Marie-Madeleine Giraud-Guille

Concentrated collagen hydrogels as dermal substitutes

Collagen hydrogels first appeared promising for skin repair. Unfortunately, their extensive contraction and their poor mechanical properties constituted major disadvantages toward their utilization as permanent graft. The present study has investigated a way to correct these drawbacks by increasing the collagen concentration in controlled conditions. Concentrated collagen hydrogels (CCH) at 1.5, 3 and 5mg/ml were obtained. The effect of raised collagen concentration on contraction, cell growth and remodeling activities was evaluated for 21 days in culture. Subsequently, in vivo integration of CCH and normal collagen hydrogels (NCH) was assessed. Compared to NCH, CCH contraction was delayed and smaller. At day 21, surface area of CCH at 3mg/ml was 18 times more important than that of NCH. Whatever the initial fibroblast density, CCH favored cell growth that reached about 10 times the initial cell number at day 21; cell proliferation was inhibited in NCH. Gelatinase A activities appeared lower in CCH than within NCH. In vivo studies in rats revealed a complete hydrolysis of NCH 15 days after implantation. In contrast, CCH at 3mg/ml was still present after 30 days. Moreover, CCH showed cell colonization, neovascularization and no severe inflammatory response. Our results demonstrate that concentrated collagen hydrogels can be considered as new candidates for dermal substitution because they are is easy to handle, do not contract drastically, favor cell growth, and can be quickly integrated in vivo.

Water-mediated structuring of bone apatite

It is well known that organic molecules from the vertebrate extracellular matrix of calcifying tissues are essential in structuring the apatite mineral. Here, we show that water also plays a structuring role. By using solid-state nuclear magnetic resonance, wide-angle X-ray scattering and cryogenic transmission electron microscopy to characterize the structure and organization of crystalline and biomimetic apatite nanoparticles as well as intact bone samples, we demonstrate that water orients apatite crystals through an amorphous calcium phosphate-like layer that coats the crystalline core of bone apatite. This disordered layer is reminiscent of those found around the crystalline core of calcified biominerals in various natural composite materials in vivo. This work provides an extended local model of bone biomineralization.

Liquid crystallinity in condensed type I collagen solutions : a clue to the packing of collagen in extracellular matrices

We recently described a new type of assembly of collagen molecules, forming typical liquid crystalline phases in highly concentrated solutions after sonication. The present work shows that intact 300 nm long collagen molecules also form cholesteric liquid crystalline domains, but the time required is much longer, several weeks instead of several days. Differential calorimetry and X-ray diffraction show that sonication does not alter the triple-helical structure of the collagen fragments. In the viscous solutions, observed between crossed polars in optical microscopy, the textures vary as a function of the concentration. Molecules first align near the air interface at the coverslip edge, then as the concentration increases by slow evaporation of the solvent, the birefringence extends inwards and liquid crystalline domains progressively appear. For concentrations estimated to be above 100 mg/ml, typical textures and defects of cholesteric phases are obtained, at lower concentrations zig-zag extinction patterns and banded patterns are observed; all these textures are described and interpreted. The cholesteric packing of collagen fibrils in various extracellular matrices is known, and the relationship that can be made between the ordered phases obtained with collagen molecules in vitro and the related geometrical structures observed between fibrils in vivo is thoroughly discussed.

Structural aspects of fish skin collagen which forms ordered arrays via liquid crystalline states

The ability of acid-soluble type I collagen extracts from Soleidae flat fish to form ordered arrays in condensed phases has been compared with data for calf skin collagen. Liquid crystalline assemblies in vitro are optimized by preliminary treatment of the molecular population with ultrasounds. This treatment requires the stability of the fish collagen triple helicity to be controlled by X-ray diffraction and differential scanning calorimetry and the effect of sonication to be evaluated by viscosity measurements and gel electrophoresis. The collagen solution in concentrations of at least 40 mg ml(-1) showed in polarized light microscopy birefringent patterns typical of precholesteric phases indicating long-range order within the fluid collagen phase. Ultrastructural data, obtained after stabilization of the liquid crystalline collagen into a gelated matrix, showed that neutralized acid-soluble fish collagen forms cross-striated fibrils, typical of type I collagen, following sine wave-like undulations in precholesteric domains. These ordered geometries, approximating in vivo situations, give interesting mechanical properties to the material.

Liquid crystalline assemblies of collagen in bone and in vitro systems

Precise descriptions of the three-dimensional arrangements of collagen in bone are essential to understand the mechanical properties of this complex tissue. Transmission electron microscopy (TEM) analysis of decalcified human compact bone in section reveals characteristic patterns forming regular series of nested arcs. Such patterns are a direct consequence of an organization described as a twisted plywood and relate the distribution of collagen fibrils in osteons with that of molecules in cholesteric liquid crystals. The hypothesis that liquid crystalline properties are involved in the morphogenesis of dense collagen matrices was supported by data obtained in vitro. At a molecular level, acid-soluble collagen molecules spontaneously assemble, at concentrations of 50mg/ml or more, in precholesteric-banded patterns and cholesteric phases, identified by polarized light microscopy. In a more physiological context, these results were conforted, with the precursor molecule of collagen, procollagen, soluble at neutral pH. This protein spontaneously forms liquid crystalline precholesteric phases corresponding to banded patterns and birefringent cords. Stabilization of the liquid crystalline collagen, induced by pH modification and fibril formation, shows characteristic morphologies in TEM, which directly mimic arrays described in vivo. Undulating fibrils are indeed similar to crimp morphologies described in tendons and continuously twisting fibrils, and give rise to arced patterns similar to supra-molecular architectures identified in compact bone.

