Peroxisome proliferator-activated receptor γ (PPARγ) is a ligand-regulated nuclear receptor transcription factor that regulates gene expression programs controlling adipogenesis and insulin sensitization. Endogenous PPARγ ligands, which include lipids and fatty acids, bind to an orthosteric pocket within the PPARγ ligand-binding domain (LBD) and function as PPARγ agonists that activate gene programs (Itoh et al., 2008; Li et al., 2008; Malapaka et al., 2012; Kliewer et al., 1997; Kliewer et al., 1995; Waku et al., 2009; Shang et al., 2018). Synthetic small molecule PPARγ ligands, which include FDA-approved antidiabetic drugs, also bind to the same orthosteric pocket, most of which function as agonists that activate PPARγ-mediated transcription. Endogenous and synthetic ligands were originally thought to compete for binding to the PPARγ orthosteric pocket. However, we previously showed that endogenous and synthetic ligands can cobind to PPARγ, likely due to the large size and flexibility of the orthosteric pocket, and synergistically influence PPARγ structure and function (Johnson et al., 2000).

The structural mechanism of agonist-induced activation of PPARγ transcription has been revealed by structural biology studies including NMR spectroscopy and crystal structures. In the absence of ligand, the apo (ligand-free) PPARγ LBD dynamically exchanges between two or more structural conformations (Shang et al., 2020). NMR data show that a critical structural element in the LBD called activation function-2 (AF-2) helix (helix 12), which is part of the AF-2 coactivator binding surface, exchanges between active and repressive conformations that can be stabilized upon binding ligand (Hughes et al., 2012). Agonist binding to the orthosteric pocket stabilizes a solvent exposed helix 12 conformation that enables high-affinity binding of coactivators and increases transcription (Shang et al., 2019; Frkic et al., 2023). Transcriptionally neutral antagonists and repressive inverse agonists developed from orthosteric agonist ligand scaffolds bind via a similar mechanism of agonists but stabilize non-active helix 12 conformations (Frkic et al., 2018; Zheng et al., 2018; Marciano et al., 2015; Lee et al., 2002).

GW9662 and T0070907 are covalent ligands originally described as antagonists as they bind via a nucleophilic substitution mechanism to Cys285 located within the orthosteric pocket and were shown to inhibit binding of select reference PPARγ agonists (Leesnitzer et al., 2002; Hughes et al., 2014). These ligands have been used extensively by the field as covalent antagonist inhibitors to block other synthetic ligands from binding PPARγ to test for synthetic ligand specificity in functional experiments. However, we previously showed GW9662 and T0070907 do not block all ligands from binding to PPARγ Johnson et al., 2000; Hughes et al., 2016; Brust et al., 2017; MacTavish et al., 2024 — and moreover, they have distinct pharmacological PPARγ functions as a transcriptionally neutral antagonist (GW9662) and repressive inverse agonist (T0070907) (Irwin et al., 2022). Although these covalent ligands have similar pharmacological functions to orthosteric non-covalent antagonists and inverse agonists, GW9662 and T0070907 function through a different structural mechanism: they slow the rate of exchange between transcriptionally active and repressive conformations natively populated in the apo-LBD, with T0070907 having a more pronounced effect than GW9662 (Hughes et al., 2012; Orsi et al., 2023). In the transcriptionally repressive conformation stabilized by covalent inverse agonists, helix 12 adopts a solvent-occluded conformation within the orthosteric pocket that overlaps with orthosteric ligand binding poses (Figure 1; Hughes et al., 2012; Orsi et al., 2023; Shang and Kojetin, 2021; Arifi et al., 2023). These and other published studies have informed a ligand activation model whereby agonist binding to the orthosteric pocket either displaces helix 12 from a solvent occluded repressive conformation within the orthosteric pocket to a solvent exposed active conformation, or selects for an active helix 12 conformation from the dynamic LBD ensemble (Jang et al., 2017).

Figure 1

Download asset Open asset

What remains unclear is the structural basis of covalent inhibitor and synthetic ligand cobinding. This ligand cobinding mechanism was originally discovered in studies of alternate site ligand binding (Hughes et al., 2016; Brust et al., 2017; MacTavish et al., 2024; Laghezza et al., 2018; Leijten-van de Gevel et al., 2022; Choi et al., 2011; Berger et al., 2003). Structural studies have mapped the alternate ligand-binding site (Hughes et al., 2016; Brust et al., 2017) when two equivalents of a synthetic ligand bind, one to the orthosteric pocket and another to the entrance of the orthosteric pocket (Jang et al., 2017). NMR and biochemical data revealed non-covalent synthetic compounds can still bind to the PPARγ LBD in the presence of a covalent orthosteric inhibitor (Hughes et al., 2016; Brust et al., 2017; MacTavish et al., 2024). While it is presumed that the non-covalent synthetic compound adopts a non-orthosteric binding mode at an alternate site, crystal structures to verify this cobinding mechanism are still needed. Here, using structural biology studies including NMR and crystallography, we confirm that GW9662 and T0070907 do not prevent other synthetic ligands from binding to PPARγ. Furthermore, we demonstrate that certain synthetic ligands can unexpectedly adopt an orthosteric binding pose when cobound with a covalent antagonist inhibitor.

