R. Bossi scite author profile

MPS1 kinase is a key regulator of the spindle assembly checkpoint (SAC), a mitotic mechanism specifically required for proper chromosomal alignment and segregation. It has been found aberrantly overexpressed in a wide range of human tumors and is necessary for tumoral cell proliferation. Here we report the identification and characterization of NMS-P715, a selective and orally bioavailable MPS1 small-molecule inhibitor, which selectively reduces cancer cell proliferation, leaving normal cells almost unaffected. NMS-P715 accelerates mitosis and affects kinetochore components localization causing massive aneuploidy and cell death in a variety of tumoral cell lines and inhibits tumor growth in preclinical cancer models. Inhibiting the SAC could represent a promising new approach to selectively target cancer cells.

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Discovery of Entrectinib: A New 3-Aminoindazole As a Potent Anaplastic Lymphoma Kinase (ALK), c-ros Oncogene 1 Kinase (ROS1), and Pan-Tropomyosin Receptor Kinases (Pan-TRKs) inhibitor

Menichincheri

et al. 2016

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Anaplastic lymphoma kinase (ALK) is a receptor tyrosine kinase responsible for the development of different tumor types. Despite the remarkable clinical activity of crizotinib (Xalkori), the first ALK inhibitor approved in 2011, the emergence of resistance mutations and of brain metastases frequently causes relapse in patients. Within our ALK drug discovery program, we identified compound 1, a novel 3-aminoindazole active on ALK in biochemical and in cellular assays. Its optimization led to compound 2 (entrectinib), a potent orally available ALK inhibitor active on ALK-dependent cell lines, efficiently penetrant the blood-brain barrier (BBB) in different animal species and highly efficacious in in vivo xenograft models. Moreover, entrectinib resulted to be strictly potent on the closely related tyrosine kinases ROS1 and TRKs recently found constitutively activated in several tumor types. Entrectinib is currently undergoing phase I/II clinical trial for the treatment of patients affected by ALK-, ROS1-, and TRK-positive tumors.

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Crystal Structures of Anaplastic Lymphoma Kinase in Complex with ATP Competitive Inhibitors

et al. 2010

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Anaplastic lymphoma kinase (ALK) is a receptor tyrosine kinase involved in the development of several human cancers and, as a result, is a recognized target for the development of small-molecule inhibitors for the treatment of ALK-positive malignancies. Here, we present the crystal structures of the unphosphorylated human ALK kinase domain in complex with the ATP competitive ligands PHA-E429 and NVP-TAE684. Analysis of these structures provides valuable information concerning the specific characteristics of the ALK active site as well as giving indications about how to obtain selective ALK inhibitors. In addition, the ALK-KD-PHA-E429 structure led to the identification of a potential regulatory mechanism involving a link made between a short helical segment immediately following the DFG motif and an N-terminal two-stranded beta-sheet. Finally, mapping of the activating mutations associated with neuroblastoma onto our structures may explain the roles these residues have in the activation process.

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Cross-Talk and Ammonia Channeling between Active Centers in the Unexpected Domain Arrangement of Glutamate Synthase

et al. 2000

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The outstanding property of glutamate synthase is the ability to coordinate the activity of its various functional sites to avoid wasteful consumption of L-glutamine. The structure reveals two polypeptide segments that connect the catalytic centers and embed the ammonia tunnel, thus being ideally suited to function in interdomain signaling. Depending on the enzyme redox and ligation states, these signal-transducing elements may affect the active site geometry and control ammonia diffusion through a gating mechanism.