Fibrillogenesis in Dense Collagen Solutions: A Physicochemical Study

Fibrillogenesis, the formation of collagen fibrils, is a key factor in connective tissue morphogenesis. To understand to what extent cells influence this process, we systematically studied the physicochemistry of the self-assembly of type I collagen molecules into fibrils in vitro. We report that fibrillogenesis in solutions of type I collagen, in a high concentration range close to that of living tissues (40-300 mg/ml), yields strong gels over wide pH and ionic strength ranges. Structures of gels were described by combining microscopic observations (transmission electron microscopy) with small- and wide-angle X-ray scattering analysis, and the influence of concentration, pH, and ionic strength on the fibril size and organization was evaluated. The typical cross-striated pattern and the corresponding small-angle X-ray scattering 67-nm diffraction peaks were visible in all conditions in the pH 6 to pH 12 range. In reference conditions (pH 7.4, ionic strength=150 mM, 20 degrees C), collagen concentration greatly influences the overall macroscopic structure of the resultant fibrillar gels, as well as the morphology and structure of the fibrils themselves. At a given collagen concentration, increasing the ionic strength from 24 to 261 mM produces larger fibrils until the system becomes biphasic. We also show that fibrils can form in acidic medium (pH approximately 2.5) at very high collagen concentrations, beyond 150 mg/ml, which suggests a possible cholesteric-to-smectic phase transition. This set of data demonstrates how simple physicochemical parameters determine the molecular organization of collagen. Such an in vitro model allows us to study the intricate process of fibrillogenesis in conditions of molecular packing close to that which occurs in biological tissue morphogenesis.

Twisted liquid crystalline supramolecular arrangements in morphogenesis.

Supramolecular assemblies following liquid crystalline cholesteric geometries have been described in biological systems from optical properties observed in polarized-light microscopy and structural data obtained in electron microscopy. Major biological macromolecules are discussed, including structural polymers of the extracellular matrix, genetic material in nuclei and chromosomes, and proteins of the cytoplasm. The liquid crystalline assembly properties of biological polymers have been demonstrated by experiments in vitro with molecules at basic structural levels, such as molecular chains of cellulose and chitin, triple helices of collagen, and double helices of DNA, and also with entities at higher states of organization as they appear in cells and tissues, such as cellulose and chitin crystallites, and collagen fibrils. It appears that the building of cellular and extracellular edifices implies self-ordering processes of the liquid crystalline type and that the study of these mesomorphic states will help resolve basic questions about the structure and morphogenesis of densely packed biological structures.

Production of ordered collagen matrices for three-dimensional cell culture

The aim of this study was to produce collagen gels with controlled fibrillar order as matrices for cell culture. Their structural characterization and colonization by human dermal fibroblasts arc presently reported. Ordered matrices are obtained by using the property of type I collagen monomers to self-assemble in liquid crystalline arrays by slow evaporation of acidic solutions at high concentrations. Induction of fibrillogenesis concomittent with the stabilization of the supramolecular order is then obtained, within petri dishes, by gelation of the viscous preparations under ammoniac vapours. For comparison, dermal equivalents, in which collagen compaction depends on fibroblasts contraction, are made according to the method of Bell et al. (Proc. Natl. Acad. Sci. 76(3) (1979) 1274). The fibrillar arrangement of the collagen network in the samples is determined by polarizing optical microscopy and by transmission electron microscopy. Whereas dermal equivalents exhibit heterogeneous distributions of fibrils, two differents types of order are obtained in the stabilized liquid crystalline collagen samples, namely aligned, i.e. nematic, at 20 mg/ml, or crimped, i.e. precholesteric, at 40 mg/ml. The morphology and behaviour of fibroblasts seeded on the surface of the matrices are analysed from day 1 to day 21. The cells are viable, proliferate at the surface of ordered matrices and migrate up to 400 microm in depth. Production of concentrated and ordered collagen matrices provides new perspectives to study the behaviour of cells in a valorized three-dimensional context where the fibrillar organization becomes close to in vivo situations.

Plywood structures in nature

Abstract Ordered fibrous composites, also known as plywood structures, are frequently encountered in natural systems, mostly in skeletal or protective extracellullar tissues where mineral deposition often occurs. A major challenge in the field of materials science is the possibility to copy supramolecular assemblies described in biological structures. To do this the different structural levels of natural plywoods need to be precisely described and this approach has enabled the definition of organic networks as stabilized analogues of liquid crystals. Recently, there have been successful attempts at mimicking supramolecular ordering with extracellular polymers

Liquid crystalline phases of sonicated type I collagen

Summary— The assembly properties of concentrated solutions of type I collagen molecules are compared before and after a 5‐min sonication, breaking the 300‐nm triple helices into short segments of about 20 nm, with a strong polydispersity. The collagen concentration of these solutions, sonicated or not, was increase up to 100 mg/ml by slow evaporation of the solvent. Whereas the non‐sonicated solutions remain isotropic, the sonicated solutions transform after a few hours into a twisted liquid crystalline phase, well recognizable in polarizing microscopy. The evidence of a twisted assembly of collagen triple helices in vitro is new and relevant in a biological context since it was reported in various collagen matrices.