Self-aligned fibrous scaffolds for automechanoinduction of cell cultures

Abstract

Self-aligned fibrous scaffolds are disclosed. The scaffolds are capable of automechanoinduction of cell cultures and methods to induce authomechanoinduction in cancer cells and stem cells are disclosed as well.

Claims

1. A biocompatible scaffold for multi-dimensional cultivation of cells, said scaffolds capable of automechanoinduction and comprising: aligned fibers oriented to form a scaffold with open porosity for the cultured cells, wherein the fibers have a diameter of 5-100 nm, and an aspect ratio more than 10000:1, said fibers being made of non-cytotoxic, non-carcinogenic inorganic metal oxide, and said fibers being self-aligned into the scaffold during its manufacturing process.

2. The scaffold according to claim 1, wherein the open porosity is in a range of 70-99%.

3. The scaffold according to claim 2, wherein the open porosity is 85-95%.

4. The scaffold according to claim 1, wherein the fibers have a length of 10-20 mm.

5. The scaffold according to claim 1, wherein the diameter of the fibers is 20-50 nm.

6. The scaffold according to claim 1, wherein the fibers have aspect ratio more than 20000:1.

7. The scaffold according to claim 1, wherein the fibers are coated with a bioinert material.

8. The scaffold according to claim 7, wherein the bioinert material is non-functionalized graphene.

9. The scaffold according to claim 1, wherein the metal oxide is selected from the group consisting of silica, titania, zirconia and alumina.

10. The scaffold of according to claim 9, wherein the fibers are of aluminum oxide.

11. The scaffold of claim 1, wherein the scaffold is for cultivation of stem cells and the scaffold is capable of inducing automechanoinduction of neural differentiation of the stem cells.

12. The scaffold of claim 1, wherein the scaffold is for cultivation of cancer cells and the scaffold is capable of inducing automechanoinduction of gene expressions in the cancer cells to make them suitable as tumor models.

13. A method to induce automechanoinduction of neural differentiation of stem cells by cultivating the stem cells on a scaffold of claim 1.

14. A method to induce automechanoinduction of gene expressions in cancer cells by cultivating the cancer cells on a scaffold of claim 1.

Description

BRIEF DESCRIPTION OF DRAWINGS

(1) FIG. 1 shows the fine structure of the self-aligned fibrous scaffold made of metal oxide (alumina) nanofibers of 40 nm diameter.

(2) FIG. 2 A, B shows contour morphology of the hMSC cultured on control (A) and new scaffolds (B), exhibiting preferential orientation.

(3) FIG. 3A, B shows images of the MDA-MB231 cancer cells cultures on the control (A) and new scaffolds (B).

(4) FIGS. 4 A and B shows gene expression heat maps for PBMC (A) and for hMSC (B) cultured on the scaffolds (all relative to control; note logaritmic scale which proves few orders of magnitude differences).

DETAILED DESCRIPTION OF THE INVENTION

Definitions

(5) For the reasons of clarity, the terminology used in this description means: Fiber refers to a fiber made of a non-cytotoxic, non-carcinogenic metal oxide, but not from polymers or bioactive ceramics (such as hydroxyapatite). Automechanoinduction means an induction of a mechanical stimulus to a cell or tissue from their own interaction with the substrate or media, without application of an external force, comprising that this induction leads to changes in cells or tissues behavior, structure, functionality, morphology, or any other relevant property. Automechanoinduction also excludes application of specific culture media, where said changes in cells or tissues are caused by e.g. adjustment of biochemical or chemical composition. Bioinert means a material which does not enter into biochemical reactions with live cells leading to changes in their shape, functionality, proliferation or fate, neither undergoes a destruction or transformations (bioresorbtion). Scaffold refers to a structure comprising a self-aligned network of fibers made in situ. Randomly oriented fibers refers to any fiber scaffold not fitting the description of the present invention, i.e. such fibers that have not been actively aligned or that do not follow any designed pattern of orientation to each other. Self-aligned fibers refers to a structure that consists of one or more fibers that are highly oriented in parallel to each other during the structure manufacturing process, i.e. not during the separate packing of the fibers info the structure (assembly) after the fibers have been manufactured otherwise. Ultra-high anisotropy refers to a self-aligned fibers scaffold which fibers have aspect ratios (length to diameter) of 10000:1 and more.

