Patent Abstract:
bioengineered tissue graft scaffolds and method for producing such scaffolds are provided . the scaffolds are useful to replace or repair damaged mammalian tissues and organs .

Detailed Description:
cholecyst and small intestine tissue was obtained from market weight pigs , slaughtered at duffy &# 39 ; s meats abattoir , gort . co . galway . porcine specimens were fixed immediately post mortem by total immersion in 10 % neutral buffered formalin ( nbf ) for light microscopy and 3 % glutaraldehyde fixative for electron microscopy . whole cholecysts were punctured and drained of bile before immersion in fixatives , while small intestinal samples were cut into approximately 10 cm long sections before immersion in fixative . samples were subsequently transported to a suitable laboratory environment for further tissue processing . before fixation had fully occurred ( 2 hours ), samples were further processed to allow for total fixation and for the isolation of extra cellular matrix . this process resulted in the procurement of whole tissue and delaminated extra cellular matrix , for light and electron microscopy . before delamination occurred whole samples were take for analysis , and thickness measurement were taken via an ap - 6500 micrometer screw gauge . cholecyst and small intestine were removed from the pig gut . cholecysts were excised from the liver leaving the cystic duct intact . liver tissue was still connected to the cholecyst following excision and the cholecyst wall was distended with bile ( see fig1 ). cholecysts measured approximately 10 cm from fundus to neck . 10 cm segments of small intestine was isolated from the pig jejunum and excised from the adjoining omentum ( fig2 ). it was subsequently opened with a longitudinal incision to reveal the inner mucosal surface ( see fig2 ). liver tissue was trimmed away from the cholecyst and the cystic duct removed to allow the bile to drain through the neck from the cholecyst lumen ( fig3 ). the fundus and neck regions were subsequently removed ( fig4 ) and the tissue opened via a longitudinal incision to reveal the mucosal surface ( fig4 ) the mucosa and lamina propria , the luminal surface layers were removed as a single entity using a pair of forceps . cholecyst , although derived from the embryonic foregut tube , lacks muscularis mucosae or submucosa . below the mucosa and lamina propria is the muscularis layer . this layer was removed by mechanical delamination , using the blunt handle of a scalpel ; scraping the tissue in one direction . similar delaminarion procedure for scraping was also applied to remove the mucosa and lamina propria of the intestinal . the serosal and adipose tissue layers on the outer side of cem and sis were removed from the cholecyst and small intestine . these were removed as a single layer using a forceps . for the removal of these layers from the small intestine it was necessary to first immerse the tissue in 10 % neutral buffered formalin for i minute to prevent repeated tearing during delamination . samples obtained from the cholecyst and intestine submucosa ( fig5 ) were cut into pieces approximately 1 . 5 cm 2 , these were fixed overnight in 10 % nbf for light microscopy and overnight in 3 % glutaraldehyde fixative for electron microscopy . exactly the same procedure fixing was carried out for the laminated cholecyst and small intestine samples . following 24 - 48 hour fixation in 10 % nbf all samples intended for light microscopy were placed in distilled water and prepared for paraffin embedding , however , samples to be stained with toluidine blue were processed according to the procedures used for transmission electron microscopy . two methods of paraffin wax embedding were investigated : 1 . samples were dehydrated and infiltrated with paraffin via an automated processing microwave — micromed t / t mega microwave processing lab station 2 . samples were dehydrated in graded alcohols and infiltrated with paraffin by hand . samples were placed in polymer cassettes measuring approx . 3 cm × 2 cm . these were housed in a cylinder provided with the processing oven and immersed in a dehydrating fluid supplied with the machine — j . f . c . solution in a 2 . 5 litre bottle ( available from hacker instruments ). samples were processed in this solution for approx 40 minutes at 72 ° c . samples were then removed from the fluid and immersed in molten paraffin wax for a further 30 minutes at 72 ° c . samples were rinsed 3 × phosphate buffered saline ( pbs ), then passed through a series of graded alcohols : pbs is not essential , as distilled water or even tap water may also be used . samples were then placed in cassettes and immersed in xylene 3 × 7 minutes and then immersed in molten paraffin wax for 45 minutes . microwave processed and hand processed samples were then placed in individual steel moulds and subsequently set in paraffin wax blocks overnight at 4 ° c . paraffin embedded sections were cut on a hm 200 ergostar microtome and placed on glass slides in a 37 ° c . incubator overnight . simple staining was performed to elucidate the structure of both laminated