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7. Structural characterization of macro domain-containing Thoeris antiphage defense systems.

Author

Shi Y, Masic V, Mosaiab T, Rajaratman P, Hartley-Tassell L, Sorbello M, Goulart CC, Vasquez E, Mishra BP, Holt S, Gu W, Kobe B, and Ve T

Subjects
Bacteriophages, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Bacterial Proteins genetics, Models, Molecular, NAD metabolism, Protein Binding, Protein Domains
Abstract

Thoeris defense systems protect bacteria from infection by phages via abortive infection. In these systems, ThsB proteins serve as sensors of infection and generate signaling nucleotides that activate ThsA effectors. Silent information regulator and SMF/DprA-LOG (SIR2-SLOG) containing ThsA effectors are activated by cyclic ADP-ribose (ADPR) isomers 2'cADPR and 3'cADPR, triggering abortive infection via nicotinamide adenine dinucleotide (NAD + ) depletion. Here, we characterize Thoeris systems with transmembrane and macro domain (TM-macro)-containing ThsA effectors. We demonstrate that ThsA macro domains bind ADPR and imidazole adenine dinucleotide (IAD), but not 2'cADPR or 3'cADPR. Combining crystallography, in silico predictions, and site-directed mutagenesis, we show that ThsA macro domains form nucleotide-induced higher-order oligomers, enabling TM domain clustering. We demonstrate that ThsB can produce both ADPR and IAD, and we identify a ThsA TM-macro-specific ThsB subfamily with an active site resembling deoxy-nucleotide and deoxy-nucleoside processing enzymes. Collectively, our study demonstrates that Thoeris systems with SIR2-SLOG and TM-macro ThsA effectors trigger abortive infection via distinct mechanisms.

Published
2024
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8. New Perspectives on Escherichia coli Signal Peptidase I Substrate Specificity: Investigating Why the TasA Cleavage Site Is Incompatible with LepB Cleavage.

Author

Musik JE, Poole J, Day CJ, Haselhorst T, Jen FE, Ve T, Masic V, Jennings MP, and Zalucki YM

Subjects
Humans, Substrate Specificity, Tryptophan metabolism, Amino Acid Sequence, Protein Sorting Signals, Escherichia coli metabolism, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism
Abstract

Escherichia coli signal peptidase I (LepB) has been shown to inefficiently cleave secreted proteins with aromatic amino acids at the second position after the signal peptidase cleavage site (P2'). The Bacillus subtilis exported protein TasA contains a phenylalanine at P2', which in B. subtilis is cleaved by a dedicated archaeal-organism-like signal peptidase, SipW. We have previously shown that when the TasA signal peptide is fused to maltose binding protein (MBP) up to the P2' position, the TasA-MBP fusion protein is cleaved very inefficiently by LepB. However, the precise reason why the TasA signal peptide hinders cleavage by LepB is not known. In this study, a set of 11 peptides were designed to mimic the inefficiently cleaved secreted proteins, wild-type TasA and TasA-MBP fusions, to determine whether the peptides interact with and inhibit the function of LepB. The binding affinity and inhibitory potential of the peptides against LepB were assessed by surface plasmon resonance (SPR) and a LepB enzyme activity assay. Molecular modeling of the interaction between TasA signal peptide and LepB indicated that the tryptophan residue at P2 (two amino acids before the cleavage site) inhibited the active site serine-90 residue on LepB from accessing the cleavage site. Replacing the P2 tryptophan with alanine (W26A) allowed for more efficient processing of the signal peptide when the TasA-MBP fusion was expressed in E. coli. The importance of this residue to inhibit signal peptide cleavage and the potential to design LepB inhibitors based on the TasA signal peptide are discussed. IMPORTANCE Signal peptidase I is an important drug target, and understanding its substrate is critically important to develop new bacterium-specific drugs. To that end, we have a unique signal peptide that we have shown is refractory to processing by LepB, the essential signal peptidase I in E. coli, but previously has been shown to be processed by a more human-like signal peptidase found in some bacteria. In this study, we demonstrate how the signal peptide can bind but is unable to be processed by LepB, using a variety of methods. This can inform the field on how to better design drugs that can target LepB and understand the differences between bacterial and human-like signal peptidases., Competing Interests: The authors declare no conflict of interest.

Published
2023
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9. Cyclic ADP ribose isomers: Production, chemical structures, and immune signaling.

