Your search keyword '"Fibrillin-1 chemistry"' showing total 17 results

1. Development of a mix-and-read assay for human asprosin using antibody-oligonucleotide probes and thermofluorimetric analysis.

Author

Hu J and Easley CJ

Subjects

Humans, Immunoassay methods, Antibodies immunology, Antibodies chemistry, Oligonucleotides chemistry, Adipokines, Fibrillin-1 chemistry

Abstract

Adipose tissue, or fat tissue, can now be classified as an endocrine organ as it responds to stimuli by secreting a range of hormones, termed adipokines, which regulate the functions of various other tissues and organs. Because novel adipokines continue to be discovered and characterized by researchers, there is an enduring need for the development of new analytical assays that target these hormones. Discovered recently, asprosin is an adipokine hormone secreted by white adipose tissue (WAT) during fasting which has been implicated for its important effects on the liver, skeletal muscle, hypothalamus, pancreas, and possibly other tissues. While standard immunoassays have been developed, the continued surge in research on asprosin's function would greatly benefit from an assay with homogeneous, mix-and-read workflow, and the nanomolar clinical range makes this goal more feasible. In this work, we developed such an assay for asprosin using our thermofluorimetric analysis (TFA) methods with antibody-oligonucleotide conjugate probes. The assay, achievable in less than one hour, was successfully validated by quantifying native levels of asprosin in human serum collected from fasting, nonfasting, type II diabetic, and obese donors.

Published

2024

2. Microfibril-associated glycoprotein 4 forms octamers that mediate interactions with elastogenic proteins and cells.

Author

Wozny MR, Nelea V, Siddiqui IFS, Wanga S, de Waard V, Strauss M, and Reinhardt DP

Subjects

Humans, Adipokines, Calcium metabolism, Glycoproteins, HEK293 Cells, Models, Molecular, Mutation, Missense, Protein Binding, Protein Multimerization, Cryoelectron Microscopy, Extracellular Matrix Proteins metabolism, Extracellular Matrix Proteins chemistry, Extracellular Matrix Proteins genetics, Fibrillin-1 metabolism, Fibrillin-1 genetics, Fibrillin-1 chemistry, Microfibrils metabolism, Microfibrils chemistry, Microfibrils ultrastructure, Tropoelastin metabolism, Tropoelastin chemistry, Tropoelastin genetics

Abstract

Microfibril-associated glycoprotein 4 (MFAP4) is a 36-kDa extracellular matrix glycoprotein with critical roles in organ fibrosis, chronic obstructive pulmonary disease, and cardiovascular disorders, including aortic aneurysms. MFAP4 multimerises and interacts with elastogenic proteins, including fibrillin-1 and tropoelastin, and with cells via integrins. Structural details of MFAP4 and its potential interfaces for these interactions are unknown. Here, we present a cryo-electron microscopy structure of human MFAP4. In the presence of calcium, MFAP4 assembles as an octamer, where two sets of homodimers constitute the top and bottom halves of each octamer. Each homodimer is linked together by an intermolecular disulphide bond. A C34S missense mutation prevents disulphide-bond formation between monomers but does not prevent octamer assembly. The atomic model, built into the 3.55 Å cryo-EM map, suggests that salt-bridge interactions mediate homodimer assembly, while non-polar residues form the interface between octamer halves. In the absence of calcium, an MFAP4 octamer dissociates into two tetramers. Binding studies with fibrillin-1, tropoelastin, LTBP4, and small fibulins show that MFAP4 has multiple surfaces for protein-protein interactions, most of which depend upon MFAP4 octamer assembly. The C34S mutation does not affect these protein interactions or cell interactions. MFAP4 assemblies with fibrillin-1 abrogate MFAP4 interactions with cells., (© 2024. The Author(s).)

Published

2024

3. Presence of microfibril associated glycoprotein 4 and type V collagen and the possible absence of fibrillin-1 in bead-like structures in elastofibroma.

