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| United States Patent Application |
20110059292
|
| Kind Code
|
A1
|
|
Wicker; Ryan
; et al.
|
March 10, 2011
|
HYDROGEL CONSTRUCTS USING STEREOLITHOGRAPHY
Abstract
A preferred embodiment of the present invention provides a method and
system for building cost-efficient biocompatible hydrogel constructs
using stereolithography. Hydrogel constructs may be used in, for example,
multi-lumen nerve regeneration conduits and other tissue engineering
scaffolds with embedded channel architecture that facilitate tissue
regeneration through possible incorporation of precisely located
bioactive agents, cells, and other desired inert and/or active chemical
agents and devices. Another preferred embodiment of the present invention
provides a method of fabricating a hydrogel construct comprising:
solidifying a first solution into a first construct layer with a first
energy dosage using stereolithography, the first solution comprising: a
first polymer; and a first photoinitiator, wherein the first polymer and
first photoinitiator are of a first concentration.
| Inventors: |
Wicker; Ryan; (El Paso, TX)
; Medina; Francisco; (El Paso, TX)
; Arcaute; Karina; (El Paso, TX)
; Ochoa; Luis; (El Paso, TX)
; Elkins; Christopher; (Redwood City, CA)
; Mann; Brenda; (Salt Lake City, UT)
|
| Family ID:
|
37186025
|
| Appl. No.:
|
12/862546
|
| Filed:
|
August 24, 2010 |
Related U.S. Patent Documents
| | | | |
|---|
|
| Application Number | Filing Date | Patent Number |
|---|
| | 10907984 | Apr 22, 2005 | 7780897 |
| | 12862546 | | |
|
|
| Current U.S. Class: |
428/137 ; 264/401 |
| Current CPC Class: |
B29C 67/0055 20130101; B29C 67/0062 20130101; B29L 2031/7532 20130101; C12M 25/14 20130101; B33Y 30/00 20141201; B33Y 70/00 20141201; B33Y 10/00 20141201; B33Y 80/00 20141201; Y10T 428/24322 20150115 |
| Class at Publication: |
428/137 ; 264/401 |
| International Class: |
B32B 3/10 20060101 B32B003/10; B29C 35/08 20060101 B29C035/08 |
Claims
1-27. (canceled)
28. A method of fabricating a hydrogel construct comprising: solidifying
one or more solutions into three or more hydrogel construct layers such
that: (i) the plurality of hydrogel construct layers are coupled together
to form the construct; and (ii) at least one lumen or channel extends
through at least two of the three or more hydrogel construct layers;
where each of the one or more solutions comprise a hydrogel polymer and a
photoiniator.
29. The method of claim 28, where the three or more hydrogel construct
layers are solidified such that two or more lumens or channels extend
through at least two of the three or more hydrogel construct layers.
30. The method of claim 29, where at least two of the two or more lumens
or channels connect within the construct.
31. The method of claim 28, where at least one of the three or more
layers is solidified from two or more different solutions.
32. The method of claim 28, where at least one of the hydrogel polymer(s)
is a derivative of poly(ethylene glycol).
33. The method of claim 30, where at least one of the photoinitiator(s)
is selected from the group consisting of UV photoinitiators and
visible-light photoinitiators.
34. The method of claim 28, where at least one of the photoinitiator(s)
is selected from the group consisting of: 2-hydroxy-2-methyl-1
phenyl-1-propanone,
2-hydroxy-1-[4-(2-hydroxehtoxy)phenyl]-2-methyl-1-propanone,
2,2-dimethoxy-2-phenyl-acetophenone, and any combination thereof.
35. The method of claim 28, where at least one of the one or more
solutions includes one or more materials selected from the group
consisting of: biocompatible media, water, a buffer, phosphate-buffered
saline, cell culture media, and any combination thereof.
36. The method of claim 28, where the construct is cytocompatible.
37. The method of claim 30, where at least one of the hydrogel construct
layers has a thickness that is different from the thickness of at least
one other of the three or more hydrogel construct layers.
38. The method of claim 30, where at least one of the three or more
hydrogel construct layers is a partial layer.
39. The method of claim 28, further comprising cleaning the hydrogel
construct.
40. The method of claim 28, further comprising curing/drying the hydrogel
construct.
41. The method of claim 28, where at least one of the one or more
solutions includes an additive selected from the group consisting of
imbedded devices and imbedded materials, bioactive ingredients and cells,
and any combination thereof.
42. The method of claim 28, where the one or more solutions are
solidified using stereolithography.
43. A hydrogel construct comprising: three or more hydrogel construct
layers coupled together to form the construct; and where at least one
lumen or channel extends through at least two of the three or more
hydrogel construct layers.
44. The construct of claim 43, where two or more lumens extend through at
least two of the three or more hydrogel construct layers.
45. The construct of claim 44, where at least two of the two or more
lumens or channels connect within the construct.
46. The construct of claim 45, where at least one of the three or more
layers comprises two or more materials.
47. The construct of claim 28, where at least one of the three or more
layers comprises a derivative of poly(ethylene glycol).
Description
BACKGROUND
[0001] The present invention relates to the general field of rapid
prototyping technology, and in particular, to stereolithography methods
and systems.
