Eggshell Membrane as a Bioactive Agent in Polymeric Nanotopographic
Scaffolds for Enhanced Bone Regeneration
Daun Kim†1, Yonghyun Gwon†1, Sunho
Park1, Sujin Kim1, Woochan
Kim1, Kwidug Yun*2, Jangho
Kim*1
1 Department of Rural and Biosystems Engineering,
Chonnam National University, Gwangju 61186, Republic of Korea
2 Department of Prosthodontics, School of Dentistry,
Chonnam National University, Gwangju, 61649, Republic of Korea.
+D.K. and Y.G. contributed equally to this work.
* Corresponding authors: Correspondence should be
addressed to J.K.
(rain2000@jnu.ac.kr ) or
Y.G. (ykd@chonnam.ac.kr )
Abstract
A bone regeneration scaffold is typically designed as a platform to
effectively heal a bone defect while preventing soft tissue
infiltration. Despite the wide variety of scaffold materials currently
available, such as collagen, critical problems in achieving bone
regeneration remain, including a rapid absorption period and low tensile
strength as well as high costs. Inspired by extracellular matrix protein
and topographical cues, we developed a polycaprolactone-based scaffold
for bone regeneration using a soluble eggshell membrane protein (SEP)
coating and a nanotopography structure for enhancing the physical
properties and bioactivity. The scaffold exhibited adequate flexibility
and mechanical strength as a biomedical platform for bone regeneration.
The highly aligned nanostructures and SEP coating were found to regulate
and enhance cell morphology, adhesion, proliferation, and
differentiation in vitro . In a calvarial bone defect mouse model,
the scaffolds coated with SEP applied to the defect site promoted bone
regeneration along the direction of the nanotopography in vivo .
These findings demonstrate that bone-inspired nanostructures and SEP
coatings have high potential to be applicable in the design and
manipulation of scaffolds for bone regeneration.
Keywords: biomimetic, eggshell membrane, nanotopography, bone
regeneration, tissue engineering
1.Introduction
Bone defects are frequent pathological problems of orthopedic and
odontology diseases worldwide (Giannoudis, Dinopoulos, & Tsiridis,
2005). In particular, bone loss due to massive trauma can exceed the
critical size, beyond which self-healing is difficult. The current gold
standard for treating these critical-size defects is an autogenous bone
graft. However, autogenous bone grafts suffer from several limitations,
including the high cost of surgery, complicated microsurgery techniques,
and limited treatment of large bone defects (H. N. Kim et al., 2013;
Lichte, Pape, Pufe, Kobbe, & Fischer, 2011; Lim, Suh, Kim, Choung, &
Chung, 2011; McMahon, Wang, Skoracki, & Mathur, 2013; Wang, Kim,
Vunjak-Novakovic, & Kaplan, 2006). Consequently, an effective platform
is required to achieve the goals of bone regeneration (BR) (J. Kim et
al., 2014). Several types of scaffolds have been introduced as an
effective treatment method for BR. For example, the BR membrane, which
is mainly used for alveolar BR during implant in the odontology field,
guides the induction of surrounding bone tissue and promotes BR while
preventing soft tissue invasion (Chiapasco, Casentini, & Zaniboni,
2008; Fujihara, Kotaki, & Ramakrishna, 2005; H, Hammerle, & Karring,
1998; Rakhmatia, Ayukawa, Furuhashi, & Koyano, 2013). The general
conditions required for a BR scaffold are as follows: (1) excellent
biocompatibility and adhesion to tissue cells, (2) porosity to maintain
the permeation of nutrient sources, (3) blocking ability to inhibit the
migration of regenerative inhibitory cells, (4) space maintenance
ability to provide sufficient growth space for cells, (5) excellent
mechanical strength and flexibility, and (6) ease of operation (Elgali,
Omar, Dahlin, & Thomsen, 2017).
BR scaffolds can be generally classified into those based on materials
with an absorption property such as collagen, and those without
absorption such as high-density polytetrafluoroethylene (d-PTFE) and
titanium (Kasaj et al., 2008; Rakhmatia, Ayukawa, Atsuta, Furuhashi, &
Koyano, 2015; Sheikh et al., 2017; Song, Kim, & Kim, 2007). However,
the efficiency of these scaffolds to regenerate bone defects is still
limited owing to quick absorption, low mechanical strength, and
secondary surgery, as mentioned above. To overcome these disadvantages,
researchers have focused on scaffolds based on polymers to prepare
synthetic BR scaffolds, including poly(lactide-co-glycolic acid) (PLGA),
polyglycolic acid (PGA), polylactic acid (PLA), and polycaprolactone
(PCL) (G. Chen et al., 2013; Gentile, Chiono, Tonda-Turo, Ferreira, &
Ciardelli, 2011; Shim et al., 2013; Shim et al., 2014; Zhang et al.,
2016). Among these, PCL is widely used in the biomedical field owing to
its advantageous properties such as biodegradability, biocompatibility,
high rigidity, and flexibility. In addition, PCL is a common material
used to manufacture US Food and Drug Administration (FDA)-approved
devices and is also relatively inexpensive (Gunatillake, 2003; J. C.
Middleton., 2000; D. Kim et al., 2020). Therefore, PCL is considered to
be one of the ideal candidates for the development of scaffolds for BR.
Nevertheless, PCL still has many limitations such as its hydrophobic
property and low adhesion, which leads to low cell attachment,
proliferation, and differentiation.
Eggshells have long been treated as waste and the amount of eggshell
waste is increasing annually (Balaz, 2014; Park et al., 2016). However,
the membrane components in eggshells have proven to be useful for tissue
regeneration, and many methods have been developed to reduce eggshell
waste (Farjah, Heshmatian, Karimipour, & Saberi, 2013; Kang, Chen,
Okubayashi, & Sukigara, 2012). The eggshell membrane (ESM) is a
semi-permeable membrane with a fiber structure comprising an inner and
outer double layer located between the eggshell and the egg white (Meng
& Deng, 2016; Park et al., 2016). The constituents include both organic
and inorganic matter, with collagen (type I, V, and X), osteopontin
(OPN), fibronectin, and CaCO3 as the major components
(M. K. Sah & Rath, 2016). In addition, ESM functionally prevents the
mineralization of embryos, exchanges gases, and prevents bacteria from
penetrating the egg (jun Jia, Guo, Yu, & Dauan, 2011; Park et al.,
2016; M. K. Sah & Rath, 2016). Therefore, ESM has been mainly used in
the biomedical field for wound dressings, and has also proven to be an
efficient platform for tissue regeneration (Guha Ray et al., 2018; Kang
et al., 2012). However, raw ESM has limitations in various applications
owing to the difficulty in controlling its size and thickness.
