Inhibition of TBC1D5 activates Rab7a and can enhance the function of the retromer cargo-selective complex.
- Authors
- Seaman, Matthew N J; Mukadam, Aamir S; Breusegem, Sophia Y
- Year
- 2018
- Journal
- Journal of cell science
- PMID
- 29777037
- DOI
- 10.1242/jcs.217398
- PMCID
- PMC6031384
The retromer complex is a vital component of the endosomal protein sorting machinery necessary for sorting into both the endosome-to-Golgi retrieval pathway and also the endosome-to-cell-surface recycling pathway. Retromer mediates cargo selection through a trimeric complex comprising VPS35, VPS29 and VPS26, which is recruited to endosomes by binding to Rab7a and Snx3. Retromer function is linked to two distinct neurodegenerative diseases, Parkinson's disease and Alzheimer's disease and modulating retromer function has been proposed as an avenue to explore for a putative therapy in these conditions. We hypothesised that activating Rab7a to promote the recruitment of retromer to endosomes could positively modulate its activity. Here, we show that inhibition of the GTPase activating protein TBC1D5 can enhance Rab7a activation and lead to a gain of function for retromer.
Loss of TBC1D5 expression enhances endosomal levels of the retromer CSC. (A) HeLa cells were transiently transfected with empty GFP vector, GFP-TBC1D5 wild type (WT) or GFP-TBC1D5 R169A/Q204A (RQ) mutant. After fixation, the cells were stained with antibodies against VPS35 and VPS26. Transfected cells are marked with an asterisk. Overexpression of the wild-type TBC1D5 can displace the retromer CSC from membranes. (B) HeLa cells were treated with siRNA to silence TBC1D5 expression. The knockdown cells were mixed with control cells and seeded onto coverslips. After fixation, cells were labelled with anti-TBC1D5 and antibodies against either VPS35 or VPS26. Loss of TBC1D5 expression (in cells marked with an asterisk) results in brighter staining of the retromer CSC proteins. (C,D) HeLa cells treated with siRNA to silence TBC1D5 expression were labelled with antibodies against VPS26, TBC1D5, CIMPR or TGN46 and then imaged using an automated microscope. Loss of TBC1D5 results in ∼40% increase in VPS26 fluorescence intensity but does not markedly increase the number of VPS26-positive spots (D). No spots were counted for TGN46 as the morphology of the TGN is not punctate but ribbon-like. P-values for TBC1D5 knockdown versus control: VPS26, 1.2×10−4; CIMPR, 0.0095; TGN46, 0.0037 for total intensity values. The P-values for spot numbers are: 0.08 for VPS26 and 0.23 for CIMPR. Scale bars: 20 µm.
Loss of TBC1D5 function leads to increased levels of active Rab7a. (A) HeLa cells stably expressing GFP-tagged Rab7a-GTP were treated with siRNA to silence TBC1D5 expression. Following fixation, the cells were labelled with anti-Rab7a-GTP antibodies. Knockdown of TBC1D5 leads to increased staining of the anti-Rab7a antibody. Scale bar: 20 µm. (B) Cells stably expressing various GFP-tagged proteins were treated as in A and then imaged using an automated microscope. Only cells expressing GFP-Rab7a or GFP-Rab7a Q67L registered significant fluorescence and the knockdown of TBC1D5 results in a pronounced increase in the levels of active (GTP-bound) Rab7a. Values are mean±s.e.m. of 250 cells measured for each cell line. The P-values for control and TBC1D5 knockdown for cells expressing GFP-Rab7a are shown on the graph and demonstrate that the increase in fluorescence is statistically significant. (C) Cells expressing various GFP-tagged proteins were treated with siRNA to abolish either Rab7a or TBC1D5 expression. After fixation, the cells were labelled with antibodies against VPS26 and imaged using an automated microscope. Loss of Rab7a expression causes VPS26 (and the retromer CSC) to dissociate from endosomes, massively reducing the fluorescence intensity except where the knockdown of Rab7a is rescued by GFP-tagged Rab7a or Rab7a Q67L. Loss of TBC1D5 expression enhances VPS26 fluorescence even in cells where VPS26 fluorescence is lower due to the expression of a GDP-locked Rab7a T22N mutant. P-values are shown on the graph. (D) The number of VPS26 spots is not significantly altered after loss of TBC1D5 expression. P-values for all control versus TBC1D5-knockdown measurements were >0.1.
