Abstract
The development of vascular grafts has focused on finding a biomaterial that is non-thrombogenic, minimizes intimal hyperplasia, matches the mechanical properties of native vessels and allows for regeneration of arterial tissue. In this study, the structural and mechanical properties and the vascular cell compatibility of electrospun recombinant human tropoelastin (rTE) were evaluated as a potential vascular graft support matrix. Disuccinimidyl suberate (DSS) was used to cross-link electrospun rTE fibers to produce a polymeric recombinant tropoelastin (prTE) matrix that is stable in aqueous environments. Tubular 1 cm diameter prTE samples were constructed for uniaxial tensile testing and 4 mm small-diameter prTE tubular scaffolds were produced for burst pressure and cell compatibility evaluations from 15 wt% rTE solutions. Uniaxial tensile tests demonstrated an average ultimate tensile strength (UTS) of 0.36±0.05 MPa and elastic moduli of 0.15±0.04 MPa and 0.91±0.16 MPa, which were comparable to extracted native elastin. Burst pressures of 485 ± 25 mmHg were obtained from 4 mm ID scaffolds with 453 ± 74 μm average wall thickness. prTE supported endothelial cell growth with typical endothelial cell cobblestone morphology after 48 hours in culture. Cross-linked electrospun recombinant human tropoelastin has promising properties for utilization as a vascular graft biomaterial with customizable dimensions, a compliant matrix, and vascular cell compatibility.
Keywords: Tropoelastin, Electrospinning, Mechanical properties, Vascular grafts, Tissue Engineering
1. Introduction
Heart disease remains the leading cause of death in the Western world with nearly 81 million people affected in the United States in 2006 [1]. Bypass surgery using autografts of saphenous veins or mammary arteries remains the gold standard treatment for severe cases, but can be limited by previous vessel harvest or preexisting disease. Synthetic graft materials, such as expanded poly(tetrafluoroethylene) (ePTFE) and poly(ethylene terephthalate) (PET or Dacron®), work well for large diameter vessels, but are not viable options for grafts smaller than six millimeters in diameter [2].
The failure modes of small diameter vascular grafts have primarily been thrombosis, aneurysm, and intimal hyperplasia [3]. To address these failure modes many researchers have studied both synthetic and natural biomaterial scaffolds. Synthetic biomaterials have controllable physical and mechanical properties that are highly reproducible and are easily manufactured in large-scale quantities, but many lack the elasticity of native arteries and biocompatibility for long-term vascular cell functionality. Considerable efforts have been made to functionalize synthetic surfaces [4, 5]. Natural biomaterial scaffolds, including well-studied grafts of decellularized blood vessels [6-8], have had limited success. The decellularized bovine [6] and human [7] blood vessels had promising 5 year patency rates, yet aneurysm formation due to in vivo degradation limited their widespread use [7, 8]. Decellularized arteries, from allogenic and xenogenic sources are attractive scaffolds for tissue-engineered vascular grafts due to their mechanical and biological properties [9], yet these natural scaffolds are limited by the lack of precise manufacturing control of the physical and mechanical properties, as well as problems with inflammation and calcification [18]. To reduce concerns of inflammation of the allogenic and xenogenic sourced vascular biomaterials, the biomaterials are frequently cross-linked; yet this has led to problems of limited cell repopulation and increased stiffness of the biomaterials [19]. While stiffness and compliance mismatch alone may not lead to vascular graft failure [27-29], graft compliance has correlated to the formation of intimal hyperplasia and should be considered in biomaterial scaffold design along with the potential of cellular remodeling of the graft and cell signaling capability [20-26]. The search for a viable off-the-shelf small diameter vascular graft that can match an autograft’s performance in terms of mechanical properties, cell compatibility, and vascular healing has been the focus of many research efforts, but has remained an elusive target.
