Architecture of the linker-scaffold in the nuclear pore

Petrovic, Stefan; Samanta, Dibyendu; Perriches, Thibaud; Bley, Christopher J.; Thierbach, Karsten; Brown, Bonnie; Nie, Si; Mobbs, George W.; Stevens, Taylor; Liu, X.; Tomaleri, Giovani Pinton; Schaus, Lucas; Hoelz, André

doi:10.1126/science.abm9798

Cited by 64 publications

(54 citation statements)

References 150 publications

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“…The need for better methods to determine dynamic and variable copy numbers of Nups reliably at the level of single protein complexes under physiological conditions is further highlighted by the fact that our live-cell-based approach resulted in copy number estimates that differ from estimates derived by other approaches for four out of the ten investigated Nups. The main methods used in the field, including quantitative mass spectrometry from cell populations 23 , fitting of single protein structures into highly averaged cryo-EM densities 33 , 34 , as well as calibrated imaging of fluorescently tagged knock-in proteins in single living cells as used in our study, currently all have limitations in this regard. For example, cryo-EM based averaging often selects ‘complete’ NPCs, to obtain a ‘fully occupied’ average NPC model, whereas live-cell imaging data average NPC stoichiometry from all pores in one cell and thus include pore-to-pore variability, which can result in lower estimates.…”

Section: Discussionmentioning

confidence: 99%

“…8 ). The pseudoatomic model of the native NPC structure 27 , 28 we imposed as the endpoint of the assembly pathway does not include the Y-complex-bound fraction of Nup205 or the Nup214-bound fraction of Nup62, and thus contains only 16 of the 40 copies of Nup205 33 , 34 and 32 of the 48 copies of Nup62 35 in the fully mature NPC. How the remaining 24 copies of Nup205 and 16 copies of Nup62 are assembled remains elusive.…”

Section: Integrative Modelling Of Postmitotic Assemblymentioning

confidence: 99%

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A quantitative map of nuclear pore assembly reveals two distinct mechanisms

Otsuka

Tempkin

Zhang

et al. 2023

Nature

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Understanding how the nuclear pore complex (NPC) is assembled is of fundamental importance to grasp the mechanisms behind its essential function and understand its role during the evolution of eukaryotes1–4. There are at least two NPC assembly pathways—one during the exit from mitosis and one during nuclear growth in interphase—but we currently lack a quantitative map of these events. Here we use fluorescence correlation spectroscopy calibrated live imaging of endogenously fluorescently tagged nucleoporins to map the changes in the composition and stoichiometry of seven major modules of the human NPC during its assembly in single dividing cells. This systematic quantitative map reveals that the two assembly pathways have distinct molecular mechanisms, in which the order of addition of two large structural components, the central ring complex and nuclear filaments are inverted. The dynamic stoichiometry data was integrated to create a spatiotemporal model of the NPC assembly pathway and predict the structures of postmitotic NPC assembly intermediates.

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Section: Discussionmentioning

confidence: 99%

Section: Integrative Modelling Of Postmitotic Assemblymentioning

confidence: 99%

A quantitative map of nuclear pore assembly reveals two distinct mechanisms

Otsuka

Tempkin

Zhang

et al. 2023

Nature

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“…The integrative structure of the yeast NPC can be sub-divided into the membrane ring, inner and outer rings, a cytoplasmic export platform, the nuclear basket and the disordered FG repeats that fill the pore. The integrative structure of the yeast NPC provided insights into underlying architectural principles, mechanisms of transport across the nuclear membrane, functional regulation, and assembly/disassembly processes and broadened our understanding of the evolutionary origins of NPCs (Akey et al 2022;Petrovic et al 2022;Bley et al 2022;Zimmerli et al 2021;Allegretti et al 2020;Mosalaganti et al 2018).…”