Therefore, various processing
methods have been developed to overcome this limitation. For example, Yi
et al. (Feng Yi, Yu, Guo, Zhang, & Li, 2003) produced soluble eggshell
membrane protein (SEP) from raw ESM using organic solvents. The
fabricated SEP showed good bioactivity (e.g., adhesion and
proliferation) compared to the collagen-type scaffold. In addition, Sah
et al. (Mahesh Kumar Sah & Pramanik, 2014) demonstrated increased
adhesion and proliferation of cells in vitro by conjugating SEP
to a porous silk fibroin scaffold, which also showed good
biocompatibility in vivo. Jia et al. (J. Jia, Duan, Yu, & Lu,
2008) further confirmed that the proliferation and adhesion of cells
were improved by immobilizing PCL nanofibers using SEP, and SEP also
improved the mechanical strength. In addition, amino acid compositions
have been shown to have similar effects to SEP and raw ESM, suggesting
that coating of SEP may have great potential for improving the limited
bioactivity of PCL owing to its biomimetic role, which can offer ideal
conditions for a variety of applications (F. Yi, Guo, Zhang, Yu, & Li,
2004).
Living cells are highly sensitive to the complex, well-defined
structural extracellular matrix (ECM) environment that can regulate cell
fate and function. The ECM has various topographical characteristics
ranging from the microscale to nanoscale. Many ECM proteins interact
with a variety of factors to regulate the complex behavior of cells. The
ECM of several tissues such as the bone, nerves, and skin with a
well-ordered orientation represent geometric structures that form
directional structures that affect cell function (D.-H. Kim, Provenzano,
Smith, & Levchenko, 2012; H. N. Kim, Hong, Kim, Kim, & Suh, 2012; J.
Kim, H. N. Kim, K. T. Lim, Y. Kim, S. Pandey, et al., 2013; J. Kim, H.
N. Kim, K. T. Lim, Y. Kim, H. Seonwoo, et al., 2013). The bones consist
of collagen and hydroxyapatite, and the protein fibers of the ECM are
arranged in a complex hierarchical structure with grooves at the tens of
micro- to nanoscale (J. Kim et al., 2014; Liu, Luo, & Wang, 2016). The
fate and function of osteogenic cells depend on the structure and
orientation of the fibers in the highly aligned ECM topography.
Therefore, by mimicking the ECM structure of the bone, it would be
possible to promote BR by increasing the bioactivity property.
In this study, we used the following two strategies to promote BR.
First, a patch-type scaffold was coated with SEP to convert the
hydrophobic property to a hydrophilic property and improve the
mechanical properties. Second, inspired by the ECM of the bone, we
produced nanogrooves in the scaffold to improve the bioactivity of the
cells. We investigated the effects of SEP function and topographical
cues on the proliferation, differentiation, and morphology of osteogenic
cells. In addition, we used a calvaria bone defect mouse model to
evaluate whether our newly developed SEP-coated bone-inspired platform
can promote BR in vivo .
2.Materials and Methods
Design and Fabrication of PCL Patches and SEP-Coated PCL patches .
The UV-assisted polyurethane acrylate (PUA; Changsung Sheet, Korea)
precursor solution was dropped onto the silicon master mold containing
nanosized linear grooves (800 nm). The silicon master mold was then
covered with 100-μm-thick poly(ethyleneterephthalate) (SKC, Korea) film.
For curing, the master mold covered with the PUA precursor was exposed
to UV light (λ= 310–400 nm, 40 W) for 30 s.
The polydimethylsiloxane (PDMS) mold for manufacturing the flat/nano
structure was fabricated as follows. To fabricate the flat mold, the
silicon wafer used to fabricate the PDMS (Sylgard 184 Silicon elastomer,
Dow Corning, USA) mold was fixed to a Petri dish. The PDMS pre-polymer
was mixed with a 10% (w/w) curing agent solution and poured onto the
clean silicon wafer, which was baked at 60 ℃ for at least 4 h. The nano
mold was fabricated in the same manner as the flat mold after fixing the
PUA mother mold to the Petri dish. Before curing the PDMS solution,
bubbles were removed from the vacuum condition for 1 h.
To fabricate the ESM solution, the raw ESM was peeled off from the
eggshell by hand. The separated raw ESM was washed several times with
distilled water, dried, and then ground in a blender for 5 min. The
eggshell powder was dissolved in a hotplate with a magnetic stirrer
using 3-mercaptopropionic acid (Sigma-Aldrich, USA), acetic acid
(Daejung Chemicals & Metals, Republic of Korea), and deionized water at
120°C at 1500 rpm for 3 days. The low-pH ESM solution was adjusted to pH
5 using sodium hydroxide (NaOH, Sigma-Aldrich, USA); the neutralized ESM
was washed three times with methanol (Daejung Chemicals & Metals,
Republic of Korea) and distilled water and then dried in a vacuum oven
at 70°C for 2 h. Finally, the dried ESM powder was dissolved in a
magnetic stirrer using 10% acetic acid.
PCL beads (Mw: 80,000; Sigma-Aldrich, USA) were dissolved in
dichloromethane (18 wt.%) using a magnetic stirrer for 1 day. To
fabricate PCL patches, the PCL solution was poured onto a clean square
glass (18 mm × 18 mm) and spin-coated at 3500 rpm for 240 s. The glass
coated with PCL was pressed at ~70 kPa with flat PDMS
fabricated on a hot plate at 80°C. After the imprinting process,
fabricated flat PCL patches were cooled off at room temperature and the
PDMS mold was peeled off on the PCL patches. Using the same process, the
PCL flat patches were pressed at ~70 kPa with a nano
PDMS fabricated on a hot plate at 80°C. Likewise, the nano patches were
cooled off at room temperature and the PDMS mold was peeled off on the
PCL flat patches. The fabricated PCL flat/nano patches were dip-coated
using the SEP solution for 1 h at room temperature. After the coating,
the PCL patches were vacuum treated to remove the organic solvent
overnight.