TBC1D5 knockdown enhances the associations of the retromer CSC. (A) Cells expressing either GFP-Rab5 or GFP-Rab7a were treated with siRNA to silence TBC1D5 expression. After lysis under native conditions, the GFP-tagged proteins were recovered by immunoprecipitation (IP) using anti-GFP. The immunoprecipitated proteins were analysed by western blotting. Retromer CSC proteins were detected in the GFP-Rab7a IP but not GFP-Rab5 IP. The knockdown of TBC1D5 increased the levels of retromer CSC proteins associated with GFP-Rab7a but no changes in protein levels were observed after TBC1D5 knockdown when lysates were analysed. IP of VPS26 confirmed that TBC1D5 expression was abolished and that loss of TBC1D5 does not alter the interaction between VPS26 and VPS35. (B) Following a protocol for SILAC labelling, three HeLa cell lines were labelled over several passages with heavy or light amino acids before being subjected to TBC1D5 knockdown (in the light amino acid-labelled cells) and treated with the DSP crosslinking reagent. After lysis, VPS26 was recovered by IP and the resulting IPs analysed by mass spectrometry. Levels of the proteins in the IPs are shown as a ratio of heavy:light normalised to VPS26. The retromer CSC proteins all give values close to 1, indicating that TBC1D5 knockdown does not affect retromer CSC assembly. The TBC1D5 protein has a ratio ∼3-3.5 consistent with a knockdown of the protein. Other proteins detected generally gave ratios <1, showing that more peptides labelled with light amino acids were detected, indicating an increased level of the protein after TBC1D5 knockdown. (C) Cells expressing either GFP-VPS35 WT or GFP-VPS35 D620N (DN) were treated as in B and the lysates were treated with anti-GFP antisera. The knockdown of TBC1D5 can enhance the interaction of the VPS35 D620N mutant with Fam21. (D) Lysates from cells in C analysed by western blotting to confirm TBC1D5 knockdown.
Silencing TBC1D5 expression can rescue the impaired Fam21 interaction of the VPS35 D620N mutant. (A,B) Cells expressing either wild-type GFP-VPS35 (WT) (A) or GFP-VPS35 D620N (DN) (B) were treated with siRNA to abolish TBC1D5 expression. After fixation, the cells were labelled with antibodies against Fam21 and the CIMPR. There is a marked increase in the fluorescence staining of Fam21 in the GFP-VPS35 D620N cells after TBC1D5 knockdown. Scale bar: 20 µm. (C) Cells from A and B were imaged using an automated microscope to measure the fluorescence intensity. Knockdown of TBC1D5 can rescue the fluorescence intensity of Fam21, consistent with an increase in the association of Fam21 (and the WASH complex) with the retromer CSC. P-values for TBC1D5 KD versus control are: VPS35 WT: VPS26, 2.7×10−6; CIMPR, 1.4×10−6; Fam21, 0.0022; VPS35 D620N: VPS26, 3.0×10−8; CIMPR, 9.8×10−6; Fam21, 8.5×10−9.
Inhibition of TBC1D5 function can partially rescue the trafficking defects caused by the VPS35 D620N mutation. (A) HeLa cells expressing GFP-VPS35 D620N were treated with siRNA to silence TBC1D5 expression. After fixation, the cells were labelled with antibodies against Glut1 and the CIMPR. The localisation of Glut1 appears to be shifted away from perinuclear structures after TBC1D5 knockdown. Scale bar: 20 µm. (B) HeLa cells expressing either GFP-VPS35 wild type (WT) or the GFP-VPS35 D620N mutant were treated with siRNA to silence TBC1D5 expression and then labelled with antibodies against Glut and Snx1. The cells were imaged using an automated microscope and the overlap of the Glut1 and Snx1 antibodies measured. There is more overlap of Glut1 with Snx1 in cells expressing VPS35 D620N. The overlap is reduced upon TBC1D5 knockdown but not to levels seen in cells expressing wild-type VPS35. (C) There is no appreciable change in the Snx1 fluorescence following TBC1D5 knockdown. (D) Cells treated as in B were labelled with anti-Glut1 and anti-GM130. (E) There is no appreciable change in GM130 fluorescence after TBC1D5 knockdown. For B-E, values are mean±s.d. and P-values are shown on the graphs.