The incorporation of vascular cells with biomaterial scaffolds to produce tissue engineered grafts have been successful in animal and, recently, human trials [10-15]. Production of the scaffold by the vascular cells has been accomplished using both in vivo [11,16-17] and in vitro [12,13] methods. The in vivo methods require the graft to be grown in the recipient’s peritoneal cavity. Recent advancements of this technique include improved scaffold design to produce multilayered scaffolds and the use of cyclic stretch to improve the assembly time and organization of the extracellular matrix [16,17]. Yet these in vivo methods require a second surgical site for autologous use. The in vitro methods of L’Heureux et al., where the tissue-engineered vascular grafts were produced from autologous cells without a scaffold, have advanced to clinical trails using an arteriovenous shunt model [12, 13]. These autologous tissue-engineered grafts have promising results with primary patency rates of 78% at 1 month and 60% at 6 months and the limited failures due to thrombosis, dilation, and aneurysm [12]. The in vitro cell produced scaffolds are elegant in design, but require lengthy production times potentially limiting their clinical use.
The use of electrospinning to make biomaterials has the capability of combining natural proteins with controllable physical and mechanical properties. Electrospinning produces submicron sized fibers from suspensions of monomers or polymers from both natural proteins and synthetic polymers [30-34]. Fibers produced from monomer suspensions can then be cross-linked to produce stable polymeric structures with customizable dimensions in terms of fiber diameter and overall graft dimensions. Electrospun fibrous scaffolds made from biodegradable polymers, such as poly( -caprolactone) (PCL), polylactic acid (PLA), polyglycolic acid (PGA), and poly(lactide-co-glycolide) (PLGA) [35-38] have been proposed for use in bone, cardiac, blood vessel, and wound dressing applications [39-45]. Several groups have successfully electrospun elastin for use in tissue-engineered grafts [46-52] and support material for vein grafts [53]. Most, however, have used animal sourced elastin that is [20, 54-56] extracted from already assembled and cross-linked protein forms. While these forms of elastin may provide the biochemical signaling of elastin, they remain an animal sourced material with the associated potential for immuno-rejection leading to structural degradation and ultimate aneurismal graft failure.
Our aim is to electrospin small diameter vascular grafts containing recombinant human tropoelastin, the monomer unit of elastin, that when cross-linked mimics native elastin fibers. Elastin is the principal structural component of elastic arteries responsible for energy storage and recovery, and contributes to their unique mechanical properties [60]. End stage aneurysm disease and supravalvular aortic stenosis have been associated with the pathologic loss of elastin or deficiency in elastin expression [61-68]. Elastin, as a blood-contacting surface on stents and grafts, reduced thrombus adherence and demonstrated good long-term patency [69, 70]. Establishing an elastic fiber structure in a vascular scaffold that is similar to the arterial wall has been well recognized, as the depletion or loss of elastin has been correlated to both aneurysmal progression and severe smooth muscle cell hyperplasia in both animals and humans.[61, 64, 65, 67, 70, 82-84]. Thus, elastin is a promising, and perhaps necessary, component in vascular graft development [71, 72]. Recent work has examined a class of elastin-like recombinant polymers with self-assembly properties and cross-link sites designed into the peptide sequence [57]. The elastin-like polymer has been used to produce organized multilayer collagen reinforced vascular grafts and abdominal wall repair tissue constructs with customizable mechanical properties, which make this technology promising for many soft tissue applications [58, 59]. Our use of electrospinning will enable the customization of the dimensions and mechanical properties for the vascular graft biomaterial, and the use of tropoelastin may impart critical cell signaling to the biomaterial.
2. Materials and Methods
2.1. Materials
Human tropoelastin was optimized and expressed from a synthetic gene codon in gram quantities in a 10-liter E.coli fermentation system. Gel electrophoresis determined that the purification procedure resulted in a greater than 99% pure product (Figure 1) as well as low endotoxin levels with an average of 0.2 EU/mg (1 EU = 100 pg of endotoxin) as determined by the Kinetic-QCL Assay (Cambrex). All chemical reagents were acquired from Sigma-Aldrich unless otherwise noted.
The purified human tropoelastin protein includes all of the functional exons with the exception of exons 1, 22, and 26A (Figure 2). Exon 1 contains the signal sequence, while hydrophobic exon 22, and hydrophilic exon 26A are rarely expressed in mature elastin. The resultant tropoelastin exon structure used is the same as a natural isoform produced by normal human fetal heart cells.
