RÉSUMÉ
Oral cancer patients suffer pain at the site of the cancer. Calcitonin gene related polypeptide (CGRP), a neuropeptide expressed by a subset of primary afferent neurons, promotes oral cancer growth. CGRP also mediates trigeminal pain (migraine) and neurogenic inflammation. The contribution of CGRP to oral cancer pain is investigated in the present study. The findings demonstrate that CGRP-immunoreactive (-ir) neurons and neurites innervate orthotopic oral cancer xenograft tumors in mice. Cancer increases anterograde transport of CGRP in axons innervating the tumor, supporting neurogenic secretion as the source of CGRP in the oral cancer microenvironment. CGRP antagonism reverses oral cancer nociception in preclinical oral cancer pain models. Single-cell RNA-sequencing is used to identify cell types in the cancer microenvironment expressing the CGRP receptor components, receptor activity modifying protein 1 Ramp1 and calcitonin receptor like receptor (CLR, encoded by Calcrl). Ramp1 and Calcrl transcripts are detected in cells expressing marker genes for Schwann cells, endothelial cells, fibroblasts and immune cells. Ramp1 and Calcrl transcripts are more frequently detected in cells expressing fibroblast and immune cell markers. This work identifies CGRP as mediator of oral cancer pain and suggests the antagonism of CGRP to alleviate oral cancer pain.
Sujet(s)
Douleur cancéreuse , Tumeurs de la bouche , Hormones peptidiques , Humains , Souris , Animaux , Peptide relié au gène de la calcitonine/métabolisme , Calcitonine , Procalcitonine , Récepteurs du peptide relié au gène de la calcitonine/génétique , Récepteurs du peptide relié au gène de la calcitonine/métabolisme , Douleur cancéreuse/traitement médicamenteux , Cellules endothéliales/métabolisme , Tumeurs de la bouche/traitement médicamenteux , Microenvironnement tumoralRÉSUMÉ
Transforming growth factor-beta (TGFß) is released from cells as part of a trimeric latent complex consisting of TGFß, the TGFß propeptides, and either a latent TGFß binding protein (LTBP) or glycoprotein-A repetitions predominant (GARP) protein. LTBP1 and 3 modulate latent TGFß function with respect to secretion, matrix localization, and activation and, therefore, are vital for the proper function of the cytokine in a number of tissues. TGFß modulates stem cell differentiation into adipocytes (adipogenesis), but the potential role of LTBPs in this process has not been studied. We observed that 72â¯h post adipogenesis initiation Ltbp1, 2, and 4 expression levels decrease by 74-84%, whereas Ltbp3 expression levels remain constant during adipogenesis. We found that LTBP3 silencing in C3H/10T1/2 cells reduced adipogenesis, as measured by the percentage of cells with lipid vesicles and the expression of the transcription factor peroxisome proliferator-activated receptor gamma (PPARγ). Lentiviral mediated expression of an Ltbp3 mRNA resistant to siRNA targeting rescued the phenotype, validating siRNA specificity. Knockdown (KD) of Ltbp3 expression in 3T3-L1, M2, and primary bone marrow stromal cells (BMSC) indicated a similar requirement for Ltbp3. Epididymal and inguinal white adipose tissue fat pad weights of Ltbp3-/- mice were reduced by 62% and 57%, respectively, compared to wild-type mice. Inhibition of adipogenic differentiation upon LTBP3 loss is mediated by TGFß, as TGFß neutralizing antibody and TGFß receptor I kinase blockade rescue the LTBP3 KD phenotype. These results indicate that LTBP3 has a TGFß-dependent function in adipogenesis both in vitro and possibly in vivo. SIGNIFICANCE: Understanding the control of mesenchymal stem cell fate is crucial for the potential use of these cells for regenerative medicine.
Sujet(s)
Adipogenèse , Récepteur PPAR gamma , Adipogenèse/génétique , Animaux , Anticorps neutralisants , Différenciation cellulaire , Lipides , Souris , Souris de lignée C3H , Récepteur PPAR gamma/génétique , Récepteur PPAR gamma/métabolisme , ARN messager/génétique , Petit ARN interférent , Facteurs de transcription , Facteur de croissance transformant bêta/métabolisme , Facteur de croissance transformant bêta-3 , Facteurs de croissance transformantsRÉSUMÉ
Membrane-type 1 matrix metalloproteinase (MT1-MMP, MMP-14), a transmembrane proteinase with a short cytoplasmic tail, is a major effector of extracellular matrix remodeling. Genetic silencing of MT1-MMP in mouse (Mmp14 -/- ) and man causes dwarfism, osteopenia, arthritis, and lipodystrophy, abnormalities ascribed to defective collagen turnover. We have previously shown non-proteolytic functions of MT1-MMP mediated by its cytoplasmic tail, where the unique tyrosine (Y573) controls intracellular signaling. The Y573D mutation blocks TIMP-2/MT1-MMP-induced Erk1/2 and Akt signaling without affecting proteolytic activity. Here, we report that a mouse with the MT1-MMP Y573D mutation (Mmp14 Y573D/Y573D ) shows abnormalities similar to but also different from those of Mmp14 -/- mice. Skeletal stem cells (SSC) of Mmp14 Y573D/Y573D mice show defective differentiation consistent with the mouse phenotype, which is rescued by wild-type SSC transplant. These results provide the first in vivo demonstration that MT1-MMP modulates bone, cartilage, and fat homeostasis by controlling SSC differentiation through a mechanism independent of proteolysis.