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Structural Studies on the Synchronization of Catalytic Centers in Glutamate Synthase

Heuvel¹,

Ferrari²,

Bossi³

et al. 2002

Journal of Biological Chemistry

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The complex iron-sulfur flavoprotein glutamate synthase (GltS) plays a prominent role in ammonia assimilation in bacteria, yeasts, and plants. GltS catalyzes the formation of two molecules of L-glutamate from 2-oxoglutarate and L-glutamine via intramolecular channeling of ammonia. GltS has the impressive ability of synchronizing its distinct catalytic centers to avoid wasteful consumption of L-glutamine. We have determined the crystal structure of the ferredoxin-dependent GltS in several ligation and redox states. The structures reveal the crucial elements in the synchronization between the glutaminase site and the 2-iminoglutarate reduction site. The structural data combined with the catalytic properties of GltS indicate that binding of ferredoxin and 2-oxoglutarate to the FMN-binding domain of GltS induce a conformational change in the loop connecting the two catalytic centers. The rearrangement induces a shift in the catalytic elements of the amidotransferase domain, such that it becomes activated. This machinery, over a distance of more than 30 Å, controls the ability of the enzyme to bind and hydrolyze the ammonia-donating substrate L-glutamine.Substrate channeling is the process of direct transfer of a reaction intermediate between enzyme-active sites that catalyze sequential reactions in a biosynthetic pathway (1). The active sites can either be located on separate subunits in a multienzyme complex or in separate domains in multifunctional enzymes. Direct transfer between the enzyme-active sites prevents loss of the intermediate into solution, limits the entrance of the intermediate into competing processes, protects labile intermediates from degradation in solution, and increases the success rate of the catalytic cycle by lowering the probability of uncoupled consecutive reactions (2, 3).Glutamine amidotransferases play a central role in cellular metabolism as they provide the main route for the incorporation of nitrogen into various biomolecules. These well studied enzymes catalyze two reactions at separate catalytic centers. L-Glutamine is hydrolyzed in the glutaminase site yielding ammonia, which is, in the subsequent synthase reaction, added to an acceptor substrate that varies among the different glutamine amidotransferases. Structural and functional studies have revealed that glutamine amidotransferases function through the channeling of ammonia from the glutaminase site to the synthase site (3, 4). In phosphoribosylpyrophosphate amidotransferase channel formation appeared to be dependent on the substrate binding to the synthase site (5), whereas in, for example, asparagine synthetase B, imidazoleglycerol-phosphate synthase, and glucosamine-6-phosphate synthase permanent channels were observed (6 -8).Glutamate synthase (GltS) 1 is a key enzyme in the early stages of the assimilation of ammonia in bacteria, yeasts, and plants. The enzyme is a complex iron-sulfur flavoprotein catalyzing the reductive transfer of the amido nitrogen from Lglutamine to 2-oxoglutarate to form two molecules of L-glutamate...

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Structure of FAD-Bound l-Aspartate Oxidase: Insight into Substrate Specificity and Catalysis^,

et al. 2002

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L-Aspartate oxidase (Laspo) catalyzes the conversion of L-Asp to iminoaspartate, the first step in the de novo biosynthesis of NAD(+). This bacterial pathway represents a potential drug target since it is absent in mammals. The Laspo R386L mutant was crystallized in the FAD-bound catalytically competent form and its three-dimensional structure determined at 2.5 A resolution in both the native state and in complex with succinate. Comparison of the R386L holoprotein with the wild-type apoenzyme [Mattevi, A., Tedeschi, G., Bacchella, L., Coda, A., Negri, A., and Ronchi, S. (1999) Structure 7, 745-756] reveals that cofactor incorporation leads to the ordering of two polypeptide segments (residues 44-53 and 104-141) and to a 27 degree rotation of the capping domain. This motion results in the formation of the active site cavity, located at the interface between the capping domain and the FAD-binding domain. The structure of the succinate complex indicates that the cavity surface is decorated by two clusters of H-bond donors that anchor the ligand carboxylates. Moreover, Glu121, which is strictly conserved among Laspo sequences, is positioned to interact with the L-Asp alpha-amino group. The architecture of the active site of the Laspo holoenzyme is remarkably similar to that of respiratory fumarate reductases, providing strong evidence for a common mechanism of catalysis in Laspo and flavoproteins of the succinate dehydrogenase/fumarate reductase family. This implies that Laspo is mechanistically distinct from other flavin-dependent amino acid oxidases, such as the prototypical D-amino acid oxidase.

