Your search keyword '"Reeks J"' showing total 26 results

1. Tunable luminescence thermal stability in YVxAs1−xO4:Eu3+ through the introduction of As5+ ions for remote temperature sensing applications

Author

Piotrowski, W. M., primary, Kardach, M., additional, Sobierajska, P., additional, Watras, A., additional, Reeks, J. M., additional, Kinzhybalo, V., additional, Marciniak, L., additional, and Wiglusz, R. J., additional

Published

2023

2. Tunable luminescence thermal stability in YVxAs1−xO4:Eu3+ through the introduction of As5+ ions for remote temperature sensing applications.

Author

Piotrowski, W. M., Kardach, M., Sobierajska, P., Watras, A., Reeks, J. M., Kinzhybalo, V., Marciniak, L., and Wiglusz, R. J.

Abstract

Thermal nonradiative depopulation processes of excited levels significantly influence the potential application of phosphors. The high efficiency of thermal quenching of luminescence can limit a phosphor's potential applications as well as reduce the temperature range in which such a material can be used. This work presents a new strategy of shifting of usable temperature range of luminescent thermometer based on Eu3+ ion emission that the molar ratio of (AsO4)3− in respect to (VO4)3− increases in YVxAs1−xO4 host material. Consequently, the thermometric performance of the luminescence thermometer based on the single band intensity ratio corresponding to the 5D0 → 7F1 of Eu3+ ions upon optical excitations matching to the 1A2(1T1) → 1B1(1T2) and 1E(1T1) → 1B1(1T2) electronic transition of (VO4)3− group can be optimized. As shown, the use of YV0.25As0.75O4:Eu3+ has an extended usable temperature range in respect to YVO4:Eu3+. This improvement, coupled with its high sensitivity (>1% K−1) make YV0.25As0.75O4:Eu3+ a more stable material for luminescence thermometer applications. The presented strategy for modulating the thermal properties of luminescent thermometers through the introduction of the (AsO4)3− groups is a step towards designing thermometers with on-demand thermometric performance. [ABSTRACT FROM AUTHOR]

Published

2023

3. PKM2 in complex with Compound 10

Author

Saur, M., primary, Hartshorn, M.J., additional, Dong, J., additional, Reeks, J., additional, Bunkoczi, G., additional, Jhoti, H., additional, and Williams, P.A., additional

Published

2020

4. PKM2 in complex with Compound 5

Author

Saur, M., primary, Hartshorn, M.J., additional, Dong, J., additional, Reeks, J., additional, Bunkoczi, G., additional, Jhoti, H., additional, and Williams, P.A., additional

Published

2020

5. PKM2 in complex with Compound 6

Author

Saur, M., primary, Hartshorn, M.J., additional, Dong, J., additional, Reeks, J., additional, Bunkoczi, G., additional, Jhoti, H., additional, and Williams, P.A., additional

Published

2020

6. Beta-galactosidase in complex with PETG

Author

Saur, M., primary, Hartshorn, M.J., additional, Dong, J., additional, Reeks, J., additional, Bunkoczi, G., additional, Jhoti, H., additional, and Williams, P.A., additional

Published

2020

7. PKM2 in complex with L-threonine

Author

Saur, M., primary, Hartshorn, M.J., additional, Dong, J., additional, Reeks, J., additional, Bunkoczi, G., additional, Jhoti, H., additional, and Williams, P.A., additional

Published

2020

8. Beta-galactosidase in complex with deoxygalacto-nojirimycin

Author

Saur, M., primary, Hartshorn, M.J., additional, Dong, J., additional, Reeks, J., additional, Bunkoczi, G., additional, Jhoti, H., additional, and Williams, P.A., additional

Published

2020

9. Beta-galactosidase in complex with L-ribose

Author

Saur, M., primary, Hartshorn, M.J., additional, Dong, J., additional, Reeks, J., additional, Bunkoczi, G., additional, Jhoti, H., additional, and Williams, P.A., additional

Published

2020

10. Structure of the stapled peptide YS-01 bound to MDM2

Author

Tan, Y.S., primary, Reeks, J., additional, Brown, C.J., additional, Jennings, C.E., additional, Eapen, R.S., additional, Tng, Q.S., additional, Thean, D., additional, Ying, Y.T., additional, Gago, F.J.F., additional, Lane, D.P., additional, Noble, M.E.M., additional, and Verma, C., additional