Extracted porcine elastin was isolated as previously described [69]. Briefly, porcine carotid arteries were obtained from domestic swine of 250 lb and 6–9 months of age (Animal Technologies, Tyler, TX) to size match the diameters. The arteries were shipped overnight in phosphate-buffered saline (PBS) on ice. The gross fat was dissected away and, using aseptic techniques, the arteries were placed in 80% ethanol for a minimum of 72 h at 4°C and subsequently treated with 0.25M NaOH for 70 min with sonication at 60°C, followed by two 30-min, 4°C washes in 0.05M HEPES (pH 7.4). The extracted elastin tubular conduits were then autoclaved at 121°C for 15 min and stored at 4°C in 0.05M HEPES buffer.
2.2 Electrospinning of rTE
Tropoelastin solutions of 15 wt% rTE in 1,1,1,3,3,3-hexafluro-2-propanol (HFP) were prepared and loaded into 2 or 5 mL glass syringes depending on the volume needed for each application. 18-gage stainless steel blunt tip needles were connected to the syringes and electrically coupled to a high voltage power supply (Glassman High Voltage, Inc., High Bridge NJ). A gap distance of 12.5 cm was set from the end of the needle to the center of the collection device. A syringe pump (Harvard Apparatus) was used to advance the protein solution at 2 mL/hr to refresh the solution at the tip of the syringe needle. Fibers were spun onto mandrels of either 1 cm diameter copper tubes for mechanical testing or 4 mm diameter stainless steel rods for small diameter graft production. Mandrels were connected to ground to complete the circuit. The collection system was set to rotate at 4400 rpm and translate longitudinally 6-8 cm with a rate of 8 cm/sec driven by a custom-built device with separate drives for longitudinal and rotational control. The solution was charged to an 18.5 kV excitation potential. All electrospinning was conducted within a chemical fume hood.
2.3. Cross-linking of Electrospun rTE
Disuccinimidyl suberate, DSS, (Pierce Biotechnology-Thermo Fisher Scientific Inc.), an organic amide bond cross-linker, was used to link electrospun rTE monomers to produce polymeric tropoelastin, prTE. Cross-linking was performed in a two-stage process. The electrospun rTE samples were incubated for 4 hours in DSS suspended in 50 mL anhydrous ethyl acetate, at a ratio of 0.072 mg of DSS per mg of rTE protein at room temperature in glass tubes. A second incubation occurred for 12-18 hours at a concentration of 0.108 mg of DSS per mg of rTE protein at room temperature. prTE samples were then rinsed in anhydrous ethyl acetate for 5 minutes with a second 5 minute rinse in 70% ethanol and a final 10 minute rinse in DI water. Final products were stored in 70% ethanol.
2.4. Electrospun rTE Fiber Characterization
The tubular scaffolds electrospun from 15 wt% prTE were analyzed with electron microscopy to determine fiber diameters and evaluate the degree of fiber orientation and consistency through the thickness of the graft. Electrospun prTE samples were mounted onto scanning electron microscopy (SEM) stubs and sputter-coated with 250 Å of gold/palladium. Micrographs were taken at magnifications from 3000 to 5000X and viewed at 5 kV on an FEI Sirion XL30 SEM. Image analysis of fibers was done with a custom MATLAB® program (MathWorks®) using a Laplacian edge detection algorithm followed by a Radon transform to determine the probability distribution of fiber orientation angles relative to horizontal.
