N-Terminal Fragments of Huntingtin Longer than Residue 170 form Visible Aggregates Independently to Polyglutamine Expansion

Article type: Research Article

Authors: Chen, Moore Z.^a | Mok, Sue-Ann^b | Ormsby, Angelique R.^a | Muchowski, Paul J.^c | Hatters, Danny M.^{a; *}

Affiliations: [a] Department of Biochemistry and Molecular Biology and Bio21 Molecular Science and Biotechnology Institute, The University of Melbourne, VIC, Australia | [b] Department of Neurology, University of California San Francisco, San Francisco, CA, USA | [c] KynuRex, 634 Los Palmos Drive, San Francisco, CA, USA

Correspondence: [*] Correspondence to: Danny M. Hatters, Department of Biochemistry and Molecular Biology and Bio21 Molecular Science and Biotechnology Institute, The University of Melbourne, VIC 3010, Australia. Tel.: +61 3 8344 2530; E-mail: [email protected].

Abstract: Background: A hallmark of Huntington’s disease is the progressive aggregation of full length and N-terminal fragments of polyglutamine (polyQ)-expanded Huntingtin (Htt) into intracellular inclusions. The production of N-terminal fragments appears important for enabling pathology and aggregation; and hence the direct expression of a variety of N-terminal fragments are commonly used to model HD in animal and cellular models. Objective: It remains unclear how the length of the N-terminal fragments relates to polyQ – mediated aggregation. We investigated the fundamental intracellular aggregation process of eight different-length N-terminal fragments of Htt in both short (25Q) and long polyQ (97Q). Methods: N-terminal fragments were fused to fluorescent proteins and transiently expressed in mammalian cell culture models. These included the classic exon 1 fragment (90 amino acids) and longer forms of 105, 117, 171, 513, 536, 552, and 586 amino acids based on wild-type Htt (of 23Q) sequence length nomenclature. Results: N-terminal fragments of less than 171 amino acids only formed inclusions in polyQ-expanded form. By contrast the longer fragments formed inclusions irrespective of Q-length, with Q-length playing a negligible role in extent of aggregation. The inclusions could be classified into 3 distinct morphological categories. One type (Type A) was universally associated with polyQ expansions whereas the other two types (Types B and C) formed independently of polyQ length expansion. Conclusions: PolyQ-expansion was only required for fragments of less than 171 amino acids to aggregate. Longer fragments aggregated predominately through a non-polyQ mechanism, involving at least one, and probably more distinct clustering mechanisms.

Keywords: Aggregation, inclusion, polyglutamine, live cell imaging, Huntington’s Disease, proteolytic fragments

DOI: 10.3233/JHD-160207

Journal: Journal of Huntington's Disease, vol. 6, no. 1, pp. 79-91, 2017