RÉSUMÉ
Latent transforming growth factor ß (TGFß)-binding proteins (LTBPs) are important for the secretion, activation, and function of mature TGFß, especially so in cancer cell physiology. However, specific roles of the LTBPs remain understudied in the context of the primary tumor microenvironment. Herein, we investigated the role of LTBP3 in the distinct processes involved in cancer metastasis. By using three human tumor cell lines of different tissue origin (epidermoid HEp-3 and prostate PC-3 carcinomas and HT-1080 fibrosarcoma) and several metastasis models conducted in both mammalian and avian settings, we show that LTBP3 is involved in the early dissemination of primary cancer cells, namely in the intravasation step of the metastatic cascade. Knockdown of LTBP3 in all tested cell lines led to significant inhibition of tumor cell intravasation, but did not affect primary tumor growth. LTBP3 was dispensable in the late steps of carcinoma cell metastasis that follow tumor cell intravasation, including vascular arrest, extravasation, and tissue colonization. However, LTBP3 depletion diminished the angiogenesis-inducing potential of HEp-3 cells in vivo, which was restorable by exogenous delivery of LTBP3 protein. A similar compensatory approach rescued the dampened intravasation of LTBP3-deficient HEp-3 cells, suggesting that LTBP3 regulates the induction of the intravasation-supporting angiogenic vasculature within developing primary tumors. Using our recently developed microtumor model, we confirmed that LTBP3 loss resulted in the development of intratumoral vessels with an abnormal microarchitecture incompatible with efficient intravasation of HEp-3 carcinoma cells. Collectively, these findings demonstrate that LTBP3 represents a novel oncotarget that has distinctive functions in the regulation of angiogenesis-dependent tumor cell intravasation, a critical process during early cancer dissemination. Our experimental data are also consistent with the survival prognostic value of LTBP3 expression in early-stage head and neck squamous cell carcinomas, further indicating a specific role for LTBP3 in cancer progression toward metastatic disease.
Sujet(s)
Protéines de liaison au TGF-bêta latent/physiologie , Tumeurs/génétique , Tumeurs/anatomopathologie , Animaux , Lignée cellulaire tumorale , Embryon de poulet , Femelle , Régulation de l'expression des gènes tumoraux/effets des médicaments et des substances chimiques , Humains , Protéines de liaison au TGF-bêta latent/antagonistes et inhibiteurs , Protéines de liaison au TGF-bêta latent/génétique , Souris , Souris de lignée NOD , Souris SCID , Invasion tumorale , Métastase tumorale , Tumeurs/mortalité , Néovascularisation pathologique/génétique , Néovascularisation pathologique/anatomopathologie , Petit ARN interférent/pharmacologie , Analyse de survieRÉSUMÉ
Pulsed electromagnetic fields (PEMFs) have been documented to promote bone fracture healing in nonunions and increase lumbar spinal fusion rates. However, the molecular mechanisms by which PEMF stimulates differentiation of human bone marrow stromal cells (hBMSCs) into osteoblasts are not well understood. In this study the PEMF effects on hBMSCs were studied by microarray analysis. PEMF stimulation of hBMSCs' cell numbers mainly affected genes of cell cycle regulation, cell structure, and growth receptors or kinase pathways. In the differentiation and mineralization stages, PEMF regulated preosteoblast gene expression and notably, the transforming growth factor-beta (TGF-ß) signaling pathway and microRNA 21 (miR21) were most highly regulated. PEMF stimulated activation of Smad2 and miR21-5p expression in differentiated osteoblasts, and TGF-ß signaling was essential for PEMF stimulation of alkaline phosphatase mRNA expression. Smad7, an antagonist of the TGF-ß signaling pathway, was found to be miR21-5p's putative target gene and PEMF caused a decrease in Smad7 expression. Expression of Runx2 was increased by PEMF treatment and the miR21-5p inhibitor prevented the PEMF stimulation of Runx2 expression in differentiating cells. Thus, PEMF could mediate its effects on bone metabolism by activation of the TGF-ß signaling pathway and stimulation of expression of miR21-5p in hBMSCs.