2.5. Mechanical Properties of prTE
The mechanical properties of electrospun prTE samples were compared to extracted porcine elastin and native porcine carotid arteries. All uniaxial tensile tests were conducted on dogbone shaped specimens with a gage length of 10 mm and 4 mm grip ends. The tubular 1 cm diameter prTE samples were opened longitudinally, laid flat, and cut with a dye cutter. Four circumferential and four longitudinal sections were cut from each of the three electrospun samples. Eight longitudinal and eight circumferential samples were tested for native carotid arteries and extracted elastin conduits. All specimens were rehydrated in PBS for at least 15 minutes prior to testing. The thickness, width, and gage length were recorded. The samples were mounted on custom tensile grips on a Chatillon Vitrodyne V1000 system with a 500 gram load cell or on a MTS 858 Mini Bionix II mechanical tester with a 5 lb load cell using spring action grips. All dogbone prTE samples were tested in tension at room temperature with a crosshead speed of 2 mm/sec until failure. Force and displacement measurements were acquired at 0.1 sec intervals. Engineering stress (force/cross-sectional area, F/Acs) and strain (change in length/original length, L/Lo) were calculated and plotted. Linear regression of the slope in the stress-strain plots was used to calculate the elastic modulus (stress/strain, / ). Elastic modulus 1 was measured between 10 and 30% strain, while elastic modulus 2 was measured between the maximum strain minus 20% and the maximum strain with linear curve fits to these regions of the stress strain curve. Peak stress (MPa) and strain (%) were taken as ultimate tensile strength (UTS) and percent elongation (ultimate strain). Compliance measurements were calculated using the stress and strain data between 50 and 100 kPA. Calculated values were based on the ANSI/ISO 7148 standard for “Cardiovascular implants – tubular vascular prostheses” [73]. Radius values at these stress values were calculated using a thin-walled cylinder approximation relating pressure to stress scaled by wall thickness and initial radius (Equation 1). Compliance was measured as the change in radius relative to the initial radius over the change in pressure or stress at 100 kPA and 50 kPa for each material (Equation 2).
Equation 1 |
Equation 2 |
Where = circumferential Cauchy stress, P = pressure, t = wall thickness, r = radius, R2 = radius at P2, and R1 = radius at P1.
2.6. Burst Pressure of prTE Scaffolds
Three 4 mm inner diameter, 5 cm long electrospun prTE scaffolds were fabricated for burst pressure analysis. Scaffolds of rTE were electrospun, cross-linked and stored in 70% ethanol prior to analysis. Wall thickness was measured using handheld digital micrometers and recorded. Scaffolds were cannulated onto barbed nylon connectors and secured using cotton umbilical tape. Samples were rehydrated in PBS for at least 30 minutes prior to testing. The ends of the scaffolds were fixed in position under zero longitudinal strain/load and saline was subsequently infused at a rate of 100 mL/min until failure occurred. The pressure (mmHg) was continuously monitored by an inline pressure transducer (Cole Parmer) and recorded with a custom built LabVIEW (National Instruments) data acquisition program.
2.7. Endothelial Cell Growth on prTE Scaffolds
Porcine bone marrow derived endothelial outgrowth cells (BMEOCs) were isolated and used to assess the growth of vascular cells on the lumenal surface of electrospun prTE vascular grafts. Porcine bone marrow mononuclear cells were collected and separated as previously reported [74]. Isolated cells were differentiated into BMEOCs in endothelial cell growth media (EGM2) at 37 C and 5% CO2 in a tissue culture incubator. BMEOCs were passaged and maintained in endothelial cell growth media (EGM2) using standard techniques. BMEOCs were stained with endothelial cell specific von Wildebrand factor (vWF, DAKO).
Tubular prTE grafts were rehydrated in growth media for 1 hour. Vessels were inoculated with BMEOCs (5 × 103 cells/cm2) and held at 90 mmHg for 1 hour. Grafts were then maintained in a cell culture incubator for 48 hours in standard conditions. Grafts were fixed with 2.5% paraformaldehyde at 48 hours and evaluated for cell engraftment with DAPI nuclear stain and rhodamine phalloidin f-actin stain. Confocal images were taken with a 63X oil objective on a Zeiss Multiphoton Confocal microscope using 543 and 780 nm excitation wavelengths.
2.8. Statistical analyses
All data are expressed as the mean ± standard deviation. Student’s t-test, linear regression, and one-way ANOVA with Tukey post hoc tests were used for hypothesis testing, with p < 0.05 as the measure for statistical significance. The number of independent tests is listed for each experiment.
