I04-1-Macromolecular Crystallography (fixed wavelength)
I23-Long wavelength MX
I24-Microfocus Macromolecular Crystallography
VMXm-Versatile Macromolecular Crystallography microfocus
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Abstract: The prevalence of multi-drug resistant strains of bacteria on a global scale demands the development and implementation of novel antibacterial therapeutics. DNA gyrase is a type IIA topoisomerase enzyme involved in the regulation and maintenance of DNA topology in bacteria. Targeting DNA gyrase as inhibitors, the fluoroquinolones have become one of the most prescribed antibiotic classes globally. However, due to the emergence of fluoroquinolone resistant bacterial strains, numerous resistance mechanisms to these antibiotics have been observed. Two novel, first-in-class antibiotics have recently achieved U.S Food and Drug Administration (FDA) approval; zoliflodacin, a spiropyrimidinetrione (SPT), and gepotidacin, a Novel Bacterial Topoisomerase Inhibitor (NBTI). These approvals mark a significant shift in antibacterial drug development, as they are the first new classes of antibiotics targeting DNA gyrase approved in decades. Protein X-ray crystallography played a vital role in the lead-compound development of gepotidacin, with six crystal structures published in the Protein Data Bank (PDB). Protocols detailing DNA gyrase crystallisation in complex with DNA and antibiotics favour the microbatch under-oil method, and no structure-based fragment screening programs had been done on the S. aureus GyrB27:A56 fusion truncateCORE construct for the discovery of novel compounds. Furthermore, DNA gyrase crystals are often twinned resulting in complications in structure solution and molecular refinement. In this thesis, a 2.78 Å resolution crystal structure (PDB ID 8BP2) showed two molecules of zoliflodacin binding to an S. aureus DNA gyrase - DNA cleavage complex. Structural analysis showed zoliflodacin binds more directly with conserved GyrB residues, rather than through the water-metal ion bridge to highly mutated GyrA residues, observed in fluoroquinolone structures. Furthermore, a 2.58 Å resolution crystal structure was determined (PDB ID 9FZ6), whereby anomalous difference Fourier maps enabled the modelling of three novel manganese binding sites. Investigations into crystal twinning using the nanofocus beamline VMXm at Diamond Light Source (DLS) demonstrated that multiple complete datasets can be solved from a single, large macromolecular crystal. Extensive crystallisation optimisation saw the development of a new crystallisation protocol for the S. aureus DNA gyrase - DNA complex, through sitting drop vapour diffusion, enhancing the reliability of growing highly diffracting crystals. By achieving a robust, high-throughput crystallisation protocol, the first structure-based fragment screening campaign at XChem (DLS) on the S. aureus GyrB27:A56 fusion truncateCORE construct was completed, soaking over 500 crystals with small drug-like fragments for structure determination. Following extensive refinement and model building, four fragment hits were observed in notable binding pockets; three within the thiophene pocket and one in the GyrA dimer interface pocket.
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May 2026
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I23-Long wavelength MX
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Diamond Proposal Number(s):
[23570, 27314]
Abstract: WNK kinases are chloride- and osmotic-stress-regulated protein kinases recently shown to be controlled by potassium. Prior studies demonstrated the direct binding of chloride and osmotic stress-related water in WNK kinase regulation. Here, we probe potassium binding and regulation of WNK kinases via crystallography coupled with mutagenic analysis of WNK kinase autophosphorylation and activity. Crystals of unphosphorylated WNK1 grown in cesium formate, a surrogate for potassium, yielded nonsulfur scattering peaks at 5.75 keV. Mutations were introduced into amino acids flanking the anomalous diffraction peaks. Mutations in WNK1/E388 and the corresponding WNK3/E314, probing a peak close to WNK1/I384, led to reduced inhibition by potassium while maintaining kinase autophosphorylation and substrate phosphorylation activity. Other peaks probed by mutagenesis either did not bear out as potassium regulatory sites or were not validated due to the inactivity of the mutants synthesized. Previously synthesized chloride- and water-binding mutants demonstrate correlated sensitivity to chloride and potassium. Potassium, chloride, and water are all WNK inhibitors that share a common mechanism binding the same low-activity asymmetric dimer of WNK1 kinase domains.