Characteristics of SEP-Coated PCL Patches . High-resolution
field-emission SEM images of the flat/nano surface and SEP-coated
flat/nano surface of PCL topography patches were acquired using a
JSM-7500F microscope (JEOL Ltd., Japan) at a resolution of ×5000 with an
acceleration voltage of 15 kV. AFM images of the SEP-coated PCL
topography patches were acquired using an XE-100 microscope (Park
Systems, Korea).
FT-IR was performed using a Spectrum 400 system (PerkinElmer, USA) to
confirm the chemical bond structures of the PCL topography patches,
SEP-coated PCL topography patches, and ESM solution. The contact angles
were measured by acA1300-30 μm (Basler). Water droplets were dropped
onto the surface of 5.0-μm PCL and SEP-coated PCL topography patches.
The contact angles were averaged by measuring three other samples using
ImageJ software (NIH, Bethesda, MD, USA).
The mechanical test of strain and stress of PCL and SEP-coated PCL
patches was performed using MCT-1150 tensile testers (A&D Company,
Japan) at a test speed of 100 mm/min. The bone-inspired PCL and
SEP-coated PCL patches were measured by applying load along the
direction of the aligned nanotopography. The experiments were analyzed
for 10 specimens per sample with the same interval set. The normal and
shear adhesion forces of PCL and SEP-coated PCL patches to porcine rind
were measured using the MCT-1150 instrument at a test speed of 50
mm/min. Prior to the adhesion test, the fresh porcine rind was rinsed
with deionized water. PCL patches were attached to the surface of the
porcine rind and were measured under a preload of
~0.5/cm2 by gradually increasing the
pulling weight until the adhesion force felled off.
In
Vitro Study. Adherent cells on PCL and SEP-coated PCL patches were
fixed with a 4% paraformaldehyde solution (Biosesang, Korea) for 15 min
and permeabilized with 0.2 % Triton X-100 (Biosesang, Korea). The
samples were then blocked with 3% normal goat serum (NGS; Abcam,
Cambridge, MA, USA) in phosphate-buffered saline (PBS; Biosesang,
Korea). The patches were incubated overnight at 4°C with Vinculin
(Millipore, Billerica, MA, USA). Following a wash in PBS, the patches
were stained with TRITC-conjugated phalloidin (Millipore) for 1 h and
then with 4, 6-diamidino-2-phenylindole (DAPI; Millipore) for 3 min. The
images of the stained cells were obtained using a laser confocal
scanning microscope. Osteoblast s(1 × 104cells/samples) were seeded onto the 15-mm circle samples and cultured
for 6 h, 3 days, and 5 days at 37℃ in a humidified atmosphere containing
5 % CO2. The growth medium consisted of high-glucose
Dulbecco’s modified Eagle’s medium (Cellgro, USA) supplemented with 10
% fetal bovine serum (Cellgro, USA) and 1% penicillin-streptomycin
(GenDEPOT, Houston, TX, USA). Every 3 days, the medium was replaced with
fresh growth medium. Quantitative analysis of proliferation on the PCL
and SEP-coated PCL topography patches was performed using the WST-1
assay (Takara Bio Inc., Japan). Before adding the reagent, the patches
were washed with PBS. The reaction was carried out for 4 h, and the
extracted stains were measured using an enzyme-linked immunosorbent
assay reader (iMark Microplate Absorbance Reader, Bio-Rad, Hercules) at
450 nm to quantify cell proliferation.
The cells (2 × 104 cells/samples) were seeded onto the
15-mm circle samples and cultured for 1 day. After cell proliferation,
the culture medium was replaced with osteogenic differentiation medium
(100 nM dexamethasone, 50 μm ascorbic acid, and 10 mM
β-glycerophosphate; Sigma Aldrich, USA). After 3 days, the medium was
replaced with fresh osteogenic differentiation medium. After 7 and 14
days, the cells were washed with PBS and fixed in 4% paraformaldehyde
for 15 min. Alkaline phosphatase blue membrane solution (Sigma Aldrich,
USA) staining was performed to confirm the early osteogenic
differentiation of osteoblasts on the sample surfaces. The stained cells
were de-stained with SensoLyte pNPP Alkaline Phosphatase Assay Kit
(AnaSpec, Inc., USA), and the extracted stains were measured using a
microplate reader at 405 nm to quantify the osteogenic differentiation
of osteoblasts. ARS (Sigma–Aldrich, USA) staining was performed to
confirm the later osteogenic differentiation of osteoblasts on the
sample surfaces based on the degree of mineralization. The stained cells
were de-stained with cetylpyridinium chloride (Sigma Aldrich, USA), and
the extracted stains were measured using a microplate reader at 595 nm
to quantify the osteogenic differentiation.
A thin PDMS slab was utilized to generate a cell-free area for
investigating the migration and wound-healing effects of osteoblasts on
the samples. Specifically, a 3-mm-thick PDMS sheet was cut into slabs
with a 3-mm round using a steel punch. The PDMS slabs were placed onto
the patch surface. Osteoblasts (1 × 105 cells/samples)
were cultured on the wound generation samples. The PDMS slabs were then
removed manually with sharp tweezers and the cells of the wound healing
system were observed at 24 h by immunofluorescence staining using a
fluorescence microscope (Zeiss, Germany). The cell-covered area and
migration speed in wound-healing analysis were investigated using ImageJ
software.
For western blot analysis, RIPA Cell Lysis buffer (Biosesang, Korea)
with Xpert proteinase inhibitor cocktail (GenDEPOT, Huston, TX, USA)
were used to extract proteins from the cells. Lysed protein was
incubated on ice for 30 min and then centrifuged at 13,000 rpm for 30
min at 4°C. Protein concentrations were analyzed using the DC protein
assay kit (Bio-Rad, Hercules, CA, USA) and the Lowry assay method. Equal
amounts of proteins were loaded on sodium dodecyl sulfate-polyacrylamide
gel electrophoresis gels and then transferred onto a polyvinylidene
difluoride membrane (Millipore, IPVH00010) using an electroblotting
apparatus at a constant voltage of 30 V for 1 h. The membrane was
blocked for 1 h with 5% skim milk powder in Tris-buffered saline with
Tween (TBS-T). Subsequently, the membrane was incubated with the
following primary antibodies overnight at 4°C: OPN (1:2000, Abcam,
Cambridge, MA, USA), ERK (1:1000, Santa Cruz Biotechnology, CA, USA),
FAK (1:1000, Cell Signaling Technology, Beverly, MA, USA), and GAPDH
(1:5000, Abcam, Cambridge, MA, USA). Goat anti-mouse IgG (H+L)-HRP and
goat anti-rabbit IgG (H+L)-HRP (GenDEPOT, Houston, TX, USA) were used as
the secondary antibodies at a dilution of 1:10,000 for 1 h at room
temperature, and then the membrane was washed three times for 10 min
each in TBS-T. Bands were detected using West Pico PLUS Chemiluminescent
Substrate (Thermo Scientific, Waltham, MA, USA). Quantification of the
western blot was performed using image lab 6.0 (Bio-Rad, Hercules, CA,
USA) software with normalization to the level of the entire protein.
