502H 2 0 01 3.12 03 503H 2 0. 01 2.27 C17 4-H 2 0 01 014 504HO 01 1.78 Legend to Table XX. The table lists the interactions with Ip~r2. The column headings are as nfgr The atom of pBr2 that interacts with the amino acid of the receptor. These are also #2 The amino acid in the full length rTRa that interacts with the ligand.

#3 The name of the atom in the amino acid (standard nomenclature) where the Interaction #4 The distance in A between 1p~r2 and the protein atom.

AkPPENDIX 2 WO 97/21993 PCT/US96/0779 APPENDIX 2 WO-97/21993 PCT/US96/20778 NI1.

Ni

NI

Ni

NI

C7 C7 C9 cil C14 04 N 1 03 03 C1 3 12 C4 ca C2 C4 C4 C6 C8 cia 01 13 C8 dlo 01 263-ALA 263-ALA 263-ALA 275-TH R 276-LEU 276-LEU 276-LEU 276-LEU 276-LEU 276-LEU 276-LEU 277-SER 277-SER 228-ARG 277-SER 277-SSER 277-SER 277-SER 277-SER 290-GLY 292 -LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 292-LEU 299-ILE 381 -HIS 381 -HIS 381 -HIS

CA

Cs 0

CA

C

CD1 CD 1 CD2 CD2 CD2

N

N

NH 1

N

N

CA

CA

OG

0

CG

CG

CDl CD1 C132 CD2 CD2 CD2 CD2 CD1 C02 CD2 CD2 3.81 3.81 3.63 3.54 3.38 3.73 4.00 4.05 3.80 3.70 4.01 3.67 3.62 3.23 3.07 3.24 3.77 3.34 3.92 3.50 3.95 3.83 4.07 3.99 4.09 3.58 3.50 3.96 3.71 3.74 3.94 3.97 '3.39 APPENDIX 2 WO 97/21993 WO 9721993PCT/US96/20778 T3 Atom Amino Acid Amino Acid D Stance in full length a Atom

A

01 381-HIS Coll 3.82 CS 381-HIS NE2 3.47 381-HIS NE2 3.55.

01 3 81-HIS NE2 2.70 501 388-MET CE 3.88 01 401 -PH E dE1 3.52 01 401-PHE CZ 3.32 03 502 01 2.51 04 3-H 2 0 01 N1 2-H 2 0 01 03 503 01 2.81 1104 504 01 2.73 Legend to Table XX. The table lists the interactions with T3. The column headings are as follows- #1 The atom of T3 that interacts with the amino acid of the receptor. These are also numbered in figure X.

#2 The amino acid in the full length rTRa that interacts with the ligand.

#3 The name of the atom in the amino acid (standard nomenclature) where the interaction occurs.

#4 The distance in A between T3 and the protein atom.

APPENDIX 2 WO 97/21993 PCTUS9620778 86.

Coordination Structre of Thyroid Hormone Receptor and Dimit Coordnatn SlrucureI R2 I I R ,I RR R, I R I R, I -CH.CH(NH(CO)H -H -CHI CH, -H -H -CH(CH3)2 'OH _H -H 01 Amino Acid r1u215 Seconda Slructure H3 inoAcid I 1 1 Secondary Strucure II H3 I I I H3 AioAcid I I 1 110r7t Secondary Structure H3 mino Acid I 1221 Seconda Slructur I I H3 Amino Acid I I 222 122 222 222 Secondary Structure IH3 H 3 H3 H3 mino Acid 225 Secondary Structure H3 mino Acid 228 Secondary Structure H3 mino Acid IIA_-I1_258 258 secondary Structure

I__III__II__

SlrudrH S-HO SecodArid 259 I 259 Secordary Strudur1 H5-H8 I 1 mino Acid 252 secondary Struciure HO I )6 Secondary Srucdurs lo I mino Acid 26- Amino A:id 275 ecandaryStructure IS3 I i I I mino Acid 278 1 127j 276 1 2761- Seondary St;ructurv S3 53 53 I S3 I mine Acid 277 Secondary Slrclur mine Acid 290-291 Secanclaa Structure i mino Acid I 12921 292 292 292 292 Secondary Sructure I 110001 loop 110001 loop I o0 I I I I I Tmin--- Aci -8 1 -8 SecondaryStructure I I I I Hill AioAcid I I8I 8 e cayStrucure H11 1 1 M1( t mino Acid I 4 I I I I 1 1 Secondary Sructure i I 1 i I H12 I H121 I I mino Acd tHOHM5, 4O"So5, HoHS__ Secondary Siructure

I

APPENDIX 2 WO 97/21993 PCT/US96/20778 87.