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May 2026
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I03-Macromolecular Crystallography
I23-Long wavelength MX
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Céline
Zheng-Gérard
,
Jana
Joha
,
Maria
Carrasquero
,
Kamel
El Omari
,
Edward
Lowe
,
Shirish
Dubey
,
Simon J.
Draper
,
Yu-Chi
Chang
,
Hsi-Hsien
Lin
,
Alan D.
Salama
,
Kirsty
Mchugh
,
Elena
Seiradake
Diamond Proposal Number(s):
[18069]
Open Access
Abstract: Granulomatosis with polyangiitis is a life-threatening systemic vasculitis, characterised by anti-neutrophil cytoplasmic autoantibodies (ANCA) most commonly against proteinase 3 (PR3), a protease expressed intracellularly and on the surface of neutrophils. Most cell surface PR3 is bound to the receptor CD177; however, the molecular mechanism of the interactions is not well understood. Here, we present crystal structures of CD177 in complex with PR3 and unliganded CD177. We describe a mainly hydrophobic binding interface between PR3 and CD177, involving the first two Ly6/uPAR (LU) domains of CD177. These form a globular structure which is connected to downstream domains via a flexible linker. Using a panel of PR3-ANCA-positive patient samples, we show that a significant proportion of ANCAs target the CD177-binding site of PR3 in these samples. Structure-guided mutation of the CD177-binding site on PR3 is effective in reducing PR3-ANCA binding. The results demonstrate that the CD177-binding surface of PR3 harbours a major PR3-ANCA epitope, and that the extent of binding to this surface varies between different patients.
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Feb 2026
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I04-Macromolecular Crystallography
I23-Long wavelength MX
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Diamond Proposal Number(s):
[36838]
Open Access
Abstract: Despite the theoretical advantages of phosphorus single-wavelength anomalous diffraction (P-SAD) for nucleic acid phasing, its application remains limited due to high atomic displacement parameters and an unfavourable ratio of unique reflections to anomalous scatterers. In this study, we report the crystal structure of an RNA complex composed of four strands, which was solved by experimental phasing after AlphaFold3 failed to produce reliable models. Bromine single-wavelength anomalous diffraction (Br-SAD) data were collected at 0.916 Å on beamline I04 at Diamond Light Source, while phosphorus anomalous data were obtained at 3.024 Å on beamline I23. The structure was successfully phased using bromine anomalous scattering, and phosphorus anomalous peaks corroborated the backbone positions and validated the model. Attempts to phase the structure directly from phosphorus data failed, consistent with theoretical predictions that successful SAD phasing requires a significantly higher reflection-to-scatterer ratio. The final models reveal an RNA complex stabilized by Watson–Crick and Hoogsteen base pairing, forming a pseudo-helical complex instead of the anticipated hairpin stem-loop, likely reflecting crystallization artefacts. This work demonstrates the complementary use of bromine and phosphorus anomalous signals in RNA crystallography.
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Feb 2026
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I23-Long wavelength MX
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Hannah
Best
,
Lainey J.
Williamson
,
Adam B.
Cutts
,
Marina
Galchenkova
,
Oleksandr
Yefanov
,
Nicole
Bryce-Sharron
,
Emily A.
Heath
,
Raphael
De Wijn
,
Robin
Schubert
,
Anna
Munke
,
Alessandra
Henkel
,
Bjarne
Klopprogge
,
T. Emilie S.
Scheer
,
Viviane
Kremling
,
Salah
Awel
,
Gisel
Pena
,
Juraj
Knoska
,
Anusha
Keloth
,
Julia
Maracke
,
Romain
Letrun
,
Egor
Sobolev
,
Johan
Bielecki
,
Diogo
Melo
,
Sravya
Kantamneni
,
Katerina
Doerner
,
Marco
Kloos
,
Joachim
Schulz
,
P. Lourdu
Xavier
,
Marius
Lauffer
,
Maite
Villanueva
,
Primitivo
Caballero
,
Helen
Waller-Evans
,
Emyr
Lloyd-Evans
,
Charlotte
Uetrecht
,
Richard
Bean
,
Henry N.
Chapman
,
Neil
Crickmore
,
Pierre J.