and delaminated cholecyst and small intestine . this procedure involved the use of : fluorescent staining was also employed for the unambiguous labelling of cell nuclei . slides were passed through xylene 2 × 7 minutes then through a series of graded alcohols for rehydration : slides were next immersed in mayer &# 39 ; s haematoxylin for 5 minutes , running tap water for 2 minutes then dipped once very quickly in acid alcohol before being returned to running water for 1 minute . slides were then immersed in eosin for 1 min , tap water for 30 seconds and then blotted dry . slides were then immersed in xylene for 2 minutes and a drop of dpx mounting media applied to the slide before cover slipping . slides were passed through xylene 2 × 7 minutes then through a series of graded alcohols for rehydration : slides were next immersed in celestine blue for 7 minutes , and then in running tap water for 2 minutes . slides were next immersed in mayer &# 39 ; s haematoxylin for 5 minutes , running tap water for 2 minutes then dipped once very quickly in acid alcohol before being returned to running water for 1 minute . slides are then immersed in van gieson &# 39 ; s stain for 1 . 5 minutes , tap water for 30 seconds and then blotted dry . slides were then immersed in xylene for 2 minutes and a drop of dpx mounting media applied to the slide before cover slipping . samples to be stained with toluidine blue were embedded in a polymer resin and mounted on glass slides after sections i m were cut on an ultramicrotome ( see tissue processing for transmission electron microscopy ). the toluidine blue stain consisted of a 1 % toluidine blue powder in a 1 % sodium tetra borate solution . slides were placed on a hotplate and a drop of the stain solution added to the specimen for 30 seconds . the stain was rinsed off in tap water for a further 30 seconds . slides were passed through xylene 2 × 7 minutes then through a series of graded alcohols for rehydration : the slides were gently blotted dry of excess water before adding 50 μl of a 1 : 300 dapi solution to the slides for 5 minutes at room temperature . the slides were subsequently rinsed in pbs / tween for 3 × 5 minutes . the slides were mounted with a drop of fluoromount and cover slipped . both laminated and delaminated cholecyst and small intestine samples were prepared for electron microscopy . fixation was via a 3 % glutaraldehyde fixative for at 48 hours . samples were prepared for both scanning and transmission electron microscopy . samples were removed from fixative and subjected to dehydration by immersion in graded alcohols , as given by the following dehydration procedure : pbs 5 minutes ; 10 % ethanol 5 minutes ; 25 % ethanol 5 minutes ; 50 % ethanol 5 minutes ; 70 % ethanol 5 minutes ; 90 % ethanol 5 minutes ; 100 % ethanol 5 minutes ; 100 % acetone 5 minutes . samples were placed in a desiccator overnight to allow complete dehydration . following dehydration samples were mounted on studs via carbon adhesive plaques and gold coated in an emitech k - 550x sputter coater for 2 minutes . samples were removed from fixative and cut into 2 mm × 2 mm pieces before being rinsed in pbs 3 × 5 minutes . samples were then immersed in a 1 % osmium tetroxide ( oso 4 ) pbs solution for 2 hours . samples were subsequently dehydrated in graded alcohols : samples were place in place in 10 ml glass vials to which was added propylene oxide ( c 3 h 6 o ) for 20 minutes , this was removed and then a 50 : 50 mixture of propylene oxide and embedding resin was added . sample remained in this solution for 8 hours on a luckham multimix major roller . resin for embedding was taab spurr , which was prepared immediately before use according to supplied instruction . samples were placed in this resin for 24 hours in 10 ml glass vials on the roller . samples were then placed in taab c094 embedding capsules and incubated for 48 hours at 60 ° c . blocks were then trimmed and cut on a reichert — jung ultracut microtome . sections for toluidine blue staining were cut to 1 μm in thickness , these sections were used as scout sections for the identification of a suitable area to procure sections for transmission electron microscopy . sections were placed on agar 200 copper grids and stained with heavy metals for viewing . grids were placed in a rubber slide holder and immersed in 0 . 5 % uranyl acetate ( uo 2 ( ch 3 coo ) 2 2h 2 o ), ( ch 3 coo ) 2 . 2h 2 o ) for 40 minutes . following immersion in uranyl acetate the grids were rinsed in ultrapure h 2 o then placed in a 50 % methanol solution for 1 minute followed by a further rinse in ultrapure h 2 o . grids were then immersed reynolds in lead citrate solution for 5 minutes . the grids were placed still in their rubber holder , within a petri dish containing naoh pellets to remove carbon dioxide . the grids were finally immersed in ultrapure h 2 o for 1 minute . ( a ) light microscopy olympus bx51 fluorescent microscope . ( b ) scanning electron microscopy hitachi s - 4700 scanning electron microscope . ( c ) transmission electron microscopy hitachi h - 7600 transmission electron microscope cell numbers present in tissue were investigated using image analysis software . digital images obtained from paraffin embedded sections were accordingly stained and analysed . areas of 0 . 