Knockdown of TBC1D5 can enhance retromer function. (A) Three different cell lines were treated with siRNA to knockdown TBC1D5 expression. Following fixation, cells were labelled with antibodies against CIMPR and TGN46 and then imaged using an automated microscope. The fraction of CIMPR present in a TGN46 mask is shown graphically. For each of the cell lines, knockdown on TBC1D5 enhances the colocalisation of CIMPR with TGN46 but only the GFP-VPS35 cells demonstrate statistical significance. Values are mean±s.d. and P-values for knockdown versus control are shown for each cell line. (B) TBC1D5 expression was silenced in cells expressing GFP-VPS35 wild type or the D620N mutant. Following fixation, the cells were labelled with antibodies against Atg9A and TGN46 and then imaged using an automated microscope. The Pearson correlation coefficient for Atg9A-TGN46 mask is shown graphically. For each of the cell lines, knockdown of TBC1D5 enhances the colocalisation of Atg9A with TGN46 but only the GFP-VPS35 wild-type cells demonstrate statistical significance. Values are mean±s.d. and P-values for knockdown versus control are shown for each cell line. (C) HEK293 cells stably expressing APPswedish were treated with siRNA to silence VPS35 or TBC1D5. Cell culture medium was collected and analysed for the Aβ peptide by western blotting. Knockdown of VPS35 increases APP processing to Aβ but loss of TBC1D5 expression has the opposite effect. The data shown are from two independent experiments that were highly reproducible. Values are mean±s.d. For both the VPS35- and TBC1D5-knockdown conditions, P<0.01 using Student's t-test compared with control. (D) Representative blots of media (for Aβ and sAPPβ) and lysates (for APP, VPS35, TBC1D5 and the loading controls, GAPDH and tubulin) from C showing the reduction in Aβ detected when TBC1D5 is silenced. There is also a reduction in sAPPβ.
| Name | Type |
|---|---|
| [125I]-Protein-A local | drug |
| Alzheimer's disease | phenotype |
| amino acids | drug |
| Amyloid beta | drug |
| ANKRD27 local | gene |
| antibodies | drug |
| anti-Rab7a-GTP antibody local | drug |
| APP | gene |
| APPswedish local | variant |
| arginine | drug |
| Armus local | gene |
| ATG9A local | gene |
| Aβ peptide local | drug |
| Bis-Tris gel local | drug |
| bovine serum albumin | drug |
| calcium chloride | drug |
| Carbon local | drug |
| CD8a | gene |
| cell lysate proteins local | drug |
| CIMPR local | drug |
| CIMPR local | gene |
| D620N local | variant |
| dimethyl sulfoxide | drug |
| dithiobis(succinimidyl propionate) local | drug |
| DMEM | drug |
| DNAJC13 local | gene |
| EDTA | drug |
| elevated Rab7a-GTP signal local | phenotype |
| Endosome local | drug |
| Fam21 local | gene |
| FAM21 local | gene |
| FAM21A local | gene |
| fetal bovine serum | drug |
| G418 local | drug |
| GE Healthcare local | drug |
| gelatin | drug |
| GFP | drug |
| GFP-Rab7a local | variant |
| Glut1 local | gene |
| GLUT1 local | gene |
| glutamine | drug |
| GM130 local | drug |
| GM130 local | gene |
| GOLGA2 local | gene |
| heavy amino acids local | drug |
| Heavy isotope local | drug |
| HEK293 cells | cohort |
| HeLa | cohort |
| HeLaM local | variant |
| HEPES potassium hydroxide buffer local | drug |
| HRP-conjugated secondary antibodies local | drug |
| IGF2R local | gene |
| immune complexes | drug |
| Integrin proteins local | drug |
| Invitrogen | drug |
| KIAA1033 local | gene |
| Lamp1 local | gene |
| LAMP1 local | gene |