Author

Manik MK, Shi Y, Li S, Zaydman MA, Damaraju N, Eastman S, Smith TG, Gu W, Masic V, Mosaiab T, Weagley JS, Hancock SJ, Vasquez E, Hartley-Tassell L, Kargios N, Maruta N, Lim BYJ, Burdett H, Landsberg MJ, Schembri MA, Prokes I, Song L, Grant M, DiAntonio A, Nanson JD, Guo M, Milbrandt J, Ve T, and Kobe B

Subjects
Isomerism, NAD metabolism, Protein Domains, Receptors, Interleukin-1 chemistry, Signal Transduction, Tryptophan chemistry, Tryptophan genetics, ADP-ribosyl Cyclase chemistry, ADP-ribosyl Cyclase genetics, ADP-ribosyl Cyclase metabolism, Adaptor Proteins, Vesicular Transport chemistry, Adaptor Proteins, Vesicular Transport genetics, Adaptor Proteins, Vesicular Transport metabolism, Bacteria immunology, Bacteria virology, Bacterial Proteins chemistry, Bacterial Proteins genetics, Bacterial Proteins metabolism, Cyclic ADP-Ribose biosynthesis, Cyclic ADP-Ribose chemistry, Plant Immunity, Toll-Like Receptors chemistry, Toll-Like Receptors genetics, Toll-Like Receptors metabolism
Abstract

Cyclic adenosine diphosphate (ADP)-ribose (cADPR) isomers are signaling molecules produced by bacterial and plant Toll/interleukin-1 receptor (TIR) domains via nicotinamide adenine dinucleotide (oxidized form) (NAD + ) hydrolysis. We show that v-cADPR (2'cADPR) and v2-cADPR (3'cADPR) isomers are cyclized by O-glycosidic bond formation between the ribose moieties in ADPR. Structures of 2'cADPR-producing TIR domains reveal conformational changes that lead to an active assembly that resembles those of Toll-like receptor adaptor TIR domains. Mutagenesis reveals a conserved tryptophan that is essential for cyclization. We show that 3'cADPR is an activator of ThsA effector proteins from the bacterial antiphage defense system termed Thoeris and a suppressor of plant immunity when produced by the effector HopAM1. Collectively, our results reveal the molecular basis of cADPR isomer production and establish 3'cADPR in bacteria as an antiviral and plant immunity-suppressing signaling molecule.

Published
2022
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10. Structural basis of SARM1 activation, substrate recognition, and inhibition by small molecules.

Author

Shi Y, Kerry PS, Nanson JD, Bosanac T, Sasaki Y, Krauss R, Saikot FK, Adams SE, Mosaiab T, Masic V, Mao X, Rose F, Vasquez E, Furrer M, Cunnea K, Brearley A, Gu W, Luo Z, Brillault L, Landsberg MJ, DiAntonio A, Kobe B, Milbrandt J, Hughes RO, and Ve T

Subjects
Cytoskeletal Proteins chemistry, Cytoskeletal Proteins genetics, NAD+ Nucleosidase metabolism, Protein Domains, Armadillo Domain Proteins genetics, NAD metabolism
Abstract

The NADase SARM1 (sterile alpha and TIR motif containing 1) is a key executioner of axon degeneration and a therapeutic target for several neurodegenerative conditions. We show that a potent SARM1 inhibitor undergoes base exchange with the nicotinamide moiety of nicotinamide adenine dinucleotide (NAD + ) to produce the bona fide inhibitor 1AD. We report structures of SARM1 in complex with 1AD, NAD + mimetics and the allosteric activator nicotinamide mononucleotide (NMN). NMN binding triggers reorientation of the armadillo repeat (ARM) domains, which disrupts ARM:TIR interactions and leads to formation of a two-stranded TIR domain assembly. The active site spans two molecules in these assemblies, explaining the requirement of TIR domain self-association for NADase activity and axon degeneration. Our results reveal the mechanisms of SARM1 activation and substrate binding, providing rational avenues for the design of new therapeutics targeting SARM1., Competing Interests: Declaration of interests A.D. and J.M. are co-founders, scientific advisory board members, and shareholders of Disarm Therapeutics. B.K. is a shareholder of Disarm Therapeutics. Y. Sasaki and B.K. are consultants to Disarm Therapeutics. B.K. and T.V. receive research funding from Disarm Therapeutics. R.O.H., R.K., and T.B. are employees and shareholders in Disarm Therapeutics. S.E.A., M.F., K.C., A.B., and P.S.K. are employees of Evotec SE. R.O.H., T.B., and A.B. are inventors on a patent related to isoquinoline inhibitors of SARM1 (WO 2019/236879 Al). The authors have no additional competing financial interests., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2022
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11. Discovery of Cofactor Competitive Inhibitors against the Human Methyltransferase Fibrillarin.

Author

Shi Y, El-Deeb IM, Masic V, Hartley-Tassell L, Maggioni A, Itzstein MV, and Ve T

Abstract

Fibrillarin (FBL) is an essential and evolutionarily highly conserved S-adenosyl methionine (SAM) dependent methyltransferase. It is the catalytic component of a multiprotein complex that facilitates 2'- O -methylation of ribosomal RNAs (rRNAs), a modification essential for accurate and efficient protein synthesis in eukaryotic cells. It was recently established that human FBL (hFBL) is critical for Nipah, Hendra, and respiratory syncytial virus infections. In addition, overexpression of hFBL contributes towards tumorgenesis and is associated with poor survival in patients with breast cancer, suggesting that hFBL is a potential target for the development of both antiviral and anticancer drugs. An attractive strategy to target cofactor-dependent enzymes is the selective inhibition of cofactor binding, which has been successful for the development of inhibitors against several protein methyltransferases including PRMT5, DOT1L, and EZH2. In this work, we solved crystal structures of the methyltransferase domain of hFBL in apo form and in complex with the cofactor SAM. Screening of a fluorinated fragment library, via X-ray crystallography and 19F NMR spectroscopy, yielded seven hit compounds that competed with cofactor binding, two of which resulted in co-crystal structures. One of these structures revealed unexpected conformational variability in the cofactor binding site, which allows it to accommodate a compound significantly different from SAM. Our structural data provide critical information for the design of selective cofactor competitive inhibitors targeting hFBL, and preliminary elaboration of hit compounds has led to additional cofactor site binders.

