Affinage

WASHC2C

WASH complex subunit 2C · UniProt Q9Y4E1

Length
1341 aa
Mass
147.2 kDa
Annotated
2026-06-11
10 papers in source corpus 5 papers cited in narrative 5 extracted findings
Cross-family judge vs UniProt: Affinage preferred faithfulness: 6/6 claims corpus-supported (100%)

Mechanistic narrative

Synthesis pass · prose summary of the discoveries below

WASHC2C (FAM21C/VPEF) is an endosomal trafficking factor that couples the retromer cargo-recognition machinery to the actin-nucleating WASH complex to drive cargo sorting into recycling pathways (PMID:26041286, PMID:27816670). Its C-terminal tail directly bridges retromer to the WASH pentamer on endosomal membranes, and this interaction is required for recycling of cargo such as β1- and β2-adrenergic receptors from endosomes to the plasma membrane, with FKBP15 acting as a WASHC2C-binding partner that selectively governs β1-AR recycling (PMID:27816670). The WASH–WASHC2C–retromer assembly mediates endosomal membrane fission and routes cargo into Rab11- and Rab22-positive recycling compartments (PMID:26041286). Through a CP-interacting (CPI) domain, WASHC2C binds and inhibits the actin-capping protein CAPZA1, promoting F-actin remodeling that supports cell invasion and migration; mutation of the CPI domain abolishes both CAPZA1 binding and the pro-invasive effect (PMID:35096613). WASHC2C additionally localizes to cell-surface lipid rafts and cytoplasmic vesicles and is required for fluid-phase (macropinocytic) endocytosis (PMID:18550675). In reconstituted supported-lipid-bilayer assays, WASHC2C does not alter retromer oligomerization state, indicating its bridging role does not operate by potentiating retromer assembly (PMID:32651229).

Mechanistic history

Synthesis pass · year-by-year structured walk · 5 steps
  1. 2008 Medium

    Established WASHC2C as a membrane trafficking factor by showing it localizes to lipid rafts and recycling-endosome vesicles and is required for fluid-phase endocytosis, defining its cellular compartment before its molecular role was known.

    Evidence siRNA knockdown with virus penetration and dextran uptake assays plus confocal colocalization with Rab5a/Rab11/caveolin and lipid raft fractionation

    PMID:18550675

    Open questions at the time
    • Molecular partners and the basis of vesicle recruitment not yet identified
    • Mechanism linking surface lipid-raft pool to intracellular recycling vesicles unresolved
  2. 2015 Medium

    Placed WASHC2C within a defined molecular machine by showing it recruits both WASH and retromer to early endosomes to drive membrane fission and sorting into Rab11/Rab22 recycling pathways, answering how it acts mechanistically in trafficking.

    Evidence Live single-particle imaging plus dominant-negative and siRNA functional interference of WASH/FAM21/retromer with Rab11/Rab22 colocalization

    PMID:26041286

    Open questions at the time
    • Which structural region mediates each interaction not yet mapped
    • Direct versus indirect recruitment of retromer not distinguished
  3. 2016 Medium

    Mapped the bridging function to the WASHC2C C-tail and connected it to physiological cargo, showing the C-tail couples retromer to the WASH pentamer to recycle β-adrenergic receptors, and identified FKBP15 as a cargo-selective binding partner.

    Evidence siRNA knockdown of FAM21C and FKBP15 with radioligand receptor-recycling assays and epistasis against SNX3, Rab7a, SNX27

    PMID:27816670

    Open questions at the time
    • Structural basis of the C-tail–retromer interface not resolved
    • How FKBP15 confers cargo selectivity for β1-AR unknown
  4. 2020 Medium

    Tested whether WASHC2C bridging works by promoting retromer assembly and found it does not affect retromer oligomerization in vitro, refining the model of how the C-tail engages retromer.

    Evidence Quantitative single-particle fluorescence microscopy on supported lipid bilayers with purified retromer, SNX3, RAB7, and WASHC2C retromer-binding segments

    PMID:32651229

    Open questions at the time
    • Negative result; does not define what the bridging interaction does accomplish mechanically
    • Full-length WASHC2C and the WASH pentamer were not included in the reconstitution
  5. 2022 Medium

    Extended WASHC2C beyond cargo sorting to direct actin regulation by showing its CPI domain binds and inhibits CAPZA1 to promote F-actin remodeling and tumor cell invasion, linking it to cytoskeletal dynamics and disease relevant phenotypes.

    Evidence Co-immunoprecipitation, actin capping assays, CPI-domain mutagenesis, invasion/migration assays, and xenograft models

    PMID:35096613

    Open questions at the time
    • Whether CAPZA1 inhibition is coupled to retromer/WASH-dependent sorting at endosomes not established
    • Reciprocal/endogenous validation of the interaction limited to single-lab co-IP

Open questions

Synthesis pass · forward-looking unresolved questions
  • How WASHC2C integrates its retromer-bridging, WASH-recruitment, and CAPZA1-inhibitory activities into a single coordinated fission/sorting event, and the structural basis of these interfaces, remain unresolved.
  • No structural model of the C-tail–retromer or CPI–CAPZA1 interfaces
  • Whether actin regulation and cargo sorting are mechanistically coupled is untested