Coordination Structure of Thyroid Hormone Receptor and Triac Coorlnetlon Structure I R, mino Acid Secondary Siructure mino Acid Seconday Sircture R7! R3 IRS R R' R-1 21 .H -H -H -OH -H -H 01 215 H3 H 3 I I I *F H3 I I I I3 219 1 S221 222 222212221 222 1 H3 I H3 I H3 Amino Acid Secondary Structure I Amino Acid Secondary Structure Amino Acid Secondary Structure I Amino Acid 225 Secondary Structure H3 mino Acid 228 Secondary Structure H3 mino Acid 258 Secondary Structure Hs-H I H-He mino Acid 259 Secondary Structure HG I IHS-H8 mino Acid' 282 Secondary Structure HS-H8 mino Acid 2e3 Secondary Structure HS-Hmino Acid 260 Sewndary Struure loop minoAid 275 Secondary Sructure S3 I I I I mino Acid 278 270 27_ 27_ Secondary Structure S3 S3 S3 S3 I m Acid 277 AIrudE 2 noAdd 1 1 290--291n

I*

SecondaD: Structure I l I II mino Acid 12921 292 __292_1 292 Secondary Structure 1100 1000 0 f TOOP mnoAcid 299 Secondary Strucure He mino Acid 1 13811 381 1 Secondary Structure I _lH11H I mino Acid 388 SeodaySructure t mino Acid 401 1401 1 Secondary Siructure H12 I M12 1 minoAcid 1401IS02.HoHSo

MSO

Secondary Structura I APPENDIX 2 WO 97/21993 PCTIUS96/20778 88.

Coordination Srncrure of Thyroid Hormone Receptor and IpBr2 coordination Struclure I R, IR, I RsIPR.,I R R' IR. R I IX _CH2.CH(NH (CO H -H -Br -Or -H *H -OH -H *H 0 mino Acid 215 Seconda Structure H3 mino Acid 218 218 Secondary Structure H3 H3 I mino Acid 219 Secondary Structure H3 mino Acid 221 Secondary Structure I H3 mino Acid 222 12221 222 1 222 Secondary Structure H3 H3 I H3 H3 mino Acid 225 Seconda Structure H3 minoAcid 228 Secondary Structure H3 mino Acid 1 258 258 Secondary Structure I Hfs.H8IHS-H81 mino Acid 259 259 Secandary Structure H5-1H HH I mino Acid 282 Secondary Structure H8mino Acid 263 Secondary Stricture HS-H mino Acid 266 Secondary Structure 1000 AminoA:id 275 Secondary Structirs mino Acid 278 276 I 278 278 Secondary Structure S3 S3 S3 S3 minoAcid 277 Secondary Structure Acdd 290-291 Seoni Slruur" Inefti AminoAcd 2_21 292 1 9 292 22 292 Secondary Structure I_ __299 l loop loop I 1oo I lo mino Acid, I I I I Secondary Structur His I mino Acid __11 351 Seconday Structure _I H-8 mino Acid 38a Secondary Structure Hil mino Acid 401 14 Secondar Structure H12 I H121 I mino Add IWo14SOz, PON 5 63 I Secondary Structure APPENDIX 2 WO 97/21993 PCTIUS96/20778 Coordination Structre of Thyroid Hormone Receptor and T3 Coordlnation Stncture IR I Rj R I R R R-7 I *CHI.CH(NHz)(COdH *H :r -x -H -H -t -OH *H 0 mino Acid II 215 Secondary Structure I 1 I IQ minoAcid L 218II II 218 Secondary Structure I IH3I I 1 H3 minoAcid I I I 219 Secondary Structure I H3 mino Acid 4 2211 Secondary StruturO F H3 AioAcid I I I I I I222 1 222) 222 1 222 gecondary struc-ure !_1I I I I I H3 H J 3 H 3 minoAcid 1 225 1 Secondary Structure H2 AioAcid 228 Secondary_____aure I H3 minoAcid r 5 I I I25 I8 I Secondary Structure I mino Acid 1 2 259 Secondary Structure AioAcid 262 Secondary Strucure HS__ mino Acid 253 Secondary Struclure HS-H_ mino Acid 282 Secondary Structure Homino Acid 275 secondary structure S3 Seconda Structure S3 S3 S3 S3 Acid 2 77 u e A Qlru llra

