A conserved structural element in the RNA helicase UPF1 regulates its catalytic 
activity in an isoform-specific manner

Gowravaram, Manjeera; Bonneau, Fabien; Kanaan, Joanne; Maciej, Vincent D.; Fiorini, Francesca; Raj, Saurabh; Croquette, Vincent; Le Hir, Herve; Chakrabarti, Sutapa

doi:10.1093/nar/gky040

Item

ITEM ACTIONSEXPORT

Add to Basket

Local TagsRelease HistoryDetailsSummary

Released

Journal Article

A conserved structural element in the RNA helicase UPF1 regulates its catalytic activity in an isoform-specific manner

MPS-Authors

/persons/resource/persons77784

Bonneau, Fabien
Conti, Elena / Structural Cell Biology, Max Planck Institute of Biochemistry, Max Planck Society;

External Resource

https://academic.oup.com/nar/article-lookup/doi/10.1093/nar/gky040#supplementary-data
(Supplementary material)

Fulltext (restricted access)

There are currently no full texts shared for your IP range.

Fulltext (public)

gky040.pdf
(Publisher version), 6MB

Supplementary Material (public)

There is no public supplementary material available

Citation

Gowravaram, M., Bonneau, F., Kanaan, J., Maciej, V. D., Fiorini, F., Raj, S., et al. (2018). A conserved structural element in the RNA helicase UPF1 regulates its catalytic activity in an isoform-specific manner. Nucleic Acids Research (London), 46(5), 2648-2659. doi:10.1093/nar/gky040.

Cite as: https://hdl.handle.net/21.11116/0000-0002-797E-A

Abstract

The RNA helicase UPF1 is a key component of the nonsense mediated mRNA decay (NMD) pathway. Previous X-ray crystal structures of UPF1 elucidated the molecular mechanisms of its catalytic activity and regulation. In this study, we examine features of the UPF1 core and identify a structural element that adopts different conformations in the various nucleotide- and RNA-bound states of UPF1. We demonstrate, using biochemical and singlemolecule assays, that this structural element modulates UPF1 catalytic activity and thereby refer to it as the regulatory loop. Interestingly, there are two alternatively spliced isoforms of UPF1 in mammals which differ only in the lengths of their regulatory loops. The loop in isoform 1 (UPF11) is 11 residues longer than that of isoform 2. We find that this small insertion in UPF11 leads to a two-fold increase in its translocation and ATPase activities. To determine the mechanistic basis of this differential catalytic activity, we have determined the X-ray crystal structure of the helicase core of UPF11 in its apo-state. Our results point toward a novel mechanism of regulation of RNA helicases, wherein alternative splicing leads to subtle structural rearrangements within the protein that are critical to modulate enzyme movements and catalytic activity.