Published

2016

11. Crystal structure of an archaeal CRISPR-associated Cas6 nuclease

Author

Reeks, J., primary, Liu, H., additional, White, M.F., additional, and Naismith, J.H., additional

Published

2013

12. The structure of Csa5 from Sulfolobus solfataricus.

Author

Reeks, J., primary, Anderson, L., additional, White, M.F., additional, and Naismith, J.H., additional

Published

2013

13. SSO1725, a protein involved in the CRISPR/Cas pathway

Author

Reeks, J., primary, Liu, H., additional, Naismith, J., additional, White, M., additional, and McMahon, S., additional

Published

2010

14. Fragment-Based Discovery of a Series of Allosteric-Binding Site Modulators of β-Glucocerebrosidase.

Author

Palmer N, Agnew C, Benn C, Buffham WJ, Castro JN, Chessari G, Clark M, Cons BD, Coyle JE, Dawson LA, Hamlett CCF, Hodson C, Holding F, Johnson CN, Liebeschuetz JW, Mahajan P, McCarthy JM, Murray CW, O'Reilly M, Peakman T, Price A, Rapti M, Reeks J, Schöpf P, St-Denis JD, Valenzano C, Wallis NG, Walser R, Weir H, Wilsher NE, Woodhead A, Bento CF, and Tisi D

Subjects

Humans, Crystallography, X-Ray, Structure-Activity Relationship, Models, Molecular, Small Molecule Libraries chemistry, Small Molecule Libraries pharmacology, Small Molecule Libraries metabolism, Glucosylceramidase metabolism, Glucosylceramidase antagonists & inhibitors, Glucosylceramidase chemistry, Drug Discovery, Allosteric Site

Abstract

β-Glucocerebrosidase (GBA/GCase) mutations leading to misfolded protein cause Gaucher's disease and are a major genetic risk factor for Parkinson's disease and dementia with Lewy bodies. The identification of small molecule pharmacological chaperones that can stabilize the misfolded protein and increase delivery of degradation-prone mutant GCase to the lysosome is a strategy under active investigation. Here, we describe the first use of fragment-based drug discovery (FBDD) to identify pharmacological chaperones of GCase. The fragment hits were identified by using X-ray crystallography and biophysical techniques. This work led to the discovery of a series of compounds that bind GCase with nM potency and positively modulate GCase activity in cells.

Published

2024

15. Design, clinical applications and post-surgical assessment of bioresorbable 3D-printed craniofacial composite implants.

Author

Targońska S, Dobrzyńska-Mizera M, Di Lorenzo ML, Knitter M, Longo A, Dobrzyński M, Rutkowska M, Barnaś S, Czapiga B, Stagraczyński M, Mikulski M, Muzalewska M, Wyleżoł M, Rewak-Soroczyńska J, Nowak N, Andrzejewski J, Reeks J, and Wiglusz RJ

Subjects

Humans, Absorbable Implants, Bone Substitutes chemistry, Skull surgery, Polyesters chemistry, Male, Prosthesis Design, Biocompatible Materials chemistry, Female, Printing, Three-Dimensional, Durapatite chemistry

Abstract

This study details the design, fabrication, clinical trials' evaluation, and analysis after the clinical application of 3D-printed bone reconstruction implants made of nHAp@PLDLLA [nanohydroxyapatite@poly(L-lactide- co -D,L-lactide)] biomaterial. The 3D-printed formulations have been tested as bone reconstruction Cranioimplants in 3 different medical cases, including frontal lobe, mandibular bone, and cleft palate reconstructions. Replacing one of the implants after 6 months provided a unique opportunity to evaluate the post-surgical implant obtained from a human patient. This allowed us to quantify physicochemical changes and develop a spatial map of osseointegration and material degradation kinetics as a function of specific locations. To the best of our knowledge, hydrolytic degradation and variability in the physicochemical and mechanical properties of the biomimetic, 3D-printed implants have not been quantified in the literature after permanent placement in the human body. Such analysis has revealed the constantly changing properties of the implant, which should be considered to optimize the design of patient-specific bone substitutes. Moreover, it has been proven that the obtained composition can produce biomimetic, bioresorbable and bone-forming alloplastic substitutes tailored to each patient, allowing for shorter surgery times and faster patient recovery than currently available methods.

