A complete compendium of crystal structures for the human SEPT3 subgroup reveals functional plasticity at a specific septin interface

Danielle Karoline Silva do Vale Castro; Sabrina Matos de Oliveira da Silva; Humberto D'Muniz Pereira; Joci Neuby Alves Macedo; Diego Antonio Leonardo; Napoleão Fonseca Valadares; Patricia Suemy Kumagai; José Brandão-Neto; Ana Paula Ulian Araújo; Richard Charles Garratt

doi:10.1107/S2052252520002973

A complete compendium of crystal structures for the human SEPT3 subgroup reveals functional plasticity at a specific septin interface

IUCrJ. 2020 Mar 28;7(Pt 3):462-479. doi: 10.1107/S2052252520002973. eCollection 2020 May 1.

Affiliations

¹ Instituto de Física de São Carlos, Universidade de São Paulo, Avenida Joao Dagnone 1100, São Carlos-SP 13563-723, Brazil.
² Instituto de Química de São Carlos, Universidade de São Paulo, Avenida Trabalhador São-carlense 400, São Carlos-SP 13566-590, Brazil.
³ Federal Institute of Education, Science and Technology of Rondonia, Rodovia BR-174, Km 3, Vilhena-RO 76980-000, Brazil.
⁴ Departamento de Biologia Celular, Universidade de Brasília, Instituto de Ciências Biológicas, Brasília-DF 70910900, Brazil.
⁵ Diamond Light Source, Diamond House, Harwell Science and Innovation Campus, Didcot OX11 0DE, United Kingdom.

Abstract

Human septins 3, 9 and 12 are the only members of a specific subgroup of septins that display several unusual features, including the absence of a C-terminal coiled coil. This particular subgroup (the SEPT3 septins) are present in rod-like octameric protofilaments but are lacking in similar hexameric assemblies, which only contain representatives of the three remaining subgroups. Both hexamers and octamers can self-assemble into mixed filaments by end-to-end association, implying that the SEPT3 septins may facilitate polymerization but not necessarily function. These filaments frequently associate into higher order complexes which associate with biological membranes, triggering a wide range of cellular events. In the present work, a complete compendium of crystal structures for the GTP-binding domains of all of the SEPT3 subgroup members when bound to either GDP or to a GTP analogue is provided. The structures reveal a unique degree of plasticity at one of the filamentous interfaces (dubbed NC). Specifically, structures of the GDP and GTPγS complexes of SEPT9 reveal a squeezing mechanism at the NC interface which would expel a polybasic region from its binding site and render it free to interact with negatively charged membranes. On the other hand, a polyacidic region associated with helix α5', the orientation of which is particular to this subgroup, provides a safe haven for the polybasic region when retracted within the interface. Together, these results suggest a mechanism which couples GTP binding and hydrolysis to membrane association and implies a unique role for the SEPT3 subgroup in this process. These observations can be accounted for by constellations of specific amino-acid residues that are found only in this subgroup and by the absence of the C-terminal coiled coil. Such conclusions can only be reached owing to the completeness of the structural studies presented here.

Keywords: GTP binding/hydrolysis; X-ray crystallography; filaments; protein structure; septins.

Grants and funding

This work was funded by Fundação de Amparo à Pesquisa do Estado de São Paulo grants 2014/15546-1, 2012/00268-0, 2010/20290-5, 2008/58316-5, 2008/58316-5, 2016/19734-2, and 2017/07709-6 .