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accessStructural insight into an anti-BRIL Fab as a G-protein-coupled receptor crystallization chaperone
aR&D Division, Kyowa Kirin Co. Ltd, Tokyo, Japan, bR&D Division, Kyowa Kirin Co. Ltd, Shizuoka, Japan, cCMC R&D Center, Kyowa Kirin Co. Ltd, Shizuoka, Japan, dDepartment of Cell Biology, Graduate School of Medicine, Kyoto University, Kyoto, Japan, and eRIKEN, SPring-8 Center, Hyogo, Japan
*Correspondence e-mail: jun.saito.su@kyowakirin.com
of G-protein-coupled receptors (GPCRs) is key for the successful development of efficient drugs targeting GPCRs. BRIL is a thermostabilized apocytochrome b562 (with M7W/H102I/R106L mutations) from Escherichia coli and is often used as a GPCR fusion protein for expression and crystallization. SRP2070Fab, an anti-BRIL antibody Fab fragment, has been reported to facilitate and enhance the crystallization of BRIL-fused GPCRs as a crystallization chaperone. This study was conducted to characterize the high-resolution of the BRIL–SRP2070Fab complex. The structure of the BRIL–SRP2070Fab complex was determined at 2.1 Å resolution. This high-resolution structure elucidates the binding interaction between BRIL and SRP2070Fab. When binding to BRIL, SRP2070Fab recognizes conformational epitopes, not linear epitopes, on the surface of BRIL helices III and IV, thereby binding perpendicularly to the helices, which indicates stable binding. Additionally, the packing contacts of the BRIL–SRP2070Fab are largely due to SRP2070Fab rather than BRIL. The accumulation of SRP2070Fab molecules by stacking is remarkable and is consistent with the finding that stacking of SRP2070Fab is predominant in known crystal structures of BRIL-fused GPCRs complexed with SRP2070Fab. These findings clarified the mechanism of SRP2070Fab as a crystallization chaperone. Moreover, these data will be useful in the structure-based drug design of membrane-protein drug targets.
Keywords: crystal structure; crystal packing; apocytochrome b562; GPCRs; crystallization chaperones; anti-BRIL Fabs.
PDB reference: BRIL–SRP2070Fab complex, 7xrz
1. Introduction
G-protein-coupled receptors (GPCRs) are the largest family of membrane proteins and regulate many physiological functions associated with the nervous and cardiovascular systems, metabolism and inflammation, among others (Venkatakrishnan et al., 2013![[Venkatakrishnan, A. J., Deupi, X., Lebon, G., Tate, C. G., Schertler, G. F. X. & Babu, M. M. (2013). Nature, 494, 185-194.]](../../../../../../logos/arrows/d_arr.gif "Venkatakrishnan, A. J., Deupi, X., Lebon, G., Tate, C. G., Schertler, G. F. X. & Babu, M. M. (2013). Nature, 494, 185-194."){kind=small}
). Therefore, GPCRs have been an important target in drug development. Since the 1990s, structure elucidation of the drug candidate–target protein complex has widely been used to optimize hit compounds to lead compounds by rational design based on the obtained structural information, an approach called structure-based drug design (SBDD; Lee et al., 2018; Shoichet & Kobilka, 2012). Although is key for the success of SBDD, technical difficulties continue to persist, especially for membrane-protein targets involved in protein production, purification or crystallization. SBDD has extensively been applied to GPCRs since 2007, when the first of a human GPCR was determined (Cherezov et al., 2007; Rasmussen et al., 2007). X-ray crystallography was almost the only available method for the of GPCRs until the development of single-particle cryo-electron microscopy (cryo-EM) analysis in 2017; recently, an increasing number of structures have been determined by cryo-EM analysis (García-Nafría & Tate, 2021).