RÉSUMÉ
Latent-transforming growth factor beta-binding protein 3 (LTBP-3) is important for craniofacial morphogenesis and hard tissue mineralization, as it is essential for activation of transforming growth factor-ß (TGF-ß). To investigate the role of LTBP-3 in tooth formation we performed micro-computed tomography (micro-CT), histology, and scanning electron microscopy analyses of adult Ltbp3-/- mice. The Ltbp3-/- mutants presented with unique craniofacial malformations and reductions in enamel formation that began at the matrix formation stage. Organization of maturation-stage ameloblasts was severely disrupted. The lateral side of the incisor was affected most. Reduced enamel mineralization, modification of the enamel prism pattern, and enamel nodules were observed throughout the incisors, as revealed by scanning electron microscopy. Molar roots had internal irregular bulbous-like formations. The cementum thickness was reduced, and microscopic dentinal tubules showed minor nanostructural changes. Thus, LTBP-3 is required for ameloblast differentiation and for the formation of decussating enamel prisms, to prevent enamel nodule formation, and for proper root morphogenesis. Also, and consistent with the role of TGF-ß signaling during mineralization, almost all craniofacial bone components were affected in Ltbp3-/- mice, especially those involving the upper jaw and snout. This mouse model demonstrates phenotypic overlap with Verloes Bourguignon syndrome, also caused by mutation of LTBP3, which is hallmarked by craniofacial anomalies and amelogenesis imperfecta phenotypes.
Sujet(s)
Amélogenèse/génétique , Émail dentaire/malformations , Protéines de liaison au TGF-bêta latent/génétique , Améloblastes/métabolisme , Amélogenèse imparfaite/génétique , Animaux , Émail dentaire/ultrastructure , Génotype , Mâle , Souris , Souches mutantes de souris , Microscopie électronique à balayage , Mutation , Ostéochondrodysplasies/génétique , Phénotype , Calcification dentaire/génétique , Facteur de croissance transformant bêta/génétique , Microtomographie aux rayons XRÉSUMÉ
Marfan syndrome (MFS) is an autosomal dominant disorder of connective tissue, caused by mutations of the microfibrillar protein fibrillin-1, that predisposes affected individuals to aortic aneurysm and rupture and is associated with increased TGFß signaling. TGFß is secreted from cells as a latent complex consisting of TGFß, the TGFß propeptide, and a molecule of latent TGFß binding protein (LTBP). Improper extracellular localization of the latent complex can alter active TGFß levels, and has been hypothesized as an explanation for enhanced TGFß signaling observed in MFS. We previously reported the absence of LTBP-3 in matrices lacking fibrillin-1, suggesting that perturbed TGFß signaling in MFS might be due to defective interaction of latent TGFß complexes containing LTBP-3 with mutant fibrillin-1 microfibrils. To test this hypothesis, we genetically suppressed Ltbp3 expression in a mouse model of progressively severe MFS. Here, we present evidence that MFS mice lacking LTBP-3 have improved survival, essentially no aneurysms, reduced disruption and fragmentation of medial elastic fibers, and decreased Smad2/3 and Erk1/2 activation in their aortas. These data suggest that, in MFS, improper localization of latent TGFß complexes composed of LTBP-3 and TGFß contributes to aortic disease progression.
Sujet(s)
Anévrysme de l'aorte thoracique/métabolisme , Protéines de liaison au TGF-bêta latent/métabolisme , Syndrome de Marfan/complications , Syndrome de Marfan/génétique , Complexes multiprotéiques/métabolisme , Facteur de croissance transformant bêta/métabolisme , Analyse de variance , Animaux , Anévrysme de l'aorte thoracique/étiologie , ADN complémentaire/biosynthèse , Fibrilline-1 , Fibrillines , Immunohistochimie , Protéines de liaison au TGF-bêta latent/déficit , Souris , Protéines des microfilaments/génétique , Muscles lisses vasculaires/cytologie , Réaction de polymérisation en chaine en temps réelRÉSUMÉ
The LTBPs (or latent transforming growth factor ß binding proteins) are important components of the extracellular matrix (ECM) that interact with fibrillin microfibrils and have a number of different roles in microfibril biology. There are four LTBPs isoforms in the human genome (LTBP-1, -2, -3, and -4), all of which appear to associate with fibrillin and the biology of each isoform is reviewed here. The LTBPs were first identified as forming latent complexes with TGFß by covalently binding the TGFß propeptide (LAP) via disulfide bonds in the endoplasmic reticulum. LAP in turn is cleaved from the mature TGFß precursor in the trans-golgi network but LAP and TGFß remain strongly bound through non-covalent interactions. LAP, TGFß, and LTBP together form the large latent complex (LLC). LTBPs were originally thought to primarily play a role in maintaining TGFß latency and targeting the latent growth factor to the extracellular matrix (ECM), but it has also been shown that LTBP-1 participates in TGFß activation by integrins and may also regulate activation by proteases and other factors. LTBP-3 appears to have a role in skeletal formation including tooth development. As well as having important functions in TGFß regulation, TGFß-independent activities have recently been identified for LTBP-2 and LTBP-4 in stabilizing microfibril bundles and regulating elastic fiber assembly.