Crystal structures of PPARγ bound to covalent and non-covalent synthetic ligands have shown overlapping ligand binding modes, indicating the covalent ligands should block binding of the non-covalent ligands. We and others have posited that cobinding of a non-covalent synthetic ligand to the PPARγ LBD prebound to a covalent ligand (GW9662 or T0070907) would reveal an alternate site binding mode, different from the crystallized binding modes. To our surprise, the non-covalent ligand can bind via its native orthosteric binding mode by pushing the covalent ligand aside, or slightly adapt its binding mode within the orthosteric pocket. Our structural analysis of non-covalent ligand cobinding with a covalent ligand reveals several important observations and conclusions.

Each of the non-covalent synthetic ligands utilizes unique mechanisms to cobind with the covalent ligands, as inferred from our crystal structures in which pre-formed crystals of the PPARγ LBD were soaked with non-covalent synthetic ligands BVT.13 cobinds to a region of the orthosteric pocket that only slightly overlaps with the orthosteric covalent ligand binding pose, adopting a cobinding pose that is similar to when soaked into apo-PPARγ LBD crystals. MRL24 and nTZDpa cobinding pushes the covalent orthosteric ligand into a different conformation, allowing these ligands to adopt their orthosteric binding modes in the cobound state. This finding was surprising for MRL24 in particular, as its orthosteric binding mode overlaps considerably with the orthosteric covalent ligand binding mode. In contrast, SR1664 cobinding occurs to the so-called alternate site, located at the entrance to the orthosteric pocket.

In our previous study, we observed synthetic and natural/endogenous ligand co-binding via co-crystallography where preformed crystals of PPARγ LBD bound to unsaturated fatty acids (UFAs) were soaked with a synthetic ligand, which pushed the bound UFA to an alternate site within the orthosteric ligand-binding pocket (Johnson et al., 2000). In the scenario of synthetic ligand cobinding with a covalent inhibitor, it is possible that soaking a covalent inhibitor into preformed crystals where the PPARγ LBD is already bound to a non-covalent ligand may prove to be difficult. The covalent inhibitor would need to flow through solvent channels within the crystal lattice, which may not be a problem. However, upon reaching the entrance surface to the orthosteric ligand-binding pocket, it may be difficult for the covalent inhibitor to gain access to the region of the orthosteric pocket required for covalent modification as the larger non-covalent ligand could block access. This potential order of addition problem may not be a problem for studies in solution or in cells, where the non-covalent ligand can more freely exchange in and out of the orthosteric pocket and over time the covalent reaction would reach full occupancy.

Our data provide support to structural model where in the absence of ligand, the PPARγ LBD exchanges between a transcriptionally repressive conformation where helix 12 is solvent occluded within the orthosteric pocket and a solvent exposed active conformation (Hughes et al., 2012). T0070907 binding slows the rate of exchange between these two conformations, stabilizing a long-lived active and repressive state (Irwin et al., 2022). GW9662-bound PPARγ LBD also samples active and repressive states, as observed by PRE NMR (Hughes et al., 2012), although the active conformation is more abundantly populated (McCoy et al., 2007). Agonist binding occurs via a two-step mechanism involving a fast encounter complex binding step at the entrance to the orthosteric pocket followed by a slow conformational change where the ligand translocates into the orthosteric pocket (Jang et al., 2017). Our NMR data here show that non-covalent ligand cobinding to T0070907-bound PPARγ LBD selects for an active conformation, as the repressive conformation NMR peak disappears. This indicates non-covalent ligand cobinding prevents the LBD from adopting a transcriptionally repressive helix 12 conformation within orthosteric pocket, explaining why non-covalent ligand cobinding of MRL24 and other PPARγ agonists with a covalent ligand activates PPARγ transcription (Hughes et al., 2016; Brust et al., 2017; MacTavish et al., 2024). Another way to test this structural model could be through the use of covalent PPARγ inverse agonist analogs with graded activity (Orsi et al., 2023), where one might posit that covalent inverse agonist analogs that shift the LBD conformational ensemble towards a fully repressive LBD conformation may better inhibit synthetic ligand cobinding.

Our findings may have profound implications as these GW9662 and T0070907 have been used in many published studies as covalent inhibitors to block ligand binding to PPARγ to test for binding and functional specificity in cells. As of May 2024, more than 1900 citations referring to ‘GW9662 or T0070907’ are reported in PubMed. Nearly 1000 of these publications were published in 2015 or later, after the original report that GW9662 and T0070907 are not effective inhibitors of ligand binding (Hughes et al., 2016), yet many in the field continue to use these compounds as covalent inhibitors. Our findings strongly suggest GW9662 and T0070907 should not be used as antagonists to block binding of other synthetic PPARγ ligands. On the other hand, GW9662 and T0070907 display unique pharmacological properties as a transcriptionally neutral antagonist and repressive inverse agonist, respectively Irwin et al., 2022, and thus it would be appropriate to use these compounds as pharmacological ligands. It may be possible to use the crystal structures we obtained to guide structure-informed design of covalent inhibitors that would physically block cobinding of a synthetic ligand. This could be the potential mechanism of a newer generation covalent antagonist inhibitor we developed, SR16832, that more completely inhibit alternate site ligand binding of an analog of MRL20, rosiglitazone and the UFA docosahexaenoic acid (DHA) MacTavish et al., 2024 and thus may be a better choice for the field to use as a covalent ligand inhibitor of PPARγ.

