Molecular Determinants and Specificity of mRNA with Alternatively-Spliced UPF1 Isoforms, Influenced by an Insertion in the 'Regulatory Loop'

Monikaben Padariya; Robin Fahraeus; Ted Hupp; Umesh Kalathiya

doi:10.3390/ijms222312744

Molecular Determinants and Specificity of mRNA with Alternatively-Spliced UPF1 Isoforms, Influenced by an Insertion in the 'Regulatory Loop'

Int J Mol Sci. 2021 Nov 25;22(23):12744. doi: 10.3390/ijms222312744.

Authors

Monikaben Padariya¹, Robin Fahraeus^{1

2

3

4}, Ted Hupp^{1

5}, Umesh Kalathiya¹

Affiliations

¹ International Centre for Cancer Vaccine Science, University of Gdansk, ul. Kładki 24, 80-822 Gdansk, Poland.
² Inserm UMRS1131, Institut de Génétique Moléculaire, Université Paris 7, Hôpital St. Louis, F-75010 Paris, France.
³ Department of Medical Biosciences, Umeå University, Building 6M, 90185 Umeå, Sweden.
⁴ Regional Centre for Applied Molecular Oncology (RECAMO), Masaryk Memorial Cancer Institute, Zlutykopec 7, 65653 Brno, Czech Republic.
⁵ Institute of Genetics and Cancer, University of Edinburgh, Edinburgh EH4 2XR, UK.

Abstract

The nonsense-mediated mRNA decay (NMD) pathway rapidly detects and degrades mRNA containing premature termination codons (PTCs). UP-frameshift 1 (UPF1), the master regulator of the NMD process, has two alternatively-spliced isoforms; one carries 353-GNEDLVIIWLR-363 insertion in the 'regulatory loop (involved in mRNA binding)'. Such insertion can induce catalytic and/or ATPase activity, as determined experimentally; however, the kinetics and molecular level information are not fully understood. Herein, applying all-atom molecular dynamics, we probe the binding specificity of UPF1 with different GC- and AU-rich mRNA motifs and the influence of insertion to the viable control over UPF1 catalytic activity. Our results indicate two distinct conformations between 1B and RecA2 domains of UPF1: 'open (isoform_2; without insertion)' and 'closed (isoform_1; with insertion)'. These structural movements correspond to an important stacking pattern in mRNA motifs, i.e., absence of stack formation in mRNA, with UPF1 isoform_2 results in the 'open conformation'. Particularly, for UPF1 isoform_1, the increased distance between 1B and RecA2 domains has resulted in reducing the mRNA-UPF1 interactions. Lower fluctuating GC-rich mRNA motifs have better binding with UPF1, compared with AU-rich sequences. Except CCUGGGG, all other GC-rich motifs formed a 4-stack pattern with UPF1. High occupancy R363, D364, T627, and G862 residues were common binding GC-rich motifs, as were R363, N535, and T627 for the AU-rich motifs. The GC-rich motifs behave distinctly when bound to either of the isoforms; lower stability was observed with UPF1 isoform_2. The cancer-associated UPF1 variants (P533L/T and A839T) resulted in decreased protein-mRNA binding efficiency. Lack of mRNA stacking poses in the UPF1_P533T system significantly decreased UPF1-mRNA binding efficiency and increased distance between 1B-RecA2. These novel findings can serve to further inform NMD-associated mechanistic and kinetic studies.

Keywords: AU-rich; GC-rich; NMD; PTC; UPF1; alternatively spliced; degradation; isoform; mRNA; molecular dynamics; motifs; regulatory loop; stability.

MeSH terms

Alternative Splicing*
Gene Expression Regulation*
Humans
Nonsense Mediated mRNA Decay*
Phosphorylation
Protein Binding
Protein Isoforms
RNA Helicases / genetics
RNA Helicases / metabolism*
RNA, Messenger / genetics
RNA, Messenger / metabolism*
Trans-Activators / genetics
Trans-Activators / metabolism*

Substances

Protein Isoforms
RNA, Messenger
Trans-Activators
RNA Helicases
UPF1 protein, human

Grants and funding

2020/36/C/NZ2/00108/National Science Center