A network of transcriptional and signaling events is activated by FGF to induce chondrocyte growth arrest and differentiation

Activating mutations in FGF receptor 3 (FGFR3) cause several human dwarfism syndromes by affecting both chondrocyte proliferation and differentiation. Using microarray and biochemical analyses of FGF-treated rat chondrosarcoma chondrocytes, we show that FGF inhibits chondrocyte proliferation by initiating multiple pathways that result in the induction of antiproliferative functions and the down-regulation of growth-promoting molecules. The initiation of growth arrest is characterized by the rapid dephosphorylation of the retinoblastoma protein (pRb) p107 and repression of a subset of E2F target genes by a mechanism that is independent of cyclin E–Cdk inhibition. In contrast, hypophosphorylation of pRb and p130 occur after growth arrest is first detected, and may contribute to its maintenance. Importantly, we also find a number of gene expression changes indicating that FGF promotes many aspects of hypertrophic differentiation, a notion supported by in situ analysis of developing growth plates from mice expressing an activated form of FGFR3. Thus, FGF may coordinate the onset of differentiation with chondrocyte growth arrest in the developing growth plate

FGF signaling targets the pRb-related p107 and p130 proteins to induce chondrocyte growth arrest

Unregulated FGF signaling affects endochondral ossification and long bone growth, causing several genetic forms of human dwarfism. One major mechanism by which FGFs regulate endochondral bone growth is through their inhibitory effect on chondrocyte proliferation. Because mice with targeted mutations of the retinoblastoma (Rb)-related proteins p107 and p130 present severe endochondral bone defects with excessive chondrocyte proliferation, we have investigated the role of the Rb family of cell cycle regulators in the FGF response. Using a chondrocyte cell line, we found that FGF induced a rapid dephosphorylation of all three proteins of the Rb family (pRb, p107, and p130) and a blockade of the cells in the G1 phase of the cell cycle. This cell cycle block was reversed by inactivation of Rb proteins with viral oncoproteins such as polyoma large T (PyLT) antigen and Adenovirus E1A. Expression of a PyLT mutant that efficiently binds pRb, but not p107 and p130, allowed the cells to be growth inhibited by FGF, suggesting that pRb itself is not involved in the FGF response. To investigate more precisely the role of the individual Rb family proteins in FGF-mediated growth inhibition, we used chondrocyte micromass culture of limb bud cells isolated from mice lacking Rb proteins individually or in combination. Although wild-type as well as Rb−/− chondrocytes were similarly growth inhibited by FGF, chondrocytes null for p107 and p130 did not respond to FGF. Furthermore, FGF treatment of metatarsal bone rudiments obtained from p107−/−;p130−/− embryos failed to inhibit proliferation of growth plate chondrocytes, whereas rudiments from p107-null or p130-null embryos showed only a slight inhibition of growth. Our findings indicate that p107 and p130, but not pRb, are critical effectors of FGF-mediated growth inhibition in chondrocytes

Two NEMO-like Ubiquitin-Binding Domains in CEP55 Differently Regulate Cytokinesis

International audience(F.A.) HIGHLIGHTS CEP55 contains two NEMO-like NOA and UBZ domains CEP55 NOA and UBZ are crucial for the CEP55 function in cytokinetic coordination UBZ CEP55 functions as cargo receptor to the midbody in a ubiquitin-dependent manner UBZ CEP55 preferentially binds non-degradative linear and K63 polyubiquitin chains Said Halidi et al., iScience 20, SUMMARY CEP55 regulates the final critical step of cell division termed cytokinetic abscission. We report herein that CEP55 contains two NEMO-like ubiquitin-binding domains (UBDs), NOA and ZF, which regulate its function in a different manner. In vitro studies of isolated domains showed that NOA adopts a dimeric coiled-coil structure, whereas ZF is based on a UBZ scaffold. Strikingly, CEP55 knocked-down HeLa cells reconstituted with the full-length CEP55 ubiquitin-binding defective mutants, containing structure-guided mutations either in NOA CEP55 or ZF CEP55 domains, display severe abscission defects. In addition, the ZF CEP55 can be functionally replaced by some ZF-based UBDs belonging to the UBZ family, indicating that the essential function of ZF CEP55 is to act as ubiquitin receptor. Our work reveals an unexpected role of CEP55 in non-degradative ubiquitin signaling during cytokinetic abscis-sion and provides a molecular basis as to how CEP55 mutations can lead to neurological disorders such as the MARCH syndrome

Immunodeficiency, auto-inflammation and amylopectinosis in humans with inherited HOIL-1 and LUBAC deficiency