[0002] Rapid prototyping (RP) technologies, also known as Solid Freeform
Fabrication (SFF), layered manufacturing and other similar technologies
enable the manufacture of complex three-dimensional (3D) parts. RP
technologies, in particular, generally construct parts by building one
layer at a time. RP technologies are commonly used to build parts and
prototypes for use in, for example, the toy, automotive, aircraft and
medical industries. Oftentimes prototypes made by RP technologies aid in
research and development and provide a low cost alternative to
traditional prototyping. In a few cases, RP technologies have been used
in medical applications such as those associated with reconstructive
surgery and tissue engineering (TE).
[0003] Stereolithography (SL) is one of the most widely used RP
technologies known in the art. The resolution of SL machines and the
ability of SL to manufacture highly complex 3D objects, make SL ideal for
building both functional and non-functional prototypes. In particular, SL
techniques provide an economical, physical model of objects quickly and
prior to making more expensive finished parts. The models are readily
customizable and changes may be easily implemented.
[0004] SL generally involves a multi-stage process. For example, the first
stage involves designing and inputting a precise mathematical geometric
description of the desired structure's shape into one of many
computer-aided design (CAD) programs and saving the description in the
standard transform language (STL) file format. In the second stage, the
STL file is imported into SL machine-specific software (RP software). The
RP software slices the design into layers and determines the placement of
support structures to hold each cross-section in place while building the
structure layer by layer. By computing build parameters, the RP software
controls the part's fabrication. In the layer preparation stage, the
build parameters for the desired part are translated into machine
language. Finally, the machine language controls the SL machine to build
a desired part and its support structure layer by layer. SL machines
typically focus an ultraviolet (UV) laser onto a cross-section of a
liquid photopolymer resin. The laser, in turn, selectively cures a resin
to form a structure, such as anatomical shapes (i.e., organs and
tissues), layer by layer. Ultimately, the part is cleaned, the support
structure is removed and the part is post-cured (typically exposed to UV)
prior to completion. The operator may, however, need to sand, file or use
some other finishing technique on the part in order to provide a specific
surface finish to the structure, which may include painting, plating
and/or coating the structure's surface.
[0005] SL technologies known in the art generally include, for example, a
laser, a liquid level sensing system, laser beam optics and controllable
scanning mirror system, a vertically movable platform, a single resin
retaining receptacle or vat and a recoating device. During the laser
scanning phase, a series of optics and controllable scanning mirrors
typically raster a UV laser beam to solidify a photocurable polymer
resin. The subject 3D part is first attached to the platform by building
a support structure with the platform in its topmost position. This step
allows for misalignment between the platform and the surface of the
liquid resin--once constructed, the base support structure is parallel
with the surface of the liquid. When building the subject part
simultaneously with its required support structure and after the laser
beam completes a layer, the platform typically is vertically traversed
downward a distance equal to the build layer thickness. After the
platform is vertically traversed downward and prior to selectively curing
the next layer, a recoating device is typically traversed horizontally
across the part leaving a uniform layer of liquid polymer. The recoating
device ensures that trapped spaces within the part are filled with liquid
resin (which may be required for future build layers) and maintains a
constant build layer thickness. The process repeats as each layer is
built. Complex-shaped parts are thus manufactured by repeating the
layering process. Once complete, the part is typically raised out of the
liquid resin, the support structure is removed from the part, the part is
cleaned and then post-cured. The operator may, however, need to sand,
file or use some other finishing technique on the part in order to
provide a specific surface finish to the structure, which may include
painting, plating and/or coating the structure's surface.
[0006] Certain RP technologies facilitate the fabrication of parts used in
medical applications. Such parts require additional design
considerations. TE techniques, in particular, rely on the use of a
scaffold, a framework that provides structural support for cells while
those cells regenerate the tissue. These scaffolds may also provide
signals to the cells to elicit particular desired behaviors. One of the
most challenging problems in TE is providing adequate nutrition to cells
seeded within implanted scaffolds. TE techniques known in the art have
shown that the diffusion of oxygen and nutrients is not sufficient to
sustain cell viability beyond distances of approximately 75 microns in
the body. Accordingly, TE techniques must retain precise control over the
resulting 3D geometry in order to design favorable diffusion into a
scaffold and thus maintain cell viability. Although SL has the resolution
and speed to make highly complex 3D structures economically, SL has not
been used to aid in TE because SL resins known in the art are not
certified for implantation in humans. Other systems known in the art for
creating complex 3D TE scaffolds are time-consuming and complicated and
therefore are not conducive to mass manufacturing. Accordingly, what is
desired is a system and method of quickly building and mass producing
biocompatible and implantable constructs with precise control over
placement of scaffold materials and bioactive agents and cells to promote
favorable tissue regeneration and nutrient diffusion within a scaffold in
an economical manner possibly with SL technologies.
[0007] Hydrogels are currently being used for a number of different TE
applications, particularly for soft tissues. Hydrogels are biocompatible
materials with high water content and are suitable as scaffolding
materials because of their similarity, both mechanically and
structurally, to extracellular matrices. In addition, hydrogels exhibit
favorable diffusion characteristics and are currently used in
photolithographic processes using manual lithographic masking techniques
as well as a variety of other processes. There are enumerable TE
applications that can benefit from precisely manufacturing hydrogel
constructs with bioactive agents and cells. Hydrogels, however, are not
currently adequately supported by layered manufacturing (LM) technologies
using SL.