V

-Amino Acid j f j 290-291 Secondary Structure lo Amino Acid I 1292r 292 292 1 292 1292 Secondary Strcture I I 1 0oop0l... l oop 1 100D loop Amino Acid 299 1 2 1 #SecndaryStructure H8 x A A o;A 3131 3511 Secondary Struc:uro 15_ 1 HI I Amino Acid Secondary Structure AmioI I 01_ 1401 Amino Acid 401 401 1 Cinuita I JC~UIIUQI V\IYI Y U i .I I I I I I Amlnn Add I NHd2C ~cWan~,dflfI i I 1 M T 1 t N 0 Secondary Structure______ APPENDIX 2

Claims (10)

1. A crystal of a TR LBD comprising: o a TR LBD and a TR LBD ligand, wherein said crystal was formed at a temperature ranging from about 18 0 C to about 2500, and diffracts with at least a 3.0 angstrom resolution. 00

2. The crystal of claim 1, wherein said TR LBD has at least 200 amino acids.

3. The crystal of claim 2, wherein said TR LBD is from a TR protein selected ci from the group consisting of TR amino acid sequence 122 to 410 of rat TR-a, 157 to 410 rat TR-a and 202 to 461 TR-f3.

4. The crystal of claim 2, wherein said TR LBD ligand is a compound being of a formula: 'R '6 R5 R 6 \/X/\R1O R 'R 3 'R 2 R3 2 wherein R, is -O-CH 2 00 2 H, -NHCH 2 C0 2 H, -CO 2 H, -CH 2 C0 2 H, -CH 2 CH 2 C0 2 H, -CH 2 CH 2 CH 2 00 2 H, -CH 2 CH(NH 2 )CO 2 H, -CH 2 CH[NHCOCHM 2 CO 2 H, -CH 2 CH[NHCO(CH 2 15 CH 3 ]CO 2 H, -CH 2 CH[NH-FMOC]00 2 H, -CH 2 CH[NH-tBOC]CO 2 H, or a carboxylate connected to the ring with a 0 to 3 carbon linker, -P0 3 H 2 -0H 2 P0 3 H 2 -CH 2 CH 2 PO 3 H 2 -CH 2 CHNH 2 PO 3 H 2 -CH 2 CH[NH-COCH-1 2 ]PO 3 H- 2 -CH 2 CHIINHCO(CH 2 1