Diffraction data and crystal structures have been deposited in the PDB under accession codes 8ZFN, 8ZFO, 8ZFP, 8ZFQ, 8ZFR, 8ZFS, and 8ZFT. Other data generated and analyzed during the current study are in Figure 3—source data 1.

1. 1. Shang J
   2. Kojetin DJ

   (2024) RCSB Protein Data Bank

   ID 8ZFN. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with GW9662 and BVT.13.

   https://www.wwpdb.org/pdb?id=pdb_00008zfn
2. 1. Shang J
   2. Kojetin DJ

   (2024) RCSB Protein Data Bank

   ID 8ZFO. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with GW9662 and nTZDpa.

   https://www.wwpdb.org/pdb?id=pdb_00008zfo
3. 1. Shang J
   2. Kojetin DJ

   (2024) RCSB Protein Data Bank

   ID 8ZFP. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with GW9662 and MRL24.

   https://www.wwpdb.org/pdb?id=pdb_00008zfp
4. 1. Shang J
   2. Kojetin DJ

   (2024) RCSB Protein Data Bank

   ID 8ZFQ. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with T0070907 and BVT.

   https://www.wwpdb.org/pdb?id=pdb_00008zfq
5. 1. Shang J
   2. Kojetin DJ

   (2024) RCSB Protein Data Bank

   ID 8ZFR. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with T0070907 and nTZDpa.

   https://www.wwpdb.org/pdb?id=pdb_00008zfr
6. 1. Shang J
   2. Kojetin DJ

   (2024) RCSB Protein Data Bank

   ID 8ZFS. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with T0070907 and MRL24.

   https://www.wwpdb.org/pdb?id=pdb_00008zfs
7. 1. Shang J
   2. Kojetin DJ

   (2024) RCSB Protein Data Bank

   ID 8ZFT. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with T0070907 and SR1664.

   https://www.wwpdb.org/pdb?id=pdb_00008zft

1. 1. Tomioka D
   2. Hashimoto H
   3. Sato M
   4. Shimizu T

   (2011) RCSB Protein Data Bank

   ID 3B0R. Human PPAR gamma ligand binding dmain complexed with GW9662 in a covalent bonded form.

   https://www.wwpdb.org/pdb?id=pdb_00003b0r
2. 1. Shang J
   2. Fuhrmann J
   3. Brust R
   4. Kojetin DJ

   (2018) RCSB Protein Data Bank

   ID 6C1I. Crystal Structure of Human PPARgamma Ligand Binding Domain in Complex with T0070907.

   https://www.wwpdb.org/pdb?id=pdb_00006c1i
3. 1. Shang J
   2. Kojetin DJ

   (2022) RCSB Protein Data Bank

   ID 8FHE. Crystal structure of PPARgamma ligand-binding domain in complex with N-CoR peptide and GW9662.

   https://www.wwpdb.org/pdb?id=pdb_00008fhe
4. 1. Shang J
   2. Kojetin DJ

   (2019) RCSB Protein Data Bank

   ID 6ONI. Crystal structure of PPARgamma ligand binding domain in complex with N-CoR peptide and inverse agonist T0070907.

   https://www.wwpdb.org/pdb?id=pdb_00006oni
5. 1. Bruning JB
   2. Nettles KW

   (2007) RCSB Data Bank

   ID 2Q6S. 2.4 angstrom crystal structure of PPAR gamma complexed to BVT.13 without co-activator peptides.

   https://www.wwpdb.org/pdb?id=pdb_00002q6s
6. 1. Bruning JB
   2. Nettles KW

   (2007) RCSB Protein Data Bank

   ID 2Q5P. Crystal Structure of PPARgamma bound to partial agonist MRL24.

   https://www.wwpdb.org/pdb?id=pdb_00002q5p
7. 1. Bruning JB
   2. Nettles KW

   (2007) RCSB Protein Data Bank

   ID 2Q5S. Crystal Structure of PPARgamma bound to partial agonist nTZDpa.

   https://www.wwpdb.org/pdb?id=pdb_00002q5s
8. 1. Jang JY

   (2015) RCSB Protein Data Bank

   ID 5DWL. Human PPARgamma ligand binding dmain in complex with SR1664.

   https://www.wwpdb.org/pdb?id=pdb_00005dwl
9. 1. Marciano DP
   2. Kamenecka T
   3. Griffin PR
   4. Bruning JB

   (2014) RCSB Protein Data Bank

   ID 4R2U. Crystal Structure of PPARgamma in complex with SR1664.

   https://www.wwpdb.org/pdb?id=pdb_00004r2u
10. 1. Shang J
    2. Kojetin DJ

    (2019) RCSB Protein Data Bank

    ID 6ONJ. Crystal structure of PPARgamma ligand binding domain in complex with TRAP220 peptide and agonist rosiglitazone.

    https://www.wwpdb.org/pdb?id=pdb_00006onj

1. 1. Acton JJ III
   2. Black RM
   3. Jones AB
   4. Moller DE
   5. Colwell L
   6. Doebber TW
   7. MacNaul KL
   8. Berger J
   9. Wood HB