[0008] Embedded channels may be important to build angiogenic structures
or roadways between proliferative structures located within hydrogel
scaffolds. Thus, biological and architectural cues need to be assessed to
fabricate cytocompatible scaffolds. For example, gradients of growth
factors have been found to direct cell migration and neurite extension,
and ultimately enhance tissue regeneration in both guided angiogenesis
and subsequent vasculogenesis in vivo and peripheral nerve regeneration.
Several agents, such as vascular endothelial growth factor (VEGF), for
example, exert potent angiogenic effects. In the case of VEGF, these
effects are several-fold, ranging from marrow stimulation of endothelial
precursor production and release to local selective recruitment of
precursors and enhanced, for example, vascular permeability which in turn
enhances vascular bud formation.
[0009] Once initiated, a vascular bud is potentially guided by gradients
that allow permeability in the target bud direction and stabilization of
the adjacent sides. Several stabilizing agents have been identified in
vitro. These agents, such as angiopoietin 2, serve to prevent aberrant
budding and to guide the bud in the direction of high permeability. When
provided nonspecifically, these agents suppress bud formation. Thus, a
gradient in VEGF will facilitate guided bud formation and propagation. A
reverse gradient of angiopoietin 2 should stabilize directional control
of angiogenesis and prevent nonspecific turns or termination. Further,
extracellular matrix (ECM) elements have been shown to either facilitate
(hyaluronic acid) or inhibit (polymerized collagen) directional
angiogenesis through specific cellular receptors. Thus, what is desired
is exogenously engineered gradients of biologic agents and/or ECM that
will potentially facilitate induction and directional propagation of
angiogenesis in an engineered implantable, cytocompatible scaffold.
[0010] One particular need in the art is a system and method to create
complex nerve guidance conduits. Currently, peripheral nerve repair is
accomplished by using a nerve autograft. Autografting involves taking a
portion of a nerve from one location in the body (a donor site) and
placing it in another part of the body exhibiting a specified need. There
are several drawbacks to autografting including, for example, requiring
multiple surgical sites and a considerable risk of neuroma formation at
the donor site. Oftentimes, results from autografting have been variable
and more often altogether unsuccessful.
[0011] Nerve guidance conduits (NGCs) offer a promising alternative to
autografting. NGCs are tubes that are sutured to nerve stumps to bridge
the gap and aid in guiding sprouting axons from the regenerating nerve
toward their target. NGCs retain neurotrophic factors and other compounds
secreted by the damaged nerve, thus aiding in regeneration and preventing
the infiltration of fibrous tissue. There are currently two types of NGCs
available, one made of collagen and the other made of polyvinylalcohol (a
hydrogel). These NGCs, however, are simple, single material and single
lumen conduits that fail to recreate the 3D structure of the nerve.
[0012] Multi-lumen conduits are desirable because they mimic the natural
peripheral nerve structure and increase surface area for neurite
attachment/extension and support cell attachment/migration. Multi-lumen
conduits thus allow for more precisely located growth factors and support
cells within a tissue scaffold. Although multi-lumen conduits made with
poly(lactic-co-glycolic acid) have previously been made, the techniques
used to make such scaffolds are difficult to scale-up to a manufacturing
level, do not allow for cells to be homogeneously seeded within the
conduit during its manufacture, and do not allow the mechanical
properties of and bioagents within the construct to vary throughout the
construct, which is afforded by layered manufacturing.
[0013] Thus, systems known in the art fail to mass produce complex,
multiple material 3D constructs with embedded channel architecture from
hydrogels using SL technology. Accordingly, what is desired is a low
cost, efficient and easy-to-use system which has the ability to fabricate
hydrogel constructs with embedded channels of virtually any orientation.
What is further desired is a system which enables scaffold fabrication
with internal channel architecture including any variable channel
orientation. What is still further desired is the ability to fabricate
multiple material hydrogel constructs that enable the construction of
precise scaffolds with variable hydrogel scaffold materials both within
and across layers.
[0014] In addition, what is still desired is the ability to fabricate
multiple material hydrogel constructs with precisely placed bioactive
agents and cells both within and across layers. What is further desired
is a simple method for manufacturing multi-lumen conduits of bioactive
hydrogels as potential scaffolds for peripheral nerve regeneration. What
is still further desired is a simple method for manufacturing complex
bioactive hydrogel constructs as potential scaffolds for guided
angiogenesis and adipose tissue generation. What is also still further
desired is a simple method for fabricating multi-material constructs that
may serve as TE scaffolds.
SUMMARY OF THE INVENTION
[0015] One aspect of the present invention overcomes the aforementioned
limitations in an effective and efficient manner, thus expanding the use
of RP in various applications and improves SL functionality. In another
aspect, the present invention will accommodate these needs and provide
further improvements in TE, chemical sensing, biological sensing and
numerous other applications requiring complex, three-dimensional,
multi-material, multi-element and/or multi-color, biocompatible
manufacturing. In still another aspect, the present invention provides a
multi-material SL system that builds angiogenic structures or roadways
between proliferative structures for use in, for example, guided
angiogenesis to restore vascular function. In yet another aspect, the
present invention provides a SL system for constructing bioactive,
multi-lumen nerve guidance conduits. In still another aspect, the present
invention provides a system for fabricating tissue scaffolds such as, for
example, tissue scaffolds for promoting adipose tissue population and
growth.