In Vivo Animal Study . The
animal study was approved by the Ethics Committee of Chonnam National
University (CNU IACUC-YB-2019-37). Twenty-two male mice (C57Bl/6N) were
assigned into two groups of 11 mice each: uncoated PCL topography
patches and SEP-coated PCL topography patches. The mice were fully
anesthetized with an intraperitoneal injection of zoletil (0.006 cc/10
g) and rumpun (0.004 cc/10 g), and then the head was shaved and
disinfected. The bones were exposed by incising the skin approximately
3.0 cm above the calvarial bone. A 3-mm bone defect was made on the
right and left sides of the revealed calvarial bone using an electric
drill. Patches were placed onto the calvarial bone defects. After
suturing the skin, the ambient temperature was raised, and the mice were
woken up from the anesthesia. The mice were sacrificed 3 weeks after
surgery to obtain tissues including the defect region and the calvaria
bone.
Calvaria bone tomography was performed with Skyscan001172 (Skyscan,
Konitch, Belgium) microcomputed tomography (μ-CT) at a resolution of
11.38 pixels and exposure time of 316 ms, with an energy source of 80 kV
and current of 124 uA. An average of 488 slices of calvarial bone was
scanned. The μ-CT images were analyzed using MIMICS 14.0 3D imaging
software (Materialise’s Interactive Medical Image Control System,
Leuven, Belgium). The calvarial bone specimens were fixed in 10%
formalin and decalcified in a 0.5 M ethylenediaminetetraacetic acid (pH
7.4) solution at room temperature for 7 days. After the specimens were
embedded in paraffin, they were cut into 5-mm-thick sections and then
stained with H&E. Images were obtained by Aperio ImagesScope (Leica,
CA, USA) software.
Statistical Analysis. Student’s t-tests were used for statistical
analysis. All quantitative results are presented as mean ± standard
deviation.
3.Results
3.1. Design and Characteristics of the SEP-Coated PCL Flat Patch
Inspired by the collagen-based ESM, to improve the low bioactivity and
poor mechanical properties of PCL, it was coated with SEP as a protein
signal. Toward this end, we first designed PCL-based patches with a flat
topography to promote BR using capillary force lithography technology
and dip coating. Figure 1 a shows a schematic of the SEP-coated
PCL flat patch and optical images of a fabricated patch (see the
Experimental Section for the detailed design process).
Scanning electron microscopy (SEM) images of the fabricated flat patch
surface showed the spotless, clean topography of the flat structure.
SEP-coated flat topography surfaces were identical to the uncoated flat
topography surfaces (Figure 1 b). Atomic force microscopy (AFM)
observations were made to further examine the detailed morphologies the
SEP-coated flat topography, demonstrating a higher-order structure than
the uncoated flat topography patch. Although the height of the surface
was increased by the SEP coating, the surface was irregular because of
dip coating (Figure 1 c). The functional groups between SEP and
the PCL flat topography were investigated by Fourier transform-infrared
(FT-IR) spectroscopy. The absorption bands in the spectrum of PCL with a
flat topography showed CH2 asymmetric stretching at 2945
cm−1, symmetric stretching at 2866
cm−1, C=O stretching vibration at 1721
cm−1, and stretching of C-O at 1160
cm−1. The absorption bands in the spectrum of SEP
typically showed O-H stretching at 3338 cm−1 and C=O
stretching (amine II) at 1638 cm−1. The SEP-coated PCL
flat patch exhibited the characteristics of both the PCL flat topography
and SEP adsorption bands (Figure 1 d). The contact angles of the
uncoated PCL flat patches (hereafter referred to as “flat”) and
SEP-coated PCL flat patches (hereafter referred to as “e-flat”) were
73.20° and 34.37°, respectively (Figure 1 e), confirming the
change in surface properties when PCL flat patches with hydrophobic
properties were coated with SEP.
A platform for effective BR must have good mechanical properties to
withstand the pressure of the soft tissue and to ensure sufficient space
for new tissue (Elgali et al., 2017). Therefore, the tensile strength of
the patch was measured using a tensile tester to evaluate the ability to
withstand the pressure of the soft tissue following SEP coating while
maintaining sufficient tissue space. The e-flat patch (14.04 MPa) showed
greater mechanical stresses than the flat patch (~10.61
MPa (Figure 1 f). To analyze the effect of SEP on the tissue
adhesion performance, we measured the normal and shear adhesion forces
of the PCL patches on a porcine rind tissue surface under a preload of
~0.5/cm2. As shown in Figure
1 g, the e-flat topography displayed higher normal (1.16
N/cm2) and shear (0.046 N/cm2)
adhesion forces compared to those of the flat topography (normal: 0.76
N/cm2, shear: 0.042 N/cm2).