Published

2024

16. A randomised controlled dismantling trial of sleep restriction therapies for chronic insomnia disorder in middle childhood: effects on sleep and anxiety, and possible contraindications.

Author

Cain N, Richardson C, Bartel K, Whittall H, Reeks J, and Gradisar M

Subjects

Child, Female, Humans, Male, Sleepiness, Treatment Outcome, Anxiety complications, Anxiety therapy, Contraindications, Sleep Initiation and Maintenance Disorders therapy, Parasomnias

Abstract

Sleep restriction therapies likely drive improvement in insomnia in middle childhood via increases in homeostatic sleep pressure (e.g., evening sleepiness). Increased evening sleepiness may also dampen comorbid anxiety symptoms; and reduced wakefulness in bed may reduce worry. However, sleep restriction therapies have never been evaluated as a standalone intervention in this population. The mechanism of action needs testing, as do effects on anxiety, and cognitive performance and parasomnias (possible contraindications). This randomised controlled trial evaluated the efficacy of two "doses" of sleep restriction therapy (sleep restriction therapy, bedtime restriction therapy), compared to a control condition (time in bed regularisation). A total of 61 children (mean [SD, range] age 9.1 [2.1, 6-14] years; 54% female) with chronic insomnia disorder received two weekly 60-min treatment sessions with a psychologist. Sleep, sleepiness, anxiety, worry, cognitive performance, and parasomnias were measured pre-treatment, across treatment, and at 4-weeks post-treatment. Both the sleep and bedtime restriction groups experienced reductions in total sleep time (d = 1.38-2.27) and increases in evening sleepiness (d = 1.01-1.47) during the 2-week treatment, and improvements in insomnia (i.e., sleep onset latency; d = 1.10-1.21), relative to the control group. All groups reported improved anxiety and worry, yet there were no differences between the control and restriction groups (all p > 0.658). Time in bed increased at the 1-month follow-up, and benefits to sleep and insomnia were maintained. There were no adverse effects on cognitive functioning (all p > 0.259), nor parasomnia occurrence (all p > 0.740). These results suggest that sleep restriction therapies are brief, yet effective, standalone interventions for insomnia in middle childhood, and improvements are likely due to increased sleepiness, not sleep regularisation., (© 2022 European Sleep Research Society.)

Published

2022

17. Fragment-Based Discovery of a Novel, Brain Penetrant, Orally Active HDAC2 Inhibitor.

Author

Tamanini E, Miyamura S, Buck IM, Cons BD, Dawson L, East C, Futamura T, Goto S, Griffiths-Jones C, Hashimoto T, Heightman TD, Ishikawa S, Ito H, Kaneko Y, Kawato T, Kondo K, Kurihara N, McCarthy JM, Mori Y, Nagase T, Nakaishi Y, Reeks J, Sato A, Schöpf P, Tai K, Tamai T, Tisi D, and Woolford AJ

Abstract

Fragment-based ligand discovery was successfully applied to histone deacetylase HDAC2. In addition to the anticipated hydroxamic acid- and benzamide-based fragment screening hits, a low affinity (∼1 mM) α-amino-amide zinc binding fragment was identified, as well as fragments binding to other regions of the catalytic site. This alternative zinc-binding fragment was further optimized, guided by the structural information from protein-ligand complex X-ray structures, into a sub-μM, brain penetrant, HDAC2 inhibitor ( 17 ) capable of modulating histone acetylation levels in vivo ., Competing Interests: The authors declare no competing financial interest., (© 2022 American Chemical Society.)