Several inactive-state GPCR structures bound to antagonists or inverse agonists have been determined by X-ray crystallography, whereas most active-state GPCR structures coupled to heterotrimeric G proteins have been determined by cryo-EM analysis (Congreve et al., 2020). This tendency is attributed to the range of tractable particle sizes using current cryo-EM technology (García-Nafría & Tate, 2021). Therefore, while the number of GPCR structures determined by cryo-EM analysis is expected to continue to increase, X-ray crystallography will remain the method of choice for elucidating GPCR structures below 50 kDa. Another advantage of X-ray crystallography for SBDD is the high throughput of complex with numerous ligands. SBDD is generally performed in the optimization stage of candidate compounds, with several compounds being screened in the analysis. A series of candidate compound structures bound to a target GPCR can quickly be determined by utilizing the soaking method, in which the compounds are soaked into apoprotein crystals of the GPCR; hence, X-ray crystallography can be used to accelerate SBDD for GPCRs (Rucktooa et al., 2018). Thus, X-ray crystallography and cryo-EM serve as complementary methods in assessing the structure–function relationships of GPCRs and for use in SBDD.
BRIL, an engineered four-helix bundle protein, is a thermostabilized apocytochrome b562 protein from Escherichia coli that is derived from cytochrome b562 and stabilized as an apoprotein without the cofactor heme by introducing M7W/H102I/R106L mutations (Chu et al., 2002). BRIL has been widely used as a GPCR fusion protein since 2012. Structural flexibility can be reduced and thermostability can be improved by replacing the flexible loop of GPCRs with BRIL, which is often necessary for expression and crystallization (Chun et al., 2012; Xiang et al., 2016). Several optimizations are required to obtain GPCR constructs suitable for crystallization: (i) the deletion of N-terminal and/or C-terminal domains (Hollenstein et al., 2013; Jaakola et al., 2008; Huang et al., 2013; Warne et al., 2011), (ii) the implementation of point mutations to improve thermal stability (Vaidehi et al., 2016) and (iii) the insertion of a fusion protein into the third intracellular loop or into the N-terminus (Xiang et al., 2016). BRIL is often chosen as a fusion partner, and approximately 20% of reported GPCR structures have been determined as BRIL fusion mutants (Xiang et al., 2016).
We recently reported an anti-BRIL antibody fragment (SRP2070Fab) that facilitates and enhances the crystallization of BRIL-fused GPCRs and demonstrated that SRP2070Fab can be a versatile crystallization chaperone for BRIL-fused GPCRs (Miyagi et al., 2020). The structures of two BRIL-fused GPCRs, namely 5HT1B bound to ergotamine and AT2R bound to an angiotensin II analog, were determined by complexing the GPCRs with SRP2070Fab. Our study also showed that no undesired structural change occurred on the binding of SRP2070Fab and that this approach can be applied for structural analyses of GPCRs regardless of whether the receptors adopt active or inactive conformations. However, the structures of AT2R or 5HT1B complexed with SRP2070Fab had low resolution, which was a limitation for characterizing detailed structural features such as the precise interactions within epitopes and paratopes or crystal-packing contacts.
More recently, a series of semi-synthetic anti-BRIL antibodies (sABs) have been reported as tools for the of BRIL-fused membrane proteins, and the structure of BAG2, an affinity-matured sAB, bound to BRIL was determined at 1.9 Å resolution (Mukherjee et al., 2020). These studies raise expectations that anti-BRIL antibodies may be promising tools for the structural study of membrane proteins.
In this study, we characterized the high-resolution of the BRIL–SRP2070Fab complex, which provides a clearer understanding of the BRIL recognition sites and the crystal-packing interactions. This information clarified the differences between SRP2070Fab and other anti-BRIL antibodies and revealed the advantages of SRP2070Fab as a crystallization chaperone.