3.2. In Vitro Effects of the SEP-Coated PCL Flat Patch on
Osteoblasts
SEP is known to affect living cell bioactivity (Bae et al., 2015; F. Yi
et al., 2004). Therefore, the effects of the PCL flat patches on
osteoblasts were evaluated to confirm the influence of SEP on cell
function (e.g., cell shape and focal adhesion) at the single-cell level
by immunostaining. As shown in Figure 2a, SEP greatly influenced the
osteoblasts as evidenced by the extensive cytoskeletal structure on the
substrate. The single cells on a flat topography showed a random shape
and orientation. The cells on the e-flat topography showed a wider
morphology than those on the flat topography. The cell elongation factor
(CEF; long axis/short axis) was measured to quantify the observed cell
polarity. Surprisingly, the CEF of cells on the e-flat topography
patches was reduced compared to that on the flat topography patches. We
also analyzed the nuclei of the cells based on calculation of the
nuclear elongation factor (NEF; long axis/short axis), since SEP has
been reported to affect the structure and function of the nucleus in the
substrate (J. Kim, H. N. Kim, K. T. Lim, Y. Kim, H. Seonwoo, et al.,
2013). There were substantially more nuclei in cells on the e-flat
topography than in cells on the flat topography. Therefore, the NEF of
the e-flat topography was lower than that of the flat topography. We
also calculated the cell shape index (CSI; cell area/cell
perimeter2) and nucleus shape index (NSI; nucleus
area/nucleus perimeter2) as alternative morphological
indices (J. Kim, H. N. Kim, K. T. Lim, Y. Kim, H. Seonwoo, et al.,
2013). The cells on the e-flat topography showed a higher CSI value than
those on the flat topography, whereas the NSI of cells was lower on the
e-flat topography (Figure 2b). The elongation factor and spreading area
showed a positive correlation (Figure 2c), indicating that the body and
nucleus of cells can interact closely to regulate their behavior.
Staining of focal adhesion markers was performed to confirm cell
adhesion. With SEP coating, the cells were attached to the flat
substrate over a wider range (Figure 2d). Accordingly, it was confirmed
that the focal adhesion clustering size and number were higher in the
e-flat structure by approximately 1.6 and 3.7 times, respectively. After
6 h, more cells adhered to the e-flat topography patch than to the flat
topography patch. After 3 days of cell culture, cell proliferation was
slightly higher than that observed at 6 h of cell culture, and quite
high proliferation was observed after 5 days. There was no significant
difference between the two groups according to the SEP coating, but good
proliferation was observed (Figure 2e).
The ESM is composed of both organic (80–85%) and inorganic (15–20%)
constituents, including OPN, collagen, fibronectin, and
CaCO3, which could promote BR. OPN is a human bone
component, collagen type I has high osteocompatibility, and fibronectin
is related to the adhesion and differentiation of cells.
CaCO3 facilitates bone formation (M. K. Sah & Rath,
2016). Therefore, we conducted alkaline phosphatase (ALP; an early BR
marker) and alizarin red S (ARS; a late BR marker) to confirm BR. For
ALP activation, osteoblasts were cultured for 7 days in an osteogenic
induction medium, and the ALP enzyme of differentiated cells was stained
in each patch. Higher ALP activity was observed on the e-flat topography
than on the flat topography (Figure 2 f). For mineralization
assessment, osteoblasts were cultured for 14 days in an osteogenic
induction medium. ARS staining revealed higher calcium levels on the
e-flat topography than on the flat topography (Figure 2 g). Our
results demonstrated that SEP coating could successfully regulate
cellular behavior with potential to repair tissue in vivo or to
be used as a regenerative synthetic ECM.
3.3. Design and Characteristics of the SEP-Coated PCL Nanopatch
The results summarized above demonstrated that SEP improves the
mechanical properties and bioactivity of PCL flat patches. We next
attempted to mimic the nanostructure of the ECM to further improve the
function (e.g., morphology and differentiation) of cells on a structural
orientation. Similar to the design of the flat patch topography, using
capillary force lithography technology and dip-coating, we designed a
PCL-based nanotopography patch to promote BR regeneration.Figure 3 a shows a schematic of the fabrication method of
flexible PCL nanostructure (hereafter “Nano”) and SEP-coated flexible
PCL nanostructure (hereafter “e-Nano”) patches inspired by the bone
ECM. The SEM images of the fabricated nanopatch surfaces showed a
spotless, clean topography of the nanostructures with 800-nm grooves.
SEP-coated nanotopography surfaces were similar to the uncoated
nanotopography surfaces (Figure 3 b). We performed AFM
observations to further examine the detailed morphologies the SEP-coated
nanotopography, which showed a higher-order structure than the uncoated
nanotopography (Figure 3 c). The functional groups between the
SEP and PCL (uncoated) nanotopography were investigated by FT-IR
spectroscopy. The absorption bands in the spectrum of the PCL
nanotopography showed CH2 asymmetric stretching at 2944
cm−1, symmetric stretching at 2866
cm−1, C=O stretching vibration at 1721
cm−1, and stretching of C-O at 1161
cm−1. The absorption bands in the spectrum of the SEP
nanotopography typically showed O-H stretching at 3338
cm−1 and C=O stretching (amine II) at 1638
cm−1. The E-Nano patch showed both the PCL
nanotopography and SEP adsorption band characteristics (Figure
3 d). The contact angles of the Nano patches were also measured to
determine the change in surface properties when coated with SEP. Nano
and E-Nano patches showed contact angles of 81.72° and 35.01°,
respectively. (Figure 3 e).
The tensile strength of the nanopatches was measured when loaded along
the aligned nanotopography direction. Interestingly, when the load was
applied toward the orientation of the aligned topography, the
nanotopography showed greater mechanical stresses than the flat
topography and increased by approximately 3 MPa with SEP coating (i.e.,
Nano: ~14.69 MPa and E-Nano: ~16.81 MPa)
(Figure 3 f). To analyze the effect SEP and the nanotopography
on tissue adhesion, we measured the normal and shear adhesion forces of
the PCL nanopatches on a porcine rind tissue surface under a preload of
~0.5/cm2. As shown in Figure
3 g, the e-Nano patch displayed higher normal (1.32
N/cm2) and shear (0.080 N/cm2)
adhesion forces compared with the Nano patches (normal: 1.00
N/cm2, shear: 0.056 N/cm2), likely
due to the increase in the adhesion force imparted by the conjugation of
PCL patches and SEP.
3.4. In Vitro Effects of the SEP-Coated PCL Nanopatch on
Osteoblasts
A nanostructure is well known to affect cellular morphology and
function, and SEP coating is known to affect cell function and behavior
(J. Kim et al., 2017; J. Kim, H. N. Kim, K. T. Lim, Y. Kim, H. Seonwoo,
et al., 2013; Mahesh Kumar Sah & Pramanik, 2014; F. Yi et al., 2004).