Author

Nishida H, Sasaki T, Taga Y, Murasawa Y, Simizu S, Matsushita S, Isogai Z, Hattori S, Daa T, Nagamine N, Sekine A, and Fujiwara S

Subjects

Extracellular Matrix, Extracellular Matrix Proteins chemistry, Fibrillin-1 chemistry, Fibrillins chemistry, Collagen Type V, Microfibrils chemistry, Fibroma chemistry, Fibroma metabolism

Abstract

Competing Interests: Conflict of Interest The authors have no conflict of interest to declare.

Published

2023

4. POGLUT2 and POGLUT3 O-glucosylate multiple EGF repeats in fibrillin-1, -2, and LTBP1 and promote secretion of fibrillin-1.

Author

Williamson DB, Sohn CJ, Ito A, and Haltiwanger RS

Subjects

Amino Acid Motifs, Fibrillin-1 chemistry, Fibrillin-1 genetics, Fibrillin-2 chemistry, Fibrillin-2 genetics, Glycosylation, Humans, Latent TGF-beta Binding Proteins chemistry, Latent TGF-beta Binding Proteins genetics, Marfan Syndrome enzymology, Marfan Syndrome genetics, Protein Translocation Systems, Signal Transduction, Fibrillin-1 metabolism, Fibrillin-2 metabolism, Latent TGF-beta Binding Proteins metabolism, Marfan Syndrome metabolism

Abstract

Fibrillin-1 (FBN1) is the major component of extracellular matrix microfibrils, which are required for proper development of elastic tissues, including the heart and lungs. Through protein-protein interactions with latent transforming growth factor (TGF) β-binding protein 1 (LTBP1), microfibrils regulate TGF-β signaling. Mutations within the 47 epidermal growth factor-like (EGF) repeats of FBN1 cause autosomal dominant disorders including Marfan Syndrome, which is characterized by disrupted TGF-β signaling. We recently identified two novel protein O-glucosyltransferases, Protein O-glucosyltransferase 2 (POGLUT2) and 3 (POGLUT3), that modify a small fraction of EGF repeats on Notch. Here, using mass spectral analysis, we show that POGLUT2 and POGLUT3 also modify over half of the EGF repeats on FBN1, fibrillin-2 (FBN2), and LTBP1. While most sites are modified by both enzymes, some sites show a preference for either POGLUT2 or POGLUT3. POGLUT2 and POGLUT3 are homologs of POGLUT1, which stabilizes Notch proteins by addition of O-glucose to Notch EGF repeats. Like POGLUT1, POGLUT2 and 3 can discern a folded versus unfolded EGF repeat, suggesting POGLUT2 and 3 are involved in a protein folding pathway. In vitro secretion assays using the N-terminal portion of recombinant FBN1 revealed reduced FBN1 secretion in POGLUT2 knockout, POGLUT3 knockout, and POGLUT2 and 3 double-knockout HEK293T cells compared with wild type. These results illustrate that POGLUT2 and 3 function together to O-glucosylate protein substrates and that these modifications play a role in the secretion of substrate proteins. It will be interesting to see how disease variants in these proteins affect their O-glucosylation., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2021

5. Insights into the biophysical forces between proteins involved in elastic fiber assembly.

Author

O'Neill Moore S, Grubb TJ, and Kothapalli CR

Subjects

Amino Acid Oxidoreductases chemistry, Animals, Extracellular Matrix Proteins chemistry, Fibrillin-1 chemistry, Humans, Hydrophobic and Hydrophilic Interactions, Mice, Models, Chemical, Protein Binding, Rats, Receptors, Cell Surface chemistry, Tropoelastin chemistry, Amino Acid Oxidoreductases metabolism, Elastic Tissue chemistry, Extracellular Matrix Proteins metabolism, Fibrillin-1 metabolism, Receptors, Cell Surface metabolism, Tropoelastin metabolism