1 mm 2 were identified and cells within counted . area grids overlapped into that of the previous area . 10 counts were taken per slide section . eighteen individual slides were analysed , nine being sections cut from the isolated small intestine submucosa and nine from the isolated cholecyst extra cellular matrix . mtgase ( activa ® wm , ajinomoto co . inc . ), which had been purified by cation - exchange chromatography can be used at various concentrations for cross - linking the isolated tissue . the specific activity of mtgase was determined to be 27000 nmol putrescine incorporated / mg / hour . the mtgase was supplied in 20 mg ( dry weight ) samples , which were subsequently dissolved in 20 ml of deionised h 2 o and stored at − 20 ° c . various concentrations of mtgase ( 0 . 01 - 0 . 03 %) can be used cross - link tissue at 45 ° c . the tissue is then cooled to room temperature ( 22 ° c .). two independent studies were carried out in order to appraise the behaviour of 3t3 fibroblasts when in contact with mtgase , with emphasis on its capacity to support cell adhesion and cell growth . firstly , to facilitate the investigation of any adverse effect on cell viability and cell proliferation in the presence of mtgase , 3t3 fibroblasts were cultured in 6 - well tissue culture plates containing 3ml of dulbecco &# 39 ; s modified eagle medium ( dmem ) supplemented with 10 % fetal bovine serum ( fbs ) and 1 % penicillin / streptomycin ( pen / strep ), in addition to 0 . 05 %, 0 . 005 % and 0 . 0005 % mtgase ( control wells were comprised of medium and cells only ). cells were seeded at a density of 1 × 10 5 cells / well and cultures were maintained at 37 ° c . in a 5 % co 2 humidified incubator for up to 72 hours . experiments utilised triplicate samples per concentration variant , and cell viability and cell proliferation were examined using trypan blue staining and alamarblue ™ assays , respectively , after 24 and 72 hours incubation . a second study was carried out in order to evaluate the cytocompatibility of 4 % w / v gelatin gels cross - linked with 0 . 01 - 0 . 03 % mtgase , after 24 , 48 and 72 hours incubation . tissue culture grade polystyrene was used as a control substrate . thin gels ( cross - linked and untreated ) were cast in 6 - well tissue culture plates under sterile conditions . all sterile equipment , including magnetic stirrers and containers were utilized and production was carried out in laminar flow cabinets . both the protein and the enzyme were passed through sterile filters to ensure sterility . the gels were stabilised at room temperature for 5 hours followed by rinsing with 1 % pen / strep solution and hank &# 39 ; s balanced salt solution ( hbss , sigma chemicals ). 3t3 fibroblasts were seeded on each substrate at a cell density of 1 × 10 5 cells / well and grown in dmem medium supplemented with 10 % fbs and 1 % pen / strep . three samples were employed with each concentration variant , and cell viability and cell proliferation were examined using trypan blue exclusion methods and alamarblue ™ assays , respectively , after 24 , 48 and 72 hours incubation at 37 ° c . in a 5 % co 2 humidified incubator . in further embodiments of the invention , such as those exemplified in fig2 - 28 , cem was isolated from the cholecysts of 12 - 18 month old market weight pigs within 2 hours of animal slaughter . the cem isolation technique involved draining the bile from the cholecyst , removing the fundus and neck regions and cutting the remaining cylindrical piece of tissue to create a rectangular section of cholecyst . the mucosal layer was removed in long wiping motions with a blunt edge , the tissue was turned over and the serosal side was pealed off with a forceps , leaving the extra cellular matrixl layer . isolated cem was rinsed in phosphate buffered solution ( pbs ) ( sigma - aldrich , dublin , ireland . all reagents were purchases from sigma - aldrich ireland , unless otherwise stated ). orientation of the excised tissue was recorded during the isolation procedure and isolated samples of cem were cut into asymmetrical sections , which facilitated later identification of the mucosal and serosal sides of the material and the orientation of each sample . cem from five cholecysts was fixed in 2 % glutaraldehyde / pbs for 24 hours at room temperature and pressure . two samples , measuring approximately 10 mm * 10 mm , were isolated from the central region of each cholecyst and prepared for sem analysis through dehydration in graded alcohols ( 30 %- 100 %) followed by two 15 minute exchanges in absolute alcohol and chemical drying in hexamethyldisilazane ( hmds ). one serosal - side - up and one mucosal - side - up sample from each organ was mounted on carbon stubs and a 4 nm thick coating of gold was applied with the ion beam sputter coater ( emitech k550 , emitech ltd ., kent , england ). the low voltage , high resolution sem ( s - 4700 hitachi scientific instruments , berkshire england ) was used to capture photomicrographs of both the mucosal and serosal sides at 15 kv and at magnifications ranging from 1 , 000 × to 15 , 000 ×. three stereo pairs captured from random locations on each side of each sample at 15 , 000 × and at angles of 0 ° and 5 ° were used to create virtual three dimensional images of the surface topography . elevation height , a three - dimensional feature , was quantified by viewing the stereo pairs under a stereoscope and using the formula : where z is feature height , a is half of the angle of the stereo pair and p is the parallax , the latter of which was measured with a stereo viewer . one of the images from each pair was then used to measure pore and fiber diameters on the surface with image analysis software ( image pro ®, media cybernetics , berkshire , england ). due to the non - uniform non - circular shape of pores on the material surface pore diameter measurements were taken at the widest part of the pore and always in the vertical direction . in all cases 10 features were measured per photomicrograph or stereo pair and the location of particular features measured were chosen by superimposing a numbered grid on the photomicrograph and using statistical tables of random numbers to select locations from which to take measurements . asymmetrical samples of cem ( n = 5 ), fixed similarly to those for sem analysis , were viewed under circularly polarised light with the metripol birefringence imaging module ® ( oxford cryosystems ltd ., oxford , england ), which was attached to a light microscope ( prior ). the polarisation module , consisting of a series of specialised filters , an analyser and a rotating polariser , was used to produce a ray of polarised light which split into two mutually perpendicular vibrating rays as it passed through the birefringent cem specimen . retardance of one ray relative to that of the other was then measured by the microscope . for each area of cem examined 50 views were captured by a ccd camera at 3 . 6 ° intervals and merged to create a composite image of the area ; this process was facilitated by the rotating polariser . composite images captured by the microscope consisted of three images : an orientation image depicting collagen orientation , a birefringence image , demonstrating levels of birefringence of the area under investigation and an intensity image representing light intensity . data in these images was stored as pixels whereby , pixel colours corresponded to a given legend and represented collagen fiber angle for the particular pixel . to calculate the preferred collagen fiber orientation the number of pixels of a particular colour in the orientation images was quantified using image analysis software ( image pro ®) and the percentage area of the sample under the microscope with fibers oriented at a particular angle was calculated . all samples were examined at 40 × and 100 ×, but for image analysis and statistical analysis purposes five composite images of each sample were captured at random locations at 100 × and the orientation images were analysed . in all cases filter 5 which operates at a wavelength of 600 nm was used to polarise the light and all images were taken on the slow axis of the indicatrix . heart valves , whose collagen fiber orientation has previously been characterised , were used as a control ( 18 ). equi - biaxial mechanical tests were preformed on sections of cem to identify the stiffness of the material along the axes parallel and perpendicular to the preferred collagen fiber orientation , as elucidated by polarised light microscopy . a biaxial fixture was designed in conjunction with zwick gmbh & amp ; co . kg ( ulm , germany ) and consisted of 4 100n load cells , attached to a clamping mechanism via poly - paraphenylene terephthalamide ( kevlar ®, dupont engineering fibers , geneva , switzerland ) pulley cables . the clamping mechanism was a combination of four fishing hooks on each side of the sample , connected by kevlar ® and attached to the pulley cables via a small stainless steel tab . all samples tested were clamped prior to loading onto the biaxial fixture in an effort to reduce mounting strains . the biaxial fixture was attached to the z5000 zwick universal testing machine ( zwick gmbh & amp ; co . kg ). samples of isolated cem ( n = 8 ), approximately 2 cm * 2 cm , were biaxially loaded parallel to and perpendicular to the directions of preferred collagen fiber orientation . a preload of 0 . 01n was applied to all load cells prior to commencing each test and all samples were fully loaded and unloaded twice to precondition . cem samples were loaded three times at a strain rate of 1 . 27 mm / min to 1 . 2n . all tests were carried out in the water bath at 37 ° c . cem thickness was 0 . 