Published

2022

18. Structure-Based Design of Potent and Orally Active Isoindolinone Inhibitors of MDM2-p53 Protein-Protein Interaction.

Author

Chessari G, Hardcastle IR, Ahn JS, Anil B, Anscombe E, Bawn RH, Bevan LD, Blackburn TJ, Buck I, Cano C, Carbain B, Castro J, Cons B, Cully SJ, Endicott JA, Fazal L, Golding BT, Griffin RJ, Haggerty K, Harnor SJ, Hearn K, Hobson S, Holvey RS, Howard S, Jennings CE, Johnson CN, Lunec J, Miller DC, Newell DR, Noble MEM, Reeks J, Revill CH, Riedinger C, St Denis JD, Tamanini E, Thomas H, Thompson NT, Vinković M, Wedge SR, Williams PA, Wilsher NE, Zhang B, and Zhao Y

Subjects

Animals, Antineoplastic Agents chemical synthesis, Antineoplastic Agents metabolism, Bone Neoplasms drug therapy, Cell Line, Tumor, Cell Proliferation drug effects, Crystallography, X-Ray, Drug Stability, Female, Humans, Isoindoles chemical synthesis, Isoindoles metabolism, Macaca fascicularis, Male, Mice, Inbred BALB C, Mice, Nude, Microsomes, Liver metabolism, Molecular Structure, Protein Binding, Structure-Activity Relationship, Xenograft Model Antitumor Assays, Mice, Antineoplastic Agents pharmacology, Isoindoles pharmacology, Osteosarcoma drug therapy, Protein Multimerization drug effects, Proto-Oncogene Proteins c-mdm2 metabolism, Tumor Suppressor Protein p53 metabolism

Abstract

Inhibition of murine double minute 2 (MDM2)-p53 protein-protein interaction with small molecules has been shown to reactivate p53 and inhibit tumor growth. Here, we describe rational, structure-guided, design of novel isoindolinone-based MDM2 inhibitors. MDM2 X-ray crystallography, quantum mechanics ligand-based design, and metabolite identification all contributed toward the discovery of potent in vitro and in vivo inhibitors of the MDM2-p53 interaction with representative compounds inducing cytostasis in an SJSA-1 osteosarcoma xenograft model following once-daily oral administration.

Published

2021

19. Discriminative SKP2 Interactions with CDK-Cyclin Complexes Support a Cyclin A-Specific Role in p27KIP1 Degradation.

Author

Salamina M, Montefiore BC, Liu M, Wood DJ, Heath R, Ault JR, Wang LZ, Korolchuk S, Baslé A, Pastok MW, Reeks J, Tatum NJ, Sobott F, Arold ST, Pagano M, Noble MEM, and Endicott JA

Subjects

Binding Sites, CDC2-CDC28 Kinases chemistry, CDC2-CDC28 Kinases genetics, CDC2-CDC28 Kinases metabolism, Cyclin A genetics, Cyclin A metabolism, Cyclin E chemistry, Cyclin E genetics, Cyclin E metabolism, Cyclin-Dependent Kinase 2 genetics, Cyclin-Dependent Kinase 2 metabolism, Cyclin-Dependent Kinase Inhibitor p27 genetics, Cyclin-Dependent Kinase Inhibitor p27 metabolism, Gene Expression Regulation, HEK293 Cells, Humans, Protein Binding, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Interaction Domains and Motifs, Proteolysis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, S-Phase Kinase-Associated Proteins genetics, S-Phase Kinase-Associated Proteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Signal Transduction, Cyclin A chemistry, Cyclin-Dependent Kinase 2 chemistry, Cyclin-Dependent Kinase Inhibitor p27 chemistry, G1 Phase Cell Cycle Checkpoints, S-Phase Kinase-Associated Proteins chemistry

Abstract

The SCF SKP2 ubiquitin ligase relieves G1 checkpoint control of CDK-cyclin complexes by promoting p27KIP1 degradation. We describe reconstitution of stable complexes containing SKP1-SKP2 and CDK1-cyclin B or CDK2-cyclin A/E, mediated by the CDK regulatory subunit CKS1. We further show that a direct interaction between a SKP2 N-terminal motif and cyclin A can stabilize SKP1-SKP2-CDK2-cyclin A complexes in the absence of CKS1. We identify the SKP2 binding site on cyclin A and demonstrate the site is not present in cyclin B or cyclin E. This site is distinct from but overlapping with features that mediate binding of p27KIP1 and other G1 cyclin regulators to cyclin A. We propose that the capacity of SKP2 to engage with CDK2-cyclin A by more than one structural mechanism provides a way to fine tune the degradation of p27KIP1 and distinguishes cyclin A from other G1 cyclins to ensure orderly cell cycle progression., (Copyright © 2021 The Author(s). Published by Elsevier Ltd.. All rights reserved.)