Abstract

Elastogenesis is a complex process beginning with transcription, translation, and extracellular release of precursor proteins leading to crosslinking, deposition, and assembly of ubiquitous elastic fibers. While the biochemical pathways by which elastic fibers are assembled are known, the biophysical forces mediating the interactions between the constituent proteins are unknown. Using atomic force microscopy, we quantified the adhesive forces among the elastic fiber components, primarily between tropoelastin, elastin binding protein (EBP), fibrillin-1, fibulin-5, and lysyl oxidase-like 2 (LOXL2). The adhesive forces between tropoelastin and other tissue-derived proteins such as insoluble elastin, laminin, and type I collagens were also assessed. The adhesive forces between tropoelastin and laminin were strong (1767 ± 126 pN; p < 10-5vs. all others), followed by forces (≥200 pN) between tropoelastin and human collagen, mature elastin, or tropoelastin. The adhesive forces between tropoelastin and rat collagen, EBP, fibrillin-1, fibulin-5, and LOXL2 coated on fibrillin-1 were in the range of 100-200 pN. The forces between tropoelastin and LOXL2, LOXL2 and fibrillin-1, LOXL2 and fibulin-5, and fibrillin-1 and fibulin-5 were less than 100 pN. Introducing LOXL2 decreased the adhesive forces between the tropoelastin monomers by ∼100 pN. The retraction phase of force-deflection curves was fitted to the worm-like chain model to calculate the rigidity and flexibility of these proteins as they unfolded. The results provided insights into how each constituent's stretching under deformation contributes to structural and mechanical characteristics of these fibers and to elastic fiber assembly.

Published

2020

6. Three Novel Variants identified in FBN1 and TGFBR2 in seven Iranian families with suspected Marfan syndrome.

Author

Bitarafan F, Razmara E, Khodaeian M, Keramatipour M, Kalhor A, Jafarinia E, and Garshasbi M

Subjects

Adult, Child, Female, Fibrillin-1 chemistry, Humans, Iran, Male, Marfan Syndrome pathology, Middle Aged, Pedigree, Protein Domains, Receptor, Transforming Growth Factor-beta Type II chemistry, Fibrillin-1 genetics, Marfan Syndrome genetics, Mutation, Missense, Receptor, Transforming Growth Factor-beta Type II genetics

Abstract

Background: Marfan syndrome (MFS) is a multi-systemic autosomal dominant disease of the connective tissue characterized by the early development of thoracic aneurysms/dissections, along with various manifestations of the ocular and skeletal systems. Due to the genetic and clinical heterogeneity, the clinical diagnosis of this disorder is challenging. Loss-of-function mutations in FBN1 (encodes fibrillin-1) lead to MFS type 1. Also, similar mutations in transforming growth factor β receptor 2 (TGFBR2) gene cause MFS type 2. Both proteins involve in TGF-β signaling., Methods: In this study, genetic screening using a panel involving 14 genes, especially FBN1 and TGFBR2, were performed on seven representatives affected members of seven unrelated Iranian families suspected with MFS. To confirm the variants, Sanger sequencing was applied to other affected/unaffected members of the families., Results: A total of 13 patients showed MFS manifestations. Using genetic screening, two novel and three previously reported variants in FBN1 were identified. We also detected two variants (a novel and a previously reported variant) in the TGFBR2 gene., Conclusion: In this study, we introduce three novel variants identified through gene screening in seven Iranian MFS families. This report is expected to considerably improve genetic counseling for Iranian MFS families. Early precise molecular diagnosis can be helpful for better management and improving the life expectancy of these patients., (© 2020 The Authors. Molecular Genetics & Genomic Medicine published by Wiley Periodicals LLC.)

Published

2020

7. Genetic and molecular mechanism for distinct clinical phenotypes conveyed by allelic truncating mutations implicated in FBN1.