   (2005) Benzoyl 2-methyl indoles as selective PPARγ modulators

   Bioorganic & Medicinal Chemistry Letters 15:357–362.

   https://doi.org/10.1016/j.bmcl.2004.10.068

   • Google Scholar
2. 1. Adams PD
   2. Afonine PV
   3. Bunkóczi G
   4. Chen VB
   5. Davis IW
   6. Echols N
   7. Headd JJ
   8. Hung LW
   9. Kapral GJ
   10. Grosse-Kunstleve RW
   11. McCoy AJ
   12. Moriarty NW
   13. Oeffner R
   14. Read RJ
   15. Richardson DC
   16. Richardson JS
   17. Terwilliger TC
   18. Zwart PH

   (2010) PHENIX: a comprehensive Python-based system for macromolecular structure solution

   Acta Crystallographica. Section D, Biological Crystallography 66:213–221.

   https://doi.org/10.1107/S0907444909052925

   • PubMed
   • Google Scholar
3. 1. Agirre J
   2. Atanasova M
   3. Bagdonas H
   4. Ballard CB
   5. Baslé A
   6. Beilsten-Edmands J
   7. Borges RJ
   8. Brown DG
   9. Burgos-Mármol JJ
   10. Berrisford JM
   11. Bond PS
   12. Caballero I
   13. Catapano L
   14. Chojnowski G
   15. Cook AG
   16. Cowtan KD
   17. Croll TI
   18. Debreczeni JÉ
   19. Devenish NE
   20. Dodson EJ
   21. Drevon TR
   22. Emsley P
   23. Evans G
   24. Evans PR
   25. Fando M
   26. Foadi J
   27. Fuentes-Montero L
   28. Garman EF
   29. Gerstel M
   30. Gildea RJ
   31. Hatti K
   32. Hekkelman ML
   33. Heuser P
   34. Hoh SW
   35. Hough MA
   36. Jenkins HT
   37. Jiménez E
   38. Joosten RP
   39. Keegan RM
   40. Keep N
   41. Krissinel EB
   42. Kolenko P
   43. Kovalevskiy O
   44. Lamzin VS
   45. Lawson DM
   46. Lebedev AA
   47. Leslie AGW
   48. Lohkamp B
   49. Long F
   50. Malý M
   51. McCoy AJ
   52. McNicholas SJ
   53. Medina A
   54. Millán C
   55. Murray JW
   56. Murshudov GN
   57. Nicholls RA
   58. Noble MEM
   59. Oeffner R
   60. Pannu NS
   61. Parkhurst JM
   62. Pearce N
   63. Pereira J
   64. Perrakis A
   65. Powell HR
   66. Read RJ
   67. Rigden DJ
   68. Rochira W
   69. Sammito M
   70. Sánchez Rodríguez F
   71. Sheldrick GM
   72. Shelley KL
   73. Simkovic F
   74. Simpkin AJ
   75. Skubak P
   76. Sobolev E
   77. Steiner RA
   78. Stevenson K
   79. Tews I
   80. Thomas JMH
   81. Thorn A
   82. Valls JT
   83. Uski V
   84. Usón I
   85. Vagin A
   86. Velankar S
   87. Vollmar M
   88. Walden H
   89. Waterman D
   90. Wilson KS
   91. Winn MD
   92. Winter G
   93. Wojdyr M
   94. Yamashita K

   (2023) The CCP4 suite: integrative software for macromolecular crystallography

   Acta Crystallographica. Section D, Structural Biology 79:449–461.

   https://doi.org/10.1107/S2059798323003595

   • PubMed
   • Google Scholar
4. 1. Arifi S
   2. Marschner JA
   3. Pollinger J
   4. Isigkeit L
   5. Heitel P
   6. Kaiser A
   7. Obeser L
   8. Höfner G
   9. Proschak E
   10. Knapp S
   11. Chaikuad A
   12. Heering J
   13. Merk D

   (2023) Targeting the alternative vitamin E metabolite binding site enables noncanonical PPARγ modulation

   Journal of the American Chemical Society 145:14802–14810.

   https://doi.org/10.1021/jacs.3c03417

   • PubMed
   • Google Scholar
5. 1. Bae H
   2. Jang JY
   3. Choi SS
   4. Lee JJ
   5. Kim H
   6. Jo A
   7. Lee KJ
   8. Choi JH
   9. Suh SW
   10. Park SB

   (2016) Mechanistic elucidation guided by covalent inhibitors for the development of anti-diabetic PPARγ ligands

   Chemical Science 7:5523–5529.

   https://doi.org/10.1039/c6sc01279e

   • PubMed
   • Google Scholar
6. 1. Berger JP
   2. Petro AE
   3. Macnaul KL
   4. Kelly LJ
   5. Zhang BB
   6. Richards K
   7. Elbrecht A
   8. Johnson BA
   9. Zhou G
   10. Doebber TW
   11. Biswas C
   12. Parikh M
   13. Sharma N
   14. Tanen MR
   15. Thompson GM
   16. Ventre J
   17. Adams AD
   18. Mosley R
   19. Surwit RS
   20. Moller DE

   (2003) Distinct properties and advantages of a novel peroxisome proliferator-activated protein [gamma] selective modulator

   Molecular Endocrinology 17:662–676.