Published

2021

20. Fragment-based drug discovery using cryo-EM.

Author

Saur M, Hartshorn MJ, Dong J, Reeks J, Bunkoczi G, Jhoti H, and Williams PA

Subjects

Carrier Proteins chemistry, Carrier Proteins metabolism, High-Throughput Screening Assays, Humans, Membrane Proteins chemistry, Membrane Proteins metabolism, Reproducibility of Results, Thyroid Hormones chemistry, Thyroid Hormones metabolism, beta-Galactosidase chemistry, beta-Galactosidase metabolism, Thyroid Hormone-Binding Proteins, Cryoelectron Microscopy methods, Drug Discovery methods

Abstract

Recent advances in electron cryo-microscopy (cryo-EM) structure determination have pushed the resolutions obtainable by the method into the range widely considered to be of utility for drug discovery. Here, we review the use of cryo-EM in fragment-based drug discovery (FBDD) based on in-house method development. We demonstrate not only that cryo-EM can reveal details of the molecular interactions between fragments and a protein, but also that the current reproducibility, quality, and throughput are compatible with FBDD. We exemplify this using the test system β-galactosidase (Bgal) and the oncology target pyruvate kinase 2 (PKM2)., (Copyright © 2020 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published

2020

21. Tuning the Binding Affinity and Selectivity of Perfluoroaryl-Stapled Peptides by Cysteine-Editing.

Author

Verhoork SJM, Jennings CE, Rozatian N, Reeks J, Meng J, Corlett EK, Bunglawala F, Noble MEM, Leach AG, and Coxon CR

Subjects

Amino Acid Sequence, Cysteine metabolism, Humans, Peptides chemical synthesis, Peptides metabolism, Protein Binding, Protein Conformation, Proto-Oncogene Proteins c-mdm2 chemistry, Proto-Oncogene Proteins c-mdm2 genetics, Proto-Oncogene Proteins c-mdm2 metabolism, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Tumor Suppressor Protein p53 chemistry, Tumor Suppressor Protein p53 genetics, Tumor Suppressor Protein p53 metabolism, Cysteine chemistry, Fluorocarbons chemistry, Peptides chemistry

Abstract

A growing number of approaches to "staple" α-helical peptides into a bioactive conformation using cysteine cross-linking are emerging. Here, the replacement of l-cysteine with "cysteine analogues" in combinations of different stereochemistry, side chain length and beta-carbon substitution, is explored to examine the influence that the thiol-containing residue(s) has on target protein binding affinity in a well-explored model system, p53-MDM2/MDMX, which is constituted by the interaction of the tumour suppressor protein p53 and proteins MDM2 and MDMX, which regulate p53 activity. In some cases, replacement of one or more l-cysteine residues afforded significant changes in the measured binding affinity and target selectivity of the peptide. Computationally constructed homology models indicate that some modifications, such as incorporating two d-cysteine residues, favourably alter the positions of key functional amino acid side chains, which is likely to cause changes in binding affinity, in agreement with measured surface plasmon resonance data., (© 2019 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2019

22. Benzene Probes in Molecular Dynamics Simulations Reveal Novel Binding Sites for Ligand Design.

Author

Tan YS, Reeks J, Brown CJ, Thean D, Ferrer Gago FJ, Yuen TY, Goh ET, Lee XE, Jennings CE, Joseph TL, Lakshminarayanan R, Lane DP, Noble ME, and Verma CS

Subjects

Binding Sites, Ligands, Models, Molecular, Molecular Dynamics Simulation, Protein Binding, Benzene chemistry

Abstract

Protein flexibility poses a major challenge in binding site identification. Several computational pocket detection methods that utilize small-molecule probes in molecular dynamics (MD) simulations have been developed to address this issue. Although they have proven hugely successful at reproducing experimental structural data, their ability to predict new binding sites that are yet to be identified and characterized has not been demonstrated. Here, we report the use of benzenes as probe molecules in ligand-mapping MD (LMMD) simulations to predict the existence of two novel binding sites on the surface of the oncoprotein MDM2. One of them was serendipitously confirmed by biophysical assays and X-ray crystallography to be important for the binding of a new family of hydrocarbon stapled peptides that were specifically designed to target the other putative site. These results highlight the predictive power of LMMD and suggest that predictions derived from LMMD simulations can serve as a reliable basis for the identification of novel ligand binding sites in structure-based drug design.