Author

Lin M, Liu Z, Liu G, Zhao S, Li C, Chen W, Coban Akdemir Z, Lin J, Song X, Wang S, Xu Q, Zhao Y, Wang L, Zhang Y, Yan Z, Liu S, Liu J, Chen Y, Zuo Y, Yang X, Sun T, Yang XZ, Niu Y, Li X, You W, Qiu B, Ding C, Liu P, Zhang S, Carvalho CMB, Posey JE, Qiu G, Lupski JR, Wu Z, Zhang J, and Wu N

Subjects

Adolescent, Adult, Child, Female, Fibrillin-1 chemistry, Fibrillin-1 metabolism, HEK293 Cells, Humans, Lipodystrophy pathology, Marfan Syndrome pathology, Progeria pathology, Protein Domains, Smad2 Protein genetics, Smad2 Protein metabolism, Fibrillin-1 genetics, Lipodystrophy genetics, Marfan Syndrome genetics, Mutation, Phenotype, Progeria genetics

Abstract

Background: The molecular and genetic mechanisms by which different single nucleotide variant alleles in specific genes, or at the same genetic locus, cause distinct disease phenotypes often remain unclear. Allelic truncating mutations of FBN1 could cause either classical Marfan syndrome (MFS) or a more complicated phenotype associated with Marfanoid-progeroid-lipodystrophy syndrome (MPLS)., Methods: We investigated a small cohort, encompassing two classical MFS and one MPLS subjects from China, whose clinical presentation included scoliosis potentially requiring surgical intervention. Targeted next generation sequencing was performed on all the participants. We analyzed the molecular diagnosis, clinical features, and the potential molecular mechanism involved in the MPLS subject in our cohort., Results: We report a novel de novo FBN1 mutation for the first Chinese subject with MPLS, a more complicated fibrillinopathy, and two subjects with more classical MFS. We further predict that the MPLS truncating mutation, and others previously reported, is prone to escape the nonsense-mediated decay (NMD), while MFS mutations are predicted to be subjected to NMD. Also, the MPLS mutation occurs within the glucogenic hormone asprosin domain of FBN1. In vitro experiments showed that the single MPLS mutation p.Glu2759Cysfs*9 appears to perturb proper FBN1 protein aggregation as compared with the classical MFS mutation p.Tyr2596Thrfs*86. Both mutations appear to upregulate SMAD2 phosphorylation in vitro., Conclusion: We provide direct evidence that a dominant-negative interaction of FBN1 potentially explains the complex MPLS phenotypes through genetic and functional analysis. Our study expands the mutation spectrum of FBN1 and highlights the potential molecular mechanism for MPLS., (© 2019 The Authors. Molecular Genetics & Genomic Medicine published by Wiley Periodicals, Inc.)

Published

2020

8. A disease-associated mutation in fibrillin-1 differentially regulates integrin-mediated cell adhesion.

Author

Del Cid JS, Reed NI, Molnar K, Liu S, Dang B, Jensen SA, DeGrado W, Handford PA, Sheppard D, and Sundaram AB

Subjects

Amino Acid Motifs, Amino Acid Substitution, Animals, Cell Line, Tumor, Humans, Mice, Protein Domains, Cell Adhesion, Fibrillin-1 chemistry, Fibrillin-1 genetics, Fibrillin-1 metabolism, Integrins chemistry, Integrins genetics, Integrins metabolism, Marfan Syndrome genetics, Marfan Syndrome metabolism, Marfan Syndrome pathology, Mutation, Missense

Abstract

Fibrillins serve as scaffolds for the assembly of elastic fibers that contribute to the maintenance of tissue homeostasis and regulate growth factor signaling in the extracellular space. Fibrillin-1 is a modular glycoprotein that includes 7 latent transforming growth factor β (TGFβ)-binding protein-like (TB) domains and mediates cell adhesion through integrin binding to the RGD motif in its 4th TB domain. A subset of missense mutations within TB4 cause stiff skin syndrome (SSS), a rare autosomal dominant form of scleroderma. The fibrotic phenotype is thought to be regulated by changes in the ability of fibrillin-1 to mediate integrin binding. We characterized the ability of each RGD-binding integrin to mediate cell adhesion to fibrillin-1 or a disease-causing variant. Our data show that 7 of the 8 RGD-binding integrins can mediate adhesion to fibrillin-1. A single amino acid substitution responsible for SSS (W1570C) markedly inhibited adhesion mediated by integrins α5β1, αvβ5, and αvβ6, partially inhibited adhesion mediated by αvβ1, and did not inhibit adhesion mediated by α8β1 or αIIbβ3. Adhesion mediated by integrin αvβ3 depended on the cell surface expression level. In the SSS mutant background, the presence of a cysteine residue in place of highly conserved tryptophan 1570 alters the conformation of the region containing the exposed RGD sequence within the same domain to differentially affect fibrillin's interactions with distinct RGD-binding integrins., (© 2019 Del Cid et al.)