BRIEF DESCRIPTION OF THE DRAWINGS
[0016] The above and further advantages of the invention may be better
understood by referring to the following description in conjunction with
the accompanying drawings, in which:
[0017] FIG. 1 is a schematic of a typical SL machine known in the art; and
[0018] FIG. 2A depicts the chemical composition of a preferred hydrogel
used in an aspect of the present invention;
[0019] FIGS. 2B and C depict the preferred chemical compositions preferred
photoinitiators used in an aspect of the present invention;
[0020] FIG. 3 illustrates a preferred working environment for building
hydrogel construct with a typical SL machine (shown with an optional
glass slide for measuring gel thickness);
[0021] FIGS. 4A and 4B illustrate the cure depth or hydrogel thickness
curves for preferred photoinitiators and hydrogel solutions used in an
aspect of the present invention;
[0022] FIG. 4C illustrates a preferred laser vector pattern used to
determine hydrogel thicknesses in accordance with an aspect of the
present invention;
[0023] FIG. 5 illustrates the relationship between gel thickness and
energy dosage for a preferred solution used in an aspect of the present
invention;
[0024] FIG. 6 depicts a typical UV-VIS absorption spectrum for preferred
photoinitiators used in an aspect of the present invention;
[0025] FIGS. 7A-C depict exemplary 3D tissue engineered scaffolds
fabricated with I-2959 in accordance with an aspect of the present
invention;
[0026] FIG. 8A depicts the vector file from the SL machine software
depicting the path of the laser beam during the build process in
accordance with an aspect of the present invention;
[0027] FIGS. 8B and 8C depict an exemplary 3D tissue engineered scaffolds
fabricated with HMPP in accordance with an aspect of the present
invention;
[0028] FIG. 9A depicts a CAD model of a preferred nerve guidance conduit;
[0029] FIG. 9B depicts the vector file from the SL machine software
depicting the path of the laser beam during the build process in
accordance with an aspect of the present invention; and
[0030] FIG. 9C-9F depict exemplary 3D multi-lumen nerve guidance conduits
fabricated in accordance with a preferred embodiment of the present
invention.
DETAILED DESCRIPTION OF THE INVENTION
[0031] While the making and using of various embodiments of the present
invention are discussed in detail below, it should be appreciated that
the present invention provides many applicable inventive concepts that
can be embodied in a wide variety of specific contexts. The specific
embodiments discussed herein are merely illustrative of specific ways to
make and use the invention and do not delimit the scope of the invention.
[0032] A typical prior art SL machine 10, as illustrated in FIG. 1,
generally includes a UV laser beam 12, a liquid level sensing system 14,
optics 16 and controllable scanning mirror system 18, a vertically
movable platform 20 and a resin retaining receptacle or vat 22. The vat
22 houses, for example, a liquid photocurable polymer resin 24 and,
generally, the SL machine 10 rasters a UV laser beam 12 across the resin
through a series of optics 16 and a controllable scanning mirror system
18. In most designs, the subject three-dimensional (3D) part 26 is
usually first attached to the platform 20 by building a base support
structure 28 while the platform 20 is still in its topmost position. The
support structure 28 is usually made up of fine filaments that support
the subject part's 26 overhangs and are manufactured simultaneously using
the same resin 24. Prior art designs typically incorporate a recoating
device, recoating blade or other sweeping device 29 that sweeps or
horizontally translates across the surface of the liquid after the
platform 20 and subject part 26 have been traversed downward a distance
equal to the build layer thickness. Thus, the recoating device 29
facilitates uniform liquid layers on the surface of the subject part 26
and eliminates trapped gases or bubbles and/or trapped volumes left on or
underneath the platform 20 and/or the subject part 26 both before and
during the building process.
[0033] Referring still to the prior art SL machine 10 depicted in FIG. 1,
after the SL machine 10 rasters the UV laser beam 12 and completes a
given layer (which also includes waiting a sufficient time for the
reaction to finish after the laser beam has completed its scan), the
platform 20 is vertically traversed downward a distance equal to the
build layer thickness typically between but not limited to 2 and 6 mils
or optionally traversed downward a distance greater than the build layer
thickness in order to dip the subject part 26 into the resin 24 and fill
any internal part cavities. Once dipping the subject part 26 is
completed, if dipping is optionally performed, the platform 20 is then
traversed upward until the top of the subject part attached to the
platform is located a distance equal to the build layer thickness from
the surface of the resin 24. The build layer thickness usually depends on
the type of build desired. Prior to beginning a new reaction with the
laser 12, a recoating device 29 typically traverses the liquid resin 24
surface as described previously, and the SL machine 10 waits a prescribed
amount of time for the liquid resin to reach a state of equilibrium (so
that essentially all waves and any other movement of the liquid resin has
stopped) prior to starting the next layer. The process repeats as each
layer is built. The materials used within the layer may be varied in a
number of different configurations including, for example, the materials
used to manufacture the layers can be varied both within and across the
layers. Complex-shaped parts are thus manufactured by repeating the
layering process. Once complete, the subject part 26 is typically raised
out of the liquid polymer resin 24, the support structures 28 are removed
and the subject part 26 is cleaned (preferably with a typical cleaning
solution or a cytocompatible solution) and post-cured, usually in a UV
oven (not shown). However, it should be understood that support
structures 28 may be removed before, during, and/or after the cleaning
and curing/drying processes.