Mechanism profile

Synthesis pass · controlled-vocabulary classification · explore literature graph →
Molecular activity
GO:0060090 molecular adaptor activity 2 GO:0008092 cytoskeletal protein binding 1 GO:0098772 molecular function regulator activity 1
Localization
GO:0005768 endosome 3 GO:0005886 plasma membrane 1 GO:0031410 cytoplasmic vesicle 1
Pathway
R-HSA-5653656 Vesicle-mediated transport 2 R-HSA-9609507 Protein localization 1
Partners
CAPZA1FKBP15
Complex memberships
WASH complex

Evidence

Reading pass · 5 per-paper findings extracted from the source corpus
Year Finding Method Journal Conf PMIDs
2008 VPEF (WASHC2C/FAM21C) was detected on cell surface lipid rafts and on vesicle-like structures in the cytoplasm, and knockdown of VPEF blocked vaccinia virus penetration and intracellular transport of dextran, indicating VPEF mediates fluid phase (macropinocytic) endocytosis. Intracellular VPEF-containing vesicles partially colocalized with Rab11 but not Rab5a or caveolin, placing VPEF in recycling endosome trafficking. siRNA knockdown with virus penetration and dextran uptake assays; confocal colocalization with Rab5a, Rab11, caveolin markers; cell surface lipid raft fractionation Journal of virology Medium 18550675
2015 VPEF/FAM21C (WASHC2C) recruits WASH and retromer protein complexes to early endosomes, and this WASH–VPEF/FAM21–retromer complex mediates endosomal membrane fission and cargo sorting into Rab11- and Rab22-positive recycling pathways. Functional interference with VPEF/FAM21 blocked sorting of vaccinia virus-containing vesicles prior to membrane fusion. Live single-particle fluorescence imaging; functional interference assays (dominant-negative constructs, siRNA knockdown) of WASH, FAM21, retromer components; colocalization with Rab11, Rab22, early endosome markers Journal of virology Medium 26041286
2016 The C-tail of FAM21C (WASHC2C) is required for complexing retromer to the WASH pentamer on endosomal membranes, and this FAM21C–retromer–WASH interaction is necessary for recycling of WT β1-AR and β2-AR from endosomes to the plasma membrane. Additionally, FKBP15 was identified as a FAM21C-binding endosomal protein that selectively regulates WT β1-AR (but not β2-AR) recycling. siRNA knockdown of FAM21C and FKBP15; receptor recycling assays (radioligand binding); epistasis with SNX3, Rab7a, SNX27 Cellular signalling Medium 27816670
2020 Retromer-binding segments of WASHC2C were used in a reconstituted supported-lipid-bilayer system, and neither WASHC2C segments nor other accessory factors substantially affected retromer oligomerization state, indicating that WASHC2C does not potentiate retromer oligomerization on membranes. Quantitative single-particle fluorescence microscopy on supported lipid bilayers with purified fluorescently-labeled retromer, SNX3, RAB7, and retromer-binding segments of WASHC2C The Journal of biological chemistry Medium 32651229
2022 FAM21C (WASHC2C) interacts with CAPZA1 (capping protein alpha-1) via its CP-interacting (CPI) domain, and this binding inhibits the actin-filament capping capacity of CAPZA1, thereby promoting F-actin cytoskeleton remodeling, cell invasion and migration. Mutation of the CPI domain on FAM21C abolished its interaction with CAPZA1 and eliminated the pro-invasive effect. Co-immunoprecipitation; actin capping assays; CPI-domain mutagenesis; in vitro invasion/migration assays; in vivo xenograft models Frontiers in oncology Medium 35096613

Source papers

Stage 0 corpus · 10 papers · ranked by NIH iCite citations
Year Title Journal Citations PMID
2008 A novel cellular protein, VPEF, facilitates vaccinia virus penetration into HeLa cells through fluid phase endocytosis. Journal of virology 80 18550675
2010 Evolutionary conservation of the WASH complex, an actin polymerization machine involved in endosomal fission. Communicative & integrative biology 33 20714399
2015 Intracellular Transport of Vaccinia Virus in HeLa Cells Requires WASH-VPEF/FAM21-Retromer Complexes and Recycling Molecules Rab11 and Rab22. Journal of virology 30 26041286
2017 Effects of probiotics on ghrelin and lungs in children with acute lung injury: A double-blind randomized, controlled trial. Pediatric pulmonology 18 29193877
2016 Two barcodes encoded by the type-1 PDZ and by phospho-Ser312 regulate retromer/WASH-mediated sorting of the ß1-adrenergic receptor from endosomes to the plasma membrane. Cellular signalling 16 27816670
2020 Retromer forms low order oligomers on supported lipid bilayers. The Journal of biological chemistry 14 32651229
2022 FAM21C Promotes Hepatocellular Carcinoma Invasion and Metastasis by Driving Actin Cytoskeleton Remodeling via Inhibiting Capping Ability of CAPZA1. Frontiers in oncology 6 35096613
2017 Genetic analysis of VCP and WASH complex genes in a German cohort of sporadic ALS-FTD patients. Neurobiology of aging 6 28551275
2025 Transcriptome Analysis Reveals Circadian Rhythmic Regulation of Lipid Metabolism and Immune Function in Chicken Livers. Animals : an open access journal from MDPI 1 41301950
2025 Association of the endosomal sorting processes cargo selection and membrane tubulation with human reward system reactivity. European archives of psychiatry and clinical neuroscience 0 41081810

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