Published

2016

23. CRISPR interference: a structural perspective.

Author

Reeks J, Naismith JH, and White MF

Subjects

Crystallography, Models, Molecular, Nucleic Acid Conformation, RNA Processing, Post-Transcriptional, Repetitive Sequences, Nucleic Acid

Abstract

CRISPR (cluster of regularly interspaced palindromic repeats) is a prokaryotic adaptive defence system, providing immunity against mobile genetic elements such as viruses. Genomically encoded crRNA (CRISPR RNA) is used by Cas (CRISPR-associated) proteins to target and subsequently degrade nucleic acids of invading entities in a sequence-dependent manner. The process is known as 'interference'. In the present review we cover recent progress on the structural biology of the CRISPR/Cas system, focusing on the Cas proteins and complexes that catalyse crRNA biogenesis and interference. Structural studies have helped in the elucidation of key mechanisms, including the recognition and cleavage of crRNA by the Cas6 and Cas5 proteins, where remarkable diversity at the level of both substrate recognition and catalysis has become apparent. The RNA-binding RAMP (repeat-associated mysterious protein) domain is present in the Cas5, Cas6, Cas7 and Cmr3 protein families and RAMP-like domains are found in Cas2 and Cas10. Structural analysis has also revealed an evolutionary link between the small subunits of the type I and type III-B interference complexes. Future studies of the interference complexes and their constituent components will transform our understanding of the system.

Published

2013

24. Structure of a dimeric crenarchaeal Cas6 enzyme with an atypical active site for CRISPR RNA processing.

Author

Reeks J, Sokolowski RD, Graham S, Liu H, Naismith JH, and White MF

Subjects

Amino Acid Sequence, Archaeal Proteins genetics, Base Sequence, Crystallography, X-Ray, Inverted Repeat Sequences genetics, Models, Molecular, Molecular Sequence Data, RNA, Archaeal genetics, RNA, Archaeal metabolism, Ribonucleases genetics, Sequence Homology, Amino Acid, Sulfolobus solfataricus genetics, Sulfolobus solfataricus metabolism, Archaeal Proteins chemistry, Archaeal Proteins metabolism, Catalytic Domain genetics, RNA Processing, Post-Transcriptional genetics, RNA, Archaeal chemistry, Ribonucleases chemistry, Ribonucleases metabolism, Sulfolobus solfataricus enzymology

Abstract

The competition between viruses and hosts is played out in all branches of life. Many prokaryotes have an adaptive immune system termed 'CRISPR' (clustered regularly interspaced short palindromic repeats) which is based on the capture of short pieces of viral DNA. The captured DNA is integrated into the genomic DNA of the organism flanked by direct repeats, transcribed and processed to generate crRNA (CRISPR RNA) that is loaded into a variety of effector complexes. These complexes carry out sequence-specific detection and destruction of invading mobile genetic elements. In the present paper, we report the structure and activity of a Cas6 (CRISPR-associated 6) enzyme (Sso1437) from Sulfolobus solfataricus responsible for the generation of unit-length crRNA species. The crystal structure reveals an unusual dimeric organization that is important for the enzyme's activity. In addition, the active site lacks the canonical catalytic histidine residue that has been viewed as an essential feature of the Cas6 family. Although several residues contribute towards catalysis, none is absolutely essential. Coupled with the very low catalytic rate constants of the Cas6 family and the plasticity of the active site, this suggests that the crRNA recognition and chaperone-like activities of the Cas6 family should be considered as equal to or even more important than their role as traditional enzymes.