[0034] In order to attach newly formed layers to previously cured layers,
it is crucial to maintain a certain liquid photocurable resin 24
chemistry, layer thickness and laser energy so that the laser 12 is
capable of curing beyond the layer thickness into previously cured layers
(also known as "laser overcure"). Cure depth, a fundamental
characteristic of liquid photocurable resins 24, measures the penetration
depth of a laser at which the laser successfully cures the liquid
photocurable resin 24 for a given laser energy. As described earlier, in
a typical commercial SL machine 10 a series of optics 16 focuses and
directs the laser 12 onto the liquid surface while the scanning mirrors
18 controls the laser's movement in the X-Y plane across the vat 22.
Because commercial SL machines 10 accommodate a dynamic scanning mirror
system, photochemical reactions are controlled by varying the scan speed
of the laser 12 (for a fixed laser power). Thus, understanding and
characterizing the cure depth behavior of the liquid photocurable resins
24 is necessary for successfully fabricating 3D objects using SL and its
scanning mirror system 18 as seen, for example, in the later-described
example.
[0035] Additionally, in order to successfully fabricate embedded channels
and features that are opened or closed in and/or between cured layers,
for example, the particular characteristics of the hydrogel solution
(e.g., a photoinitiator (PI), poly(ethylene glycol) (PEG) and distilled
water solution) need to be characterized. Certain unique characteristics
must be exhibited in order to allow for successful fabrication. For
example, some hydrogel solutions exhibit characteristics, such as
hydrogel thickness or cure depth, that may potentially vary widely as a
function of PI type and concentration, energy dosage and polymer
concentration in the hydrogel solution as also demonstrated in the
later-described example.
[0036] Polymers that may be used in the present invention include any
number of polymers with photoreactive functional groups and are capable
of forming a hydrogel construct. These polymers include natural,
synthetic, and semi-synthetic polymers known to those of skill in the
art, and may be degradable or non-degradable. One exemplary polymer is
derivatized PEG having functional groups such as acrylate, methacrylate,
or vinyl sulfone. The PEG may have a molecular weight between about 1000
and 20,000, preferably between about 1000 and 10,000. The PEG may be a
straight linear chain with a functional group on either end, such as PEG
diacrylate, or may be a multi-armed PEG. Other polymers which may be used
include, for example, derivatized polyvinyl alcohol, hyaluronic acid,
chondroitin sulfate, and collagen. For example, methacrylated hyaluronic
acid and methacrylated chondroitin sulfate have both been
photocrosslinked into hydrogels. Other useful polymers capable of forming
hydrogels following photocrosslinking are well-known to those of skill in
the art. The concentration of the polymer in solution is preferably
between about 1% and 30% (w/v).
[0037] Various biocompatible fluids may be used in conjunction with
aspects of the present invention, including water, buffer (such as
phosphate-buffered saline) and cell culture media. When cells or
bioactive factors are included in the polymer solution, the fluid is
preferably at a pH of about 7.0 to 7.8, most preferably about 7.4.
[0038] Various PIs may be used in conjunction with a preferred embodiment
of the present invention and are generally known to those of skill in the
art of photocrosslinking. The PI preferably has an absorption in the UV
wavelength range, and more preferably in the long UV wavelength range.
Preferred PIs, include but are not limited to,
2,2-dimethyl-2-phenylacetophenone,
2-hydroxy-2-methyl-1-phenyl-1-propanone (HMPP), and
2-hydroxy-1-[4-(2-hydroxyethoxy)phenyl]-2-methyl-1-propanone (Irgacure
2959, Ciba-Geigy). The concentration of the PI in the polymer solution is
preferably below about 5%, and more preferably below about 1%,
particularly when cells are present in the polymer solution. It should be
understood by those skilled in the art that other PIs, such as other
UV-PIs and visible PIs, may also be used in accordance with aspects of
the present invention.
[0039] Bioactive factors, such as adhesion ligands, growth factors, and
cytokines, may be incorporated into the scaffold during the
photocrosslinking process by including them in the polymer solution.
These bioactive factors may be attached to the scaffold during the
photocrosslinking process through functional groups attached to the
factors, or may simply be trapped within the hydrogel during the process.
The bioactive factors are preferably incorporated at a concentration
effective to elicit the desired biological response.
[0040] Cells may be included in the polymer solution prior to the
photocrosslinking process, thereby being homogeneously seeded within the
scaffold following photocrosslinking of the hydrogel (or seeded into the
scaffold after construction). The cell density may be wide-ranging
depending on the particular application for which the scaffold will be
used, but will typically not be more than about 50.times.10.sup.6
cells/ml in the polymer solution.
[0041] In accordance with one aspect of the present invention, a complete
TE cytocompatible hydrogel implant or construct was fabricated by first
creating a desired nerve regeneration conduit computer-aided design (CAD)
drawing. The design is saved in a standard transform language (STL) file
format and imported in SL machine-specific software to create SL vector
files or SL machine command files. Contemporaneously, hydrogel and PI
selection occurs depending on the desired design criteria. A solution is
prepared combining the hydrogel in distilled water and PI. Optionally,
the solution may incorporate additives including, for example, bioactive
agents, live cells, other chemicals, devices for implantation or any
combination thereof. The solution may undergo several characterization
tests including, for example, tests for evaluating mechanical,
photo-chemical and cytocompatibility properties. After the initial design
and testing phases are complete, the SL process may begin. After
initialization of the SL machine, including laser power adjustment, SL
machine-specific parameter determination, the hydrogel receptacle (or
other existing receptacle), is placed at a desired height on the building
platform. After determining the receptacle and solution volume required
for a desired build layer thickness, the build process begins. Keeping in
mind that build layer thickness may be varied as the build process
continues, certain material volumes and machine parameters may need to be
altered.