Sujet(s)
Protéines de liaison au TGF-bêta latent/physiologie , Animaux , Matrice extracellulaire/physiologie , Fibrillines , Humains , Protéines des microfilaments/physiologie , Isoformes de protéines/physiologie , Transduction du signal , Facteur de croissance transformant bêta/physiologieRÉSUMÉ
Mutations in the gene for the latent transforming growth factor beta binding protein 4 (LTBP4) cause autosomal recessive cutis laxa type 1C. To understand the molecular disease mechanisms of this disease, we investigated the impact of LTBP4 loss on transforming growth factor beta (TGFß) signaling. Despite elevated extracellular TGFß activity, downstream signaling molecules of the TGFß pathway, including pSMAD2 and pERK, were down-regulated in LTBP4 mutant human dermal fibroblasts. In addition, TGFß receptors 1 and 2 (TGFBR1 and TGFBR2) were reduced at the protein but not at the ribonucleic acid level. Treatment with exogenous TGFß1 led to an initially rapid increase in SMAD2 phosphorylation followed by a sustained depression of phosphorylation and receptor abundance. In mutant cells TGFBR1 was co-localized with lysosomes. Treatment with a TGFBR1 kinase inhibitor, endocytosis inhibitors or a lysosome inhibitor, normalized the levels of TGFBR1 and TGFBR2. Co-immunoprecipitation demonstrated a molecular interaction between LTBP4 and TGFBR2. Knockdown of LTBP4 reduced TGFß receptor abundance and signaling in normal cells and supplementation of recombinant LTBP4 enhanced these measures in mutant cells. In a mouse model of Ltbp4 deficiency, reduced TGFß signaling and receptor levels were normalized upon TGFBR1 kinase inhibitor treatment. Our results show that LTBP4 interacts with TGFBR2 and stabilizes TGFß receptors by preventing their endocytosis and lysosomal degradation in a ligand-dependent and receptor kinase activity-dependent manner. These findings identify LTBP4 as a key molecule required for the stability of the TGFß receptor complex, and a new mechanism by which the extracellular matrix regulates cytokine receptor signaling.
Sujet(s)
Cutis laxa/génétique , Protéines de liaison au TGF-bêta latent/métabolisme , Protein-Serine-Threonine Kinases/métabolisme , Récepteurs TGF-bêta/métabolisme , Animaux , Études cas-témoins , Cellules cultivées , Modèles animaux de maladie humaine , Régulation négative , Endocytose/génétique , Femelle , Fibroblastes/cytologie , Fibroblastes/métabolisme , Humains , Immunoprécipitation , Protéines de liaison au TGF-bêta latent/génétique , Mâle , Souris , Souris knockout , Mutation , Phosphorylation , Protein-Serine-Threonine Kinases/génétique , Récepteur de type I du facteur de croissance transformant bêta , Récepteur de type II du facteur de croissance transformant bêta , Récepteurs TGF-bêta/génétique , Transduction du signal , Protéine Smad2/génétique , Protéine Smad2/métabolismeRÉSUMÉ
Inherited dental malformations constitute a clinically and genetically heterogeneous group of disorders. Here, we report on four families, three of them consanguineous, with an identical phenotype, characterized by significant short stature with brachyolmia and hypoplastic amelogenesis imperfecta (AI) with almost absent enamel. This phenotype was first described in 1996 by Verloes et al. as an autosomal recessive form of brachyolmia associated with AI. Whole-exome sequencing resulted in the identification of recessive hypomorphic mutations including deletion, nonsense and splice mutations, in the LTBP3 gene, which is involved in the TGF-beta signaling pathway. We further investigated gene expression during mouse development and tooth formation. Differentiated ameloblasts synthesizing enamel matrix proteins and odontoblasts expressed the gene. Study of an available knockout mouse model showed that the mutant mice displayed very thin to absent enamel in both incisors and molars, hereby recapitulating the AI phenotype in the human disorder.