3. Results and Discussion
Electrospinning has proven to be a valuable tool to produce biomimetic scaffolds for use in tissue engineering. Electrospun vascular graft materials have included natural proteins, such as collagen and elastin, and biodegradable polymers either as stand alone materials or as blends with other polymers or natural proteins [33, 56, 76]. The number of materials used for electrospinning is increasing as well as the design complexity with multilayered constructs [16, 58, 59, 77, 78] and materials with tunable mechanical properties [59, 78, 79]. Elastin is emerging as an important component of vascular graft development with our increased understanding that synthetic polymers alone pose problems with compliance mismatch and foreign body response [56]. Elastin has unique properties making it a natural choice as a component in vascular scaffold biomaterials that require long-term durability, antithrombogenic properties, and elasticity. Elastin is highly insoluble with a half life of greater than 70 years; it modulates cell function reducing the thrombogenic potential of the surface; and it is highly elastic thus adding compliance to the structure of the biomaterial [80]. Electrospinning of tropoelastin into a biomaterial was first reported in 2005 [51]. Widespread use of tropoelastin for biomaterial development has been limited by the availability of monomeric tropoelastin. Since 2005, the use of tropoelastin has increased and has been incorporated into additional vascular graft scaffolds [78, 80] and coatings on stent struts [81]. The current work describes methods of electrospinning recombinant human tropoelastin into tubular grafts, cross-linking the material into a stable polymer, and characterizing its structural, mechanical, and cell compatibility properties.
3.1. Morphology and Substructure of prTE Fibers
To produce purely electrospun prTE tubular scaffolds, 15 wt% solutions of rTE were electrospun onto rotating mandrels and cross-linked. Conduits were 4-10 cm in length, 4 mm in diameter, with wall thicknesses of 0.43-0.65 mm (Figure 3A). The wall thickness was dependent on the volume of the rTE solution used. The prTE fibers were randomly oriented as determined using image analysis to calculate the probability distribution function of fiber orientation angles relative to horizontal (Figure 4). The average fiber diameters (580 94 nm) and fiber structure (Figure 3B) of the electrospun protein was maintained throughout the thickness of the graft (data not shown).
3.2. Mechanical Properties of prTE
Uni-axial tensile testing of prTE samples from 15 wt% rTE produced stress-strain curves (Figure 5) for both the longitudinal and circumferential sample orientations. The curves were similar for the two orientations showing a bimodal stress-strain relationship in which the modulus was dependent on the percent strain. The transition in moduli values occurred between 40 and 50% strain. The only mechanical property that was significantly different between the longitudinal and circumferential orientations of electrospun prTE was the elastic modulus 2 (t-test, p < 0.01). The remaining mechanical properties (UTS, % elongation, and elastic modulus 1) were not significantly different (t-test, p > 0.05) between the two orientations (Figure 6). Combining electrospun prTE’s longitudinal and circumferential orientations measurements, the average UTS, elastic modulus 1 and percent elongation were 0.36 ± 0.05 MPa, 0.15 ± 0.04 MPa, and 77 ± 5%, respectively. Elastic modulus 2 values were not combined because they were significantly different between orientations.
Ultimate tensile strength (UTS), percent elongation, and elastic moduli for electrospun prTE were compared to extracted porcine elastin and native porcine carotid arteries for the longitudinal (L) and circumferential (C) orientations (Figure 6). The electrospun prTE samples had UTS values of 0.34 ± 0.14 MPa (C) and 0.38 ± 0.05 MPa (L). The UTS values for the electrospun prTE were comparable to extracted porcine elastin in the longitudinal direction, yet significantly different to circumferential extracted elastin and both native carotid artery specimens (ANOVA, Tukey post hoc, p < 0.05). The percent elongation at failure of the electrospun prTE was 79 ± 6% (C) and 75 ± 5% (L), which was significantly lower than the control materials in both orientations (ANOVA, Tukey post hoc, p < 0.01). The average elastic moduli of electrospun prTE were 0.15 ± 0.05 MPa (C) and 0.15 ± 0.03 MPa (L) for elastic modulus 1 and 0.82 ± 0.11 MPa, (C) and 0.99 ± 0.17 MPa (L) for elastic modulus 2 which were comparable to extracted elastin in the longitudinal direction for elastic modulus 1 and in both orientations for elastic modulus 2. Both prTE elastic moduli were significantly different from the native carotid materials (ANOVA, Tukey post hoc, p < 0.05)
Average compliance values for electrospun prTE, extracted elastin, and native carotid arteries were 20.2 2.6, 32.0 3.1 and 3.4 0.5 % respectively, which were all significantly different (ANOVA, Tukey post hoc, p < 0.01). Extracted elastin lacks collagen and therefore is expected to have greater compliance. The compliance of electrospun prTE fell between extracted elastin and native carotid arteries. This allows for the addition of stiffer materials, such as collagen, to the biomaterial to both strengthen the vessel in terms of UTS while maintaining compliance equivalent to native vessels.