5 CH 3 ]PO 3 H 2 -CH 2 CH[NH-FMOC]P0 3 H 2 -CH- 2 CH[N-tBO3C]P0 3 H- 2 or a phosphate or phosphonate connected to the ring with a 0 to 3 carbon linker, WA'Fi~cm\69862S\69B62S sp~i.do. r_ I -SO 3 H, -CH 2 SO 3 H, -CH 2 CH 2 SO 3 H, -CH 2 CHNH 2 SO 3 ,H, -CH 2 CH[NHCOCH) 2 ]SO 3 H, -CH 2 CH[NHCO(CH 2 15 CH 3 ]S0 3 H 2 S-CH 2 CH[NH-FMOC]SO 3 H, -CH 2 CH[NH-tBOC]SO 3 H, or a sulfate or sulfite connected to the ring with a 0 to 3 carbon linker, 00 or acts as the functional equivalent of CH 2 CH(NH 2 )CO 2 H of T3 in the molecular o 0 recognition domain when bound to a TR, wherein said R 1 can be optionally substituted with an amine, wherein R 2 is SH, halogen, CF 3 OH, NH 2 SH, CH 3 -Et, or acts as the functional equivalent of H in the molecular recognition domain when bound to a TR, wherein R 3 is halogen, -CF 3 -OH, -NH 2 -N3, -SH, -CH 3 -Et, or acts as the functional equivalent of I in the molecular recognition domain when bound to a TR, wherein R 5 is halogen, -CF 3 -OH, -NH 2 -N 3 -SH, -CH 3 -Et, or acts as the functional equivalent of I in the molecular recognition domain when bound to a TR, and R 3 can be identical to R 5 wherein R 6 is halogen, -CF 3 -OH, -NH 2 -SH, -CH 3 or acts as the functional equivalent of H in the molecular recognition domain when bound to a TR, and R 2 can be identical to R 6 wherein R 2 is halogen, -CF 3 -OH, -NH 2 -N 3 -SH, -CH 3 -Et, or acts as the functional equivalent of H in the molecular recognition domain when bound to a TR, Y:\MarNKI NO DELETE2003220708.doc I 92 n wherein R 3 is any hydrophobic group, including C halogen, -CF 3 -SH, alkyl, aryl, 5- or 6-membered heterocyclic, cyano, Jb or acts as the functional equivalent of I in the molecular recognition domain when bound to a TR, 0 wherein R 4 is 00 halogen, -CF 3 -OH, -NH 2 NH 3 -N(CH 3 3 carboxylate, phosphonate, phosphate or sulfate, -SH, -CH 3 -Et, or alkyl, aryl or 5- or 6-membered N heterocyclic aromatic attached through urea or carbamate linkages to O or N or S S 10 at the R 4 position, or acts as the functional equivalent of OH in the molecular Srecognition domain when bound to a TR, wherein R 5 is -OH, -NH 2 -N(CH 3 2 -SH, -NH 3 -N(CH 3 3 carboxylate, phosphonate, phosphate, sulfate, branched or straight chain alkyl having 1 to 9 carbons, substituted or unsubstituted aryl, wherein said substituted aryl is substituted with halogen or 1 to 5 carbon alkyl and wherein said aryl is optionally connected to the ring by a -CH 2 aromatic heterocycle having 5 to 6 atoms, wherein said heterocycle may be substituted with one or more groups selected from -OH, -NH 2 -SH, -NH 3 -N(CH 3 3 carboxylate, phosphonate, phosphate, sulfate, heteroalkyl, heteroaryl, arylalkyl, heteroaryl alkyl, polyaromatic, polyheteroaromatic, wherein said R 5 may be substituted with polar or charged groups. wherein R 6 is halogen, -CF 3 -OH, -NH 2 -SH, -CH 3 -Et, or acts as the functional equivalent of H in the molecular recognition domain when bound to a TR, wherein X is O, S, SO 2 NH, NR 7 CH 2 CHR 7 CR 7 R 7 wherein R 7 is alkyl, aryl or 5- or

6-membered heterocyclic aromatic, and wherein said TR LBD ligand has an apparent Kd for binding TR LBD of 1pM or less. Y:\MaryNKI NO DELETE\2003220708.doc I 93 n 5. The crystal of claim 2, wherein said crystal of TR LBD ligand has the Sfollowing unit cell dimensions in angstroms: a=117.00 b=80.00 2%, to c=63.00 at a P angle of 120.00 2% degrees and a monoclinic space group C2. oo 6. The crystal of claim 5, wherein said crystal coordinates said TR LBD ligand 0 o and said crystal is selected from the group consisting of crystals having one of the following sets of properties: S1) unit cell dimensions in angstroms: a=117.16, b=80.52, c=63.21, at a p angle of 120.58 degrees, a monoclinic space group C2, 2.2 angstrom resolution c and completeness value of 87.0%, 2) unit cell dimensions in angstroms: a=117.19, b=80.20, c=63.23, at a P angle of 120.60 degrees, a monoclinic space group C2, 2.0 angstrom resolution and completeness value of 82.4%, and 3) unit cell dimensions in angstroms: a=117.18, b=80.12, c=63.13, at a p angle of 120.69 degrees, a monoclinic space group C2, 2.2 angstrom resolution and completeness value of 93.7%.

7. The crystal of claim 2, wherein said crystal further comprises a human protein.

8. The crystal of claim 7, wherein said crystal has the following unit cell dimensions in angstroms: a=b=68.448 and c=130.559 at an a angle of 90.000, a p angle of 90.000 and a y angle of 120.000 and having a trigonal space group p3(1)21.

9. The crystal of claim 8, wherein said crystal further comprises a human protein. Y:\MaryKI NO DELETrE2003220708.doc 94 n

10. A crystal according to claim 1 substantially as hereinbefore described with reference to any one of the examples or drawings. DATED: 8 August 2005 00 PHILLIPS ORMONDE FITZPATRICK oo Attorneys for: Y:\Mary\NKI NO DELETE\2003220708.doc