   https://doi.org/10.1210/me.2002-0217

   • PubMed
   • Google Scholar
7. 1. Bruning JB
   2. Chalmers MJ
   3. Prasad S
   4. Busby SA
   5. Kamenecka TM
   6. He Y
   7. Nettles KW
   8. Griffin PR

   (2007) Partial agonists activate PPARgamma using a helix 12 independent mechanism

   Structure 15:1258–1271.

   https://doi.org/10.1016/j.str.2007.07.014

   • PubMed
   • Google Scholar
8. 1. Brust R
   2. Lin H
   3. Fuhrmann J
   4. Asteian A
   5. Kamenecka TM
   6. Kojetin DJ

   (2017) Modification of the orthosteric PPARγ covalent antagonist scaffold yields an improved dual-site allosteric inhibitor

   ACS Chemical Biology 12:969–978.

   https://doi.org/10.1021/acschembio.6b01015

   • PubMed
   • Google Scholar
9. 1. Choi JH
   2. Banks AS
   3. Kamenecka TM
   4. Busby SA
   5. Chalmers MJ
   6. Kumar N
   7. Kuruvilla DS
   8. Shin Y
   9. He Y
   10. Bruning JB
   11. Marciano DP
   12. Cameron MD
   13. Laznik D
   14. Jurczak MJ
   15. Schürer SC
   16. Vidović D
   17. Shulman GI
   18. Spiegelman BM
   19. Griffin PR

   (2011) Antidiabetic actions of a non-agonist PPARγ ligand blocking Cdk5-mediated phosphorylation

   Nature 477:477–481.

   https://doi.org/10.1038/nature10383

   • PubMed
   • Google Scholar
10. 1. Chrisman IM
    2. Nemetchek MD
    3. de Vera IMS
    4. Shang J
    5. Heidari Z
    6. Long Y
    7. Reyes-Caballero H
    8. Galindo-Murillo R
    9. Cheatham TE III
    10. Blayo AL
    11. Shin Y
    12. Fuhrmann J
    13. Griffin PR
    14. Kamenecka TM
    15. Kojetin DJ
    16. Hughes TS

    (2018) Defining a conformational ensemble that directs activation of PPARγ

    Nature Communications 9:1794.

    https://doi.org/10.1038/s41467-018-04176-x

    • PubMed
    • Google Scholar
11. 1. Emsley P
    2. Cowtan K

    (2004) Coot: model-building tools for molecular graphics

    Acta Crystallographica. Section D, Biological Crystallography 60:2126–2132.

    https://doi.org/10.1107/S0907444904019158

    • PubMed
    • Google Scholar
12. 1. Frkic RL
    2. Marshall AC
    3. Blayo AL
    4. Pukala TL
    5. Kamenecka TM
    6. Griffin PR
    7. Bruning JB

    (2018) PPARγ in complex with an antagonist and inverse agonist: a tumble and trap mechanism of the activation helix

    iScience 5:69–79.

    https://doi.org/10.1016/j.isci.2018.06.012

    • PubMed
    • Google Scholar
13. 1. Frkic RL
    2. Pederick JL
    3. Horsfall AJ
    4. Jovcevski B
    5. Crame EE
    6. Kowalczyk W
    7. Pukala TL
    8. Chang MR
    9. Zheng J
    10. Blayo AL
    11. Abell AD
    12. Kamenecka TM
    13. Harbort JS
    14. Harmer JR
    15. Griffin PR
    16. Bruning JB

    (2023) PPARγ corepression involves alternate ligand conformation and inflation of H12 ensembles

    ACS Chemical Biology 18:1115–1123.

    https://doi.org/10.1021/acschembio.2c00917

    • PubMed
    • Google Scholar
14. 1. Ge K
    2. Guermah M
    3. Yuan CX
    4. Ito M
    5. Wallberg AE
    6. Spiegelman BM
    7. Roeder RG

    (2002) Transcription coactivator TRAP220 is required for PPAR gamma 2-stimulated adipogenesis

    Nature 417:563–567.

    https://doi.org/10.1038/417563a

    • PubMed
    • Google Scholar
15. 1. Hughes TS
    2. Chalmers MJ
    3. Novick S
    4. Kuruvilla DS
    5. Chang MR
    6. Kamenecka TM
    7. Rance M
    8. Johnson BA
    9. Burris TP
    10. Griffin PR
    11. Kojetin DJ

    (2012) Ligand and receptor dynamics contribute to the mechanism of graded PPARγ agonism

    Structure 20:139–150.

    https://doi.org/10.1016/j.str.2011.10.018

    • PubMed
    • Google Scholar
16. 1. Hughes TS
    2. Giri PK
    3. de Vera IMS
    4. Marciano DP
    5. Kuruvilla DS
    6. Shin Y
    7. Blayo AL
    8. Kamenecka TM
    9. Burris TP
    10. Griffin PR
    11. Kojetin DJ

    (2014) An alternate binding site for PPARγ ligands

    Nature Communications 5:3571.

    https://doi.org/10.1038/ncomms4571

    • PubMed
    • Google Scholar
17. 1. Hughes TS
    2. Shang J
    3. Brust R
    4. de Vera IMS
    5. Fuhrmann J
    6. Ruiz C
    7. Cameron MD
    8. Kamenecka TM
    9. Kojetin DJ