| late-onset Alzheimer's disease | phenotype |
| Leucine | drug |
| light amino acids local | drug |
| Light isotope local | drug |
| Luminol reagents local | drug |
| Lysine local | drug |
| M6PR local | gene |
| magnesium acetate local | drug |
| membrane-permeable chemical crosslinker local | drug |
| MES/SDS buffer local | drug |
| Millipore local | drug |
| Mitophagy local | phenotype |
| nitrocellulose local | drug |
| nitrocellulose membranes | drug |
| Nitrogen local | drug |
| Nupage local | drug |
| paraformaldehyde | drug |
| Parkinson's disease | phenotype |
| penicillin | drug |
| peroxide local | drug |
| pharmacological chaperone local | drug |
| Pharmacological chaperone local | drug |
| phosphate-buffered saline | drug |
| polyethylenimine | drug |
| potassium acetate local | drug |
| primary antibody | drug |
| ProLong mounting medium local | drug |
| Protein-A Sepharose local | drug |
| PtdIns3P local | drug |
| Q66L local | variant |
| Rab21 local | gene |
| RAB21 local | gene |
| Rab32 local | gene |
| RAB32 local | gene |
| Rab38 | gene |
| Rab5 | gene |
| RAB7 local | gene |
| Rab7a local | gene |
| RAB7A local | gene |
| Rab7a Q67L local | variant |
| Rab7a T22N local | variant |
| Rab9 local | gene |
| Retromer local | drug |
| retromer complex local | drug |
| retromer CSC local | drug |
| retromer CSC local | gene |
| Retromer CSC local | drug |
| RILP local | gene |
| sAPPβ local | drug |
| secondary antibody | drug |
| Sigma local | drug |
| SILAC medium local | drug |
| siRNA | drug |
| siRNA targeting TBC1D5 local | drug |
| skimmed milk powder local | drug |
| SLC2A1 local | gene |
| small-molecule inhibitor local | drug |
| Snx1 local | gene |
| SNX1 local | gene |
| SNX2 local | gene |
| Snx27 local | gene |
| Snx3 local | gene |
| SNX3 local | gene |
| SNX5 local | gene |
| SNX6 local | gene |
| sorbitol local | drug |
| SORL1 | gene |
| SORT1 | gene |
| streptomycin | drug |
| strumpellin local | gene |
| T22N local | variant |
| TBC1D15 local | gene |
| TBC1D5 local | gene |
| TBC1D5 RQ mutant local | variant |
| TBS-based blocking buffer local | drug |
| TBST local | drug |
| TGN46 local | drug |
| TGN46 local | gene |
| TGOLN2 local | gene |
| tris(hydroxymethyl)aminomethane hydrochloride local | drug |
| Triton X-100 | drug |
| Tubulin local | gene |
| Tween20 local | drug |
| VARP local | gene |
| VPS17 local | gene |
| VPS26 local | gene |
| VPS29 local | gene |
| VPS35 local | gene |
| VPS35 D620N local | variant |
| VPS5 local | gene |
| WASHC2A local | gene |
| WASH complex local | drug |
| WASH complex local | gene |
| Whole Cell Stain Blue local | drug |
| YPT7 local | gene |
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In this knowledge base
| Title | Year | PMID |
|---|---|---|
| RNA alternative splicing impacts the risk for alcohol use disorder. | 2023 | 37217680 |
External
| Title | Authors | Journal | Year | Link |
|---|---|---|---|---|
| Role of lysosomal morphology in aging and age-related diseases. | Liu H et al. | — | 2026 | → |
| AP2A1 activates Rab7 to promote axonal autophagosome transport and slow the progression of Alzheimer's disease. | Wang Y et al. | — | 2025 | → |
| Cryo-EM structure of the human MON1A-CCZ1-RAB7A complex provides insights into nucleotide exchange mechanism. | Li X et al. | — | 2025 | → |
| EccDNA atlas in male mice reveals features protecting genes against transcription-induced eccDNA formation. | Liang X et al. | — | 2025 | → |