Sujet(s)
Amélogenèse imparfaite/génétique , Protéines de liaison au TGF-bêta latent/génétique , Ostéochondrodysplasies/génétique , Adolescent , Amélogenèse imparfaite/imagerie diagnostique , Animaux , Séquence nucléotidique , Enfant , Consanguinité , Analyse de mutations d'ADN , Femelle , Mutation avec décalage du cadre de lecture , Études d'associations génétiques , Humains , Mâle , Souris , Souris de lignée C57BL , Souris knockout , Mutation faux-sens , Ostéochondrodysplasies/imagerie diagnostique , Pedigree , Radiographie , Délétion de séquenceRÉSUMÉ
Mice deficient in Latent TGFß Binding Protein 4 (Ltbp4) display a defect in lung septation and elastogenesis. The lung septation defect is normalized by genetically decreasing TGFß2 levels. However, the elastic fiber assembly is not improved in Tgfb2(-/-) ;Ltbp4S(-/-) compared to Ltbp4S(-/-) lungs. We found that decreased levels of TGFß1 or TGFß3 did not improve lung septation indicating that the TGFß isoform elevated in Ltbp4S(-/-) lungs is TGFß2. Expression of a form of Ltbp4 that could not bind latent TGFß did not affect lung phenotype indicating that normal lung development does not require the formation of LTBP4-latent TGFß complexes. Therefore, the change in TGFß-level in the lungs is not directly related to Ltbp4 deficiency but probably is a consequence of changes in the extracellular matrix. Interestingly, combination of the Ltbp4S(-/-) mutation with a fibulin-5 null mutant in Fbln5(-/-) ;Ltbp4S(-/-) mice improves the lung septation compared to Ltbp4S(-/-) lungs. Large globular elastin aggregates characteristic for Ltbp4S(-/-) lungs do not form in Fbln5(-/-) ;Ltbp4S(-/-) lungs and EM studies showed that elastic fibers in Fbln5(-/-) ;Ltbp4S(-/-) lungs resemble those found in Fbln5(-/-) mice. These results are consistent with a role for TGFß2 in lung septation and for Ltbp4 in regulating fibulin-5 dependent elastic fiber assembly.
Sujet(s)
Plan d'organisation du corps/génétique , Tissu élastique/embryologie , Protéines de la matrice extracellulaire/physiologie , Protéines de liaison au TGF-bêta latent/physiologie , Poumon/embryologie , Facteur de croissance transformant bêta-2/métabolisme , Animaux , Tissu élastique/malformations , Élastine/métabolisme , Matrice extracellulaire/génétique , Matrice extracellulaire/métabolisme , Protéines de la matrice extracellulaire/génétique , Protéines de la matrice extracellulaire/métabolisme , Fibrillines , Protéines de liaison au TGF-bêta latent/génétique , Poumon/malformations , Mâle , Souris , Souris de lignée C57BL , Souris knockout , Protéines des microfilaments/métabolisme , Isoformes de protéines/biosynthèse , Isoformes de protéines/génétique , Protéines recombinantes/génétique , Transduction du signal/génétique , Facteur de croissance transformant bêta-2/génétiqueRÉSUMÉ
Elastic fiber assembly requires deposition of elastin monomers onto microfibrils, the mechanism of which is incompletely understood. Here we show that latent TGF-ß binding protein 4 (LTBP-4) potentiates formation of elastic fibers through interacting with fibulin-5, a tropoelastin-binding protein necessary for elastogenesis. Decreased expression of LTBP-4 in human dermal fibroblast cells by siRNA treatment abolished the linear deposition of fibulin-5 and tropoelastin on microfibrils. It is notable that the addition of recombinant LTBP-4 to cell culture medium promoted elastin deposition on microfibrils without changing the expression of elastic fiber components. This elastogenic property of LTBP-4 is independent of bound TGF-ß because TGF-ß-free recombinant LTBP-4 was as potent an elastogenic inducer as TGF-ß-bound recombinant LTBP-4. Without LTBP-4, fibulin-5 and tropoelastin deposition was discontinuous and punctate in vitro and in vivo. These data suggest a unique function for LTBP-4 during elastic fibrogenesis, making it a potential therapeutic target for elastic fiber regeneration.
Sujet(s)
Protéines de la matrice extracellulaire/métabolisme , Protéines de liaison au TGF-bêta latent/physiologie , Protéines recombinantes/métabolisme , Animaux , Cellules HEK293 , Humains , Protéines de liaison au TGF-bêta latent/métabolisme , Souris , Souris knockout , Liaison aux protéines , Interférence par ARNRÉSUMÉ
Fibrillin microfibrils are extracellular matrix structures with essential functions in the development and the organization of tissues including blood vessels, bone, limbs and the eye. Fibrillin-1 and fibrillin-2 form the core of fibrillin microfibrils, to which multiple proteins associate to form a highly organized structure. Defining the components of this structure and their interactions is crucial to understand the pathobiology of microfibrillopathies associated with mutations in fibrillins and in microfibril-associated molecules. In this study, we have analyzed both in vitro and in vivo the role of fibrillin microfibrils in the matrix deposition of latent TGF-ß binding protein 1 (LTBP-1), -3 and -4; the three LTBPs that form a complex with TGF-ß. In Fbn1(-/-) ascending aortas and lungs, LTBP-3 and LTBP-4 are not incorporated into a matrix lacking fibrillin-1 microfibrils, whereas LTBP-1 is still deposited. In addition, in cultures of Fbn1(-/-) smooth muscle cells or lung fibroblasts, LTBP-3 and LTBP-4 are not incorporated into a matrix lacking fibrillin-1 microfibrils, whereas LTBP-1 is still deposited. Fibrillin-2 is not involved in the deposition of LTBP-1 in Fbn1(-/-) extracellular matrix as cells deficient for both fibrillin-1 and fibrillin-2 still incorporate LTBP-1 in their matrix. However, blocking the formation of the fibronectin network in Fbn1(-/-) cells abrogates the deposition of LTBP-1. Together, these data indicate that LTBP-3 and LTBP-4 association with the matrix depends on fibrillin-1 microfibrils, whereas LTBP-1 association depends on a fibronectin network.