(6) The present invention will now be described in more detail hereafter with reference to the accompanying examples and figures, in which embodiments of the invention are shown. This invention may, however, be embodied in many different forms and should not be construed as limited to the embodiments set forth herein.

Practical Examples

(7) Methods Used

(8) The scaffolds were manufactured from aluminum oxide based material (however, other oxides, such as silica, titania, zirconia could also be used) and heat treated with regimes determined by a thermal analysis study [9]. These self-aligned metal oxide fibers (FIG. 1) with an average single-fiber diameter of 40 nm (TEM, HRSEM) and length of 10-20 mm (aspect ratio (10 . . . 20).Math.10.sup.3 m/40.Math.10.sup.3 m=(250000 . . . 500000):1) have 70-99% open porosity, preferably 85-95% open porosity (measured by BET and mercury porosimetry). Some of the scaffolds were also coated by graphene with catalyst-free chemical vapor deposition (CVD) at 1000 C. to demonstrate that coatings might be easily performed if required. On the contrary to other studies, graphene on the nanofibres was not functionalized in any way and became augmented to the underlying oxide fiber surface. Non-functionalized graphene was used as an example of bioinert material. Nanofibers with other average diameters like 7 and 25 nm and similar aspect ratios were also obtained, but most of the cell studies were conducted with 40 nm fiber scaffolds for consistency. No bioactive agents were added, nor other modification of the scaffolds was made, unlike most of their known studies, to exclude possible effects of bioactive additions on cells.

(9) Human MSCs were obtained from freshly isolated subcutaneous adipose tissue and characterized as reported [10]. Cancer cell lines MDA-MB231, Caco2, WM239A and Kelly, were obtained from ATCC. Cells were grown in culture media (DMEM) with 10% FBS (fetal bovine serum), 1 mg/ml penicillin and 0.1 mg/ml streptomycin at 37 C. in 5% CO.sub.2. The scaffolds were pre-treated for three days before the cells seeding by complete medium with changing the medium for fresh every 24 hours to saturate them by active components adsorbed from liquid phase (CellIn Technologies, Estonia).

(10) For visualization of the cells, specific to filamentous actin (F-actin) phalloidin tagged by FITC (Sigma) was used. For hMSCs, pooled cells from three individuals with passage number below 5 were seeded on the scaffolds in 12-well plate (410.sup.4 cells per well). For cancer cells, 510.sup.4 cells were added to the each well with scaffolds. Similar cells grown on a flat glass at the same density and cell culture conditions were considered as the controls. The cells were fixed by 4% PFA at 48 h after seeding, washed by PBS (phosphate buffered saline) and permeabilized by 0.3% TRITON X-100 in PBS for 5 minutes. Phalloidin-FITC (1:100) staining lasted for 18 h at 4 C. for scaffolds and 2 h at RT for controls. To stain the cells nucleus, cells were incubated for 10 minutes with Hoechst 33342 (Invitrogen, 1 g/ml). After a final wash, the phalloidin-stained cells were analyzed by Nikon Eclipse 80i microscope (CellIn Technologies, Estonia).

(11) Calculation of the orientations of hMSC seeded was used with ImageJ software and Orientation-J Distribution plug-in (version 1.50 g, National Institute of Health, USA). Original microscope images were converted into 8-bit color images and the pixels/distance ratio was calibrated based on the microscope camera bar. The images were threshold first by HSV color and then by brightness into binary images using Li algorithm. The orientation parameters were calculated with 5 pixel Gaussian window size and approximation with a cubic spline gradient. Finally, these data were treated with SigmaPlot software (Systat GmbH, Germany) into polar form.