| Mapping of endosomal proximity proteomes reveals Retromer as a hub for RAB GTPase regulation. | Antón-Plágaro C et al. | — | 2025 | → |
| Methamphetamine and Methamphetamine-Induced Neuronal Exosomes Modulate the Activity of Rab7a via PTEN to Exert an Influence on the Disordered Autophagic Flux Induced in Neurons. | Qiu H et al. | — | 2025 | → |
| Neurons Specialize in Presynaptic Autophagy: A Perspective to Ameliorate Neurodegeneration. | Mishra AK et al. | — | 2025 | → |
| Noncanonical roles of ATG5 and membrane atg8ylation in retromer assembly and function. | Paddar MA et al. | — | 2025 | → |
| PKD3 localizes to late endosomes to maintain Rab7-dependent endolysosomal homeostasis. | Gutiérrez-Galindo E et al. | — | 2025 | → |
| Rab7a is required to degrade select blood-brain barrier junctional proteins after ischemic stroke. | Cottarelli A et al. | — | 2025 | → |
| The hereditary spastic paraplegia type 21 (SPG21) protein is a RAB7A effector that promotes noncanonical mTORC1-catalyzed TFEB phosphorylation and cytoplasmic retention. | Kunselman JM et al. | — | 2025 | → |
| VPS35-Retromer: Multifunctional Roles in Various Biological Processes - A Focus on Neurodegenerative Diseases and Cancer. | Fan X et al. | — | 2025 | → |
| γ-secretase facilitates retromer-mediated retrograde transport. | Takeo Y et al. | — | 2025 | → |
| Assembly and fission of tubular carriers mediating protein sorting in endosomes. | Gopaldass N et al. | — | 2024 | → |
| Autophagy captures the retromer-TBC1D5 complex to inhibit receptor recycling. | Carosi JM et al. | — | 2024 | → |
| Collapse of late endosomal pH elicits a rapid Rab7 response via the V-ATPase and RILP. | Mulligan RJ et al. | — | 2024 | → |
| Endocytosis and Alzheimer's disease. | Zadka Ł et al. | — | 2024 | → |
| Retromer-mediated recruitment of the WASH complex involves discrete interactions between VPS35, VPS29, and FAM21. | Romano-Moreno M et al. | — | 2024 | → |
| Structural basis for coupling of the WASH subunit FAM21 with the endosomal SNX27-Retromer complex. | Guo Q et al. | — | 2024 | → |
| Systematic Analysis of Biological Processes Reveals Gene Co-expression Modules Driving Pathway Dysregulation in Alzheimer's Disease. | Adeoye T et al. | — | 2024 | → |
| The role of membrane trafficking and retromer complex in Parkinson's and Alzheimer's disease. | Abdul-Rahman T et al. | — | 2024 | → |
| VPS34 Governs Oocyte Developmental Competence by Regulating Mito/Autophagy: A Novel Insight into the Significance of RAB7 Activity and Its Subcellular Location. | Liu W et al. | — | 2024 | → |
| VPS35 and retromer dysfunction in Parkinson's disease. | Rowlands J et al. | — | 2024 | → |
| EMP3 sustains oncogenic EGFR/CDK2 signaling by restricting receptor degradation in glioblastoma. | Martija AA et al. | — | 2023 | → |
| Identification of influential observations in high-dimensional survival data through robust penalized Cox regression based on trimming. | Sun H et al. | — | 2023 | → |
| Receptor Recycling by Retromer. | Carosi JM et al. | — | 2023 | → |
| Regulation of Endosomal Trafficking by Rab7 and Its Effectors in Neurons: Clues from Charcot-Marie-Tooth 2B Disease. | Mulligan RJ et al. | — | 2023 | → |
| RNA alternative splicing impacts the risk for alcohol use disorder. | Li R et al. | — | 2023 | → |
| Role of Ceramides and Sphingolipids in Parkinson's Disease. | Vos M et al. | — | 2023 | → |
| Structural basis for coupling of the WASH subunit FAM21 with the endosomal SNX27-Retromer complex | Guo Q et al. | — | 2023 | — |
