An Intein-based Strategy for the Production of Tag-free Huntingtin Exon 1 Proteins Enables New Insights into the Polyglutamine Dependence of Httex1 Aggregation and Fibril Formation

Vieweg, Sophie; Ansaloni, Annalisa; Wang, Zhe Ming; Warner, John B.; Lashuel, Hilal A.

doi:10.1074/jbc.m116.713982

Cited by 31 publications

(54 citation statements)

References 62 publications

(71 reference statements)

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“…It is possible that addition of the fluorescent tag changes the biophysical properties of Htt ex1 oligomers, leading to formation of the toxic species similarly to what is observed with the addition of the FLAG tag at the amino terminus end of the protein . Indeed, recent in vitro data indicate that untagged Htt ex1 can behave differently than the tagged versions . In addition, we found the CFP‐tagged proteins produced a very weak fluorescent signal, especially for the soluble 25Q construct.…”

Section: Resultssupporting

confidence: 52%

“…42 Indeed, recent in vitro data indicate that untagged Htt ex1 can behave differently than the tagged versions. 45 In addition, we found the CFP-tagged proteins produced a very weak fluorescent signal, especially for the soluble 25Q construct. This signal is so low that it is on par or even below that emanating from red vacuolar pigment due to the ade2-1 mutation in the W303 strain 46 (Figure 1C).…”

Section: The Presence Of a Fp Tag Unmasks Expanded Htt Ex1 Toxicitymentioning

confidence: 86%

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Polyglutamine toxicity in yeast uncovers phenotypic variations between different fluorescent protein fusions

Jiang

Gregorio

Duennwald

et al. 2016

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The palette of fluorescent proteins (FPs) available for live-cell imaging contains proteins that strongly differ in their biophysical properties. FPs cannot be assumed to be equivalent and in certain cases could significantly perturb the behavior of fluorescent reporters. We employed Saccharomyces cerevisiae to comprehensively study the impact of FPs on the toxicity of polyglutamine (polyQ) expansion proteins associated with Huntington's disease. The toxicity of polyQ fusion constructs is highly dependent on the sequences flanking the polyQ repeats. Thus, they represent a powerful tool to study the impact of fluorescent fusion partners. We observed significant differences on polyQ aggregation and toxicity between commonly used FPs. We gener-

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Section: Resultssupporting

confidence: 52%

Section: The Presence Of a Fp Tag Unmasks Expanded Htt Ex1 Toxicitymentioning

confidence: 86%

Polyglutamine toxicity in yeast uncovers phenotypic variations between different fluorescent protein fusions

Jiang

Gregorio

Duennwald

et al. 2016

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“…Other studies suggest that the Nt17 interaction with the polyQ domain influences the structure of Httex1 in ways that favor the population of aggregation-prone conformational intermediates (17,24,25). Consistent with these studies, N-terminal Htt fragments lacking Nt17 show reduced aggregation rates compared with those containing Nt17 with similar polyQ repeat lengths (19,26). In addition to its role in Htt aggregation, this domain has been implicated in the regulation of full-length protein-protein interactions (21,(27)(28)(29)(30), subcellular localization (10), and toxicity (31).…”

Section: Introductionsupporting

confidence: 55%

N-terminal phosphorylation of Huntingtin: A molecular switch for regulating Htt aggregation, helical conformation, internalization and nuclear targeting

Fares

et al. 2018

Preprint

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Phosphorylation of exon1 of the Huntingtin protein (Httex1) has been shown to play important roles in regulating the structure, toxicity and cellular properties of N-terminal fragments and the full-length Huntingtin protein. Here, we investigated and compared the effect of bona fide phosphorylation at S13 and/or S16 on the structure, aggregation, membrane binding, and subcellular properties of mutant Httex1-Q18A. We show that serine phosphorylation at either S13 or S16 strongly disrupts the amphipathic α-helix of the N-terminus, inhibits the aggregation of mutant Httex1 and prompts the internalization and nuclear targeting of Httex1 preformed aggregates. In synthetic peptides phosphorylation at S13 and/or S16 strongly disrupted the amphipathic α-helix of the N-terminal 17 residues (Nt17) of Httex1 and Nt17 membrane binding. Our studies on peptides bearing a different combination of phosphorylation sites within Nt17 revealed a novel phosphorylation-dependent switch for regulating the structure of Httex1 involving crosstalk between phosphorylation at T3 and S13 or S16. Together, our results provide novel insights into the role of phosphorylation in regulating Httex1 structure and function in health and disease and underscore the critical importance of identifying enzymes responsible for regulating Htt phosphorylation and their potential as therapeutic targets for the treatment of Huntington's disease.

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“…The resulting HTT open reading frames encoded within this series of constructs have either an Nterminal FLAG-octapeptide between the START methionine and the N-terminal methionine of the HTT amino acid sequence, or have the FLAGoctapeptide linked to the extreme C-terminus of HTT via a Gly-Gly-Ser-Gly linker ( Figure 1C). As subtle changes to the exon 1 amino acid sequence of the HTT protein have been shown to give rise to changes to biophysical properties of the protein (21,22), the C-terminally FLAG-tagged constructs allow expression of a "clean" exon 1 sequence.…”

Section: Cloning Of Htt Expression Constructsmentioning

confidence: 99%

Design and characterisation of mutant and wild-type huntingtin proteins produced from a toolkit of scalable eukaryotic expression systems

Harding

Loppnau

Ackloo

et al. 2018

Preprint

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The gene mutated in Huntington's disease (HD) patients encodes the 348 kDa huntingtin (HTT) protein. The pathogenic HD CAG-expansion mutation causes a polyglutamine (polyQ) tract at the N-terminus of the HTT protein to expand above a critical threshold of ~35 glutamine residues. The effect of HD mutations on HTT is not well understood, in part due to difficulties in carrying out biochemical, biophysical and structural studies of this large protein. To facilitate such studies, we have generated expression constructs for the scalable production of HTT in multiple eukaryotic expression systems. Our set of HTT expression clones comprises both N and C-terminally FLAGtagged HTT constructs with polyQ lengths representative of the general population, HD patients, juvenile HD patients as well as the more extreme polyQ expansions used in some HD tissue and animal models. These reagents yield milligram quantities of pure recombinant HTT protein, including many of the previously mapped posttranslational modifications. We have characterised both apo and HTT-HAP40 complex samples produced using this HD resource, demonstrating that this toolkit can be used to generate physiologically meaningful complexes of HTT. We demonstrate how these resources can produce sufficient material for protein-intensive experiments such as small angle X-ray scattering (SAXS), providing biochemical insight into HTT protein structure. The work outlined in this manuscript and the tools generated, lay a foundation for further biochemical and structural A toolkit of HTT protein resources 2 work on the HTT protein and its functional interactions with other biomolecules.

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An Intein-based Strategy for the Production of Tag-free Huntingtin Exon 1 Proteins Enables New Insights into the Polyglutamine Dependence of Httex1 Aggregation and Fibril Formation

Cited by 31 publications

References 62 publications

Polyglutamine toxicity in yeast uncovers phenotypic variations between different fluorescent protein fusions

Polyglutamine toxicity in yeast uncovers phenotypic variations between different fluorescent protein fusions

N-terminal phosphorylation of Huntingtin: A molecular switch for regulating Htt aggregation, helical conformation, internalization and nuclear targeting

Design and characterisation of mutant and wild-type huntingtin proteins produced from a toolkit of scalable eukaryotic expression systems

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