Published

2019

9. Variability in gene-based knowledge impacts variant classification: an analysis of FBN1 missense variants in ClinVar.

Author

Baudhuin LM, Kluge ML, Kotzer KE, and Lagerstedt SA

Subjects

Alleles, Amino Acid Sequence, Binding Sites, Calcium metabolism, Fibrillin-1 chemistry, Gene Frequency, Genotype, Humans, Mutation, Missense, Protein Binding, Protein Interaction Domains and Motifs, Databases, Genetic, Fibrillin-1 genetics, Genetic Association Studies methods, Genetic Predisposition to Disease, Genetic Variation

Abstract

Gene-specific knowledge can enhance genetic variant classification, but may not be routinely incorporated into clinical laboratory practice. For example, FBN1 variants associated with Marfan syndrome may be variably classified depending on knowledge of FBN1-specific critical regions. In order to assess variability in classification of FBN1 variants, 674 FBN1 missense variants from 18 ClinVar submitters were compared and reanalyzed using FBN1-specific criteria and ACMG/AMP 2015 guidelines for variant interpretation. Conflicting variant classifications occurred in 30.7% of the missense variants that had multiple submitters. There were 451 classifications of 361 critical residue missense variants, with 80.0% (361/451) classified as likely pathogenic or pathogenic [(L)P]. Non-cysteine critical residue variants were less likely to be classified as (L)P [55.3% (78/141)] than cysteine variants [91.3% (283/310)] and were more likely to lack evidence citing the functional significance of the amino acid impacted. Application of FBN1-specific knowledge allowed for reclassification or discrepancy resolution in 65/361 (18.0%) critical residue variants. There were 522 classifications of 313 unique missense variants not known to impact a critical residue. Of these, 31.6% (165/522) were likely overclassified as either (L)P or uncertain significance (VUS), especially when minor allele frequency (MAF) was taken into account, and we reclassified or resolved classification discrepancies in 128/313 (40.9%) of these variants. Our results provide a refined framework and resource for FBN1 variant classification, and further supports the more global implications of combining gene-based knowledge with ACMG/AMP criteria and appropriate MAF cutoffs for variant classification that extend beyond FBN1.

Published

2019

10. Fibrillin protein pleiotropy: Acromelic dysplasias.

Author

Sakai LY and Keene DR

Subjects

Fibrillin-1 chemistry, Genetic Predisposition to Disease, Humans, Limb Deformities, Congenital, Musculoskeletal Development, Mutation, Protein Domains, Bone Diseases, Developmental genetics, Contracture genetics, Fibrillin-1 genetics, Skin Diseases, Genetic genetics

Abstract

The fibrillins are large extracellular matrix molecules that polymerize to form microfibrils. Fibrillin microfibrils are distinctive architectural elements that are both ubiquitous in the connective tissue space and also unique, displaying tissue-specific patterns. Mutations in the genes for fibrillin-1 (FBN1) result in multiple distinct pleiotropic disorders. Most of the more than 3000 mutations known today in FBN1 cause the Marfan syndrome. Marfan mutations can occur in any of the 56 domains that compose fibrillin-1. In contrast, rare mutations in FBN1 that are confined to only certain domains cause several different types of acromelic dysplasia. These genetic disorders demonstrate that specific domains of fibrillin-1 perform roles important to musculoskeletal growth. Many of the phenotypes of acromelic dysplasias are the opposite of those found in Marfan syndrome. Knowledge of the functions and structural organization of fibrillin molecules within microfibrils is required to understand how one protein and one gene can be the basis for multiple genetic disorders., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2019

11. Identification and characterization of a novel FBN1 gene variant in an extended family with variable clinical phenotype of Marfan syndrome.