2. Materials and methods
2.1. Expression and purification of BRIL
The amino-acid sequence of BRIL used in the present study was the same as that reported previously (Chu et al., 2002). The gene encoding a Tobacco etch virus (TEV) protease cleavage site and BRIL (Ala1–Leu106) was synthesized and subcloned into pET-28a(+) using BamHI and HindIII. 6×His-tagged BRIL was expressed in the E. coli BL21 (DE3) strain cultured in Luria–Bertani medium. The cultured cells were harvested and lysed after induction with isopropyl β-D-1-thiogalactopyranoside. 6×His-tagged BRIL was first purified by nickel-affinity The protein bound to the Ni–NTA agarose resin was eluted with 100 mM Tris–HCl pH 7.6, 300 mM NaCl, 300 mM imidazole, 5 mM 3-mercapto-1,2-propanediol. The 6×His tag was cleaved with TEV protease and removed by collecting the flowthrough fraction from the Ni–NTA agarose resin. Further purification was performed by anion-exchange using a Mono 5/50 GL column (Cytiva) and the peak fractions containing BRIL were collected.
2.2. Preparation of SRP2070Fab
SRP2070Fab was prepared according to the method reported previously (Miyagi et al., 2020). Briefly, hybridomas producing SRP2070 were intraperitoneally administered to MRL/lpr mice. Ascites was collected from the hybridoma-administered mice and SRP2070 was purified by ammonium sulfate precipitation and protein G After cleaving SRP2070 with papain, the Fc fragment was removed by collecting the flowthrough fraction from the protein A column. SRP2070Fab was further purified by (SEC) on a Superdex 200 10/300 GL column equilibrated with phosphate-buffered saline.
2.3. Purification of BRIL–SRP2070Fab
BRIL and SRP2070Fab were mixed in a 1:1.2 molar ratio for 1 h on ice before further purification of the complex by SEC using a Superdex 200 Increase 10/300 GL column equilibrated with SEC buffer consisting of 20 mM Tris–HCl pH 7.6, 2 mM 3-mercapto-1,2-propanediol. Concentrated BRIL–SRP2070Fab (∼20 mg ml−1) was used in crystallization experiments.
2.4. Crystallization and of BRIL–SRP2070Fab
Initial crystallization trials were performed by the sitting-drop vapor-diffusion method using a Mosquito crystallization robot (SPT Labtech). All drops were formed by mixing 100 nl protein solution with an equal volume of reservoir solution in 96-well plates, and the drops were equilibrated against 50 µl reservoir solution. Initial crystallization screening using JCSG+ (Molecular Dimensions), ProPlex (Molecular Dimensions) and The PEGs II Suite (Qiagen) revealed several promising hit conditions. Crystals of the BRIL–SRP2070Fab complex were finally obtained using a condition composed of 18%(w/v) polyethylene glycol (PEG) 6000, 100 mM Tris–HCl pH 8.5 at 4°C (Supplementary Fig. S1 and Table S1), which was optimized from a hit from the ProPlex screen. The crystals were cryoprotected by soaking them in a solution containing 20%(v/v) glycerol before flash-cooling in liquid nitrogen.
Diffraction data for the BRIL–SRP2070Fab were collected on the X10SA beamline at the Swiss Light Source (SLS) and were processed using XDS (Kabsch, 2010) and AIMLESS (Evans & Murshudov, 2013). The initial phase was determined by using MOLREP (Vagin & Teplyakov, 2010) and Phaser (McCoy et al., 2007). The structures of BRIL (PDB entry 1m6t; Chu et al., 2002) and of Fab derived from mouse IgG1 (PDB entry 1f58; Stanfield et al., 1999) were used as search models. The initial structural model was refined by rigid-body and with REFMAC5 (Murshudov et al., 2011). The model of the structure was repeatedly corrected using Coot to be consistent in electron density (Emsley et al., 2010). The interfaces between BRIL and SRP2070Fab and within the crystal packing were analyzed with PISA (Krissinel & Henrick, 2007) and Molecular Operating Environment (MOE, version 2020.0901; Chemical Computing Group ULC). The buried surface area (BSA) on complex formation was calculated by PISA according to the equation BSAAB = (ASAA + ASAB − ASAAB)/2, where BSAXY is the buried surface area when molecules X and Y form a complex and ASAX is the total accessible surface area of molecule X. Structural figures were prepared using the CCP4mg molecular-graphics software (Potterton et al., 2002) and PyMOL version 0.99 (DeLano, 2002).