The mechanical properties of electrospun proteins are dependent on the specific proteins selected, the protein concentration, electrospinning parameters, cross-linkers, and fiber orientation [51, 76, 85-87]. The mechanical properties of the circumferential and longitudinal orientations of the prTE materials were similar, where the only measured significant difference was in the elastic modulus 2 of electrospun prTE. UTS values of prTE electrospun materials were between the values of native extracted elastin in the longitudinal and circumferential directions and were much lower than the native carotid artery [88-93]. These results were expected due to the random (non-oriented) nature of the electrospun prTE fibers compared with the oriented fibers of native elastin [94], and due to the presence of collagen in the native matrix. Additionally, the elastic modulus 1 of electrospun prTE, measured on the initial linear slope of the stress-strain curve, were comparable to the extracted elastin. Native elastic fibers (composed of elastin and fibrillin-1) contribute significantly to the material properties of native elastic arteries [95] in this initial linear slope region of the stress-strain curve. Native arteries are true composites of matrix proteins and the transition in elastic modulus is primarily due to elastin and collagen’s unique mechanical contributions working in concert. Therefore, the incorporation of prTE into a collagen scaffold is likely to increase the compliance of the vascular graft. The material properties of the electrospun prTE biomaterials were significantly different from the electrospun human tropoelastin by Li et al. [51]. The prTE had lower average UTS (0.36 MPa vs. 13 MPa) and average elastic moduli (0.15 MPa (elastic modulus 1) and 0.91 MPa (elastic modulus 2) vs. 289 MPa), yet a higher average percent elongation at failure (77% vs. 15%). It should be noted that only a single mechanical test was reported for Li’s electrospun tropoelastin due to limited availability of protein [51]. The prTE materials were more elastic with a lower failure stress than Li’s previously reported electrospun tropoelastin [51]. These disparities could be due to significant differences in electrospinning methods, testing methods, and cross-linking strategies. Our electrospinning parameters differ from Li et al., in several ways, including lower concentration of tropoelastin, higher accelerating voltage, and a smaller gap distance, which resulted in smaller and cylindrically-shaped fibers [96] for our prTE. The mechanical property evaluation by Li et al. utilized a unique testing system designed to evaluate textiles, which included the measured material weight to calculate stress. This measurement can be variable due to differences in the hydration of the tropoelastin. Our engineering stress calculations were based on the measured initial cross-sectional area. Additionally, to crosslink the tropoelastin Li et al. used hexamethylene diisocyanate (HMDI), which binds lysine or hydroxylysine residues, but may also react with nucleophilic functional groups such as amines, alcohols, and protonated acids. HMDI has been shown to react with side chains of lysine, cysteine, histidine and tyrosine and may as well react to arginine, and aspartic acid. Nonspecific binding of residues by HMDI may affect the functionality and water content [97], thus altering the mechanical properties of cross-linked tropoelastin. DSS in comparison is specific to amines on lysine residues with an 8 atom bridge resulting in a 11.4 Angstrom crosslink arm. The specificity of DSS to lysine [98] leaves the cell binding domains available on the molecule as well as results in improved consistency of mechanical properties.
The mechanical properties were comparable to extracted elastin scaffolds, but still lack the tensile strength to support in vivo arterial pressures. For vascular graft applications, the tensile strengths of the prTE scaffolds must be further increased by reinforcement or co-spinning with either collagen or synthetic materials.