Sujet(s)
Fibronectines/métabolisme , Régulation de l'expression des gènes/physiologie , Protéines de liaison au TGF-bêta latent/métabolisme , Protéines des microfilaments/métabolisme , Animaux , ADN complémentaire/génétique , ADN complémentaire/métabolisme , Fibrilline-1 , Fibrilline-2 , Fibrillines , Fibroblastes/métabolisme , Fibronectines/génétique , Protéines de liaison au TGF-bêta latent/génétique , Poumon/cytologie , Souris , Souris knockout , Protéines des microfilaments/génétique , Muscles lisses vasculaires/cytologie , Myocytes du muscle lisse/métabolisme , ARN/génétique , ARN/métabolisme , Réaction de polymérisation en chaine en temps réelRÉSUMÉ
The latent TGF-ß binding proteins (LTBP-1 -3, and -4) assist in the secretion and localization of latent TGF-ß molecules. Ltbp3(-/-) and Ltbp4S(-/-) mice have distinct phenotypes and only in the lungs does deficiency of either Ltbp-3 or Ltbp-4 cause developmental abnormalities. To determine if these two LTBPs have additional common functions, we generated mice deficient for both Ltbp-3 and Ltbp-4S. The only novel defect in Ltbp3(-/-);Ltbp4S(-/-) mice was an early lethality compared to mice with single mutations. In addition lung abnormalities were exacerbated and the terminal air sac septation defect was more severe in Ltbp3(-/-);Ltbp4S(-/-) mice than in Ltbp4S(-/-) mice. Decreased cellularity of Ltbp3(-/-);Ltbp4S(-/-) lungs was correlated with higher rate of apoptosis in newborn lungs of Ltbp3(-/-);Ltbp4S(-/-) animals compared to WT, Ltbp3(-/-), and Ltbp4S(-/-) mice. No differences in the maturation of the major lung cell types were discerned between the single and double mutant mice. However, the distribution of type 2 cells and myofibroblasts was abnormal, and myofibroblast segregation in some areas might be an indication of early fibrosis. We also observed differences in ECM composition between Ltbp3(-/-);Ltbp4S(-/-) and Ltbp4S(-/-) lungs after birth, reflected in decreased incorporation of fibrillin-1 and -2 in Ltbp3(-/-);Ltbp4S(-/-) matrix. The function of the lungs of Ltbp3(-/-);Ltbp4S(-/-) mice after the first week of life was potentially further compromised by macrophage infiltration, as proteases secreted from macrophages might exacerbate developmental emphysema. Together these data indicate that LTBP-3 and -4 perform partially overlapping functions only in the lungs.
Sujet(s)
Protéines de liaison au TGF-bêta latent/métabolisme , Poumon/embryologie , Poumon/métabolisme , Animaux , Apoptose , Différenciation cellulaire , Élastine/biosynthèse , Fibroblastes/métabolisme , Régulation de l'expression des gènes au cours du développement , Inflammation/métabolisme , Inflammation/anatomopathologie , Protéines de liaison au TGF-bêta latent/déficit , Protéines de liaison au TGF-bêta latent/génétique , Poumon/anatomopathologie , Souris , Microfibrilles/métabolisme , PhénotypeRÉSUMÉ
The majority of human skeletal dysplasias are caused by dysregulation of growth plate homeostasis. As TGF-beta signaling is a critical determinant of growth plate homeostasis, skeletal dysplasias are often associated with dysregulation of this pathway. The context-dependent action of TFG-beta signaling is tightly controlled by numerous mechanisms at the extracellular level and downstream of ligand-receptor interactions. However, TGF-beta is synthesized as an inactive precursor that is cleaved to become mature in the Golgi apparatus, and the regulation of this posttranslational intracellular processing and trafficking is much less defined. Here, we report that a cysteine-rich protein, E-selectin ligand-1 (ESL-1), acts as a negative regulator of TGF-beta production by binding TGF-beta precursors in the Golgi apparatus in a cell-autonomous fashion, inhibiting their maturation. Furthermore, ESL-1 inhibited the processing of proTGF-beta by a furin-like protease, leading to reduced secretion of mature TGF-beta by primary mouse chondrocytes and HEK293 cells. In vivo loss of Esl1 in mice led to increased TGF-beta/SMAD signaling in the growth plate that was associated with reduced chondrocyte proliferation and delayed terminal differentiation. Gain-of-function and rescue studies of the Xenopus ESL-1 ortholog in the context of early embryogenesis showed that this regulation of TGF-beta/Nodal signaling was evolutionarily conserved. This study identifies what we believe to be a novel intracellular mechanism for regulating TGF-beta during skeletal development and homeostasis.