We report the clinical description and molecular dissection of a new fatal human inherited disorder characterized by chronic auto-inflammation, invasive bacterial infections and muscular amylopectinosis. Patients from two kindreds carried biallelic loss-of-expression and loss-of-function mutations in HOIL1, a component the linear ubiquitination chain assembly complex (LUBAC). These mutations resulted in impairment of LUBAC stability. NF-κB activation in response to interleukin-1β (IL-1β) was compromised in the patients’ fibroblasts. By contrast, the patients’ mononuclear leukocytes, particularly monocytes, were hyperresponsive to IL-1β. The consequences of human HOIL-1 and LUBAC deficiencies for IL-1β responses thus differed between cell types, consistent with the unique association of auto-inflammation and immunodeficiency in these patients. These data suggest that LUBAC regulates NF-κB-dependent IL-1β responses differently in different cell types

Human OTULIN haploinsufficiency impairs cell-intrinsic immunity to staphylococcal alpha-toxin

The molecular basis of interindividual clinical variability upon infection with Staphylococcus aureus is unclear. We describe patients with haploinsufficiency for the linear deubiquitinase OTULIN, encoded by a gene on chromosome 5p. Patients suffer from episodes of life-threatening necrosis, typically triggered by S. aureus infection. The disorder is phenocopied in patients with the 5p- (Cri-du-Chat) chromosomal deletion syndrome. OTULIN haploinsufficiency causes an accumulation of linear ubiquitin in dermal fibroblasts, but tumor necrosis factor receptor-mediated nuclear factor kappa B signaling remains intact. Blood leukocyte subsets are unaffected. The OTULIN-dependent accumulation of caveolin-1 in dermal fibroblasts, but not leukocytes, facilitates the cytotoxic damage inflicted by the staphylococcal virulence factor alpha-toxin. Naturally elicited antibodies against alpha-toxin contribute to incomplete clinical penetrance. Human OTULIN haploinsufficiency underlies life-threatening staphylococcal disease by disrupting cell-intrinsic immunity to alpha-toxin in nonleukocytic cells.Peer reviewe

INTERACTIONS AU NIVEAU DES DOMAINES INTRACELLULAIRES DES SOUS-UNITES ALPHA3A, ALPHA6A ET BETA1A DES INTEGRINES

LES ADHESIONS FOCALES (AF) CONSTITUENT UN LIEN ESSENTIEL ENTRE LA MATRICE EXTRACELLULAIRE ET LE CYTOSQUELETTE, AINSI QUE LE SITE DE TRANSMISSION DE SIGNAUX PAR LES INTEGRINES. LES INTEGRINES 31 ET 61, RECEPTEURS DES LAMININES, DIFFERENT DANS LEUR SPECIFICITE DE RECONNAISSANCE : LA LAMININE 1 SE LIE A L'INTEGRINE 61 SEULEMENT ET L'ADHERENCE DES CELLULES A CE SUBSTRAT ENTRAINE LA FORMATION D'AF DISTINCTES DE CELLES FORMEES SUR D'AUTRES ISOFORMES DE LAMININE LIANT A LA FOIS 31 ET 61. L'INTEGRINE 31 POURRAIT DONC REGULER DE MANIERE TRANSDOMINANTE L'INTEGRINE 61. AFIN DE TESTER CETTE HYPOTHESE, DES PEPTIDES REPRESENTANT LE DOMAINE INTRACELLULAIRE DES SOUS-UNITES 3A OU 6A D'INTEGRINES ONT ETE INJECTES DANS DES FIBROBLASTES VIVANTS ADHERES A LA LAMININE 1. SEULE LA MICROINJECTION DU PEPTIDE 3A ENTRAINE UNE REORGANISATION SPECIFIQUE DES AF, RAPPELANT CELLES FORMEES LORS DE L'ACTIVATION DU RECEPTEUR 31 PAR SES LIGANDS. DE PLUS, DES ETUDES PAR RESONANCE PLASMONIQUE DE SURFACE (SPR) PERMETTENT DE DETECTER UNE INTERACTION DIRECTE ENTRE LES PEPTIDES CORRESPONDANT AUX DOMAINES INTRACELLULAIRES DES SOUS-UNITES 3A ET 1A D'INTEGRINE. ENFIN, UN CRIBLAGE DE BANQUE D'ADNC AVEC LE DOMAINE INTRACELLULAIRE DE LA SOUS-UNITE 3A COMME AMORCE DANS LE SYSTEME DOUBLE HYBRIDE CHEZ LA LEVURE, A PERMIS L'IDENTIFICATION DE PLUSIEURS PARTENAIRES D'INTERACTION. PARMI CEUX-CI, LA PROTEINE DRAL/FHL2 INTERAGIT AVEC L'INTEGRINE 31 IN VIVO. EN CONCLUSION, DIFFERENTES INTERACTIONS SPECIFIQUES AU DOMAINE INTRACELLULAIRE DE LA SOUS-UNITE 3A, CONTRIBUENT A LA REGULATION DE L'ORGANISATION DES AF PAR L'INTEGRINE 31. PAR AILLEURS, NOUS AVONS EXAMINE LA CONTRIBUTION DU DOMAINE INTRACELLULAIRE DE LA SOUS-UNITE 1A DANS LE PHENOMENE DE CLUSTERING DES INTEGRINES. DES ANALYSES EN SPR REVELENT UNE AFFINITE DU DOMAINE INTRACELLULAIRE DE 1A POUR LUI-MEME. DES EXPERIENCES EN GEL FILTRATION ET EN SDS-PAGE MONTRENT QUE CE DOMAINE FORME DES MULTIMERES QUI, D'APRES DES MESURES EN DICHROISME CIRCULAIRE, ADOPTENT UNE STRUCTURE EN HELICE . L'OLIGOMERISATION ET LE CHANGEMENT DE STRUCTURE SECONDAIRE DU DOMAINE INTRACELLULAIRE DE LA SOUS-UNITE 1A POURRAIENT INTERVENIR DE MANIERE ACTIVE DANS L'AGREGATION DES INTEGRINES ET LA FORMATION DES AF.PARIS-BIUSJ-Thèses (751052125) / SudocCentre Technique Livre Ens. Sup. (774682301) / SudocPARIS-BIUSJ-Physique recherche (751052113) / SudocSudocFranceF