(12) Immunologic response for peripheral blood mononuclear cells (PBMCs) was evaluated using PBMCs from healthy donors, isolated using Ficoll-Paque gradient fractionation (CellIn Technologies, Estonia). 210.sup.6 cells were used for each analysis. RNAs were extracted directly from scaffolds by TRIzol (Ambion) reagent following 24 h cells growth on the scaffold, according to the manufacturer's recommendations. cDNAs were synthesized from DNase-treated (Ambion) RNA by RevertAid Reverse Transcriptase (Thermo Fisher Scientific) with addition of RiboLock (Thermo Fisher Scientific) according to the manufacturer's recommendations. cDNA quality was verified by RT-PCR by using GAPDH primers and HOT FIREpol Master Mix (Solis Biodyne, Estonia). RT-qPCR was performed in triplicates using EvaGreen qPCR mix plus no Rox (Solis Biodyne, Estonia) and the LightCycler 480 Real-Time PCR System (Roche Applied Science). The fold of change was calculated relatively to the control (cells grown without scaffolds) after normalization to GAPDH expression, using 2-Ct method (double difference of Ct). The values are respectively Ct=Ct(gene of interest)Ct(GAPDH), and Ct=Ct(treated)Ct(control). For visualization, the data were normalized to the cells grown without scaffold materials (control), converted to log scale and represented as a heat map (LionSolver 2.1, Reactive Search s.r.l., Italy). The minimal mapping error is achieved by minimizing sum of coordinates normalized with respect to the maximum and minimum along each dimension (in this case, decimal logarithm of relative expressions).

(13) Secretome ELISA analysis was done from cell culture media collected with soluble factors expression was analysed 24 h after initiation of cell culture (Protobios, Estonia). The levels of IL6, IL8/CXCL8, CCL2, IL1B, IL2, IL4, IL12, TNF and IFN secreted into the growth medium were measured using Human IL-6 DuoSet ELISA Development Kit (R&D System, Wiesbaden, Germany), Human IL-8 Standard ABTS ELISA Development Kit (Peprotech, Rock Hill, N.J., USA), Human CCL2/MCP-1 DuoSet (R&D System), Human IL-1/IL-1F2 DuoSet ELISA Development Kit (R&D System, Wiesbaden, Germany), Human IL-2 ELISA Development Kit (Peprotech, Rock Hill, N.J., USA), Human IL-4 Standard ABTS (PeproTech, Rock Hill, N.J., USA), Human IL-12 ELISA Development Kit (Peprotech, Rock Hill, N.J., USA), Human TNF ELISA Development Kit (Peprotech, Rock Hill, N.J., USA), Human IFN- ELISA Development Kit (Peprotech, Rock Hill, N.J., USA), and Human Standard ABTS ELISA Development Kit (Peprotech), respectively. The ELISA analysis was performed using high binding ELISA plates (Greiner BioOne) at RT according to the manufacturer's instructions. Optical density was measured using photospectrometer Spectramax 340 PC (Molecular Devices) at the wavelength 450 nm.

Example 1. Human Mesenchymal Stem Cells Cultured on New Scaffolds of this Invention Exhibit Preferential Orientation

(14) The morphology, adhesion and distribution of viable hMSC after 3 days of culture on horizontally oriented new scaffolds and on control (glass) are demonstrated in FIGS. 2A and B. The scaffolds under present invention were clearly guiding cells to line up along the fibers with a spindle-like shape and more than usually elongated lamellipodia extensions. High aspect ratio cellular orientations are developed throughout the scaffold, allowing directional connection between individual cells and formation of cells network. This confirms scaffolds do not impede the normal growth of stem cells. Furthermore, elongated morphology of hMSC and its high polarization create pre-requisites for preferential specific (e. g. neuronal or myogenic) lineage differentiation.