Section: Area Of Focus No 6: Pdb-dev Integrative Structures Largely R...mentioning

confidence: 99%

Electron microscopy holdings of the Protein Data Bank: the impact of the resolution revolution, new validation tools, and implications for the future

et al. 2022

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As a discipline, structural biology has been transformed by the three-dimensional electron microscopy (3DEM) “Resolution Revolution” made possible by convergence of robust cryo-preservation of vitrified biological materials, sample handling systems, and measurement stages operating a liquid nitrogen temperature, improvements in electron optics that preserve phase information at the atomic level, direct electron detectors (DEDs), high-speed computing with graphics processing units, and rapid advances in data acquisition and processing software. 3DEM structure information (atomic coordinates and related metadata) are archived in the open-access Protein Data Bank (PDB), which currently holds more than 11,000 3DEM structures of proteins and nucleic acids, and their complexes with one another and small-molecule ligands (~ 6% of the archive). Underlying experimental data (3DEM density maps and related metadata) are stored in the Electron Microscopy Data Bank (EMDB), which currently holds more than 21,000 3DEM density maps. After describing the history of the PDB and the Worldwide Protein Data Bank (wwPDB) partnership, which jointly manages both the PDB and EMDB archives, this review examines the origins of the resolution revolution and analyzes its impact on structural biology viewed through the lens of PDB holdings. Six areas of focus exemplifying the impact of 3DEM across the biosciences are discussed in detail (icosahedral viruses, ribosomes, integral membrane proteins, SARS-CoV-2 spike proteins, cryogenic electron tomography, and integrative structure determination combining 3DEM with complementary biophysical measurement techniques), followed by a review of 3DEM structure validation by the wwPDB that underscores the importance of community engagement.

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“…Each nuclear pore is composed of 500 to 1000 copies of nucleoporin protein as well as PA that accumulate at stalled nuclear pore complexes [ 115 ]. Recently, the architecture of the nuclear pore has been described at high resolution [ 116 , 117 ]. In T cells and cancer cells, serum starvation led to the specific production of saturated and monounsaturated 16 carbon atoms PA species by DGKα, suggesting that these molecular species of PA might have been produced in the nucleus in non-proliferative conditions [ 19 , 20 , 21 ].…”

Section: Membrane Morphology Changes During Cancer and T Cell Biologi...mentioning

confidence: 99%

DGKα, Bridging Membrane Shape Changes with Specific Molecular Species of DAG/PA: Implications in Cancer and Immunosurveillance

Bozelli

Epand

2022

Cancers

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Cancer immunotherapy has revolutionized the oncology field. Despite the success, new molecular targets are needed to increase the percentage of patients that benefits from this therapy. Diacylglycerol kinase α (DGKα) has gathered great attention as a potential molecular target in immunotherapy because of its role in cancer proliferation and immunosuppression. DGKα catalyzes the ATP-dependent phosphorylation of diacylglycerol (DAG) to produce phosphatidic acid (PA). Since both lipids are potent signaling messengers, DGKα acts as a switch between different signaling pathways. Its role in cancer and immunosuppression has long been ascribed to the regulation of DAG/PA levels. However, this paradigm has been challenged with the identification of DGKα substrate acyl chain specificity, which suggests its role in signaling could be specific to DAG/PA molecular species. In several biological processes where DGKα plays a role, large membrane morphological changes take place. DGKα substrate specificity depends on the shape of the membrane that the enzyme binds to. Hence, DGKα can act as a bridge between large membrane morphological changes and the regulation of specific molecular species of DAG/PA. Bearing in mind the potential therapeutic benefits of targeting DGKα, here, the role of DGKα in cancer and T cell biology with a focus on the modulation of its enzymatic properties by membrane shape is reviewed. The goal is to contribute to a global understanding of the molecular mechanisms governing DGKα biology. This will pave the way for future experimentation and, consequently, the design of better, more potent therapeutic strategies aiming at improving the health outcomes of cancer patients.

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Architecture of the linker-scaffold in the nuclear pore

Cited by 64 publications

References 150 publications

A quantitative map of nuclear pore assembly reveals two distinct mechanisms

A quantitative map of nuclear pore assembly reveals two distinct mechanisms

Electron microscopy holdings of the Protein Data Bank: the impact of the resolution revolution, new validation tools, and implications for the future

DGKα, Bridging Membrane Shape Changes with Specific Molecular Species of DAG/PA: Implications in Cancer and Immunosurveillance

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