| 2000 |
The isolated tandem DH/PH domain of p190RhoGEF activates RhoA in vitro (GDP release and protein binding assays), but not Rac1 or Cdc42, establishing RhoA-specific GEF activity. Full-length p190RhoGEF fails to activate RhoA in vitro, suggesting autoinhibition requiring unknown binding partners to unmask exchange activity in vivo. p190RhoGEF directly interacts with microtubules via its C-terminal region adjacent to the DH/PH domain, shown by in vitro and in vivo binding experiments. |
In vitro GDP release assay, protein binding assay, immunofluorescence, in vitro and in vivo microtubule binding experiments |
The Journal of biological chemistry |
High |
11058585
|
| 2003 |
FAK directly interacts with p190RhoGEF in neuronal cells and brain tissue extracts. The FAK C-terminal focal adhesion targeting (FAT) domain binds the C-terminal coiled-coil domain of p190RhoGEF, identified by two-hybrid assay and deletion mutagenesis. A FAK FAT domain mutation (Leu-1034 to Ser) disrupts this interaction. FAK activity promotes p190RhoGEF tyrosine phosphorylation and RhoA GTP loading downstream of laminin/integrin and IGF-1 receptor stimulation. |
Co-immunoprecipitation, co-localization, yeast two-hybrid, deletion mutagenesis, dominant-negative inhibition (FRNK), RhoA GTP-loading assay |
The Journal of biological chemistry |
High |
12702722
|
| 2001 |
14-3-3η and 14-3-3ε are binding partners of p190RhoGEF, identified by yeast two-hybrid screen and confirmed biochemically by co-immunoprecipitation and co-localization. A phosphorylation-independent binding site (I1370QAIQNL) in p190RhoGEF was mapped; deletion of this site abolishes 14-3-3η interaction in vitro and prevents 14-3-3η-mediated alteration of p190RhoGEF cytoplasmic aggregation in cells. |
Yeast two-hybrid, co-immunoprecipitation, co-localization with fluorescent fusion proteins, deletion mutagenesis |
The Journal of biological chemistry |
High |
11533041
|
| 2001 |
p190RhoGEF binds directly and specifically to the 68-nucleotide destabilizing element in the 3' UTR of NF-L (neurofilament light) mRNA via its C-terminal domain (clone 39), demonstrated by Northwestern blot, gel-shift, and cross-linkage assays. Expression of p190RhoGEF in stably transfected neuronal cells increased the half-life of wild-type NF-L mRNA but not of a mutant lacking the destabilizing element, establishing a functional role in NF-L mRNA stability. |
GST-fusion pulldown, Northwestern blot, gel-shift assay, RNA cross-linkage, stable transfection with mRNA half-life measurement |
The Journal of biological chemistry |
High |
11435431
|
| 2002 |
BC1 RNA (a neuronally expressed non-coding RNA) binds to the same C-terminal site of p190RhoGEF as NF-L mRNA and competes with NF-L mRNA for p190RhoGEF binding, identified by affinity chromatography and cross-competition experiments using a GST-p190RhoGEF C-terminal fusion protein. |
GST-fusion affinity chromatography, gel-shift, cross-competition binding assay |
The Journal of biological chemistry |
Medium |
12215442
|
| 2003 |
Anti-apoptotic activity of p190RhoGEF is localized to two cytoplasmic retention sequences (CRS-1 and CRS-2) in its C-terminal region that overlap with the JIP-1 and 14-3-3 binding sites. Deleting both CRS sequences abolishes cytoplasmic retention and anti-apoptotic activity of EGFP-tagged p190RhoGEF in Neuro 2a cells; restoring either CRS-1 or CRS-2 rescues both properties. |
Transfection of EGFP-tagged deletion constructs, apoptosis assay, fluorescence microscopy in Neuro 2a cells |
Brain research. Molecular brain research |
Medium |
14499478
|
| 2003 |
p190RhoGEF expression is induced by CD40 stimulation in WEHI 231 B cells. Overexpression of p190RhoGEF mimics CD40-stimulated cellular structure changes and NF-κB activation through RhoA; these effects are blocked by dominant-negative RhoA (T19N) or dominant-negative p190RhoGEF (Y1003A). |
2D gel electrophoresis identification, overexpression with dominant-negative constructs, NF-κB reporter assay |
