New one-pot synthesis of N-fused isoquinoline derivatives by palladium-catalyzed C–H arylation: potent inhibitors of nucleotide pyrophosphatase-1 and -3

Ausekle, Elina; Ejaz, Syeda Abida; Khan, Shafi Ullah; Ehlers, Peter; Villinger, Alexander; Lecka, Joanna; Sévigny, Jean; Iqbal, Jamshed; Langer, Peter

doi:10.1039/c6ob02236g

Cited by 43 publications

(40 citation statements)

References 71 publications

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“…7). 91 However, selectivity data vs. other ecto-nucleotidases have not been provided. The SAR studies showed that two methoxy groups at the 2-and 3-positions of the isoquinoline scaffold are important for the inhibitory activity.…”

Section: Non-nucleotide-based Npp1 Inhibitorsmentioning

confidence: 99%

Nucleotide pyrophosphatase/phosphodiesterase 1 (NPP1) and its inhibitors

Lee

Müller

2017

Med. Chem. Commun.

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Ecto-nucleotide pyrophosphatase/phosphodiesterase 1 (NPP1, EC 3.1.4.1) is a metalloenzyme that belongs to the NPP family, which comprises seven subtypes (NPP1-7). NPP1 hydrolyzes a wide range of phosphodiester bonds, in nucleoside triphosphates, (cyclic) dinucleotides, and nucleotide sugars yielding nucleoside 5'-monophosphates as products. Its main substrate is ATP which is cleaved to AMP and diphosphate. The enzyme is involved in various biological processes including bone mineralization, soft-tissue calcification, insulin receptor signalling, cancer cell proliferation and immune modulation. Therefore, NPP1 inhibitors have potential as novel drugs, for (immuno)oncology. In the last two decades several inhibitors of NPP1 derived from nucleotide- or non-nucleotide scaffolds have been developed. The most potent and selective NPP1-inhibitory substrate analog is adenosine 5'-α,β-methylene-γ-thiotriphosphate ( = 20 nM -Nph-5'-TMP, human membrane-bound NPP1). Non-nucleotide-derived NPP1 inhibitors comprise polysulfonates, polysaccharides, polyoxometalates and small heterocyclic compounds. The polyoxometalate [TiWCoO] (PSB-POM141) is the most potent and selective NPP1 inhibitor described to date ( = 1.46 nM ATP, human soluble NPP1); it displays an allosteric mechanism of inhibition and represents a useful pharmacological tool for evaluating the potential of NPP1 as a novel drug target.

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Section: Non-nucleotide-based Npp1 Inhibitorsmentioning

confidence: 99%

Nucleotide pyrophosphatase/phosphodiesterase 1 (NPP1) and its inhibitors

Lee

Müller

2017

Med. Chem. Commun.

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“…In order to investigate the putative binding mode of the selective inhibitors in the homology models of human TNAP, human IAP, human NPP1 and human NPP3, docking studies were carried out. The crystal structure of any of the proteins was not available at the protein databank, therefore, homology models were prepared by our research group . Since these homology modelled structures do not contain any co‐crystallized ligand in their active sites, the site finder of MOE program was used for selection of binding site before molecular docking studies.…”

Section: Resultsmentioning

confidence: 99%

“…Cell Transfection and Preparation of Membrane Fractions: The process of cell transfection was carried out initially by transfecting human alkaline phosphatase ( h ‐TNAP & h ‐IAP) expressing plasmids or human nucleotide pyrophosphatase/phosphodiesterase ( h ‐NPP1 & h ‐NPP3), expressing plasmids into the COS‐7 cells, respectively, in 10‐cm plates using Lipofectamine. In the next step, the cells were transferred to Dulbecco's modified Eagle's medium (DMEM) containing 6 µg of plasmid DNA and 24 µL of Lipofectamine reagent.…”

Section: Methodsmentioning

confidence: 99%

“…Selection of Protein Structure: Ligand‐bound crystallographic structures of h ‐TNAP, h ‐IAP, h ‐NPP1 and h ‐NPP3 are not available in the Protein Data Bank (PDB) so in this study, recently reported homology models from our group were used for docking . The site finder of MOE software was used for selections of binding site before carrying out docking studies, as catalytic zinc ions were important in respect of interactions within the active site .…”

Section: Methodsmentioning

confidence: 99%

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Deazapurine Analogues Bearing a 1H‐Pyrazolo[3,4‐b]pyridin‐3(2H)‐one Core: Synthesis and Biological Activity

et al. 2018

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A new methodology for the synthesis of fluorinated and non‐fluorinated 1H‐pyrazolo[3,4‐b]pyridin‐3‐ones was developed. The reactions proceed by cyclization of electron‐rich 3‐amino‐1H‐pyrazol‐5(4H)‐ones with 1,3‐diketones and the products were obtained in good to excellent yields and with excellent regioselectivity. The products, which can be regarded as deazapurine analogues, were tested for the alkaline phosphatase (h‐TNAP and h‐IAP) and nucleotide pyrophosphatase/phosphodiesterase (h‐NPP1 and h‐NPP3) inhibition profile. Most of the derivatives exhibited selective and potent inhibition on tissue non‐specific and intestinal alkaline phosphatase and nucleotide pyrophosphatase (NPP1 and NPP3) enzymes. Possible binding modes of the most potent inhibitors were studied by molecular docking analysis.

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“…Despite these multiple possible roles, the biochemistry of NPP3 has not been extensively characterized, and the determinants of its substrate specificity are unknown. The 3D structures of all the other mammalian NPPs have been elucidated [11,[22][23][24][25][26][27][28], whereas NPP3 has been the subject of modeling studies to assist isozyme-specific inhibitor design [29][30][31]. Here, we report the crystal structure of human NPP3 as well as its complex with a substrate analog, and explore the dimerization properties of this enzyme.…”

Section: Introductionmentioning

confidence: 99%