[0042] For example, to begin the building phase, an initial amount of
solution is added into the receptacle, either by hand or by way of an
automated system free of human intervention (or alternatively, the
solution is contained in a fixed material vat similar to those found in
existing commercial systems). Part building begins in accordance with the
layer specific build file or machine command file using a machine adapted
to perform SL including, for example, the SL machine schematically
depicted in FIG. 3 without the optional glass slide. As each hydrogel
construct layer is complete, the platform is traversed vertically a
distance equal to the desired build layer thickness (which can be varied
throughout the build).
[0043] In accordance with a preferred embodiment of the present invention,
each hydrogel construct layer (or portion of a layer) may be fabricated
to reflect a certain characteristic. As mentioned earlier, unique
characteristics, such as hydrogel thickness or cure depth, vary widely as
a function of PI type and concentration, energy dosage and polymer
concentration in the hydrogel solution as also demonstrated in the
later-described example. Thus, by changing PI type, PI concentration,
polymer type, polymer concentration, solution type or solution
concentration or energy dosage, the hydrogel solution generally exhibits
a unique characteristic. Accordingly, in a preferred embodiment, although
the entire hydrogel construct may be made of essentially the same
material, distinct construct layers (or a portion of a layer), for
example, exhibit unique physical and biological characteristics depending
on the altered characteristics of the hydrogel solution used to fabricate
that particular construct layer (or portion of a layer). Alternatively,
it may be desired to build a layer (or a portion of a part layer) within
or across the current part layer with altogether different materials.
Keeping in mind that each layer may be built in a number of different
configurations including, for example, partial layers, layers built in
any one dimension or in multiple dimensions and cross-layers built
between layers in any dimensions, a preferred embodiment of the present
invention provides a system of fabricating virtually endless combinations
of single material and multi-material hydrogel constructs, allowing
different parts of the same hydrogel construct to exhibit a desired
characteristic.
[0044] As each part layer is completed, solution is added or removed
accordingly to or from, respectively, from the receptacle to accommodate
variable build layers (or portions of a build layer) and layer thickness
(or thickness of a portion of a layer), using a receptacle fill/remove
system (or alternatively, the platform could be traversed down into a
single vat of material). The preferred building process is repeated using
the build or machine command file until the part is complete. Finally,
after removing all of the solution, the subject part is separated from
the receptacle (or, alternatively the subject part is separated from an
existing build platform or from an optional build platform such as a
glass slide as seen in FIG. 3), the subject part is cleaned, optionally
undergoes a finishing process that may include cutting or trimming the
hydrogel construct, rinsing with a cytocompatible solution, and finally
inspected for quality control. Accordingly, a completed TE hydrogel
implant is cytocompatible and fabricated using SL. TE hydrogel implants
additionally may promote, for example, adipose tissue population and
growth (or nerve regeneration or guided angiogenesis and ultimately
vasculogenesis).
[0045] Although the below-described example primarily references PEG, it
should be understood by those skilled in the art that other hydrogels may
also be used in accordance with the present invention. For example, a
natural polymer, synthetic polymer or some combination thereof may also
be used. Natural polymer hydrogels include polymers such as anionic
polymers (for example, hyaluronic acid, alginic acid, pectin,
carrageenan, chondroitin sulfate, dextran sulfate), cationic polymers
(for example, chitosan and polylysine), amphipathic polymers (such as
collagen, gelatin, carboxymethyl chitin and fibrin) and neutral polymers
(for example, dextran, agarose and pullulan) and their derivatives.
[0046] Synthetic polymer hydrogels, on the other hand, include, for
example, polymers such as polyesters: poly(ethylene glycol)-poly(lactic
acid)-poly(ethylene glycol); poly(ethylene
glycol)-poly(lactic-co-glycolic acid)-poly(ethylene glycol);
poly(ethylene glycol)-polycaprolactone-poly(ethylene glycol); poly(lactic
acid)-poly(ethylene glycol)-poly(lactic acid); poly(hydroxyl butyrate);
poly(propylene fumerate-co-ethylene glycol).+-.acrylate end groups; and
poly(poly(ethylene glycol)/poly(butylene oxide)terephthalate).
[0047] Synthetic polymer hydrogels may include, for example, other
polymers such as: poly(ethylene glycol)-bis-(poly(lactic acid)-acrylate);
poly(ethylene glycol).+-.cyclodextrins; poly(ethylene
glycol)-g-poly(acrylamide-co-Vamine); polyacrylamide; poly(N-isopropyl
acrylamide-co-acrylic acid); poly(N-isopropyl acrylamide-co-ethyl
methacrylate); poly(vinyl acetate)/poly(vinyl alcohol); poly(N-vinyl
pyrrolidone); poly(methyl methacrylate-co-hydroxyethyl methacrylate);
polyacrylonitrile-co-allyl sulfonate);
poly(biscarboxy-phenoxy-phosphazene); and poly(glucosylethyl
methacrylate-sulfate).