PP2A-Mediated Dephosphorylation of p107 Plays a Critical Role in Chondrocyte Cell Cycle Arrest by FGF

FGF signaling inhibits chondrocyte proliferation, a cell type-specific response that is the basis for several genetic skeletal disorders caused by activating FGFR mutations. This phenomenon requires the function of the p107 and p130 members of the Rb protein family, and p107 dephosphorylation is one of the earliest distinguishing events in FGF-induced growth arrest. To determine whether p107 dephoshorylation played a critical role in the chondrocyte response to FGF, we sought to counteract this process by overexpressing in RCS chondrocytes the cyclin D1/cdk4 kinase complex. CyclinD/cdk4-expressing RCS cells became resistant to FGF-induced p107 dephosphorylation and growth arrest, and maintained significantly high levels of cyclin E/cdk2 activity and of phosphorylated p130 at later times of FGF treatment. We explored the involvement of a phosphatase in p107 dephosphorylation. Expression of the SV40 small T-Ag, which inhibits the activity of the PP2A phosphatase, or knockdown of the expression of the PP2A catalytic subunit by RNA interference prevented p107 dephosphorylation and FGF-induced growth arrest of RCS cells. Furthermore, an association between p107 and PP2A was induced by FGF treatment. Our data show that p107 dephosphorylation is a key event in FGF-induced cell cycle arrest an

Role of Optineurin in the Mitochondrial Dysfunction: Potential implications in Neurodegenerative Diseases and Cancer

International audienceOptineurin (Optn) is a 577 aa protein encoded by the Optn gene. Mutations of Optn are associated with normal tension glaucoma and amyotrophic lateral sclerosis, and its gene has also been linked to the development of Paget's disease of bone and Crohn's disease. Optn is involved in diverse cellular functions, including NF-κB regulation, membrane trafficking , exocytosis, vesicle transport, reorganization of actin and microtubules, cell cycle control, and autophagy. Besides its role in xenophagy and autophagy of aggregates, Optn has been identified as a primary autophagy receptor, among the five adaptors that translocate to mitochondria during mitophagy. Mitophagy is a selective macroauto-phagy process during which irreparable mitochondria are degraded, preventing accumulation of defective mitochondria and limiting the release of reactive oxygen species and proapoptotic factors. Mitochondrial quality control via mitophagy is central to the health of cells. One of the important surveillance pathways of mitochondrial health is the recently defined signal transduction pathway involving the mitochondrial PTEN-induced putative kinase 1 (PINK1) protein and the cytosolic RING-between-RING ubiquitin ligase Parkin. Both of these proteins, when mutated, have been identified in certain forms of Parkinson's disease. By targeting ubiquitinated mitochondria to autophagosomes through its association with autophagy related proteins, Optn is responsible for a critical step in mitophagy. This review reports recent discoveries on the role of Optn in mito-phagy and provides insight into its link with neurodegenerative diseases. We will also discuss the involvement of Optn in other pathologies in which mitophagy dysfunctions are involved including cancer