Journal of immunology |
Medium |
12496377
|
| 2008 |
delta-Catenin interacts with p190RhoGEF in the cytoplasm at low cell density, reducing RhoA activity. At high cell density, E-cadherin outcompetes p190RhoGEF for delta-catenin binding, shifting delta-catenin to the plasma membrane and restoring RhoA activity. Ectopic E-cadherin expression in mouse embryonic fibroblasts decreased delta-catenin's effect on RhoA activity reduction. |
Co-immunoprecipitation, immunofluorescence, RhoA activity assay, ectopic E-cadherin expression |
Biochemical and biophysical research communications |
Medium |
18930028
|
| 2010 |
Human RGNEF (the human homologue of p190RhoGEF) directly interacts with human NFL mRNA in vitro by gel-shift assay. In tissue lysates, RGNEF-NFL mRNA interaction was detected by IP-RT-PCR only in ALS patient samples, not in neuropathologically normal controls. |
Gel-shift assay (in vitro), IP-RT-PCR (in tissue lysates) |
Amyotrophic lateral sclerosis |
Medium |
19488899
|
| 2011 |
Rgnef forms a complex with FAK in human colon carcinoma cells. Upon gastrin stimulation, Rgnef-FAK interaction is required for FAK translocation to focal adhesions, paxillin tyrosine phosphorylation, cell motility, and invadopodia formation. Overexpression of the Rgnef C-terminal region (aa 1279–1582) disrupts endogenous Rgnef-FAK interaction and blocks these events; a version lacking the FAK binding site (aa 1302–1582) does not. Rgnef-C-expressing cells form smaller, less invasive tumors in vivo. |
shRNA knockdown, co-immunoprecipitation, dominant-negative C-terminal fragment competition, phosphorylation assays, orthotopic tumor implantation |
Cancer research |
High |
21224360
|
| 2012 |
Genetic knockout of Rgnef in mouse embryo fibroblasts (Rgnef-/- MEFs) significantly inhibits haptotaxis migration, wound closure motility, focal adhesion number, and RhoA GTPase activation after fibronectin-integrin stimulation. These phenotypes are rescued by epitope-tagged Rgnef re-expression, establishing Rgnef as essential for RhoA regulation downstream of integrins. |
Conditional knockout (floxed Rgnef × CMV-Cre), primary MEF isolation, haptotaxis assay, wound closure assay, focal adhesion quantification, RhoA GTP-loading assay, rescue by re-expression |
PloS one |
High |
22649559
|
| 2013 |
Rgnef plays a non-canonical, upstream scaffolding role in promoting FAK localization to peripheral adhesions and FAK-Y397 activation upon fibronectin binding, independent of its GEF catalytic activity. A PH domain mutation in Rgnef blocks adhesion formation, FAK localization, and FAK/paxillin phosphorylation without disrupting the Rgnef-FAK interaction. A GEF-inactive Rgnef mutant rescues FAK-Y397 phosphorylation and adhesion localization but not paxillin-Y118 phosphorylation, indicating paxillin-pY118 requires Rgnef GEF activity through a distinct mechanism. |
Rgnef-null MEFs, site-directed mutagenesis (PH domain and GEF-inactive mutants), immunofluorescence, phosphotyrosine immunoblotting, rescue experiments |
Journal of cell science |
High |
24006257
|
| 2015 |
Rgnef is a new effector for Gα13 downstream of gastrin and the CCK2 receptor in DLD-1 colon carcinoma cells. Rgnef co-immunoprecipitates with activated Gα13Q226L but not Gα12Q229L; the Rgnef C-terminal region (aa 1279–1582) is sufficient for this interaction and its exogenous expression blocks Gα13-stimulated SRE activity. Point mutations in the Rgnef C-terminal region disrupt Gα13 association but not Gαq association. Gα13 depletion reduces gastrin-induced FAK-pY397 and paxillin-pY31. |
Co-immunoprecipitation, shRNA depletion of Gα13, SRE-luciferase reporter assay, point mutagenesis of Rgnef C-terminus, RhoA GTP-binding assay |
The Journal of biological chemistry |
High |
25922072
|
| 2017 |