Author

Ergoren MC, Turkgenc B, Teralı K, Rodoplu O, Verstraeten A, Van Laer L, Mocan G, Loeys B, Tetik O, and Temel SG

Subjects

Adolescent, Adult, Amino Acid Sequence, Base Sequence, Child, Computer Simulation, Family, Female, Fibrillin-1 chemistry, Heterozygote, Humans, Male, Pedigree, Phenotype, Fibrillin-1 genetics, Marfan Syndrome genetics, Marfan Syndrome pathology, Mutation genetics

Abstract

Marfan syndrome (MFS) is a multi-systemic autosomal dominant condition caused by mutations in the gene (FBN1) coding for fibrillin-1. Mutations have been associated with a wide range of overlapping phenotypes. Here, we report on an extended family presenting with skeletal, ocular and cardiovascular clinical features. The 37-year-old male propositus, who had chest pain, dyspnea and shortness of breath, was first diagnosed based on the revised Ghent criteria and then subjected to molecular genetic analyses. FBN1 sequencing of the proband as well as available affected family members revealed the presence of a novel variant, c.7828G>C (p.Glu2610Gln), which was not present in any of the unaffected family members. In silico analyses demonstrated that the Glu2610 residue is part of the conserved DINE motif found at the beginning of each cbEGF domain of FBN1. The substitution of Glu2610 with Gln decreased fibrillin-1 production accordingly. Despite the fact that this variation appears to be primarily responsible for the etiology of MFS in the present family, our findings suggest that variable clinical expressions of the disease phenotype should be considered critically by the physicians.

Published

2019

12. [Mutation analysis of FBN1 gene in a child with Marfan syndrome].

Author

Jiang L, Zhang D, Xiao Y, Wang Q, Gong B, Guo X, Huang M, and Yang Z

Subjects

Amino Acid Sequence, Base Sequence, Child, DNA Mutational Analysis, Fibrillin-1 chemistry, Humans, Male, Molecular Sequence Data, Sequence Alignment, Fibrillin-1 genetics, Marfan Syndrome genetics

Abstract

Objective: To detect potential mutations of fibrillin-1 (FBN1) gene in a child with Marfan syndrome (MFS) and explore its molecular pathogenesis., Methods: The 66 exons of the FBN1 gene were analyzed by direct sequencing. SIFT and PolyPhen-2 were used to predict the structural and functional changes at the protein level., Results: A novel heterozygous mutation c.3998 G>A (p.Cys1333Tyr) was found in exon 32 in the child. The same mutation was not found among his unaffected family members and 683 healthy controls. Multiple sequence alignment showed that this novel mutation was located in a highly conserved region of the FBN1 protein across various species and may induce structural change to a functional domain., Conclusion: The novel c.3998G>A (p.Cys1333Tyr) mutation of the FBN1 gene probably predisposed the MFS in the child. Above finding has enriched the spectrum of FBN1 mutations.

Published

2018

13. Truncated C-terminus of fibrillin-1 induces Marfanoid-progeroid-lipodystrophy (MPL) syndrome in rabbit.

Author

Chen M, Yao B, Yang Q, Deng J, Song Y, Sui T, Zhou L, Yao H, Xu Y, Ouyang H, Pang D, Li Z, and Lai L

Subjects

Amino Acid Sequence, Animals, Aorta pathology, Base Sequence, Cartilage pathology, Dilatation, Pathologic, Ear pathology, Elastic Tissue metabolism, Eye pathology, Fibrillin-1 genetics, Fibrillin-1 metabolism, Glucose metabolism, Growth and Development, Heterozygote, Lipodystrophy congenital, Muscle, Skeletal pathology, Phenotype, Rabbits, Skin pathology, Wasting Syndrome pathology, Fibrillin-1 chemistry, Lipodystrophy pathology, Marfan Syndrome pathology