Published

2013

25. Structure of the archaeal Cascade subunit Csa5: relating the small subunits of CRISPR effector complexes.

Author

Reeks J, Graham S, Anderson L, Liu H, White MF, and Naismith JH

Subjects

Archaeal Proteins genetics, Archaeal Proteins metabolism, CRISPR-Associated Proteins genetics, CRISPR-Associated Proteins metabolism, Crystallography, X-Ray, Evolution, Molecular, Models, Molecular, Protein Structure, Tertiary, RNA, Archaeal chemistry, RNA, Archaeal genetics, RNA, Archaeal metabolism, Sulfolobus solfataricus genetics, Archaeal Proteins chemistry, CRISPR-Associated Proteins chemistry, Clustered Regularly Interspaced Short Palindromic Repeats genetics, Sulfolobus solfataricus metabolism

Abstract

The Cascade complex for CRISPR-mediated antiviral immunity uses CRISPR RNA (crRNA) to target invading DNA species from mobile elements such as viruses, leading to their destruction. The core of the Cascade effector complex consists of the Cas5 and Cas7 subunits, which are widely conserved in prokaryotes. Cas7 binds crRNA and forms the helical backbone of Cascade. Many archaea encode a version of the Cascade complex (denoted Type I-A) that includes a Csa5 (or small) subunit, which interacts weakly with the core proteins. Here, we report the crystal structure of the Csa5 protein from Sulfolobus solfataricus. Csa5 comprises a conserved α-helical domain with a small insertion consisting of a weakly conserved β-strand domain. In the crystal, the Csa5 monomers have multimerized into infinite helical threads. At each interface is a strictly conserved intersubunit salt bridge, deletion of which disrupts multimerization. Structural analysis indicates a shared evolutionary history among the small subunits of the CRISPR effector complexes. The same α-helical domain is found in the C-terminal domain of Cse2 (from Type I-E Cascade), while the N-terminal domain of Cse2 is found in Cmr5 of the CMR (Type III-B) effector complex. As Cmr5 shares no match with Csa5, two possibilities present themselves: selective domain loss from an ancestral Cse2 to create two new subfamilies or domain fusion of two separate families to create a new Cse2 family. A definitive answer awaits structural studies of further small subunits from other CRISPR effector complexes.

Published

2013

26. Structure and mechanism of the CMR complex for CRISPR-mediated antiviral immunity.

Author

Zhang J, Rouillon C, Kerou M, Reeks J, Brugger K, Graham S, Reimann J, Cannone G, Liu H, Albers SV, Naismith JH, Spagnolo L, and White MF

Subjects

Archaeal Proteins isolation & purification, Archaeal Viruses immunology, Base Sequence, Crystallography, X-Ray, Macromolecular Substances chemistry, Macromolecular Substances isolation & purification, Microscopy, Electron, Models, Molecular, Molecular Sequence Data, Nucleic Acid Conformation, Protein Structure, Quaternary, Protein Structure, Tertiary, Protein Subunits chemistry, Protein Subunits isolation & purification, RNA Cleavage, RNA, Archaeal genetics, RNA, Archaeal isolation & purification, Sulfolobus solfataricus genetics, Sulfolobus solfataricus immunology, Sulfolobus solfataricus virology, Archaeal Proteins chemistry, Inverted Repeat Sequences, RNA, Archaeal chemistry, Sulfolobus solfataricus metabolism

Abstract

The prokaryotic clusters of regularly interspaced palindromic repeats (CRISPR) system utilizes genomically encoded CRISPR RNA (crRNA), derived from invading viruses and incorporated into ribonucleoprotein complexes with CRISPR-associated (CAS) proteins, to target and degrade viral DNA or RNA on subsequent infection. RNA is targeted by the CMR complex. In Sulfolobus solfataricus, this complex is composed of seven CAS protein subunits (Cmr1-7) and carries a diverse "payload" of targeting crRNA. The crystal structure of Cmr7 and low-resolution structure of the complex are presented. S. solfataricus CMR cleaves RNA targets in an endonucleolytic reaction at UA dinucleotides. This activity is dependent on the 8 nt repeat-derived 5' sequence in the crRNA, but not on the presence of a protospacer-associated motif (PAM) in the target. Both target and guide RNAs can be cleaved, although a single molecule of guide RNA can support the degradation of multiple targets., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2012