[0048] Combinations of natural and synthetic polymer hydrogels may include
polymers such as poly(polyethylene glycol-co-peptides), alginate
g-(polyethylene oxide-polypropylene oxide-polyethylene oxide),
poly(polylactic-co-glycolic acid-co-serine), collagen-acrylate,
alginate-acrylate, poly(hydroxyethly methacyrlate-g-peptide),
poly(hydroxyethyl methacyrlate/Matrigel.RTM.) and hyraluronic
acid-g-N-isopropyl acrylamide).
[0049] The SL materials used in accordance with a preferred embodiment of
the present invention may be rigid, semi-rigid, liquid (may be
encapsulated liquid) or gas (trapped gases). There are numerous examples
of curable fluid media 24 suitable for use with aspects of the present
invention. Examples of curable fluid media 24 or materials that may be
incorporated into the curable fluid media 24 include SL resins known in
the art, hydrogels, bioactive ingredients, cells, imbedded devices or
materials, photopolymer resins and powdered materials. Some types of
powdered materials may be converted from a fluid-like medium to a
cohesive cross-section by processes, such as melting and solidification.
[0050] In addition, in accordance with a preferred embodiment of the
present invention, multi-colored manufacturing may be accomplished by
mixing pigments, fluorescing particles, paints, dyes and/or other color
media into the curable fluid medium 24, thereby facilitating the
manufacture of multi-colored prototypes and models. Similarly, other
materials may, optionally, be mixed into the fluid medium 24 to alter the
strength, thermal, mechanical, optical, electrical, functional and/or
biofunctional properties thereby facilitating the manufacture of
multi-functional, multi-material, multi-colored, multi-element and/or
implantable prototypes, models and finished products. The present
invention thus facilitates using SL technology to aid in manufacturing of
parts in an endless number of materials and colors. The present invention
also facilitates manipulating certain materials to exhibit altered
properties at select locations during the building stage.
Example
[0051] Poly(ethylene glycol) (PEG) is an example of a synthetic hydrogel
material which is cytocompatible and potentially has important uses in
tissue regeneration. PEG is generally non-toxic, non-immunogenic and can
be easily cleared from the body. In addition, PEG is water soluble and
can be easily modified with photoreactive and crosslinkable groups like
acrylates or methacrylates. Thus, PEG is ideal for creating
photocrosslinkable hydrogel tissue scaffolds. The systems and methods in
accordance with an aspect of the present invention make possible, for
example, successful fabrication of 3D PEG-based scaffolds using SL.
[0052] Generally, it was found that hydrogel thicknesses vary at select
energy dosages for different scan speeds of the SL machine's UV scanning
system. In fact, hydrogel thickness was found to be a strong function of
PI type and concentration, energy dosage and PEG-dimethacrylate (PEG-dma)
concentration (for a molecular weight, M.sub.w, of 1000 PEG-dma
commercially available), especially at the low PI concentrations required
for implantation. Hydrogel thickness curves demonstrate LM for two
construct geometries where different layer thicknesses were required to
successfully fabricate the constructs. Thus, an aspect of the present
invention demonstrates, for example, the effective use of SL as a
processing technique for complex cytocompatible 3D tissue scaffolds. In
addition, other aspects of the present invention address, for example,
practical considerations associated with the use of hydrogels in LM.
[0053] In accordance with an aspect of the present invention, PEG-dma
M.sub.w 1000 was used to prepare two solutions with different
concentrations (20% and 30% w/v) in distilled water. Aliquot portions
were separated from these solutions, and different concentrations of two
PIs were added to the portions. The PIs used in this instance were
Sarcure 1121 or HMPP (2-hydroxy-2-methyl-1-phenyl-1-propanone) and
Irgacure 2959 or I-2959
(2-hydroxy-1-[4-(2-hydroxehtoxy)phenyl]-2-methyl-1-propanone). The
chemical structures of the PEG-dma and the two PIs used in this example
are shown in FIGS. 2A, 2B and 2C, respectively.
[0054] In order to obtain viable hydrogel thickness curves, the movable
platform 20 of the SL machine 10 was set a fixed height and fitted with a
laser 12, specifically a He--Cd laser (325 nm) as seen in, for example,
FIG. 3. The PEG-dma solution with PI was pipetted inside a flat-top
cylindrical container 30 and filled to the rim. A glass slide 32 was
placed on top of the container 30 and in contact with the PEG-dma
solution. The glass slide 32 acts as a substrate for hydrogel attachment
and facilitates the thickness measurements. It was determined that the
glass slide 32 filters approximately 18% of the laser 12 power.
[0055] The cylindrical container 30 with the glass slide 32 was placed on
the center of the platform 20 as depicted in FIG. 3. At the test height
of the platform 20, the laser 12 was circular with a diameter of
approximately 250-micrometers. The samples were cured by writing a vector
pattern through the glass slide 32 and into the PEG-dma container 30 at
different energy doses. FIG. 4C, for example, illustrates the vector file
of the actual laser beam trace on laser burn paper. A preferred laser
vector pattern 36 used to determine hydrogel thicknesses in accordance
with an aspect of the present invention. The pattern 36, in this example,
consisted of a series of nineteen parallel lines approximately 250
micrometers wide (the laser beam diameter) and 7.62 mm long, spaced
approximately 355-micrometers apart.