Rizkallah
,
Colin
Berry
,
Dominik
Oberthuer
Diamond Proposal Number(s):
[36446]
Open Access
Abstract: Bacillus thuringiensis (Bt) strains naturally produce pesticidal proteins as nanocrystalline inclusions that are extraordinarily stable in aqueous environments, but which dissolve selectively at specific pH conditions. These proteins have been used in agriculture for >50 years and are critical to global food security. The majority of previously determined Bt Cry protein structures lack the extended C-terminal “crystallization domain,” which is thought to stabilize crystal packing and control selective solubility in insect targets, often via manipulation of disulfide bridges. It has also recently been shown to influence toxicity and target specificity. Here, we use serial femtosecond crystallography (SFX) to determine high-resolution full-length native structures of Cry1Ca18 (1.65 Å) and Cry8Ba2 (2.27 Å) in their natural nanocrystalline state. Differences in cysteine content (19 versus 4 residues) reveal distinct in vivo crystal-stabilization strategies. Understanding Bt toxin domain architecture and natural crystal formation is essential for improving biopesticide design and advancing agricultural genetic engineering.
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Feb 2026
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I23-Long wavelength MX
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Abstract: Marine picocyanobacteria are essential drivers of global biogeochemical cycles, playing a crucial role in ecosystem functioning. Their significant phylogenetic and functional diversity allow them to thrive across various marine regions. However, the mechanisms underpinning their adaptation to diverse oceanic niches remain poorly understood, especially with changing nutrient landscapes driven by climate change and anthropogenic activities. A critical factor in their success are nutrient uptake systems, particularly ATP-binding cassette (ABC) transporters, which account for over half of their transport capabilities. This thesis explores the substrate specificity, and ecological roles of substrate-binding proteins (SBPs) associated with these transporters, highlighting how these systems aid niche adaptation in marine picocyanobacteria. SBPs are key to ABC transporter function, binding substrates with high specificity and affinity, facilitating their cellular uptake. This study integrates structural biology, genomics, biophysical studies, and environmental genomics to elucidate the functions and ecological roles of these proteins, providing insights into the adaptive strategies of marine picocyanobacteria.
Functional characterisation of three phosphate binding protein homologs (PstS), three urea binding protein homologs (UrtA) and two glycine-betaine binding protein homologs (ProX) from Synechococcus strains inhabiting distinct oceanic niches was conducted. The study of PstS homologs in WH8102 revealed that PstS1b, unique to Synechococcus clade III strains, is the highest affinity binding protein, providing a competitive advantage in ultraoligotrophic environments. Analysis of UrtA homologs in CC9311 and WH8102 revealed UrtA from CC9311 had higher binding affinity to urea compared to both UrtA proteins from WH8102. This is intriguing as CC9311 originates from a high-nutrient mesotrophic environment, contrasting with WH8102’s habitat in a nutrient-poor oligotrophic region. Investigation of ProX homologs from MITS9220 and WH8102 revealed a functional distinction between the two proteins, with MITS9220_ProX likely behaving as a generalist solute-binding protein, while WH8102_ProX acts as a specialist binding protein for higher salinity environments.
The findings of this thesis highlight the versatility and adaptability of SBP-dependent ABC transporters in marine picocyanobacteria. The study demonstrates that these transport systems modulate their substrate affinities and specificities in response to environmental conditions, facilitating niche adaptation. This research is part of a larger project aimed at characterising the full repertoire of SBPs in marine picocyanobacteria, enhancing our understanding of nutrient acquisition mechanisms in these important microorganisms. The integration of various scientific approaches in this study provides a comprehensive framework for investigating the physiological and ecological significance of ABC uptake systems, offering valuable insights into the adaptive strategies of marine microbes in the face of changing oceanic conditions.
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Oct 2025
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I03-Macromolecular Crystallography
I23-Long wavelength MX
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Open Access
Abstract: Glycine N-acyltransferase (GLYAT; EC 2.3.1.13, Accession ID: AAI12537) is a key enzyme in mammalian homeostasis that has been linked to several pathologies in humans, including cancer. Here we report the first crystal structure of a member of the GLYAT family, both in the apo form as well as bound to benzoyl-CoA. Binding of glycine could be inferred from an acetate molecule from the crystallization solution. A detailed analysis of its structure and the effects of mutations of key residues helped elucidate the catalytic mechanism, showing a general base-catalyzed reaction driven by a potential low-barrier hydrogen bond (LBHB) formed between the catalytic Glu-His dyad. This work will aid further studies of GLYAT and other members of the family.