    (2016) Probing the complex binding modes of the PPARγ partial agonist 2-chloro-n-(3-chloro-4-((5-chlorobenzo[d]thiazol-2-yl)thio)phenyl)-4-(trifluoromethyl)benzenesulfonamide (t2384) to orthosteric and allosteric sites with nmr spectroscopy

    Journal of Medicinal Chemistry 59:10335–10341.

    https://doi.org/10.1021/acs.jmedchem.6b01340

    • PubMed
    • Google Scholar
18. 1. Irwin S
    2. Karr C
    3. Furman C
    4. Tsai J
    5. Gee P
    6. Banka D
    7. Wibowo AS
    8. Dementiev AA
    9. O’Shea M
    10. Yang J
    11. Lowe J
    12. Mitchell L
    13. Ruppel S
    14. Fekkes P
    15. Zhu P
    16. Korpal M
    17. Larsen NA

    (2022) Biochemical and structural basis for the pharmacological inhibition of nuclear hormone receptor PPARγ by inverse agonists

    The Journal of Biological Chemistry 298:102539.

    https://doi.org/10.1016/j.jbc.2022.102539

    • PubMed
    • Google Scholar
19. 1. Itoh T
    2. Fairall L
    3. Amin K
    4. Inaba Y
    5. Szanto A
    6. Balint BL
    7. Nagy L
    8. Yamamoto K
    9. Schwabe JWR

    (2008) Structural basis for the activation of PPARgamma by oxidized fatty acids

    Nature Structural & Molecular Biology 15:924–931.

    https://doi.org/10.1038/nsmb.1474

    • PubMed
    • Google Scholar
20. 1. Jang JY
    2. Koh M
    3. Bae H
    4. An DR
    5. Im HN
    6. Kim HS
    7. Yoon JY
    8. Yoon HJ
    9. Han BW
    10. Park SB
    11. Suh SW

    (2017) Structural basis for differential activities of enantiomeric PPARγ agonists: Binding of S35 to the alternate site

    Biochimica et Biophysica Acta (BBA) - Proteins and Proteomics 1865:674–681.

    https://doi.org/10.1016/j.bbapap.2017.03.008

    • Google Scholar
21. 1. Johnson BA
    2. Wilson EM
    3. Li Y
    4. Moller DE
    5. Smith RG
    6. Zhou G

    (2000) Ligand-induced stabilization of PPARgamma monitored by NMR spectroscopy: implications for nuclear receptor activation

    Journal of Molecular Biology 298:187–194.

    https://doi.org/10.1006/jmbi.2000.3636

    • PubMed
    • Google Scholar
22. 1. Johnson BA

    (2018) From raw data to protein backbone chemical shifts using NMRFx processing and NMRViewJ analysis

    Methods in Molecular Biology 1688:257–310.

    https://doi.org/10.1007/978-1-4939-7386-6_13

    • PubMed
    • Google Scholar
23. 1. Kliewer SA
    2. Lenhard JM
    3. Willson TM
    4. Patel I
    5. Morris DC
    6. Lehmann JM

    (1995) A prostaglandin J2 metabolite binds peroxisome proliferator-activated receptor gamma and promotes adipocyte differentiation

    Cell 83:813–819.

    https://doi.org/10.1016/0092-8674(95)90194-9

    • PubMed
    • Google Scholar
24. 1. Kliewer SA
    2. Sundseth SS
    3. Jones SA
    4. Brown PJ
    5. Wisely GB
    6. Koble CS
    7. Devchand P
    8. Wahli W
    9. Willson TM
    10. Lenhard JM
    11. Lehmann JM

    (1997) Fatty acids and eicosanoids regulate gene expression through direct interactions with peroxisome proliferator-activated receptors alpha and gamma

    PNAS 94:4318–4323.

    https://doi.org/10.1073/pnas.94.9.4318

    • PubMed
    • Google Scholar
25. 1. Laghezza A
    2. Piemontese L
    3. Cerchia C
    4. Montanari R
    5. Capelli D
    6. Giudici M
    7. Crestani M
    8. Tortorella P
    9. Peiretti F
    10. Pochetti G
    11. Lavecchia A
    12. Loiodice F

    (2018) Identification of the first PPARα/γ dual agonist able to bind to canonical and alternative sites of PPARγ and To Inhibit Its Cdk5-Mediated Phosphorylation

    Journal of Medicinal Chemistry 61:8282–8298.

    https://doi.org/10.1021/acs.jmedchem.8b00835

    • PubMed
    • Google Scholar
26. 1. Lee G
    2. Elwood F
    3. McNally J
    4. Weiszmann J
    5. Lindstrom M
    6. Amaral K
    7. Nakamura M
    8. Miao S
    9. Cao P
    10. Learned RM
    11. Chen JL
    12. Li Y

    (2002) T0070907, a selective ligand for peroxisome proliferator-activated receptor gamma, functions as an antagonist of biochemical and cellular activities

    The Journal of Biological Chemistry 277:19649–19657.

