| 2001 |
Human UPF3A (hUpf3p) was identified as a human orthologue of S. cerevisiae Upf3p; co-immunoprecipitation of epitope-tagged proteins in HeLa cells demonstrated that hUpf2p interacts with both hUpf3p-X (UPF3B) and hUpf3p (UPF3A), and the domains required for these interactions were defined. UPF3A localizes primarily to nuclei and is a shuttling protein, indicating NMD has both nuclear and cytoplasmic components. |
Co-immunoprecipitation of epitope-tagged proteins in HeLa cells; indirect immunofluorescence for subcellular localization |
Molecular and cellular biology |
Medium |
11113196
|
| 2004 |
Crystal structure at 1.95 Å of the complex between the interacting domains of human UPF2 (MIF4G domain) and UPF3B (RNP domain) revealed that the protein-protein interface is mediated by highly conserved charged residues and involves the beta-sheet surface of the UPF3B RNP domain. The UPF3b RNP domain does not bind RNA, whereas the UPF2 construct and the complex do. The same RNP domain architecture is shared by UPF3A. |
X-ray crystallography (1.95 Å resolution); RNA-binding assays |
Nature structural & molecular biology |
High |
15004547
|
| 2006 |
Using a tethering system, UPF3A was shown to be much less active than UPF3B in inducing NMD and stimulating translation. The C-terminal domain region that discriminates UPF3A from UPF3B in NMD function mediates interaction with EJC components Y14, Magoh, BTZ, and eIF4AIII; this interaction is required for NMD induction. Translation stimulation is independent of EJC interaction and is determined by other regions of the UPF3 proteins. |
lambdaN/boxB tethering reporter assay; co-immunoprecipitation for EJC interaction mapping |
RNA (New York, N.Y.) |
Medium |
16601204
|
| 2007 |
Recombinant EJC core was sufficient to reconstitute a stable heptameric complex on RNA with UPF1, UPF2, and UPF3b. EJC proteins MAGOH, Y14, and eIF4AIII provide a composite binding site for UPF3b that bridges to UPF2 and UPF1. In the trimeric UPF complex, UPF2 and UPF3b cooperatively stimulate both ATPase and RNA helicase activities of UPF1. |
In vitro reconstitution; ATPase assay; RNA helicase assay with recombinant proteins |
Nature structural & molecular biology |
High |
18066079
|
| 2009 |
UPF3A protein levels are regulated post-transcriptionally: the presence of UPF3B promotes destabilization/reduction of UPF3A levels via a conserved UPF3B-dependent mechanism. When UPF3B is absent (e.g., due to mutations), UPF3A levels rise and partially compensate for NMD, but UPF3A also impairs NMD by competing with UPF3B for binding to UPF2. This UPF3B-dependent destabilization of UPF3A constitutes a post-transcriptional regulatory switch maintaining appropriate NMD levels. |
Western blotting of UPF3A/UPF3B levels in cells with UPF3B mutations; competitive binding assays; NMD reporter assays |
Nature structural & molecular biology |
High |
19503078
|
| 2016 |
UPF3A acts primarily as a potent NMD inhibitor, stabilizing hundreds of transcripts, rather than an NMD activator. It acquired repressor activity through impairment of a critical domain (C-terminal EJC-binding domain is weakened relative to UPF3B). Conditional knockout of UPF3A in mice causes 'hyper' NMD and leads to defects in embryogenesis and gametogenesis. UPF3A competes with UPF3B for binding to UPF2, and its NMD-inhibitory function is explained by its weaker NMD activation capacity displacing the stronger activator UPF3B. |
Loss-of-function in vitro (siRNA/shRNA) and in vivo (conditional knockout mouse); RNA-seq; NMD reporter assays; co-immunoprecipitation |
Cell |
High |
27040500
|
| 2019 |