35 mm . the results have been divided into sections , gross morphology , light microscopy , electron microscopy , cell numbers , in vitro studies . the gross morphology section addresses the gross structural characteristics of the cholecyst and small intestine submucosa following delamination and comparisons between these two scaffolds are made . the section on light microscopy deals with these two materials on a microscopic level , while the electron microscopy section investigates the ultrastructural properties of these tissues . measurements were obtained using an ap - 6500 micrometer screw gauge . relative thickness of the tissues was obtained before and after delamination of the extra cellular matrix . delaminated tissue represents the extra cellular matrix of that tissue . measurements were obtained from tissue obtained from 9 separate animals prefixation . the unprocessed cholecyst only measured an average of 0 . 4 mm , in contrast to the far thicker unprocessed small intestine , which measured an average of 4 . 9 mm . however the isolated cholecyst extra cellular matrix ( 0 . 126 mm ) transpired to be thicker than that of the isolated small intestine submucosa ( 0 . 0718 mm ). the small intestine isolated submucosa also exhibited a relatively large standard deviation in comparison with the isolated cholecyst extracellular matrix images were acquired of cholecyst and small intestine tissue before and after delamination , allowing for the comparison of gross characteristics of the tissues . the cholecyst was seen to be a relatively thin - walled organ that was easily transformed into a flattened sheet by removal of the fundus and neck region and a single longitudinal incision ( see fig7 ). the mucosa was seen to be a smooth undulating surface that was covered by a thin film of mucus and bile , which was removed along with its underlying lamina propria and poart of the muscularis layer , during the peeling process . the tissue remained highly flaccid and malleable even following extended fixation . remainder of the muscularis layer was carefully removed to expose the mucosal side surface of the cholecyst extracellular matrix . the resulting sheets were approximately 10 cm in length and 5 cm in width . the underlying serosal side layers were removed with a pair of round tipped forceps . this mesothelial layer and the adipose tissue layers were removed as a single entity , resulting in the intact extracellular matrix of the cholecyst wall . the isolated cholecyst extracellular matrix appeared as a semitransparent membrane without any remarkable surface features ( see fig8 ). it was of uniform thickness throughout its entirety and had a glistening moist appearance . the jejunum segments were tough and relatively thick walled segments of tissue ( see fig9 ). the lumen was all but obliterated by the extensive mucosa , which was thrown into numerous longitudinal ridges similar in appearance to the rugae of the stomach , no plicae circulares were observed . this mucosa was relatively difficult to remove , requiring greater force and diligence to remove than that of the cholecyst . the mucosa was clearly visible while being removed , forming a clumped mass of cellular material once removed . undigested debris also was visible within the jejunum lumen . the intestinal tissue was stiff and tended to return to the in vivo conformation spontaneously , i . e . a tubular structure . the isolated small intestine submucosa was shown to consist of a non - uniform , almost transparent film of tissue ( see fig1 ). the numerous ridges of the mucosa were still apparent at the level of the extra cellular matrix , forming local , interconnecting ridge - like thickenings along the mucosal side of the extra cellular matrix only . this extra cellular matrix scaffold also demonstrated extensive vascular tissue throughout its length , which was readily visible to the naked eye . a direct comparison between cholecyst extra cellular matrix and small intestine submucosa ( fig6 - 10 ) shows the discrepancies in surface morphology and allows the visualisation of the relative thickness between the two tissues and the amount of vascular tissue present . light microscopy revealed the microstructure of the small intestine and cholecyst tissue before and after the delaminating process . cells and cell nuclei are easily discernable from the surrounding connective tissue . epithelial cells are also evident in the micrographs , identifiable as definitive epithelia at the extremities of the tissue mucosa . haematoxylin and eosin ( h & amp ; e ) revealed the general structure of all sections , haematoxylin staining acidic structures i . e . dna of the nucleus a blue - purple colour and eosin staining the basic cytoplasmic structures a light pink colour . van gieson &# 39 ; s stain ( g ) resulted in the identification of connective tissue , staining collagen a deep red colour . nuclei are also stained blue in these images while cytoplasm and erythrocytes are stained a pale yellow colour . toluidine blue ( t ) resulted in the monochromatic staining of sections in various shades of blue , the nuclei being stained the most intensely , and the connective tissue a lighter shade of blue . scale bars were used to confirm image measurements . fig1 a demonstrates the microstructure of the laminated cholecyst attached to the liver . the mucosal surface is clearly evident as a continuous epithelium of yellow stained cells , e while the underlying