(15) Whereas response of stem cells to different substrate stiffness was studied earlier, the inventors for the first time have found the effect of such ultra-high scaffold anisotropy in a self-aligned, highly porous state, which was not previously reported. Most of known nanofiber-based scaffolds are randomly oriented or loosely packed, making a 3D nanostructure without such stiffness anisotropy [for example, U.S. Pat. No. 7,704,740, US 20060263417, US 20070269481]. Many aligned fibrous scaffolds are made of polymer fibers, the intrinsic elastic modulus of which is less than oxide ceramics by few orders of magnitude. The effect observed at scaffolds under present invention differs also substantially from known nanotopology studies, where nano-grooves or other patterns are known to support cell alignment, but without local differences in substrate stiffness.

Example 2. MDA-MB231 Cancer Cells Grown on the New Scaffold of this Invention Show Extended Microspikes and Filopodia Protrusions

(16) Several cancer cell lines were seeded on the vertical and horizontal sides of the scaffolds of present invention. Cancer cells cultured on scaffolds possess extended microspikes and actin-rich filopodia protrusions suggesting high level of membrane activity and malignant migratory cancer phenotype (FIG. 3A,B shows MDA-MB231 cancer cell growth). The initial signs of cancer cell infiltration (and hence local immobilization of the cells) were detected on vertical fibers allowing suggestion of volumetric cancer model. By cancer cell infiltration, their reduced mobility and extended filopodia formation, scaffolds allow creating more representative phenotype necessary to obtain multi-dimensional in vitro cancer model that more accurately mimics tumor genesis. Furthermore, this model differs from both known 2D and 3D cultures as it allows partial immobilization of the cells into a half-dimensional direction (into the depth), keeping them unlimited to planar mobility. The inventors call this culture as 2.5D to emphasize this difference.

Example 3. Novel Scaffolds of this Invention have an Ability to Modulate Immune Response of Peripheral Blood Mononuclear Cells

(17) Immunological profiling of any material under the influence of in vivo or in vitro environment is an important content of biocompatibility evaluation and has a critical value for future clinical translation. In addition to hMSC (Example 1), this was assessed with PBMC as they are an important part of the human peripheral immune system, responsible for transforming of the multitude of external stimuli to generate an adaptive immune response. The PBMC were grown on the scaffolds and tissue culture plastic (control) in vitro, and their inflammatory signatures were compared (FIG. 4). The mRNA expression was analyzed for genes involved in the immune reaction and a secretion of cytokines (IL1B, TNF, IFN, IL6, IL8, IL2, IL4, IL12B, and CCL2).

(18) For PBMC, clear downregulation of pro-inflammatory TNF, IL1B, IL12B, IL6, CCL2 and COX2 cytokines was detected, demonstrating the strong ability of the scaffold to modulate immune response. Interestingly at the same time upregulated CCL18, IL1RN, IDO1 and TGF1 factors were observed. These factors participate in anti-inflammatory response, pointing out to the intrinsic possible immunomodulating effect of the scaffolds caused by their structure and composition alone, without any additions of external stimuli, which also was confirmed by ELISA (data not shown).

(19) For hMSCs, the promoted mRNA expression of CXCL8, CXCL9, CXCL10 and CSF2, the chemokines participating in neutrophil, monocyte or leukocyte trafficking, were observed, indicating the possible changes in chemotaxis. Additionally, reduced expression of COX2, CCL2 and IL6 cytokines indicates a good immune tolerance of these scaffolds.

(20) The present invention provides a principally new solution overcoming the drawbacks known by prior art by providing a 2.5-dimensional biocompatible scaffold designed for various cell cultures, capable to provide novel and more efficient methods for cell and drug research as well as tissue engineering applications.

(21) Other features and uses of the invention and their associated advantages will be evident to a one skilled in the art upon reading the description and the examples.

REFERENCES

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