Therefore, analysis of osteoblasts on the PCL nanopatches was performed
to confirm the effects of SEP and nanotopographical cues on cell
function (e.g., cell shape, focal adhesion, and orientation) at the
single-cell level by immunostaining. As shown in Figure 4 a,
nanotopographical cues and SEP greatly influenced the cells as evidenced
by the aligned cytoskeletal structure on the substrate. The single cells
on the SEP coating and nanotopography showed a highly aligned shape and
orientation along a unidirectionally oriented topography substrate. In
addition, the cells adhered closely along the direction of the
substrate. The CEF of the cells of the SEP-coated nanotopography was
approximately double that of cells on the uncoated nanotopography, and
the NEF was also higher in cells on the SEP-coated nanotopography than
for those on the uncoated nanotopography. By contrast, the CSI and NSI
were lower in cells on the SEP-coated nanotopography than for those on
the uncoated nanotopography (Figure 4 b). The elongation factor
and spreading area showed a strong positive correlation (Figure
4 c), indicating that the body and nucleus of cells on the SEP coating
and nanotopographical cues can interact closely to regulate their
behavior. The cells adhered well to the SEP-coated nanostructure after 6
h. After 3 and 5 days, the cells proliferated well (Figure 4 d).
Both ALP (early) and ARS (late) staining demonstrated improved bone
differentiation in the E-Nano patch (Figure 4 e andSupporting 3b ). We confirmed osteogenesis-related protein
expression via western blotting to demonstrate BR from the
nanotopographical cues and SEP. The protein expression results showed
upregulation of OPN on the E-Nano patch relative to that on the Nano
patch. Therefore, our results demonstrated that not only the SEP coating
but also the nanostructure could successfully regulate cellular behavior
and potentially repair tissue in vivo or to be used as a
regenerative synthetic ECM.
3.5. Effect of SEP Coating and Nanotopographical Cues In Vivo
All mice used in the in vivo studies survived to the sacrifice
date, and no adverse reaction was observed. SEP-coated and uncoated flat
topography patches (5 mm diameter) were placed on the left calvarial
bone defect, and SEP-coated and uncoated nanotopography patches were
placed on the right calvarial bone defect. No infection or inflammatory
reaction was observed in any of the mice throughout the postoperative
period. The patches remained for 3 weeks without deformation. For
quantitative assessment of the nanotopography and SEP effects on bone
formation, we performed micro-computed tomography (CT) and
three-dimensional (3D)-image conversion using MIMICS 14.0 software on
new bone defects in vivo . As shown in the 3D images
(Figure 5 a), bone formation in the PCL and SEP-coated
topography patches occurred along the periphery of the bone defect and
grew along the patches. At 3 weeks, the SEP-coated PCL topography
patches group showed more bone formation than the uncoated PCL
topography patches group at the defect. The bone volume was 0.42
mm3 in the flat topography, 0.60 mm3in the E-flat topography, and 0.75 mm3 in the E-Nano
topography groups. The bone surface was 7.8 mm2 in the
flat topography, 9.39 mm2 in the E-flat topography,
and 9.77 mm2 in the E-Nano topography groups
(Figure 5 b). This suggests that SEP-coated and nanotopography
patches have potential for osteogenesis.
To confirm the BR efficacy from the SEP coating and nanotopographical
cues, hematoxylin and eosin (H&E) staining was conducted at 3 weeks
after implantation. In the uncoated flat/nanotopography patch groups,
bone formation was not observed, whereas in the SEP-coated
flat/nanotopography patch groups, bone formation was observed at the
internal space of the patch (Figure 5 a). This confirmed that
more bone formation and a dense cytoplasm occurred on SEP-coated
nanotopography structures. These results provide insight into the
importance of SEP coating and nanotopographical cues for inducing bone
tissue regeneration.
4. Discussion
Designing an effective platform that can regulate or enhance biological
function is an important challenge in the tissue regeneration field.
Various ECMs in the human body exist in the form of well-organized
nanoscale protein fibers and are naturally oriented toward their
tissue-specific functions and orientations (Bae et al., 2015; D.-H. Kim
et al., 2012; H. N. Kim et al., 2013; J. Kim et al., 2014). Thus,
nanotopography in the ordered structure of the ECM can regulate cell
morphology and function through cell surface interactions (J. Kim, H. N.
Kim, K. T. Lim, Y. Kim, H. Seonwoo, et al., 2013; Liliensiek et al.,
2010; Teixeira, Abrams, Bertics, Murphy, & Nealey, 2003). In relation
to this aspect, previous studies have shown that the fate and function
(i.e., proliferation, differentiation, and wound healing) of cells are
sensitively controlled by establishing a variety of complex and
controlled microenvironments and with appropriate stimuli (e.g.,
chemical, mechanical, protein, and topographical signals) in vivo(J. H. Chen & Simmons, 2011; Das & Zouani, 2014; H. N. Kim et al.,
2013). Regarding the fabrication of platforms with topographical cues of
the ECM in vivo , most studies have used structural stimuli such
as hierarchical structures but were faced with technical limitations on
other stimuli (J. H. Chen & Simmons, 2011; D. H. Kim et al., 2009; D.
H. Kim et al., 2010; J. Kim et al., 2017; J. Kim, H. N. Kim, K. T. Lim,
Y. Kim, S. Pandey, et al., 2013). In this study, we developed a
synthetic ECM with a SEP-coated nanotopography surface to achieve
precise control for BR.
The ESM contains organic matter such as fibronectin and collagen,
similar to the component of ECM proteins (M. K. Sah & Rath, 2016). SEP
shows a similar amino acid composition to raw ESM except for cystine and
has a slightly hydrophilic property (F. Yi et al., 2004). Accordingly,
many studies have been conducted using SEP as a platform for promoting
cell function (J. Jia et al., 2008; G. H. Kim, Min, Park, & Kim, 2008;
Mahesh Kumar Sah & Pramanik, 2014; F. Yi et al., 2004). Therefore, SEP
protein signals affect cell function and behavior. We have presented a
simple yet robust method of fabricating PCL-based nanoscale substrates
using a capillary force lithography and dip-coating technique to provide
these structural stimuli and protein signals. Capillary force
lithography technology facilitates the design and fabrication of
structural precise nano-engineered substrates. PCL was chosen for this
study because it is suitable for tissue engineering and biomedical
applications owing to the following features: (1) a biocompatible
material used to manufacture FDA-approved devices; (2) biodegradability
of approximately 2 years, making it suitable for tissues requiring
long-term regeneration; and (3) robust mechanical properties and
excellent flexibility. Therefore, we assert that the novel approach
provides better function to osteoblasts for promoting BR, resulting in
an effective platform for tissue engineering.