3. Results and discussion
A complete data set at 2.1 Å resolution was obtained from the BRIL–SRP2070Fab which belonged to C2 with unit-cell parameters a = 93.83, b = 75.24, c = 152.23 Å, β = 99.67° and contained two BRIL–SRP2070Fab complexes in the The crystallographic statistics of data collection and are summarized in Table 1.
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The overall structure of the showed that SRP2070Fab binds to BRIL by recognizing conformational epitopes, not linear epitopes, of the natively structured BRIL. All six complementarity-determining regions (CDRs) in the heavy (H) and light (L) chains cooperatively enable the recognition of BRIL, and CDR1 and CDR3 of the H chain that pinch helix IV of BRIL from both sides are remarkable compared with the others (Fig. 1a, right). Conformational epitopes, i.e. residues within 4 Å of SRP2070Fab, are extensively spread over helices III and IV of BRIL (Figs. 1b–1f). The BSA on antigen–antibody complex formation is 923.2 Å2 on average for the two BRIL–SRP2070Fab complexes in the (Supplementary Table S2a), which is larger than the average for known antigen–antibody interfaces of 534 ± 157 Å (Reis et al., 2022). Hydrophilic interactions such as hydrogen bonds and salt bridges play major roles in BRIL recognition: seven hydrogen bonds and one salt bridge are formed between the H chain and BRIL. One hydrogen bond and one salt bridge are found in CDR1, and three hydrogen bonds are found in both CDR2 and CDR3. Six hydrogen bonds are also formed between the L chain and BRIL. One hydrogen bond is formed in CDR1 and CDR2, and four hydrogen bonds are formed in CDR3. The detailed interactions are described in Supplementary Table S3. Although hydrophobic interactions contribute less to BRIL recognition, it is noteworthy that a sequence of aromatic residues, Trp94L_CDR3, Tyr33H_CDR1, Trp50H_CDR2 and Phe52H_CDR2, provide aromatic interactions with BRIL helices III and IV (Fig. 1g). Considering the number and the distance of the interactions, Asp74 and Glu92 are considered to be at the center of the (Fig. 1, Supplementary Table S3). The high-resolution structure revealed that both the epitopes and the paratopes are conformationally and spatially extended, and thus SRP2070Fab recognizes BRIL on the surface but not at a particular spot or at a linear amino-acid sequence. It is noteworthy that all six CDRs cooperatively bind to BRIL, which indicates the stability of the BRIL–SRP2070Fab complex; therefore, this aspect of SRP2070Fab may be advantageous for it to serve as a crystallization chaperone (Fig. 1, Supplementary Table S3).