Crystal structures reveal that activated Rac1·GTP and RhoA·GTP use their effector-binding surfaces to associate with the same hydrophobic surface on the p190RhoGEF PH domain. Both activated RhoA and Rac1 stimulate nucleotide exchange on RhoA·GDP by p190RhoGEF in vitro, localizing it to its substrate. This demonstrates a positive feedback (activated RhoA) and a cross-talk mechanism (activated Rac1 directly stimulates RhoA activation through p190RhoGEF). |
X-ray crystallography, in vitro nucleotide exchange assay |
Journal of structural biology |
High |
29196061
|
| 2017 |
RGNEF expression is upregulated in murine spinal motor neurons following distal sciatic nerve injury. Under cellular stress (sodium arsenite or sorbitol), RGNEF expression confers a survival benefit in HEK293T cells; the NH2-terminus domain is essential for this protective effect. Under stress, RGNEF associates with Staufen1-positive granules but not TIA-1-positive stress granules. |
In vivo nerve injury model, in vitro stress assay with deletion constructs, immunofluorescence co-localization |
Molecular and cellular neurosciences |
Medium |
28495450
|
| 2018 |
A 23-amino acid bipartite nuclear localization signal (NLS) within the Pleckstrin Homology (PH) domain of RGNEF controls its nuclear localization; deletion or mutation of this region abolishes nuclear localization. Within this NLS, an overlapping nuclear export signal (NES) promotes nuclear export in an exportin-1-dependent manner (confirmed by Leptomycin B treatment). The PH domain alone is sufficient to translocate a 160 kDa fusion protein to the nucleus. |
Deletion and point mutagenesis of NLS/NES, fluorescence microscopy of fusion proteins, Leptomycin B inhibition |
European journal of cell biology |
Medium |
30482479
|
| 2019 |
Rgnef is essential for ovarian tumor spheroid formation in vitro and tumor growth in vivo using transgenic and transplantable Rgnef knockout mouse models. Rgnef supports an NF-κB-mediated antioxidant gene signature (including Gpx4, Nqo1, Gsta4); antioxidant treatment rescues growth of Rgnef-knockout spheroids, and Rgnef re-expression facilitates NF-κB-dependent tumorsphere survival. |
Rgnef knockout mouse model, spheroid formation assay, RNA-sequencing, antioxidant rescue experiment, NF-κB reporter/pathway analysis |
Oncogene |
Medium |
31308489
|
| 2024 |
An N-terminal fragment of RGNEF (NF242) directly interacts with the RNA recognition motifs (RRMs) of TDP-43, competing with RNA binding. The IPT/TIG domain of NF242 is essential for this interaction. In a Drosophila ALS model overexpressing TDP-43, genetic expression of NF242 suppressed neuropathological phenotypes (increased lifespan, abolished motor defects, prevented neurodegeneration). Intracerebroventricular injection of AAV9/NF242 in a murine TDP-43 model (rNLS8) improved lifespan and motor phenotype and decreased neuroinflammation markers. |
Direct protein-protein interaction assay, domain deletion (IPT/TIG), Drosophila genetic epistasis model, murine AAV9 intracerebroventricular injection |
Brain : a journal of neurology |
High |
38739752
|
| 2024 |
RGNEF and TDP-43 act predominantly in an antagonistic manner to regulate expression of axon guidance genes in neuronal cells. Mechanistically, both factors affect the processivity of long intron removal (splicing), explaining their mode of transcriptomic action upon depletion. |
Comparative transcriptomics (RNA-seq) of TDP-43- and RGNEF-depleted neuronal cells, long intron processivity analysis |
FASEB journal |
Medium |
39360635
|
| 2026 |
Rgnef promotes osteoclastogenesis and attenuates osteoblastogenesis through activation of RhoA and Rac1, leading to enhanced NF-κB, MAPK, and AKT signaling. Rgnef-deficient mice show increased bone mass due to reduced osteolysis and increased osteogenesis, while Rgnef-overexpressing mice show the opposite. Rgnef-deficient mice are protected from bone loss in LPS-induced inflammation and ovariectomy models. |
Rgnef-deficient and transgenic overexpressing mice, osteoclast/osteoblast differentiation assays, RhoA/Rac1 activity assay, NF-κB/MAPK/AKT pathway analysis, in vivo bone loss models |
Experimental & molecular medicine |
Medium |
41571890
|