Allovalency revisited: An analysis of multisite phosphorylation and substrate rebinding

Locasale, Jason W.

doi:10.1063/1.2841124

Cited by 15 publications

(16 citation statements)

References 46 publications

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“…Low internal friction and fast chain reconfigurations are therefore expected for short-to-intermediate separations. In a kinetic model of ultrasensitive binding, fast reconfiguration dynamics provides more opportunities for unbound CPDs to (re)bind before pSic1 diffuses out of proximity of Cdc4 [20,21,23]. In the polyelectrostatic model, fast reconfiguration dynamics facilitates pSic1's dynamic interactions with Cdc4 through electrostatic averaging effects [22,25].…”

Section: Conformation-to-function Relationshipsmentioning

confidence: 99%

“…Different biophysical models have been proposed to explain the ultrasensitive dependence of the Sic1-Cdc4 interaction on the number of phosphorylated CPDs. A kinetic model argued that the probability of Sic1 rebinding before diffusive exit could exhibit an ultrasensitive dependence on the number of phosphorylated CPDs, dependent on the timescales of diffusion and chain dynamics [20,21]. A polyelectrostatic model suggested that long-range electrostatic interactions between the positively charged CPD binding pocket on Cdc4 and the constellation of unbound negatively charged phosphorylated CPDs on Sic1 could yield ultrasensitive binding [22,23].…”

Section: Introductionmentioning

confidence: 99%

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Integrating multiple experimental data to determine conformational ensembles of an intrinsically disordered protein

Gomes

Krzeminski

Namini

et al. 2020

Preprint

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Intrinsically disordered proteins (IDPs) have fluctuating heterogeneous conformations, which makes structural characterization challenging. Transient long-range interactions in IDPs are known to have important functional implications. Thus, in order to calculate reliable structural ensembles of IDPs, the data used in their calculation must capture these important structural features. We use integrative modelling to understand and implement conformational restraints imposed by the most common structural techniques for IDPs: NMR spectroscopy, small-angle X-ray scattering (SAXS), and single-molecule Förster Resonance Energy Transfer (smFRET). Using the disordered N-terminal region of the Sic1 protein as a test case, we find that only Paramagnetic Relaxation Enhancement (PRE) and smFRET measurements are able to unambiguously report on transient long-range interactions. It is precisely these features which lead to deviations from homopolymer statistics and divergent structural inferences in non-integrative sm-FRET and SAXS analysis. Furthermore, we find that the sequence-specific deviations from homopolymer statistics are consistent with biophysical models of Sic1 function that are mediated by phospho-sensitive binding to its partner Cdc4. To our knowledge, these are the first conformational ensembles for an IDP in physiological conditions that are simultaneously consistent with smFRET, SAXS, and NMR data.Our results stress the importance of integrating the global and local structural information provided by SAXS and Chemical Shifts, respectively, with information on specific inter-residue distances from PRE and smFRET. Our integrative modelling approach and quantitative polymer-physics-based characterization of the experimentally-restrained ensembles could be used to implement a rigorous taxonomy for the description and classification of IDPs as heteropolymers. Significance StatementIntrinsically disordered proteins (IDPs) exhibit highly dynamic and heterogeneous conformations, which impedes rigorous structural characterization and understanding of their biological functions. Sic1 regulates the yeast cell cycle through phospho-sensitive binding to its partner Cdc4 and is paradigmatic of IDPs that bind tightly without partial/transient folding. In this paper, we integrated new and existing structural data from nuclear magnetic resonance, small-angle X-ray scattering and single-molecule fluorescence to calculate conformational ensembles for Sic1 and its phosphorylated state, pSic1. Data mining of these ensembles reveal unique features distinguishing Sic1/pSic1 from homopolymer statistics, such as overall compactness and large end-to-end distance fluctuations. Integrating experiments probing disparate scales, computational modelling, and polymer physics provides new and valuable insights into the conformation-to-function relationships in IDPs.