[0056] The laser 12 drew each line in the pattern 36 twice and the energy
dosage was varied by changing the SL machine 10 parameters that control
the scan speed of the laser 12. After polymerization, the glass slide 32
was lifted off of the container 34 with the polymerized hydrogel attached
to the slide. The cured hydrogels were rinsed with distilled water to
remove any unreacted polymer and then measured with, for example, a
caliper. This procedure was repeated for all hydrogel thickness
measurements. Four sample hydrogels were cured for the PEG-dma solutions
with I-2959, and two sample gels were cured for the solutions with HMPP.
It should be noted that the measured power of the He--Cd laser 12 (rated
at 40 mW) at the fixed platform 20 height was 29.5 to 30.6 mW and 35.8 to
37.1 mW with and without the glass slide 32, respectively. The measured
laser 12 powers with the glass slide 32 were used to determine the laser
energies.
[0057] The resulting hydrogel thickness curves as a function of PI type
and concentration and the energy dose are shown in FIGS. 4A and 4B, where
FIG. 4A represents the gel thickness curve when I-2959 is used as a PI
and FIG. 4B represents the same for HMPP. The three markers used in FIGS.
4A and 4B correspond to three different energy dosages. The diamond shape
(.diamond-solid.) represents an energy level of 3.604 j/cm.sup.2 or 0.258
IPS. The square shape (.box-solid.) represents an energy level of 1.640
j/cm.sup.2 or 0.567 IPS. The triangle shape (.tangle-solidup.) represents
an energy level of 0.586 j/cm.sup.2 or 1.585 IPS.
[0058] FIGS. 4A and 4B also illustrate that there are significantly
greater gel thicknesses achieved with HMPP when compared with I-2959 for
a given PI concentration and energy dosage. It was further observed that
higher polymer concentrations typically produce thicker hydrogels.
Similarly, higher energy dosages generally produce thicker gels. Thus,
the hydrogel thickness curves aid in prescribing layer thicknesses for
fabricating complex 3D scaffolds. For example, the I-2959 affords
polymerization of thin layers and therefore the fabrication in a layer-by
layer fashion. On the other hand, HMPP may be used to successfully
fabricate single layer "large" structures.
[0059] FIG. 5 illustrates that there is a relationship between energy
dosage and hydrogel thickness for PEG solutions with 0.5% (w/v) I-2959.
The solid diamond markers (.diamond-solid.) correspond to 0.5% (w/v) of
I-2959, while the hollow diamond markers (.diamond.) correspond to 20%
(w/v) PEG-dma in distilled water. Again, as seen in FIG. 5, for the two
types of PIs tested, at low PI concentrations (<0.05%) and small
energy dosages (fast scanning speeds) the hydrogels produced were thick
and loosely crosslinked.
[0060] FIG. 6 illustrates the UV-VIS absorption spectrum of the two PIs
used in the gel thickness experiments and shows, for example, that the
hydrogel thickness has a maximum at low PI concentrations and decreases
asymptotically to a non-zero value as PI concentrations increase.
Hydrogel thickness generally begins at zero for zero PI concentration,
has a maximum at low PI concentrations, and decreases asymptotically to a
non-zero value as PI concentration increases. Hydrogel thickness starts
at zero due to the presence of polymerization inhibitors, including
monomethyl ether hydroquinone (MEHQ) and butylated hydroxytoluene (BHT),
added by the manufacturer in the PI. Measurement in the region between
zero and the maximum gel thickness are not present here as the gel is
loosely crosslinked at these PI concentrations and the measurements are
highly uncertain (and thus, the maximum gel thickness presented here
should not be viewed as an absolute maximum).
[0061] As mentioned earlier, I-2959 affords polymerization of thin layers
and therefore the fabrication in a layer-by layer fashion, while HMPP may
be used to successfully fabricate single layer "large" structures.
Accordingly, a preferred embodiment of the present invention provides SL
processing to fabricate cytocompatible parts such as those seen in FIGS.
7, 8 and 9. For example, FIG. 7A depicts the complex 3D structure with
embedded 3D channel architecture encoded in a vector file. The vector
file was in turn used to fabricate the scaffold depicted in FIGS. 7B and
7C using I-2959. As another example, FIG. 8A depicts the relatively
simple structure with multiple straight channels encoded in a vector
file. This vector file was used to fabricate the scaffold in one layer
using HMPP as in FIGS. 8B and 8C.
[0062] FIGS. 9A-9F depict other examples of multi-lumen and multi-layered
nerve guidance conduits which may be built in accordance with one aspect
of the present invention. FIG. 9A depicts a CAD model of a preferred
nerve guidance conduit while FIG. 9B depicts the vector file from the SL
machine software depicting the path of the laser beam during the build
process in accordance with an aspect of the present invention; and FIG.
9C-9F depict exemplary 3D multi-lumen nerve guidance conduits fabricated
in accordance with a preferred embodiment of the present invention.
[0063] It should be understood by those skilled in the art that there are
numerous other shapes, sizes and configurations of tissue scaffolds and
nerve guide conduits, for example, which may be fabricated using a
preferred embodiment of the present invention. Although preferred
embodiments of the present invention have been described in detail, it
will be understood by those skilled in the art that various modifications
can be made therein without departing from the spirit and scope of the
invention as set forth in the appended claims.
* * * * *