    https://doi.org/10.1074/jbc.M200743200

    • PubMed
    • Google Scholar
27. 1. Leesnitzer LM
    2. Parks DJ
    3. Bledsoe RK
    4. Cobb JE
    5. Collins JL
    6. Consler TG
    7. Davis RG
    8. Hull-Ryde EA
    9. Lenhard JM
    10. Patel L
    11. Plunket KD
    12. Shenk JL
    13. Stimmel JB
    14. Therapontos C
    15. Willson TM
    16. Blanchard SG

    (2002) Functional consequences of cysteine modification in the ligand binding sites of peroxisome proliferator activated receptors by GW9662

    Biochemistry 41:6640–6650.

    https://doi.org/10.1021/bi0159581

    • PubMed
    • Google Scholar
28. 1. Leijten-van de Gevel IA
    2. van Herk KHN
    3. de Vries R
    4. Ottenheym NJ
    5. Ottmann C
    6. Brunsveld L

    (2022) Indazole MRL-871 interacts with PPARγ via a binding mode that induces partial agonism

    Bioorganic & Medicinal Chemistry 68:116877.

    https://doi.org/10.1016/j.bmc.2022.116877

    • PubMed
    • Google Scholar
29. 1. Li Y
    2. Zhang J
    3. Schopfer FJ
    4. Martynowski D
    5. Garcia-Barrio MT
    6. Kovach A
    7. Suino-Powell K
    8. Baker PRS
    9. Freeman BA
    10. Chen YE
    11. Xu HE

    (2008) Molecular recognition of nitrated fatty acids by PPAR gamma

    Nature Structural & Molecular Biology 15:865–867.

    https://doi.org/10.1038/nsmb.1447

    • PubMed
    • Google Scholar
30. Preprint

    1. MacTavish B
    2. Zhu D
    3. Shang J
    4. Shao Q
    5. Yang ZJ
    6. Kamenecka TM
    7. Kojetin DJ

    (2024) Ligand efficacy shifts a nuclear receptor conformational ensemble between transcriptionally active and repressive states

    bioRxiv.

    https://doi.org/10.1101/2024.04.23.590805

    • Google Scholar
31. 1. Malapaka RRV
    2. Khoo S
    3. Zhang J
    4. Choi JH
    5. Zhou XE
    6. Xu Y
    7. Gong Y
    8. Li J
    9. Yong EL
    10. Chalmers MJ
    11. Chang L
    12. Resau JH
    13. Griffin PR
    14. Chen YE
    15. Xu HE

    (2012) Identification and mechanism of 10-carbon fatty acid as modulating ligand of peroxisome proliferator-activated receptors

    The Journal of Biological Chemistry 287:183–195.

    https://doi.org/10.1074/jbc.M111.294785

    • PubMed
    • Google Scholar
32. 1. Marciano DP
    2. Kuruvilla DS
    3. Boregowda SV
    4. Asteian A
    5. Hughes TS
    6. Garcia-Ordonez R
    7. Corzo CA
    8. Khan TM
    9. Novick SJ
    10. Park H
    11. Kojetin DJ
    12. Phinney DG
    13. Bruning JB
    14. Kamenecka TM
    15. Griffin PR

    (2015) Pharmacological repression of PPARγ promotes osteogenesis

    Nature Communications 6:7443.

    https://doi.org/10.1038/ncomms8443

    • PubMed
    • Google Scholar
33. 1. McCoy AJ
    2. Grosse-Kunstleve RW
    3. Adams PD
    4. Winn MD
    5. Storoni LC
    6. Read RJ

    (2007) Phaser crystallographic software

    Journal of Applied Crystallography 40:658–674.

    https://doi.org/10.1107/S0021889807021206

    • PubMed
    • Google Scholar
34. 1. Nolte RT
    2. Wisely GB
    3. Westin S
    4. Cobb JE
    5. Lambert MH
    6. Kurokawa R
    7. Rosenfeld MG
    8. Willson TM
    9. Glass CK
    10. Milburn MV

    (1998) Ligand binding and co-activator assembly of the peroxisome proliferator-activated receptor-gamma

    Nature 395:137–143.

    https://doi.org/10.1038/25931

    • PubMed
    • Google Scholar
35. 1. Norris M
    2. Fetler B
    3. Marchant J
    4. Johnson BA

    (2016) NMRFx Processor: a cross-platform NMR data processing program

    Journal of Biomolecular NMR 65:205–216.

    https://doi.org/10.1007/s10858-016-0049-6

    • PubMed
    • Google Scholar
36. 1. Orsi DL
    2. Pook E
    3. Bräuer N
    4. Friberg A
    5. Lienau P
    6. Lemke CT
    7. Stellfeld T
    8. Brüggemeier U
    9. Pütter V
    10. Meyer H
    11. Baco M
    12. Tang S
    13. Cherniack AD
    14. Westlake L
    15. Bender SA
    16. Kocak M
    17. Strathdee CA
    18. Meyerson M
    19. Eis K
    20. Goldstein JT

    (2023) Discovery and structure-based design of potent covalent PPARγ Inverse-Agonists BAY-4931 and BAY-0069

    Journal of Medicinal Chemistry 65:14843–14863.

    https://doi.org/10.1021/acs.jmedchem.2c01379

    • Google Scholar
37. 1. Ostberg T
    2. Svensson S
    3. Selén G
    4. Uppenberg J
    5. Thor M
    6. Sundbom M
    7. Sydow-Bäckman M
    8. Gustavsson AL
    9. Jendeberg L