![[Figure 1]](nj5317fig1thm.gif) | Figure 1 Structure of the BRIL–SRP2070Fab complex and the interaction between BRIL and SRP2070Fab. (a) Overall structure of the BRIL–SRP2070Fab complex. The protein structures are represented as ribbon models. BRIL is indicated in ocher, heavy (H) chain is indicated in purple and light (L) chain is indicated in light blue. (b)–(f) Interactions between BRIL and complementarity-determining regions (CDRs) are shown. The interacting side chains are shown as sticks, and hydrogen bonds and salt bridges are shown as dashed lines. (e) Asn57H_CDR2 adopts a double conformer. (g) Hydrophobic interactions between BRIL and SRP2070Fab are shown. |
To understand the properties of SRP2070Fab with regard to the crystallization of BRIL-fused membrane proteins, we explored the crystal packing of the high-resolution structure of the BRIL–SRP2070Fab complex. SRP2070Fab molecules were found to be tightly packed in the crystal, making contacts and interacting with each other. The crystal packing of the BRIL–SRP2070Fab co-complex is largely due to SRP2070Fab rather than to BRIL; that is, SRP2070Fab contributes almost 80% of the BSA due to crystal packing (Supplementary Table S2b). The results of the crystal-packing analysis showed that several BRIL–SRP2070Fab complexes stack against each other along the c axis in a face-to-face or back-to-back manner, while the complex molecules are ordered by side-by-side contacts within the ab plane (Fig. 2a). Here, the side exposing the N- and C-termini of BRIL is defined as the `face' of SRP2070Fab; that is, the face of SRP2070Fab is exposed to the receptor during fusion with BRIL (Supplementary Fig. S2). Stacking along the c axis is important because it enables perpendicular interactions with the layer of lipid or detergent mimicking the cellular membrane, which is necessary for the three-dimensional growth of membrane-protein crystals (Fig. 2b). Face-to-face stacking is predominant among all of the crystal contacts contributed by SRP2070Fab. Two BRIL–SRP2070Fab complexes facing each other are the components of an thus, they are not crystallographically equivalent and are hereafter referred to as complexes A and B (Fig. 2b). Two remarkable salt bridges, namely Glu89H_complexA–Arg188L_complexB and Glu89H_complexB–Arg155L_complexA, are found in the face-to-face stacking (Fig. 3a). Although Glu89H is involved in both salt bridges, the basic counter-residues are not conserved; this is because complexes A and B are nearly, but not perfectly, in twofold symmetry. Both of the other back-to-back stacking contacts along the c axis have the crystallographic twofold symmetries between complexes A and A or between complexes B and B. The BSA for B–B stacking is more than twice larger than that from A–A stacking; therefore, B–B stacking is more dominant in crystal packing than A–A stacking (Fig. 2b). B–B stacking is stabilized by symmetric salt bridges between Arg45L_complexB and Glu81L_complexB, while only weaker hydrogen bonds were observed between Ser60L_complexA and Glu79L_complexA at the A–A stacking boundary (Figs. 3b and 3c). The stacking interactions are summarized in Supplementary Table S2(c).
![[Figure 2]](nj5317fig2thm.gif) | Figure 2 Molecular packing of the BRIL–SRP2070Fab co-crystal. (a) Molecular packing of the BRIL–SRP2070Fab crystal along the ac plane and the ab plane. An is denoted as a rectangle drawn in black lines. Two BRIL–SRP2070Fab complexes (complexes A and B) in the are shown as a surface, while molecules outside the are shown as ribbon models. BRIL, SRP2070Fab heavy chain and SRP2070Fab light chain are shown in green, dark red and orange for complex A and in light green, pink and khaki for complex B, respectively. (b) Close-up image of the stacking along the c axis of the BRIL–SRP2070Fab crystal. Residues making contacts with neighboring complexes are depicted as spheres. Residues from neighbors outside of the are shown in gray for better distinction. The N- and C-termini of BRIL are marked by red spheres. |
![[Figure 3]](nj5317fig3thm.gif) | Figure 3 Crystal-packing interactions in the BRIL–SRP2070Fab co-crystal. Interactions observed within (a) face-to-face stacking between complexes A and B, (b) back-to-back stacking between complex A and its symmetry mate A′ and (c) back-to-back stacking between complex B and its symmetry mate B′. SRP2070Fab molecules are represented by ribbon models. The heavy and light chains of SRP2070Fab are shown in dark red and orange for complex A and in pink and khaki for complex B, respectively. Residues involved in the interactions are depicted as stick models. Salt-bridge or hydrogen-bond interactions are indicated as cyan dashed lines. |
In our previous study, crystal structures of two BRIL-fused GPCRs, 5HT1B-BRIL and AT2R-BRIL, were determined in complex with SRP2070Fab (Miyagi et al., 2020). As SRP2070Fab provides the dominant crystal packing in both crystal structures, we concluded that SRP2070Fab is a promising crystallization chaperone for BRIL-fused GPCRs. Although the packing interactions in this study are not exactly reproduced in the structures of SRP2070Fab complexed with BRIL-fused GPCRs, the conceptual principle of crystallization assistance by SRP2070Fab is commonly based on face-to-face, back-to-back or face-to-back stacking of SRP2070Fab (Supplementary Figs. S3a and S3b).