3.3. Burst Pressure of prTE Scaffolds
The electrospun prTE tubular scaffolds (n=3) had an average wall thickness of 453 74 μm and an average burst pressure of 485 25 mmHg. Scaffolds increased in size both longitudinally and circumferentially throughout the burst pressure test and test samples failed longitudinally in all cases. Saphenous vein and internal mammary artery grafts, the gold standard treatments, have reported burst pressures of 1599 877 and 3196 1264 mmHg, respectively [101]. Extracted porcine carotid elastin has a reported burst pressure of 162 ± 36 mmHg [69], which is significantly lower than the electrospun prTE, however, the UTS measurements were comparable between our electrospun and extracted elastin samples. Burst pressure differences could be due simply to differences in wall thickness or a more complex mechanism involving variations in fiber architecture, which would lead to altered loading on individual fibers during biaxial deformation of the matrix. While an average burst pressure of 485 mmHg for our electrospun graft is sufficient for initial in vivo testing of host response, higher failure pressures of at least 1500 mmHg would need to be achieved to give an ample safety factor (>10) for its widespread clinical use.
3.4. Endothelial Cell Growth on prTE Scaffolds
Organic solvents, such as HFP, facilitate the electrospinning of pure protein solutions, due to improved protein solubility and solvent volatility. HFP has been shown to affect the conformation of electrospun collagen [99], which could have a drastic effect on its stability and mechanical properties. Tropoelastin is unlikely to be affected, as it is a single chain molecule that easily regains its secondary structure on removal of denaturants. The similarity in mechanical properties of prTE and extracted native elastin indicate minimal conformational changes in the prTE. The cytotoxic effects of HFP must be considered in construct design. HFP at concentrations above 250 ppm is toxic to cells [100]. The residual solvent HFP can be present in electrospun materials, but is likely removed through post processing (heat/vacuum treatments) of the material [100]. Our electrospun materials have been shown to support vascular cell growth [96], thus indicating low residual solvent levels, but a full evaluation of residual HFP should be conducted prior to conducting in vivo implant studies.
Bone marrow derived endothelial outgrowth cells (BMEOCs) attached, spread, and grew on the 15 wt% prTE tubular scaffolds. BMEOCs stained positive for vWF indicating an endothelial cell population (Figure 7A & B). Confocal images taken at 48 hours showed cells well attached and spread on the electrospun fiber matrix. Cells formed a confluent monolayer with typical endothelial cell cobblestone morphology (Figure 7C). This supports the hypothesis that prTE is a cell compatible matrix for both endothelial cells as well as, previously reported, smooth muscle cells [102], which demonstrated positive SMC growth and proliferation on prTE over a week with logarithmic cell growth between 3 and 5 days via integrin mediated binding mechanisms.
4. Conclusions
An electrospun tubular vascular scaffold material has been developed, composed of cross-linked recombinant human tropoelastin, which has physical and mechanical properties similar to extracted arterial elastin. The graft architecture, i.e. length and diameter, of the prTE scaffold can be precisely designed and controlled. A cross-linked stable polymer assembled from recombinant human tropoelastin provides both the compliance and support of endothelial cell adhesion for a component of a vascular graft biomaterial. While the mechanical strength of the prTE scaffolds are insufficient for implantation alone, the relatively lower compliance compared to native arteries will allow for the addition of stronger, but stiffer biomaterials. This technology holds great promise for incorporation in small diameter vascular graft biomaterials.
Acknowledgements
We would like to thank Dr. Michael Rutten for isolation of the bone marrow mononuclear cells and Dr. Sean Kirkpatrick for assistance with fiber orientation code development. Tropoelastin was produced with the excellent technical assistance of Amy Jay, Cher Hawkey, and Rose Merten. This work was funded in part by the NIH R01-HL095474, NIH R01-HL103728, and the Department of the Army, Grant Nos. W81XWH-04-1-0841 and W81XWH-05-1-0586. This work does not necessarily reflect the policy of the government and no official endorsement should be inferred.
Footnotes
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