Abstract

Various clinical differences have been observed between patients with the FBN1 gene mutation and those with the classical Marfan phenotype. Although FBN1 knockout (KO) or dominant-negative mutant mice are widely used as an animal model for Marfan syndrome (MFS), these mice cannot recapitulate the genotype/phenotype relationship of Marfanoid-progeroid-lipodystrophy (MPL) syndrome, which is caused by a mutation in the C-terminus of fibrillin-1, the penultimate exon of the FBN1 gene. Here, we describe the generation of a rabbit MPL model with C-terminal truncation of fibrillin-1 using a CRISPR/Cas9 system. FBN1 heterozygous ( FBN1 Het) rabbits faithfully recapitulated the phenotypes of MFS, including muscle wasting and impaired connective tissue, ocular syndrome and aortic dilation. Moreover, skin symptoms, lipodystrophy, growth retardation and dysglycemia were also seen in these FBN1 Het rabbits, and have not been reported in other animal models. In conclusion, this novel rabbit model mimics the histopathological changes and functional defects of MPL syndrome, and could become a valuable model for studies of pathogenesis and drug screening for MPL syndrome., Competing Interests: Competing interestsThe authors declare no competing or financial interests., (© 2018. Published by The Company of Biologists Ltd.)

Published

2018

14. Structural and functional failure of fibrillin‑1 in human diseases (Review).

Author

Schrenk S, Cenzi C, Bertalot T, Conconi MT, and Di Liddo R

Subjects

Animals, Elastin metabolism, Extracellular Matrix metabolism, Humans, Intercellular Signaling Peptides and Proteins metabolism, Signal Transduction, Disease, Fibrillin-1 chemistry, Fibrillin-1 metabolism

Abstract

Fibrillins (FBNs) are key relay molecules that form the backbone of microfibrils in elastic and non‑elastic tissues. Interacting with other components of the extracellular matrix (ECM), these ubiquitous glycoproteins exert pivotal roles in tissue development, homeostasis and repair. In addition to mechanical support, FBN networks also exhibit regulatory activities on growth factor signalling, ECM formation, cell behaviour and the immune response. Consequently, mutations affecting the structure, assembly and stability of FBN microfibrils have been associated with impaired biomechanical tissue properties, altered cell‑matrix interactions, uncontrolled growth factor or cytokine activation, and the development of fibrillinopathies and associated severe complications in multiple organs. Beyond a panoramic overview of structural cues of the FBN network, the present review will also describe the pathological implications of FBN disorders in the development of inflammatory and fibrotic conditions.

Published

2018

15. The N-Terminal Region of Fibrillin-1 Mediates a Bipartite Interaction with LTBP1.

Author

Robertson IB, Dias HF, Osuch IH, Lowe ED, Jensen SA, Redfield C, and Handford PA

Subjects

Binding Sites, Fibrillin-1 metabolism, Humans, Latent TGF-beta Binding Proteins metabolism, Molecular Docking Simulation, Protein Binding, Fibrillin-1 chemistry, Latent TGF-beta Binding Proteins chemistry

Abstract

Fibrillin-1 (FBN1) mutations associated with Marfan syndrome lead to an increase in transforming growth factor β (TGF-β) activation in connective tissues resulting in pathogenic changes including aortic dilatation and dissection. Since FBN1 binds latent TGF-β binding proteins (LTBPs), the major reservoir of TGF-β in the extracellular matrix (ECM), we investigated the structural basis for the FBN1/LTBP1 interaction. We present the structure of a four-domain FBN1 fragment, EGF2-EGF3-Hyb1-cbEGF1 (FBN1 E2cbEGF1 ), which reveals a near-linear domain organization. Binding studies demonstrate a bipartite interaction between a C-terminal LTBP1 fragment and FBN1 E2cbEGF1 , which lies adjacent to the latency-associated propeptide (LAP)/TGF-β binding site of LTBP1. Modeling of the binding interface suggests that, rather than interacting along the longitudinal axis, LTBP1 anchors itself to FBN1 using two independent epitopes. As part of this mechanism, a flexible pivot adjacent to the FBN1/LTBP1 binding site allows LTBP1 to make contacts with different ECM networks while presumably facilitating a force-induced/traction-based TGF-β activation mechanism., (Copyright © 2017 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published