BAG2, another anti-BRIL Fab fragment, is also useful for characterizing the structural biology of membrane proteins (Mukherjee et al., 2020). Structural comparisons between SRP2070Fab and BAG2 (PDB entry 6cbv) complexed with BRIL clearly show a difference in the extent of BRIL recognition by the Fab fragments. Although both Fab fragments recognize conformational epitopes that are three-dimensionally spread on the BRIL surface and bind nearly at right angles to the BRIL helices, they bind to BRIL from quite different directions: SRP2070Fab recognizes helices III and IV of BRIL in the manner described above, while BAG2 recognizes helices II and III from the opposite side of BRIL (Fig. 4). Another remarkable difference is that the face of SRP2070Fab is perpendicular to BRIL, while that of BAG2 is coplanar with the BRIL helices, which would impact the crystal growth of BRIL-fused membrane proteins, assuming that the stacking of SRP2070Fab facilitates crystal growth in a direction perpendicular to the hydrophobic membrane layer. In fact, the packing of the BRIL–BAG2 is more complex than that of the SRP2070Fab–BRIL and no significant stacking can be found in the Fab portion of the BRIL–BAG2 structure (Supplementary Fig. S4).
![[Figure 4]](nj5317fig4thm.gif){kind=small} | Figure 4 Comparison of two anti-BRIL antibodies (SRP2070Fab and BAG2). The structures of BRIL–SRP2070Fab and BRIL–BAG2 (PDB entry 6cbv) are superimposed. The structures are shown in two directions. BRIL–SRP2070Fab is indicated in ocher and BRIL–BAG2 is indicated in green. |
We then determined the BRIL–SRP2070Fab structure at a high resolution that was sufficient to elucidate the detailed structural features of BRIL recognition and the crystal-packing interactions.
Smaller antibody fragments could be another candidate as crystallization chaperones owing to the highly compact crystal packing. ScFv (single-chain Fv) or Fv-clasp, which are new technologies for generating stable Fv fragments (Arimori et al., 2017), may be applicable to SRP2070.
Additionally, the high-resolution structure of the BRIL–SRP2070Fab complex can be used as a fine search model for complex structures of BRIL-fused membrane proteins and SRP2070Fab. This could be a crystallographic benefit to improve the phase given by in cases where the initial phase determined solely from the membrane-protein portion is not adequate. The high-resolution BRIL–SRP2070Fab structure is also expected to be a good starting point for structure building in cryo-EM structure determination.
We believe that our findings will provide an impetus for the of BRIL-fused membrane proteins complexed with SRP2070Fab and facilitate the SBDD of membrane-protein drug targets.
4. Conclusions
In this study, we determined the high-resolution structure of the BRIL–SRP2070Fab complex. This structure enabled us to elucidate the interactions between BRIL and SRP2070Fab. All six CDRs in the heavy and light chains cooperatively enable the recognition of BRIL. This result suggests a strong binding affinity between BRIL and SRP2070Fab. Additionally, detailed information on the crystal packing was clarified by this structure. This result confirms that SRP2070Fab promotes crystallization packing, as suggested in a previous report (Miyagi et al., 2020), indicating that SRP2070Fab is useful as a crystallization chaperone for BRIL fusion proteins.