    (2004) A new class of peroxisome proliferator-activated receptor agonists with A novel binding epitope shows antidiabetic effects

    The Journal of Biological Chemistry 279:41124–41130.

    https://doi.org/10.1074/jbc.M401552200

    • PubMed
    • Google Scholar
38. 1. Shang J
    2. Brust R
    3. Mosure SA
    4. Bass J
    5. Munoz-Tello P
    6. Lin H
    7. Hughes TS
    8. Tang M
    9. Ge Q
    10. Kamenekca TM
    11. Kojetin DJ

    (2018) Cooperative cobinding of synthetic and natural ligands to the nuclear receptor PPARγ

    eLife 7:e43320.

    https://doi.org/10.7554/eLife.43320

    • PubMed
    • Google Scholar
39. 1. Shang J
    2. Brust R
    3. Griffin PR
    4. Kamenecka TM
    5. Kojetin DJ

    (2019) Quantitative structural assessment of graded receptor agonism

    PNAS 116:22179–22188.

    https://doi.org/10.1073/pnas.1909016116

    • PubMed
    • Google Scholar
40. 1. Shang J
    2. Mosure SA
    3. Zheng J
    4. Brust R
    5. Bass J
    6. Nichols A
    7. Solt LA
    8. Griffin PR
    9. Kojetin DJ

    (2020) A molecular switch regulating transcriptional repression and activation of PPARγ

    Nature Communications 11:956.

    https://doi.org/10.1038/s41467-020-14750-x

    • PubMed
    • Google Scholar
41. 1. Shang J
    2. Kojetin DJ

    (2021) Structural mechanism underlying ligand binding and activation of PPARγ

    Structure 29:940–950.

    https://doi.org/10.1016/j.str.2021.02.006

    • PubMed
    • Google Scholar
42. 1. Waku T
    2. Shiraki T
    3. Oyama T
    4. Fujimoto Y
    5. Maebara K
    6. Kamiya N
    7. Jingami H
    8. Morikawa K

    (2009) Structural insight into PPARgamma activation through covalent modification with endogenous fatty acids

    Journal of Molecular Biology 385:188–199.

    https://doi.org/10.1016/j.jmb.2008.10.039

    • PubMed
    • Google Scholar
43. 1. Williamson MP

    (2013) Using chemical shift perturbation to characterise ligand binding

    Progress in Nuclear Magnetic Resonance Spectroscopy 73:1–16.

    https://doi.org/10.1016/j.pnmrs.2013.02.001

    • PubMed
    • Google Scholar
44. 1. Yu C
    2. Markan K
    3. Temple KA
    4. Deplewski D
    5. Brady MJ
    6. Cohen RN

    (2005) The nuclear receptor corepressors NCoR and SMRT decrease peroxisome proliferator-activated receptor gamma transcriptional activity and repress 3T3-L1 adipogenesis

    The Journal of Biological Chemistry 280:13600–13605.

    https://doi.org/10.1074/jbc.M409468200

    • PubMed
    • Google Scholar
45. 1. Zheng J
    2. Corzo C
    3. Chang MR
    4. Shang J
    5. Lam VQ
    6. Brust R
    7. Blayo AL
    8. Bruning JB
    9. Kamenecka TM
    10. Kojetin DJ
    11. Griffin PR

    (2018) Chemical crosslinking mass spectrometry reveals the conformational landscape of the activation Helix of PPARγ; a model for ligand-dependent antagonism

    Structure 26:1431–1439.

    https://doi.org/10.1016/j.str.2018.07.007

    • PubMed
    • Google Scholar

Author details

1. Jinsai Shang

   1. Department of Integrative Structural and Computational Biology, Scripps Research and The Herbert Wertheim UF Scripps Institute for Biomedical Innovation & Technology, Jupiter, United States
   2. School of Basic Medical Sciences, Guangzhou Laboratory, Guangzhou Medical University, Guangzhou, China

   Contribution

   Conceptualization, Formal analysis, Investigation, Visualization, Methodology, Writing – original draft, Writing – review and editing

   For correspondence

   shang_jinsai@gzlab.ac.cn

   Competing interests

   No competing interests declared

   "This ORCID iD identifies the author of this article:" 0000-0001-8164-1544

2. Douglas J Kojetin

   1. Department of Integrative Structural and Computational Biology, Scripps Research and The Herbert Wertheim UF Scripps Institute for Biomedical Innovation & Technology, Jupiter, United States
   2. Department of Biochemistry, Vanderbilt University, Nashville, United States
   3. Center for Structural Biology, Vanderbilt University, Nashville, United States
   4. Vanderbilt Institute of Chemical Biology, Vanderbilt University, Nashville, United States
   5. Center for Applied AI in Protein Dynamics, Vanderbilt University, Nashville, United States

   Contribution

   Conceptualization, Formal analysis, Supervision, Funding acquisition, Visualization, Methodology, Writing – original draft, Writing – review and editing

   For correspondence

   douglas.kojetin@vanderbilt.edu

   Competing interests

   No competing interests declared

   "This ORCID iD identifies the author of this article:" 0000-0001-8058-6168

• 395

  views

• 30

  downloads

• 0

  citations

Views, downloads and citations are aggregated across all versions of this paper published by eLife.