Biophysical Characterization of Interactions Involving Importin-α during Nuclear Import

Catimel, Bruno; Teh, Trazel; Fontes, Marcos R.M.; Jennings, Ian G.; Jans, David A.; Howlett, Geoffrey J.; Nice, Edouard C.; Kobe, Boštjan

doi:10.1074/jbc.m103531200

Cited by 144 publications

(159 citation statements)

References 52 publications

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“…Generation of Mutant Importin ␣ Proteins-Previous structural and in vitro analyses identified an auto-inhibitory sequence within the N-terminal IBB domain of importin ␣ (23,24,26). The structural studies suggested that this auto-inhibitory domain interacts with the NLS binding pocket by mimicking an NLS sequence (23,24).…”

Section: Resultsmentioning

confidence: 99%

“…In support of this hypothesis, in vitro binding studies have shown that importin ␣ lacking the proposed auto-inhibitory domain (⌬IBB-␣), binds more tightly to NLS-cargo than full-length importin ␣ (26), and that this auto-inhibition of full-length importin ␣ binding to NLS-cargo is relieved in the presence of importin ␤ (17,26). Further analysis of the N-terminal IBB domain of importin ␣ revealed a proposed internal NLS that could serve as an autoinhibitory sequence to regulate NLS binding through intramolecular competition for the NLS binding site (23,24). Taken together, these studies suggest a dual role for the N-terminal domain of importin ␣ in 1) binding to importin ␤ and 2) autoinhibition of NLS-cargo binding.…”

mentioning

confidence: 99%

“…The convergence of data from structural analyses and in vitro binding studies provides insight into how importin ␣ binds to and regulates interactions with NLS-cargo (17,(23)(24)(25)(26). Domain analysis has shown that importin ␣ has an N-terminal domain that binds importin ␤ (the importin ␤ binding domain or IBB), a central armadillo domain that constitutes the NLS binding pocket, and a C-terminal region that appears to be important for binding to its export receptor Cse1p/CAS (21,27).…”

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confidence: 99%

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The Auto-inhibitory Function of Importin α Is Essentialin Vivo

Harreman

Hodel²,

Fanara³

et al. 2003

Journal of Biological Chemistry

104

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Proteins that contain a classical nuclear localization signal (NLS) are recognized in the cytoplasm by a heterodimeric import receptor composed of importin/ karyopherin ␣ and ␤. The importin ␣ subunit recognizes classical NLS sequences, and the importin ␤ subunit directs the complex to the nuclear pore. Recent work shows that the N-terminal importin ␤ binding (IBB) domain of importin ␣ regulates NLS-cargo binding in the absence of importin ␤ in vitro. To analyze the in vivo functions of the IBB domain, we created a series of mutants in the Saccharomyces cerevisiae importin ␣ protein. These mutants dissect the two functions of the N-terminal IBB domain, importin ␤ binding and autoinhibition. One of these importin ␣ mutations, A3, decreases auto-inhibitory function without impacting binding to importin ␤ or the importin ␣ export receptor, Cse1p. We used this mutant to show that the auto-inhibitory function is essential in vivo and to provide evidence that this auto-inhibitory-defective importin ␣ remains bound to NLS-cargo within the nucleus. We propose a model where the auto-inhibitory activity of importin ␣ is required for NLS-cargo release and the subsequent Cse1p-dependent recycling of importin ␣ to the cytoplasm.In eukaryotes, the nuclear envelope provides an essential barrier that separates the nuclear genome from the intermediary metabolism, signaling systems, and translation machinery of the cytoplasm. Selective bi-directional transport of macromolecules across this nuclear envelope regulates critical cellular processes such as gene expression (1, 2). All nucleocytoplasmic transport of macromolecules occurs through large proteinaceous structures, called nuclear pore complexes (NPC), 1 that perforate the nuclear envelope (3, 4). These macromolecular cargoes are specifically targeted to and transported through NPCs by a family of soluble nuclear transport receptors (5, 6).The small GTPase, Ran, governs the interactions between the nuclear transport receptors and macromolecular cargoes (5, 7). Import receptors bind cargo in the absence of RanGTP, whereas export receptors bind cargo in a trimeric complex with RanGTP (5,8). This mode of regulation requires an asymmetric distribution of RanGTP, with more RanGTP in the nucleus than in the cytoplasm. To achieve this asymmetry, the Ran regulatory proteins are compartmentalized with the GTPase activating protein (RanGAP), which generates RanGDP, in the cytoplasm (9) and the guanine nucleotide exchange factor (RCC1), which generates RanGTP, in the nucleus (10).The best-characterized nuclear import process occurs via receptor recognition of a classical nuclear localization signal (NLS). This classical NLS is typified by a cluster of basic amino acids (monopartite) or two clusters of basic amino acids separated by a 10 -12 amino acid linker (bipartite) (11, 12). A heterodimeric import receptor, composed of importins ␣ and ␤ (also known as karyopherin ␣ and ␤), mediates the nuclear import of proteins that contain a classical NLS (13-15). Over the last several years many...