| Mechanisms regulating the sorting of soluble lysosomal proteins. | Meraş İ et al. | — | 2022 | → |
| The E3 ubiquitin ligase RNF115 regulates phagosome maturation and host response to bacterial infection. | Bilkei-Gorzo O et al. | — | 2022 | → |
| Canonical and Noncanonical Autophagy Pathways in Microglia. | Jülg J et al. | — | 2021 | → |
| CLN3, at the crossroads of endocytic trafficking. | Cotman SL et al. | — | 2021 | → |
| Formation of retromer transport carriers is disrupted by the Parkinson disease-linked Vps35 D620N variant. | Cui Y et al. | — | 2021 | → |
| Impaired Retrograde Transport Due to Lack of TBC1D5 Contributes to the Trafficking Defect of Lysosomal Cathepsins in Ischemic/Hypoxic Cardiomyocytes. | Cui L et al. | — | 2021 | → |
| Opposing functions for retromer and Rab11 in extracellular vesicle traffic at presynaptic terminals. | Walsh RB et al. | — | 2021 | → |
| Phosphorylation of SNX27 by MAPK11/14 links cellular stress-signaling pathways with endocytic recycling. | Mao L et al. | — | 2021 | → |
| Retromer dysfunction at the nexus of tauopathies. | Carosi JM et al. | — | 2021 | → |
| The Retromer Complex: From Genesis to Revelations. | Seaman MNJ | — | 2021 | → |
| The roles of GTPase-activating proteins in regulated cell death and tumor immunity. | He H et al. | — | 2021 | → |
| Acute inactivation of retromer and ESCPE-1 leads to time-resolved defects in endosomal cargo sorting. | Evans AJ et al. | — | 2020 | → |
| Endosomal microdomains: Formation and function. | Norris A et al. | — | 2020 | → |
| Endosomal sorting pathways in the pathogenesis of Parkinson's disease. | Cunningham LA et al. | — | 2020 | → |
| Genomic Analysis Identifies New Loci Associated With Motor Complications in Parkinson's Disease. | Ryu HS et al. | — | 2020 | → |
| Lysosomal size matters. | de Araujo MEG et al. | — | 2020 | → |
| Mechanism and evolution of the Zn-fingernail required for interaction of VARP with VPS29. | Crawley-Snowdon H et al. | — | 2020 | → |
| Screening and analysis of small molecular peptides in urine of gestational diabetes mellitus. | Hu Z et al. | — | 2020 | → |
| SKIP-HOPS recruits TBC1D15 for a Rab7-to-Arl8b identity switch to control late endosome transport. | Jongsma ML et al. | — | 2020 | → |
| TBC1D5-Catalyzed Cycling of Rab7 Is Required for Retromer-Mediated Human Papillomavirus Trafficking during Virus Entry. | Xie J et al. | — | 2020 | → |
| The secreted protein kinase CstK from <i>Coxiella burnetii</i> influences vacuole development and interacts with the GTPase-activating host protein TBC1D5. | Martinez E et al. | — | 2020 | → |
| Interaction between VPS35 and RABG3f is necessary as a checkpoint to control fusion of late compartments with the vacuole. | Rodriguez-Furlan C et al. | — | 2019 | → |
| Rab regulation by GEFs and GAPs during membrane traffic. | Lamber EP et al. | — | 2019 | → |
| Retromer and TBC1D5 maintain late endosomal RAB7 domains to enable amino acid-induced mTORC1 signaling. | Kvainickas A et al. | — | 2019 | → |
| Towards a molecular understanding of endosomal trafficking by Retromer and Retriever. | Chen KE et al. | — | 2019 | → |
| VPS29, a tweak tool of endosomal recycling. | Baños-Mateos S et al. | — | 2019 | → |
| Retromer in Synaptic Function and Pathology. | Brodin L et al. | — | 2018 | → |
| This Is the End: Regulation of Rab7 Nucleotide Binding in Endolysosomal Trafficking and Autophagy. | Stroupe C | — | 2018 | → |