Supporting information
PDB reference: BRIL–SRP2070Fab complex, 7xrz
Supplementary Tables and Figures. DOI: https://doi.org/10.1107/S205979832300311X/nj5317sup1.pdf
Acknowledgements
We thank the staff of the Swiss Light Source for conducting X-ray data collection. We thank Cactus Life Sciences, which is part of Cactus Communications, for editing and proofreading support for this manuscript. Hikaru Miyagi, Michihiko Suzuki, Mai Yasunaga and Jun-ichi Saito are employees of Kyowa Kirin Co. Ltd.
Funding information
This research has been funded by the Japanese pharmaceutical company Kyowa Kirin Co. Ltd.
References
Arimori, T., Kitago, Y., Umitsu, M., Fujii, Y., Asaki, R., Tamura-Kawakami, K. & Takagi, J. (2017). Structure, 25, 1611–1622. CrossRef CAS PubMed Google Scholar
Cherezov, V., Rosenbaum, D. M., Hanson, M. A., Rasmussen, S. G. F., Thian, F. S., Kobilka, T. S., Choi, H., Kuhn, P., Weis, W. I., Kobilka, B. K. & Stevens, R. C. (2007). Science, 318, 1258–1265. CrossRef PubMed CAS Google Scholar
Chu, R., Takei, J., Knowlton, J. R., Andrykovitch, M., Pei, W., Kajava, A. V., Steinbach, P. J., Ji, X. & Bai, Y. (2002). J. Mol. Biol. 323, 253–262. Web of Science CrossRef PubMed CAS Google Scholar
Chun, E., Thompson, A. A., Liu, W., Roth, C. B., Griffith, M. T., Katritch, V., Kunken, J., Xu, F., Cherezov, V., Hanson, M. A. & Stevens, R. C. (2012). Structure, 20, 967–976. Web of Science CrossRef CAS PubMed Google Scholar
Congreve, M., de Graaf, C., Swain, N. A. & Tate, C. G. (2020). Cell, 181, 81–91. CrossRef CAS PubMed Google Scholar
DeLano, W. L. (2002). PyMOL. https://www.pymol.org. Google Scholar
Emsley, P., Lohkamp, B., Scott, W. G. & Cowtan, K. (2010). Acta Cryst. D66, 486–501. Web of Science CrossRef CAS IUCr Journals Google Scholar
Evans, P. R. & Murshudov, G. N. (2013). Acta Cryst. D69, 1204–1214. Web of Science CrossRef CAS IUCr Journals Google Scholar
García-Nafría, J. & Tate, C. G. (2021). Biochem. Soc. Trans. 49, 2345–2355. PubMed Google Scholar
Hollenstein, K., Kean, J., Bortolato, A., Cheng, R. K. Y., Doré, A. S., Jazayeri, A., Cooke, R. M., Weir, M. & Marshall, F. H. (2013). Nature, 499, 438–443. CrossRef CAS PubMed Google Scholar
Huang, J., Chen, S., Zhang, J. J. & Huang, X. Y. (2013). Nat. Struct. Mol. Biol. 20, 419–425. CrossRef CAS PubMed Google Scholar
Jaakola, V. P., Griffith, M. T., Hanson, M. A., Cherezov, V., Chien, E. Y. T., Lane, J. R., IJzerman, A. P. & Stevens, R. C. (2008). Science, 322, 1211–1217. CrossRef PubMed CAS Google Scholar
Kabsch, W. (2010). Acta Cryst. D66, 125–132. Web of Science CrossRef CAS IUCr Journals Google Scholar
Krissinel, E. & Henrick, K. J. (2007). J. Mol. Biol. 372, 774–797. Web of Science CrossRef PubMed CAS Google Scholar
Lee, Y., Basith, S. & Choi, S. (2018). J. Med. Chem. 61, 1–46. CrossRef CAS PubMed Google Scholar