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Section: Conformation-to-function Relationshipsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Integrating multiple experimental data to determine conformational ensembles of an intrinsically disordered protein

Gomes

Krzeminski

Namini

et al. 2020

Preprint

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“…1c. The concept was developed by Klein, Pawson and Tyers in 2003 [22] and discussed and elaborated by others [23, 29]. The identical binding sites on the ligand compete for a single binding site on the receptor and only one binding site on the ligand can bind at any given time [22], which is nicely exemplified by multiple phosphorylations on an IDP binding to and competing for the same site [30].…”

Section: Allovalencymentioning

confidence: 99%

“…Please note, that the allovalency model has been discussed and expanded beyond the present formulation by Locasale [29]. …”

Section: Allovalencymentioning

confidence: 99%

Behaviour of intrinsically disordered proteins in protein–protein complexes with an emphasis on fuzziness

Olsen

Teilum

Kragelund

2017

Cell. Mol. Life Sci.

111

103

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Intrinsically disordered proteins (IDPs) do not, by themselves, fold into a compact globular structure. They are extremely dynamic and flexible, and are typically involved in signalling and transduction of information through binding to other macromolecules. The reason for their existence may lie in their malleability, which enables them to bind several different partners with high specificity. In addition, their interactions with other macromolecules can be regulated by a variable amount of chemically diverse post-translational modifications. Four kinetically and energetically different types of complexes between an IDP and another macromolecule are reviewed: (1) simple two-state binding involving a single binding site, (2) avidity, (3) allovalency and (4) fuzzy binding; the last three involving more than one site. Finally, a qualitative definition of fuzzy binding is suggested, examples are provided, and its distinction to allovalency and avidity is highlighted and discussed.

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“…This feature is found in both natural and synthetic ADs and seems a general feature corresponding to function. We suggest that these clusters function to increase the effective affinity of the AD peptides for their coactivator targets using a mechanism similar to avidity or allovalency -whereby a receptor dynamically interacts with multiple binding sites on a single ligand, effectively inhibiting the dissociation of the two molecules (Locasale, 2008;Olsen et al, 2017). This mechanism fits nicely with the dynamic and fuzzy binding of acidic activators to Med15, and presumably other coactivator targets, as well as the finding that ADcoactivator binding is driven in part by a favorable entropy change Tuttle et al, 2018).…”

Section: Discussionmentioning

confidence: 99%

A high-throughput screen for transcription activation domains reveals their sequence characteristics and permits reliable prediction by deep learning

Erijman

Kozłowski

Sohrabi-Jahromi

et al. 2019

Preprint

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Transcription activation domains (ADs) are encoded by a wide range of seemingly unrelated amino acid sequences, making it difficult to recognize features that permit their dynamic behavior, fuzzy interactions and target specificity. We screened a large set of random 30-mer peptides for AD function and trained a deep neural network (ADpred) on the AD-positive and negative sequences. ADpred correctly identifies known ADs within protein sequences and accurately predicts the consequences of mutations. We show that functional ADs are (1) located within intrinsically disordered regions with biased amino acid composition, (2) contain clusters of hydrophobic residues near acidic side chains, (3) are enriched or depleted for particular dipeptide sequences, and (4) have higher helical propensity than surrounding regions. Taken together, our findings fit the model of "fuzzy" binding through hydrophobic protein-protein interfaces, where activator-coactivator binding takes place in a dynamic hydrophobic environment rather than through combinations of sequence-specific interactions.

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Allovalency revisited: An analysis of multisite phosphorylation and substrate rebinding

Cited by 15 publications

References 46 publications

Integrating multiple experimental data to determine conformational ensembles of an intrinsically disordered protein

Integrating multiple experimental data to determine conformational ensembles of an intrinsically disordered protein

Behaviour of intrinsically disordered proteins in protein–protein complexes with an emphasis on fuzziness

A high-throughput screen for transcription activation domains reveals their sequence characteristics and permits reliable prediction by deep learning

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