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Section: Resultsmentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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The Auto-inhibitory Function of Importin α Is Essentialin Vivo

Harreman

Hodel²,

Fanara³

et al. 2003

Journal of Biological Chemistry

104

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“…The strongest affinities of natural ArmRPs were reported to be in the range of 20 nM for importin-α binding to NLS peptides [27,28]. From an initial version of a consensus ArmRP library, a binder to neurotensin was selected with a K d of 7 µM [29], but the binding mode was different from the intended canonical binding [30].…”

Section: Surface Redesign For Peptide Bindingmentioning

confidence: 99%

Computationally Designed Armadillo Repeat Proteins for Modular Peptide Recognition

Reichen

Hansen

Forzani

et al. 2016

Journal of Molecular Biology

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Armadillo repeat proteins (ArmRP) recognize their target peptide in extended conformation and bind, in a first approximation, two residues per repeat. They may thus form the basis for building a modular system, in which each repeat is complementary to a piece of the target peptide. Accordingly, preselected repeats could be assembled into specific binding proteins on demand and thereby avoid the traditional generation of every new binding molecule by an independent selection from a library.Stacked armadillo repeats, each consisting of 42 amino acids arranged in three α-helices, build an elongated superhelical structure. Here, we analyzed curvature variations in natural ArmRPs, and identified a repeat pair from yeast importin-α as having the optimal curvature geometry to be complementary to a peptide over its whole length. We employed a symmetric in silico design to obtain a uniform sequence for a stackable repeat while maintaining the desired curvature geometry.Computationally designed armadillo repeat proteins (dArmRPs) had to be stabilized by mutations to remove regions of higher flexibility, which were identified by molecular dynamics (MD) simulations in explicit solvent. Using an N-capping repeat from the consensus-design approach, two different crystal structures of dArmRP were determined. Although the experimental structures of dArmRP deviated from the designed curvature, the insertion of the most conserved binding pockets of natural ArmRPs onto the surface of dArmRPs resulted in binders against the expected peptide with low nanomolar affinities, similar to the binders from the consensus-design series.

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“…Fluorescent cargo concentrations were ≥ 100 nM in ensemble (bulk) experiments, and ∼100 pM for single molecule transport assays. At these cargo and cofactor concentrations, >99% of the cargo was expected to be complexed with importin-α and importin-β [33].…”

Section: Transport Cofactors and Ensemble Transport Experimentsmentioning

confidence: 99%

Visualizing single molecules interacting with nuclear pore complexes by narrow-field epifluorescence microscopy

Yang

Musser

2006

Methods

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The utility of single molecule fluorescence (SMF) for understanding biological reactions has been amply demonstrated by a diverse series of studies over the last decade. In large part, the molecules of interest have been limited to those within a small focal volume or near a surface to achieve the high sensitivity required for detecting the inherently weak signals arising from individual molecules. Consequently, the investigation of molecular behavior with high time and spatial resolution deep within cells using SMF has remained challenging. Recently, we demonstrated that narrow-field epifluorescence microscopy allows visualization of nucleocytoplasmic transport at the single cargo level. We describe here the methodological approach that yields 2 ms and ∼15 nm resolution for a stationary particle. The spatial resolution for a mobile particle is inherently worse, and depends on how fast the particle is moving. The signal-to-noise ratio is sufficiently high to directly measure the time a single cargo molecule spends interacting with the nuclear pore complex. Particle tracking analysis revealed that cargo molecules randomly diffuse within the nuclear pore complex, exiting as a result of a single rate-limiting step. We expect that narrow-field epifluorescence microscopy will be useful for elucidating other binding and trafficking events within cells.

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Biophysical Characterization of Interactions Involving Importin-α during Nuclear Import

Cited by 144 publications

References 52 publications

The Auto-inhibitory Function of Importin α Is Essentialin Vivo

The Auto-inhibitory Function of Importin α Is Essentialin Vivo

Computationally Designed Armadillo Repeat Proteins for Modular Peptide Recognition

Visualizing single molecules interacting with nuclear pore complexes by narrow-field epifluorescence microscopy

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