The functions and behaviors of cells are sensitive to topographic cues
such as ECM. Our in vitro analyses demonstrated that the highly
aligned nanotopographic cues affected the functions and behaviors of the
cells, adjusting their morphology along the direction of the
nanostructure. In addition, the SEP-coated topography regulated the
morphology of the cells. The cytoskeletal morphology of the osteoblasts
at the single-cell level was wider on the SEP-coated flat topography,
and the cytoskeleton showed a highly aligned and oriented morphology on
the SEP-coated nanotopography. Focal adhesion (FA) is as considered to
be a crucial factor contributing to cellular function on a
nanotopography substrate (Biggs, Richards, & Dalby, 2010; J. Kim, H. N.
Kim, K. T. Lim, Y. Kim, H. Seonwoo, et al., 2013). As shown inFigure 2 d, the SEP coating appeared to control the FA formation
of cells, which would be an important modulator of cellular functions.
In terms of the SEP-coated topography, flat patches showed a wider
morphology because of (1) the higher number of FA clusters and (2) the
thick cytoskeleton forming bunches. Nanopatches showed maximum polarity
due to the highly oriented cytoskeleton bunches and FA clusters. These
observations were supported by the increasing tendency of elongation of
the cell body and nucleus (Figure 2 b and 4 b). Kim et
al. (J. Kim, H. N. Kim, K. T. Lim, Y. Kim, H. Seonwoo, et al., 2013)
reported that the increased elongation factor of the cell was caused by
a reduction in shortening. In this study, the high CEF on the SEP-coated
nanotopography was due to the reduction of the short axis as in previous
studies. However, the effects of the flat topography according to the
long axis and short axis could not be identified owing to the widespread
distribution from the SEP coating. Therefore, the elongation rate itself
cannot provide sufficient information about the cell body except for the
aspect ratio. As an alternative, CSI and NSI contain “perimeter” and
“spreading area” as parameters, allowing for more reasonable
quantification of cellular and nuclear morphology. Versaevel et al.
(Versaevel, Grevesse, & Gabriele, 2012) reported a quantitative model
in which the cytoskeleton is regulated according to various structures
and the nucleus shape is regulated accordingly; with a lower SCI, the
shape becomes more bipolar with elongated cells. In this study, as the
cells spread from the elongated nanotopography to the aligned
orientation, the NSI decreased markedly, revealing the relationship
between the cell and nucleus morphology.
Although there was no significant difference in the proliferation of
osteoblasts between the uncoated PCL topographic cues and SEP-coated PCL
topographic cues, we found that cell attachment and proliferation
increased over time. Arias et al. (Arias et al., 2008) reported that
collagen type I of ESM inhibits BR. However, collagen type I has a
smaller ratio than collagen type I, and the Sah and Viana groups used
the ESM in the SEP and eggshell power forms to create a platform for BR
(Mahesh Kumar Sah & Pramanik, 2014; T. Viana, 2014). Indeed, bone
formation differentiation in this study was superior in the SEP-coated
PCL topography patches than in the uncoated PCL topography patches based
on both ALP and ARS staining. Therefore, ESM can inhibit BR, but can
serve as a biomaterial to promote BR when converted to a powder and
solution state.
Developing a platform to overcome the current complex surgery and
enormous cost of BR is still an important challenge. A nanotopographic
platform inspired by the structural features of bone tissue and the ECM
has been considered a promising strategy for designing functional bones.
Herein, we have proposed functional patches for BR using a biomimetic
strategy based on the PCL topography and SEP coating. By mimicking the
well-organized ECM of the bone tissue, our PCL matrix-based
nanotopographic patches can effectively induce BR by providing an
efficient environment for morphological alignment, attachment,
proliferation, and differentiation of functional osteoblasts. Ourin vivo study showed that SEP coated on PCL topographical patches
promoted BR. At 3 weeks, initial bone formation was increased in the
SEP-coated PCL topography groups (i.e., E-flat and E-Nano)
(Figure 5 a), demonstrating that SEP affects initial bone
formation. Although further in-depth study is needed to precisely
elucidate the underlying mechanisms, our findings demonstrate that SEP
could promote early bone formation and that a nanopatterned topography
resulted in superior bone formation to a flat topography. Moreover, the
SEP-coated PCL topography patches provided more accurate tissue adhesion
to the defected bone tissue than uncoated PCL topography patches
(Figure 1 g and 3 g). This finding suggests that
improved patch adhesion with SEP coating on bone tissue surfaces might
facilitate spontaneous BR along the nanotopography. Thus, PCL
topographical patches coated with SEP might be induced to begin initial
bone formation, ultimately promoting BR.
Several studies have demonstrated that a nanotopographical structure
promotes cell migration. For instance, Kim et al. reported that the
nanotopographical local density was able to control the wound-healing
process precisely through topographical contact guidance by variable
local size nanotopography. Based on these findings, we propose a
possible mechanism that the nanotopography and SEP cues will
synergistically promote the migration of osteoblasts. To assess the
recruitment of osteoblasts and evaluate their migratory behaviors on
SEP-coated PCL nanotopographical patches, we mimicked the in vivoprocess of bone repair in calvaria defects with an in vitromigration assay. We observed enhanced migratory behaviors of osteoblasts
on the SEP-coated PCL nanotopographical patches compared with the
nanotopographical patches. Interestingly, the cells on the E-Nano patch
showed a more elongated morphology compared with those on the nano-patch
(Figure 4 b). In addition, the SEP coating promoted the cell
migration rate. The cell migration distance (720 μm) and migration
velocity (35 μm/h) on the E-Nano patch were higher than those on the
Nano patch (615 μm and 28 μm/h, respectively). For the in vitrocell migration assay on the different surfaces, the cell-free area was
determined after cell migration for 1 day (Figure 5 b).
Similarly, on the SEP-nanotopographical patch, 80% of the area was
covered by the migrating MG63 cells, whereas only 60% of the area was
covered by cells on the nanotopographical patch. In general, wound
healing is governed by two distinct cell behaviors: migration and
proliferation. Thus, our results demonstrated a notable influence of the
nanotopography in the wound healing process: (i) the SEP cues
significantly promoted the migration of osteoblasts into the wound area;
(ii) the orientation of the nanotopographical structure significantly
affected the migration speed of the osteoblasts cells; and (iii) the
orientation of the nanotopographical patch and SEP cues provided an
efficient environment for constructing the structure of the native bone
ECM in which osteoblasts could proliferate and migrate to the wound
area.