Sujet(s)
Chondrocytes/métabolisme , Lame épiphysaire/métabolisme , Homéostasie , Facteur de croissance transformant bêta/métabolisme , Facteur de croissance transformant bêta/physiologie , Animaux , Différenciation cellulaire/physiologie , Chondrocytes/cytologie , Cytoplasme/métabolisme , Sélectine E/métabolisme , Furine/métabolisme , Lame épiphysaire/cytologie , Ligands , Souris , Souris knockout , Souris transgéniques , Récepteur facteur croissance fibroblaste , Sélectines/métabolisme , Sialoglycoprotéines , Transduction du signal/physiologie , Xenopus laevisRÉSUMÉ
We report recessive mutations in the gene for the latent transforming growth factor-beta binding protein 4 (LTBP4) in four unrelated patients with a human syndrome disrupting pulmonary, gastrointestinal, urinary, musculoskeletal, craniofacial, and dermal development. All patients had severe respiratory distress, with cystic and atelectatic changes in the lungs complicated by tracheomalacia and diaphragmatic hernia. Three of the four patients died of respiratory failure. Cardiovascular lesions were mild, limited to pulmonary artery stenosis and patent foramen ovale. Gastrointestinal malformations included diverticulosis, enlargement, tortuosity, and stenosis at various levels of the intestinal tract. The urinary tract was affected by diverticulosis and hydronephrosis. Joint laxity and low muscle tone contributed to musculoskeletal problems compounded by postnatal growth delay. Craniofacial features included microretrognathia, flat midface, receding forehead, and wide fontanelles. All patients had cutis laxa. Four of the five identified LTBP4 mutations led to premature termination of translation and destabilization of the LTBP4 mRNA. Impaired synthesis and lack of deposition of LTBP4 into the extracellular matrix (ECM) caused increased transforming growth factor-beta (TGF-beta) activity in cultured fibroblasts and defective elastic fiber assembly in all tissues affected by the disease. These molecular defects were associated with blocked alveolarization and airway collapse in the lung. Our results show that coupling of TGF-beta signaling and ECM assembly is essential for proper development and is achieved in multiple human organ systems by multifunctional proteins such as LTBP4.
Sujet(s)
Derme/malformations , Intestins/malformations , Protéines de liaison au TGF-bêta latent/génétique , Poumon/malformations , Mutation , Voies urinaires/malformations , Cellules cultivées , Enfant , Enfant d'âge préscolaire , Techniques de coculture , Milieux de culture conditionnés/composition chimique , ADN/génétique , ADN/isolement et purification , Derme/métabolisme , Derme/ultrastructure , Femelle , Fibroblastes/métabolisme , Régulation de l'expression des gènes au cours du développement , Hétérozygote , Homozygote , Humains , Immunohistochimie , Nourrisson , Muqueuse intestinale/métabolisme , Protéines de liaison au TGF-bêta latent/composition chimique , Poumon/métabolisme , Mâle , Appareil locomoteur , Structure tertiaire des protéines , ARN messager/métabolisme , Analyse de séquence d'ADN , Peau/cytologie , Syndrome , Voies urinaires/métabolismeRÉSUMÉ
The latent TGF-beta binding proteins (LTBP) -1, -3, and -4 are extracellular proteins that assist in the secretion and localization of latent TGF-beta. The null mutation of LTBP-4S in mice causes defects in the differentiation of terminal air-sacs, fragmented elastin, and colon carcinomas. We investigated lung development from embryonic day 14.5 (E14.5) to day 7 after birth (P7) in order to determine when the defects in elastin organization initiate and to further examine the relation of TGF-beta signaling levels and air-sac septation in Ltbp4S-/- lungs. We found that defects in elastogenesis are visible as early as E14.5 and are maintained in the alveolar walls, in blood vessel media, and subjacent airway epithelium. The air-sac septation defect was associated with excessive TGF-beta signaling and was reversed by lowering TGF-beta2 levels. Thus, the phenotype is not directly reflective of a change in TGF-beta1, the only TGF-beta isoform known to complex with LTBP-4. Reversal of the air-sac septation defect was not associated with normalization of the elastogenesis indicating two separate functions of LTBP-4 as a regulator of elastic fiber assembly and TGF-beta levels in lungs.