McCoy, A. J., Grosse-Kunstleve, R. W., Adams, P. D., Winn, M. D., Storoni, L. C. & Read, R. J. (2007). J. Appl. Cryst. 40, 658–674. Web of Science CrossRef CAS IUCr Journals Google Scholar
Miyagi, H., Asada, H., Suzuki, M., Takahashi, Y., Yasunaga, M., Suno, C., Iwata, S. & Saito, J. (2020). Sci. Rep. 10, 11669. CrossRef PubMed Google Scholar
Mukherjee, S., Erramilli, S. K., Ammirati, M., Alvarez, F. J. D., Fennell, K. F., Purdy, M. D., Skrobek, B. M., Radziwon, K., Coukos, J., Kang, Y., Dutka, P., Gao, X., Qiu, X., Yeager, M., Xu, H. E., Han, S. & Kossiakoff, A. A. (2020). Nat. Commun. 11, 1598. Web of Science CrossRef PubMed Google Scholar
Murshudov, G. N., Skubák, P., Lebedev, A. A., Pannu, N. S., Steiner, R. A., Nicholls, R. A., Winn, M. D., Long, F. & Vagin, A. A. (2011). Acta Cryst. D67, 355–367. Web of Science CrossRef CAS IUCr Journals Google Scholar
Potterton, E., McNicholas, S., Krissinel, E., Cowtan, K. & Noble, M. (2002). Acta Cryst. D58, 1955–1957. Web of Science CrossRef CAS IUCr Journals Google Scholar
Rasmussen, S. G. F., Choi, H., Rosenbaum, D. M., Kobilka, T. S., Thian, F. S., Edwards, P. C., Burghammer, M., Ratnala, V. R. P., Sanishvili, R., Fischetti, R. F., Schertler, G. F. X., Weis, W. I. & Kobilka, B. K. (2007). Nature, 450, 383–387. CrossRef PubMed CAS Google Scholar
Reis, P. B. P. S., Barletta, G. P., Gagliardi, L., Fortuna, S., Soler, M. A. & Rocchia, W. (2022). Front. Mol. Biosci. 9, 945808. CrossRef PubMed Google Scholar
Rucktooa, P., Cheng, R. K. Y., Segala, E., Geng, T., Errey, J. C., Brown, G. A., Cooke, R. M., Marshall, F. H. & Doré, A. S. (2018). Sci. Rep. 8, 41. Web of Science CrossRef PubMed Google Scholar
Shoichet, B. K. & Kobilka, B. K. (2012). Trends Pharmacol. Sci. 33, 268–272. CrossRef CAS PubMed Google Scholar
Stanfield, R. L., Cabezas, E., Satterthwait, A. C., Stura, E. A., Profy, A. T. & Wilson, I. A. (1999). Structure, 7, 131–142. CrossRef PubMed CAS Google Scholar
Vagin, A. & Teplyakov, A. (2010). Acta Cryst. D66, 22–25. Web of Science CrossRef CAS IUCr Journals Google Scholar
Vaidehi, N., Grisshammer, R. & Tate, C. G. (2016). Trends Pharmacol. Sci. 37, 37–46. CrossRef CAS PubMed Google Scholar
Venkatakrishnan, A. J., Deupi, X., Lebon, G., Tate, C. G., Schertler, G. F. X. & Babu, M. M. (2013). Nature, 494, 185–194. CrossRef CAS PubMed Google Scholar
Warne, T., Moukhametzianov, R., Baker, J. G., Nehmé, R., Edwards, P. C., Leslie, A. G. W., Schertler, G. F. X. & Tate, C. G. (2011). Nature, 469, 241–244. CrossRef CAS PubMed Google Scholar
Xiang, J., Chun, E., Liu, C., Jing, L., Al-Sahouri, Z., Zhu, L. & Liu, W. (2016). Trends Pharmacol. Sci. 37, 1055–1069. Web of Science CrossRef CAS PubMed Google Scholar
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| STRUCTURAL BIOLOGY |