The expression levels of ERK and FAK were examined to investigate cell
function-related signaling and focal adhesion-related signaling
pathways, respectively (Cheng et al., 2019; J. Kim, H. N. Kim, K. T.
Lim, Y. Kim, H. Seonwoo, et al., 2013). We performed western blotting to
analyze the cell-cell and cell-substrate relationships in more detail.
The extracellular-signal-related kinase (ERK) signal was higher for the
E-flat group (1.03) than for the flat group (0.43), indicating greater
cell-substrate interactions, and the focal adhesion kinase (FAK) signal
was also greater for the E-flat (0.71) group than for the flat group
(0.26), indicating greater cell-cell interactions (Figure 5 e,Supporting S3 a). Hence, we suggest that SEP cues may be able to
adjust the cell-substrate interactions. Namely, the expression of ERK
and FAK can be controlled by the SEP coating to induce cell body and
nucleus shape changes through cell-substrate interactions
(Figure 5 e). SEP and nanotopographical cues were found to
enhance bone differentiation and mechanical properties. The SEP-coated
nanotopographical patches showed improved mechanical factors, cell
spreading, and osteogenesis (Figure 5 f).
Finally, we propose another possible application of the SEP-coated PCL
matrix topography. First, a precisely defined nanotopography platform
with coated SEP might allow for the fabrication of substrates by
mimicking the aligned structure of other tissues (e.g., the skin,
muscle, or heart). Second, SEP-coated nanotopography patches can be used
in a variety of biomedical applications such as tissues that require
strong support owing to their robust mechanical properties and improved
adhesion to tissue bonding (Bakopoulou et al., 2019; Chamieh et al.,
2016; J. Kim et al., 2014). Therefore, our SEP-coated nanotopographic
patches might interact to enhance the behavior and function of the
cells.
Acknowledgements
This work was supported by National Research Foundation (NRF) grants
funded by the Korea Government (2016M3A9B4919374, 2019R1I1A3A0106345 and
NRF-2019M3A9H1103737). This work was also supported by a grant
(714002-7) from the Agricultural Robotics and Automation Research Center
through the Agriculture, Food and Rural Affairs Research Center Support
Program, Ministry of Agriculture, Food and Rural Affairs.
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Figure regends
Figure 1 . Fabrication and characteristic of SEP-coated PCL flat
patch. (a) Schematic of the fabrication method for the SEP-coated PCL
flat patch, including lithography and dip-coating, and optical image of
a SEP-coated flexible PCL flat patch. (b) SEM images of the uncoated
(Flat) and SEP-coated (E-flat) surfaces of the flat morphology. (c) AFM
images of the uncoated and SEP-coated surfaces of the flat morphology
(d) FT-IR analysis of the SEP, PCL flat patch, and SEP-coated PCL flat
patch. (e) Contact angle measurements of the PCL and SEP-coated PCL flat
patches. (f) Strain-stress curves of the PCL and SEP-coated PCL flat
patches. (g) Adhesion force analysis of the PCL and SEP-coated PCL flat
patch (left : normal adhesion, right: shear adhesion).
Figure 2. Effect of SEP-coated flat topography on cell
morphology, proliferation, and differentiation. (a) Immunofluorescence
image at the multi- and single-cell levels of phalloidin (red), vinculin
(green), and DAPI (blue) of osteoblasts cultured on the SEP-coated flat
topography. (b) Quantitative analysis of the cell body and nucleus (c)
Correlation of cell the body with nucleus. (d) Number and size of focal
adhesions on the SEP-coated flat topography. (e) Proliferation of cells
on the SEP-coated flat topography. (f) Alkaline phosphatase staining of
osteoblasts during osteogenesis induction on the SEP-coated flat
topography. (g) Mineralization (ARS) staining of osteoblasts during
osteogenesis on the SEP-coated flat topography.
Figure 3 . Fabrication and characteristics of the SEP-coated PCL
nanopatch. (a) Schematic for the fabrication of the SEP-coated PCL
nanopatch, including lithography and dip-coating, and optical image of a
SEP-coated flexible PCL nanopatch. (b) SEM images of uncoated (Nano) and
SEP-coated (E-nano) surfaces of the nano morphology. (c) AFM images of
uncoated and SEP-coated surfaces of the nano morphology. (d) FT-IR
analysis of the SEP, PCL nanopatch, and SEP-coated PCL nanopatch. (e)
Contact angle measurements of the PCL and SEP-coated PCL nanopatches.
(f) Tensile stress analysis of the PCL and SEP-coated PCL nanopatches.
(g) Adhesion force analysis of the PCL and SEP-coated PCL nanopatches
(left: normal adhesion, right: shear adhesion).
Figure 4 . Effect of SEP-coated nanotopography on cell
morphology, proliferation, and differentiation. (a) Immunofluorescence
images at the multi- and single-cell levels of phalloidin (red),
vinculin (green), and DAPI (blue) of osteoblasts cultured on the
SEP-coated nanotopography. (b) Quantitative analysis of the cell body
and nucleus (c) Correlation of the cell body and nucleus. (d)
Proliferation of cells on the SEP-coated nanotopography. (e) Alkaline
phosphatase staining of osteoblasts during osteogenesis induction on the
SEP-coated nanotopography. (f) Mineralization staining of osteoblasts by
osteogenesis on the SEP-coated nanotopography.
Figure 5 . Effect of SEP coating and nanotopographical cuesin vivo . (a) Representative micro-CT image, hematoxylin and eosin
(H&E) staining image, and (b) quantitative analysis of micro-CT of the
bone regeneration of SEP-coated flat and nanotopography patches after 3
weeks of repair (n = 5 per sample). (c) In vitro cell migration
on nanotopographical and SEP-coated nanotopographical patches. (d)
Quantification of cell migration distance, velocity, and covered area.
(e) Western blot analysis and quantification of the expression levels of
FAK and ERK of osteoblasts cultured on the SEP-coated flat topography
for 2 days. (f) Schematic model of SEP coating and nanotopographical cue
effects. The relative adhesion factor was obtained from the cell
spreading ratio, adhesion force, and cell differentiation factor.