Sujet(s)
Élastine/métabolisme , Protéines de liaison au TGF-bêta latent/métabolisme , Poumon/embryologie , Poumon/croissance et développement , Isoformes de protéines/métabolisme , Facteur de croissance transformant bêta/métabolisme , Animaux , Benzamides/métabolisme , Dioxoles/métabolisme , Élastine/génétique , Élastine/ultrastructure , Femelle , Protéines de liaison au TGF-bêta latent/génétique , Poumon/anatomie et histologie , Poumon/métabolisme , Mâle , Souris , Souris knockout , Phénotype , Grossesse , Isoformes de protéines/génétique , Protein-Serine-Threonine Kinases/antagonistes et inhibiteurs , Protein-Serine-Threonine Kinases/métabolisme , Alvéoles pulmonaires/physiologie , Alvéoles pulmonaires/ultrastructure , Récepteur de type I du facteur de croissance transformant bêta , Récepteurs TGF-bêta/antagonistes et inhibiteurs , Récepteurs TGF-bêta/métabolisme , Transduction du signal/physiologie , Facteur de croissance transformant bêta/génétiqueRÉSUMÉ
Transforming growth factor-beta (TGF-beta) activity is controlled at many levels including the conversion of the latent secreted form to its active state. TGF-beta is often released as part of an inactive tripartite complex consisting of TGF-beta, the TGF-beta propeptide, and a molecule of latent TGF-beta binding protein (LTBP). The interaction of TGF-beta and its cleaved propeptide renders the growth factor latent, and the liberation of TGF-beta from this state is crucial for signaling. To examine the contribution of LTBP to TGF-beta function, we generated mice in which the cysteines that link the propeptide to LTBP were mutated to serines, thereby blocking covalent association. Tgfb1(C33S/C33S) mice had multiorgan inflammation, lack of skin Langerhans cells (LC), and a shortened lifespan, consistent with decreased TGF-beta1 levels. However, the inflammatory response and decreased lifespan were not as severe as observed with Tgfb1(-/-) animals. Tgfb1(C33S/C33S) mice exhibited decreased levels of active TGF-beta1, decreased TGF-beta signaling, and tumors of the stomach, rectum, and anus. These data suggest that the association of LTBP with the latent TGF-beta complex is important for proper TGF-beta1 function and that Tgfb1(C33S/C33S) mice are hypomorphs for active TGF-beta1. Moreover, although mechanisms exist to activate latent TGF-beta1 in the absence of LTBP, these mechanisms are not as efficient as those that use the latent complex containing LTBP.
Sujet(s)
Inflammation/métabolisme , Protéines de liaison au TGF-bêta latent/métabolisme , Tumeurs/métabolisme , Facteur de croissance transformant bêta-1/métabolisme , Animaux , Cellules cultivées , Fibroblastes/cytologie , Muqueuse gastrique/cytologie , Muqueuse gastrique/métabolisme , Muqueuse gastrique/anatomopathologie , Inflammation/anatomopathologie , Muqueuse intestinale/cytologie , Muqueuse intestinale/métabolisme , Muqueuse intestinale/anatomopathologie , Cellules de Langerhans/cytologie , Cellules de Langerhans/métabolisme , Protéines de liaison au TGF-bêta latent/génétique , Souris , Souris knockout , Tumeurs/anatomopathologie , Précurseurs de protéines/génétique , Précurseurs de protéines/métabolisme , Transduction du signal/physiologie , Facteur de croissance transformant bêta-1/génétiqueRÉSUMÉ
The multifunctional cytokine transforming growth factor (TGF) beta1 is secreted in a latent complex with its processed propeptide (latency-associated peptide [LAP]). TGFbeta1 must be functionally released from this complex before it can engage TGFbeta receptors. One mechanism of latent TGFbeta1 activation involves interaction of the integrins alpha v beta6 and alpha v beta8 with an RGD sequence in LAP; other putative latent TGFbeta1 activators include thrombospondin-1, oxidants, and various proteases. To assess the contribution of RGD-binding integrins to TGFbeta1 activation in vivo, we created a mutation in Tgfb1 encoding a nonfunctional variant of the RGD sequence (RGE). Mice with this mutation (Tgfb1(RGE/RGE)) display the major features of Tgfb1(-/-) mice (vasculogenesis defects, multiorgan inflammation, and lack of Langerhans cells) despite production of normal levels of latent TGFbeta1. These findings indicate that RGD-binding integrins are requisite latent TGFbeta1 activators during development and in the immune system.
Sujet(s)
Intégrines/métabolisme , Facteur de croissance transformant bêta-1/métabolisme , Animaux , Sites de fixation , Souris , Souris knockout , Phénotype , Facteur de croissance transformant bêta-1/composition chimique , Facteur de croissance transformant bêta-1/génétique , Maladies vasculaires/génétique , Maladies vasculaires/anatomopathologie , Vésicule vitelline/vascularisation , Vésicule vitelline/anatomopathologieRÉSUMÉ
The transforming growth factor (TGF)-betas are essential in pre- and postnatal development, differentiation and morphogenesis of higher organisms. Quantitation of the levels of TGF-beta synthesis, secretion, and activation are crucial for grasping the mechanisms that control these events and ultimately control TGF-beta action. Rather than presenting a single method, we describe several methods for measuring active TGF-beta in different experimental situations. This is possible as a result of advances in transgenic mice technology that allow in vivo TGF-beta measurements in addition to the more established in vitro approaches.