In zebrafish, Upf3a (a NMD pathway member) and components of the COMPASS complex including Wdr5 are required for the genetic compensation response (GCR) triggered by mRNAs bearing a premature termination codon (PTC). The GCR is accompanied by enhancement of H3K4me3 at the transcription start site regions of compensatory genes, linking Upf3a to transcriptional upregulation of homologous genes in response to PTC-containing mRNA. |
Zebrafish knockdown vs. knockout models; transgene analysis; ChIP for H3K4me3; genetic epistasis using upf3a mutants |
Nature |
High |
30944473
|
| 2020 |
Reconstituted UPF3A expression in KM12 CRC cells (which have a frameshift mutation in UPF3A) caused down-regulation of several enzymes involved in cholesterol biosynthesis and altered phosphorylation of 85 phosphosites in 52 phosphoproteins, predominantly nuclear proteins involved in gene expression regulation and RNA splicing, suggesting UPF3A influences cellular signaling pathways beyond NMD. |
SILAC-based quantitative proteomics; phosphoproteomics in CRC cell lines with reconstituted UPF3A expression |
International journal of molecular sciences |
Medium |
32718059
|
| 2022 |
UPF3A and UPF3B share structural homology comprising an RRM-like domain (RRM-L), a NONA/paraspeckle-like domain (NOPS-L), and an extended α-helical domain; these domains are essential for RNA/ribosome-binding, RNA-induced oligomerization, and UPF2 interaction. Crystal structures of UPF2's MIF4GIII domain in complex with UPF3B or UPF3A revealed intimate binding interfaces. UPF3A binds UPF2 with ~10-fold higher affinity than UPF3B. The disease-causing UPF3B mutation Y160D in the NOPS-L domain displaces Y160 from a hydrophobic cleft in UPF2, reducing binding affinity ~40-fold. UPF3A and UPF3B compete for the same UPF2 binding site. |
X-ray crystallography; binding affinity measurements; mutagenesis; RNA/ribosome binding assays |
Nucleic acids research |
High |
35640974
|
| 2022 |
In HCT116 cells deleted for UPF3B, UPF3A strongly activates NMD; in cells lacking both UPF3A and UPF3B, NMD is only partially active. Complementation studies show the EJC-binding domain of UPF3 paralogs is dispensable for NMD; instead, the conserved 'mid' domain is consequential for NMD activity. UPF3A can activate NMD independently of EJC binding. |
CRISPR knockout cell lines; NMD reporter assays; RNA-seq; complementation with domain mutants |
The EMBO journal |
High |
35451102
|
| 2022 |
Co-depletion of UPF3A and UPF3B (but not single depletion of either) results in marked NMD inhibition and transcriptome-wide upregulation of NMD substrates, demonstrating functional redundancy between UPF3A and UPF3B. Rescue experiments show UPF2-binding or EJC-binding-deficient UPF3B largely retains NMD activity, but deletion of the middle domain combined with other mutations synergistically impairs NMD. |
siRNA knockdown and CRISPR knockout; RNA-seq; rescue experiments with domain mutants |
The EMBO journal |
High |
35451084
|
| 2023 |
In zebrafish leg1 deleterious mutants, Upf3a (but not Upf1) is essential for the homology-dependent genetic compensation response (HDGCR) induced by nonsense mutations; this occurs in an H3K4me3-independent manner. Upf3a is also responsible for correcting the expression of hundreds of genes dysregulated in leg1 mutants. |
Zebrafish single and double knockout mutants; RNA-seq (71 samples); ULI-NChIP-seq for H3K4me3; genetic epistasis |
Cell discovery |
High |
37369707
|
| 2023 |
In mouse embryonic stem cells, somatic cells, and major organs (liver, spleen, thymus), UPF3A is dispensable for NMD when UPF3B is present; UPF3A may weakly and selectively promote NMD in certain murine organs. UPF3A does not repress NMD in these contexts. |
Conditional knockout mouse (Upf3a); qRT-PCR and RNA analysis of 33 NMD targets in multiple cell lines and organs |
Life science alliance |
Medium |
36997282
|