Published
2021
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12. SARM1 is a metabolic sensor activated by an increased NMN/NAD + ratio to trigger axon degeneration.

Author

Figley MD, Gu W, Nanson JD, Shi Y, Sasaki Y, Cunnea K, Malde AK, Jia X, Luo Z, Saikot FK, Mosaiab T, Masic V, Holt S, Hartley-Tassell L, McGuinness HY, Manik MK, Bosanac T, Landsberg MJ, Kerry PS, Mobli M, Hughes RO, Milbrandt J, Kobe B, DiAntonio A, and Ve T

Subjects
Animals, Enzyme Activation, HEK293 Cells, Humans, Mice, Mice, Knockout, Models, Molecular, Molecular Dynamics Simulation, Mutagenesis, Nicotinamide-Nucleotide Adenylyltransferase genetics, Protein Conformation, Armadillo Domain Proteins genetics, Armadillo Domain Proteins metabolism, Axons pathology, Cytoskeletal Proteins genetics, Cytoskeletal Proteins metabolism, NAD metabolism, Nerve Degeneration genetics, Nerve Degeneration pathology, Nicotinamide Mononucleotide metabolism
Abstract

Axon degeneration is a central pathological feature of many neurodegenerative diseases. Sterile alpha and Toll/interleukin-1 receptor motif-containing 1 (SARM1) is a nicotinamide adenine dinucleotide (NAD + )-cleaving enzyme whose activation triggers axon destruction. Loss of the biosynthetic enzyme NMNAT2, which converts nicotinamide mononucleotide (NMN) to NAD + , activates SARM1 via an unknown mechanism. Using structural, biochemical, biophysical, and cellular assays, we demonstrate that SARM1 is activated by an increase in the ratio of NMN to NAD + and show that both metabolites compete for binding to the auto-inhibitory N-terminal armadillo repeat (ARM) domain of SARM1. We report structures of the SARM1 ARM domain bound to NMN and of the homo-octameric SARM1 complex in the absence of ligands. We show that NMN influences the structure of SARM1 and demonstrate via mutagenesis that NMN binding is required for injury-induced SARM1 activation and axon destruction. Hence, SARM1 is a metabolic sensor responding to an increased NMN/NAD + ratio by cleaving residual NAD + , thereby inducing feedforward metabolic catastrophe and axonal demise., Competing Interests: Declaration of interests A.D. and J.M. are co-founders, scientific advisory board members, and shareholders of Disarm Therapeutics. B.K. is shareholder of Disarm Therapeutics. Y. Sasaki and B.K. are consultants to Disarm Therapeutics. B.K. and T.V. receive research funding from Disarm Therapeutics. R.O.H. and T.B. are employees and shareholders in Disarm Therapeutics. K.C. and P.S.K. are employees of Evotec (UK) Ltd. The authors declare no additional competing interests., (Copyright © 2021 Elsevier Inc. All rights reserved.)

Published
2021
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13. Rare Occurrence of Incidental Finding of Noninvasive Follicular Thyroid Neoplasm With Papillary-Like Nuclear Features in Hürthle Cell Adenoma.

Author

Pigac B, Masic S, Hutinec Z, and Masic V

Subjects
Adenoma, Oxyphilic surgery, Adult, Female, Humans, Incidental Findings, Rare Diseases, Thyroid Cancer, Papillary surgery, Thyroidectomy, Treatment Outcome, Adenoma, Oxyphilic pathology, Neck Pain pathology, Thyroid Cancer, Papillary pathology, Thyroid Gland pathology
Abstract

Introduction: Hürthle cell adenoma is a rare benign lesion of the thyroid gland, however, controversies about its potential malignant behavior still remain. Among thyroid neoplasms, papillary carcinoma is the most common variant with great variety of histological subtypes demonstrating different biological behavior., Aim: To raise the awareness of possible coexistence of these two lesions and discussion about possible therapeutic approaches., Case Report: A 42 year old female patient was examined because of the pain in the thyroid area. Cytological examination suggested Hürthle cell adenoma. Subsequently, right thyroid lobectomy was performed. Intraoperative frozen sections confirmed the diagnosis, yet final histological analysis revealed encapsulated follicular variant of papillary thyroid carcinoma (EFVPTC), now reclassified as noninvasive follicular thyroid neoplasm with papillary- like nuclear features (NIFTP) within the adenoma, which was not noticed through scintigraphy, ultrasound, cytological and frozen section analysis., Conclusions: Problems concerning both diagnostic and therapeutic approach to these lesions are being discussed, since opinions reported in the literature are divided, posing great challenge for the clinician in determining adequate therapeutic procedures.

Published
2018
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