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The TB structural genomics consortium: a resource for Mycobacterium tuberculosis biology

et al. 2003

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A Covalent Modification of NADP⁺ Revealed by the Atomic Resolution Structure of FprA, a Mycobacterium tuberculosis Oxidoreductase^,

et al. 2002

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FprA is a mycobacterial oxidoreductase that catalyzes the transfer of reducing equivalents from NADPH to a protein acceptor. We determined the atomic resolution structure of FprA in the oxidized (1.05 A resolution) and NADPH-reduced (1.25 A resolution) forms. The comparison of these FprA structures with that of bovine adrenodoxin reductase showed no significant overall differences. Hence, these enzymes, which belong to the structural family of the disulfide oxidoreductases, are structurally conserved in very distant organisms such as mycobacteria and mammals. Despite the conservation of the overall fold, the details of the active site of FprA show some peculiar features. In the oxidized enzyme complex, the bound NADP+ exhibits a covalent modification, which has been identified as an oxygen atom linked through a carbonylic bond to the reactive C4 atom of the nicotinamide ring. Mass spectrometry has confirmed this assignment. This NADP+ derivative is likely to form by oxidation of the NADP+ adduct resulting from nucleophilic attack by an active-site water molecule. A Glu-His pair is well positioned to activate the attacking water through a mechanism analogous to that of the catalytic triad in serine proteases. The NADP+ nicotinamide ring exhibits the unusual cis conformation, which may favor derivative formation. The physiological significance of this reaction is presently unknown. However, it could assist with drug-design studies in that the modified NADP+ could serve as a lead compound for the development of specific inhibitors.

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R. Bossi

Targeting the Mitotic Checkpoint for Cancer Therapy with NMS-P715, an Inhibitor of MPS1 Kinase

Discovery of Entrectinib: A New 3-Aminoindazole As a Potent Anaplastic Lymphoma Kinase (ALK), c-ros Oncogene 1 Kinase (ROS1), and Pan-Tropomyosin Receptor Kinases (Pan-TRKs) inhibitor

Crystal Structures of Anaplastic Lymphoma Kinase in Complex with ATP Competitive Inhibitors

Cross-Talk and Ammonia Channeling between Active Centers in the Unexpected Domain Arrangement of Glutamate Synthase

Structural Studies on the Synchronization of Catalytic Centers in Glutamate Synthase

Structure of FAD-Bound l-Aspartate Oxidase: Insight into Substrate Specificity and Catalysis^,

The TB structural genomics consortium: a resource for Mycobacterium tuberculosis biology

A Covalent Modification of NADP⁺ Revealed by the Atomic Resolution Structure of FprA, a Mycobacterium tuberculosis Oxidoreductase^,

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R. Bossi

Targeting the Mitotic Checkpoint for Cancer Therapy with NMS-P715, an Inhibitor of MPS1 Kinase

Discovery of Entrectinib: A New 3-Aminoindazole As a Potent Anaplastic Lymphoma Kinase (ALK), c-ros Oncogene 1 Kinase (ROS1), and Pan-Tropomyosin Receptor Kinases (Pan-TRKs) inhibitor

Crystal Structures of Anaplastic Lymphoma Kinase in Complex with ATP Competitive Inhibitors

Cross-Talk and Ammonia Channeling between Active Centers in the Unexpected Domain Arrangement of Glutamate Synthase

Structural Studies on the Synchronization of Catalytic Centers in Glutamate Synthase

Structure of FAD-Bound l-Aspartate Oxidase: Insight into Substrate Specificity and Catalysis,

The TB structural genomics consortium: a resource for Mycobacterium tuberculosis biology

A Covalent Modification of NADP+ Revealed by the Atomic Resolution Structure of FprA, a Mycobacterium tuberculosis Oxidoreductase,

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Product

Resources

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Structure of FAD-Bound l-Aspartate Oxidase: Insight into Substrate Specificity and Catalysis^,

A Covalent Modification of NADP⁺ Revealed by the Atomic Resolution Structure of FprA, a Mycobacterium tuberculosis Oxidoreductase^,