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Sep 2025
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I02-Macromolecular Crystallography
I03-Macromolecular Crystallography
I04-Macromolecular Crystallography
I23-Long wavelength MX
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Jessica
Domenech
,
Nuttawan
Pramanpol
,
Claudine
Bisson
,
Sveta E.
Sedelnikova
,
Joshua R.
Barrett
,
Abdul A. A. B.
Dakhil
,
Vitaliy
Mykhaylyk
,
Ali S.
Abdelhameed
,
Stephen E.
Harding
,
David W.
Rice
,
Patrick J.
Baker
,
Juan
Ferrer
Diamond Proposal Number(s):
[300, 1218, 24447, 31850]
Open Access
Abstract: Enzymes from salt-in halophiles are stable in conditions of low water activity with applications in chiral synthesis requiring organic solvents, yet the origins of such stability remains poorly understood. Here we describe the molecular basis of the reaction mechanism and dual NADH/NADPH-specificity of D2HDH, a 2-hydroxyacid dehydrogenase from the extreme halophile Haloferax mediterranei, an organism whose proteins have to remain active in high intracellular concentrations of KCl. Halophilic adaptations of D2HDH include the expected acidic surface and a reduction in hydrophobic surface resulting from a lower lysine content. Structure determination of crystals of D2HDH grown with KCl showed that bound K+ ions were coordinated predominantly by clusters of main chain protein carbonyl ligands, with no involvement of the numerous exposed surface carboxyls. Structural comparisons identified similar sites in other halophilic proteins suggesting that the generic use of carbonyl clusters to coordinate K+ ions may also contribute in a carboxylate-independent way to the stabilisation of the folded state of the protein in its high salt environment.
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Aug 2025
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I23-Long wavelength MX
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Isabel G.
Elliott
,
Hayden
Fisher
,
H. T. Claude
Chan
,
Tatyana
Inzhelevskaya
,
C. Ian
Mockridge
,
Christine A.
Penfold
,
Patrick J.
Duriez
,
Christian M.
Orr
,
Julie
Herniman
,
Kri T. J.
Müller
,
Jonathan W.
Essex
,
Mark S.
Cragg
,
Ivo
Tews
Diamond Proposal Number(s):
[29835]
Open Access
Abstract: A promising strategy in cancer immunotherapy is activation of immune signalling pathways through antibodies that target co-stimulatory receptors. hIgG2, one of four human antibody isotypes, is known to deliver strong agonistic activity, and modification of hIgG2 hinge disulfides can influence immune-stimulating activity. This was shown for antibodies directed against the hCD40 receptor, where cysteine-to-serine exchange mutations caused changes in antibody conformational flexibility. Here we demonstrate that the principles of increasing agonism by restricting antibody conformation through disulfide modification can be translated to the co-stimulatory receptor h4-1BB, another member of the tumour necrosis factor receptor superfamily. Furthermore, we explore structure-guided design of the anti-hCD40 antibody ChiLob7/4 and show that engineering additional disulfides between opposing F(ab’) arms can elicit conformational restriction, concomitant with enhanced agonism. These results support a mode where subtle increases in rigidity can deliver significant improvements in immunostimulatory activity, thus providing a strategy for the rational design of more powerful antibody therapeutics.
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Apr 2025
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I23-Long wavelength MX
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Diamond Proposal Number(s):
[26794]
Abstract: Perlecan is an essential multi-domain, disulfide bond rich basement membrane protein. Mutations in perlecan cause Schwartz-Jampel syndrome and dyssegmental dysplasia. While there has been a large body of experimental work reported on perlecan, there is only minimal structural information available to date. There is no prior structural data for region 3 of perlecan in which some Schwartz-Jampel syndrome causing point mutations have been reported. Here, we produce constructs of the disulfide rich region 3 of perlecan along with five mutations previously reported to cause Schwatz-Jampel syndrome. Four of the mutations resulted in decreased yields and thermal stability compared to the wild-type protein. In contrast, the P1019L mutation was produced in good yields and showed higher thermal stability than the wild-type protein. The crystal structures for both the wild-type and P1019L mutation were solved. As expected, both showed laminin IV-like and laminin-type EGF-like domains, with the P1019L mutation resulting in only a minor conformational change in a loop region and no significant changes in regular secondary or tertiary structure.
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Mar 2025
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