2017

16. Extracellular Regulation of Bone Morphogenetic Protein Activity by the Microfibril Component Fibrillin-1.

Author

Wohl AP, Troilo H, Collins RF, Baldock C, and Sengle G

Subjects

Amino Acid Sequence, Animals, Bone Morphogenetic Protein 7 chemistry, Bone Morphogenetic Protein 7 genetics, Cell Line, Circular Dichroism, Fibrillin-1 chemistry, Fibrillin-1 genetics, HEK293 Cells, Humans, Microscopy, Electron, Transmission, Models, Molecular, Nanostructures chemistry, Nanostructures ultrastructure, Protein Binding, Protein Conformation, Protein Domains, Protein Structure, Secondary, Scattering, Small Angle, Surface Plasmon Resonance, X-Ray Diffraction, Bone Morphogenetic Protein 7 metabolism, Extracellular Matrix metabolism, Fibrillin-1 metabolism, Microfibrils metabolism

Abstract

Since the discovery of bone morphogenetic proteins (BMPs) as pluripotent cytokines extractable from bone matrix, it has been speculated how targeting of BMPs to the extracellular matrix (ECM) modulates their bioavailability. Understanding these processes is crucial for elucidating pathomechanisms of connective tissue disorders characterized by ECM deficiency and growth factor dysregulation. Here, we provide evidence for a new BMP targeting and sequestration mechanism that is controlled by the ECM molecule fibrillin-1. We present the nanoscale structure of the BMP-7 prodomain-growth factor complex using electron microscopy, small angle x-ray scattering, and circular dichroism spectroscopy, showing that it assumes an open V-like structure when it is bioactive. However, upon binding to fibrillin-1, the BMP-7 complex is rendered into a closed ring shape, which also confers latency to the growth factor, as demonstrated by bioactivity measurements. BMP-7 prodomain variants were used to map the critical epitopes for prodomain-growth factor and prodomain-prodomain binding. Together, these data show that upon prodomain binding to fibrillin-1, the BMP-7 complex undergoes a conformational change, which denies access of BMP receptors to the growth factor., (© 2016 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2016

17. Visualizing tropoelastin in a long-term human elastic fibre cell culture model.

Author

Halm M, Schenke-Layland K, Jaspers S, Wenck H, and Fischer F

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Cell Line, Elastic Tissue ultrastructure, Elastin chemistry, Elastin genetics, Elastin metabolism, Fibrillin-1 chemistry, Fibrillin-1 metabolism, Fibroblasts cytology, Fibroblasts metabolism, Gene Expression drug effects, Humans, Luminescent Proteins genetics, Luminescent Proteins metabolism, Microscopy, Confocal, Microscopy, Fluorescence, Real-Time Polymerase Chain Reaction, Transforming Growth Factor beta1 pharmacology, Tropoelastin chemistry, Elastic Tissue metabolism, Tropoelastin metabolism

Abstract

Elastin is an essential protein found in a variety of tissues where resilience and flexibility are needed, such as the skin and the heart. When aiming to engineer suitable implants, elastic fibres are needed to allow adequate tissue renewal. However, the visualization of human elastogenesis remains in the dark. To date, the visualization of human tropoelastin (TE) production in a human cell context and its fibre assembly under live cell conditions has not been achieved. Here, we present a long-term cell culture model of human dermal fibroblasts expressing fluorescence-labelled human TE. We employed a lentiviral system to stably overexpress Citrine-labelled TE to build a fluorescent fibre network. Using immunofluorescence, we confirmed the functionality of the Citrine-tagged TE. Furthermore, we visualized the fibre assembly over the course of several days using confocal microscopy. Applying super resolution microscopy, we were able to investigate the inner structure of the elastin-fibrillin-1 fibre network. Future investigations will allow the tracking of TE produced under various conditions. In tissue engineering applications the fluorescent fibre network can be visualized under various conditions or it serves as a tool for investigating fibre degradation processes in disease-in-a-dish-models.

Published

2016