lamina propria , l . p ., and its underlying muscularis appears deep red in colour , cholecyst extracellular matxix , ecm lies in between the muscularis and the adeventetia in the region attached to the liver , l . t ., here the serosal layer is replaced by a thick connective tissue called adventitia , ad . a central venule in liver tissue is also seen , c . v . fig1 b , presents the typical microstructure of small intestinal wall with mucosal epithelial cells , lamina propria , submucosa , thick muscle and serosal layer . the different layers in the part of cholecyst wall that is not attached to the liver , can be clearly seen in the histology fig1 a & amp ; b . the cholecyst wall is lined on its luminal surface with a simple columnar epithelium . the mucosa rests on a basement membrane , which is continuous with the lamina propria . lamina propria is rich in fenestrated capillaries and small venules . external to the lamina propria is a thin muscularis layer with numerous smooth muscle bundles interlaced with collagenous fibres running in longitudinal and circumferential directions of the cholecyst wall . muscularis layer is followed by a relatively acellular ecm made of loosely braided collagen bundles . in the portion of cholecyst , which is in direct contact with the liver , this fibrous ecm connects to the liver . elsewhere , this layer is covered by a relatively thick adipose tissue innervated with large blood and lymphatic vessels . this tissue is also reported to have autonomic nerves that innervate the muscular layer ( ref ). the adipose tissue is covered by serosa , which is made of thin layers of loose connective tissue and peritoneal mesothelium . the submucosa is lacking and its muscularis layer , unlike that of intestine , is not made of purely muscular tissue . instead , it is made of varying amounts of muscle tissue arranged loosely intertwined with collagenous fibres . in other words , a separate muscularis externa is not evident . as shown in fig1 ( a ) the extensive mucosa of the jejunum and the arrangement of the intestinal villi , vi . a large longitudinal fold , l . f ., is also strikingly evident in the centre of the image . also is seen is the large discrepancy in the submucosal thickness throughout the tissue . the vascular nature of the submucosa , s . m ., is indicated by the presence of numerous arterioles , ar , and a large venule , vn . this micrograph also demonstrates the organisation of the external muscle layers , the inner circular , i . c ., and outer longitudinal , o . l ., clearly visible . ( b ) the connective tissue of an expanded region of the jejunum submucosa , s . m . large bundles of red stained collagen , c . b ., are visible within this layer , as are numerous vessels of the portal system , ar the muscularis mucosae , m . m ., is seen in the right of the micrograph , separating the mucosa , m , from the underlying submucosa fig1 shows ( a ) the jejunum submucosa can be seen to extend up into a prominent fold , into the mucosa , m , the submucosa being thicker here than the submucosa not associated with the fold . the cellularity of the small intestinal submucosa is demonstrated by the presence of numerous arterioles , ar , and cell clusters , c . c ., probably fibroblasts . the two muscular layers , the muscularis mucosae , m . m ., and the muscularis externa , m . e ., are also visible . ( b ) demonstrates the presence of glands of brunner , b . g ., within the submucosa of the duodenum . here the connective tissue content of the submucosa is reduced and the cellular content markedly increased , the ecm only present in scant bundles and a thin layer adjacent to the inner circular smooth muscle , i . c ., the outer longitudinal muscle , o . l ., and serosa , se , is also evident . as shown in fig1 the porcine submucosa , s . m ., was abundant in collagenous connective tissue , c . b ., and remarkably less cellular than other layers , the tissue contained relatively few arterioles and venules , ve , yet scattered cells are observable within the connective tissue matrix of the submucosa ( b ), though other areas contained very few cells ( a ). occasionally delamination produced imperfection , such as the submucosal damage , se . r , evident in micrograph ( b ) and the artefacts , at , observable in micrograph ( b ). the collegenous nature of the porcine cholecyst extracellular matrix is evident in fig1 ( a ) from the pink staining of the extra cellular matrix connective tissue . very few cell nuclei are observable . ( b ) the muscularis mucosae , m . m ., has been preserved on the delaminated small intestine submucosa . large bundles of collagen , c . b ., are evident , as is a paired arteriole and venule , a + v . electron microscopy revealed the fine ultrastructure of the extra cellular matrix scaffolds , fiber orientation , and density and cellularisation were observed via scanning electron microscopy ( sem ) and transmission electron microscopy ( tem ). scale bars and magnification factors are included in the ultramicrographs . the fine ultrastructure of the extra cellular matrix can be seen in fig1 ( a ) collagen bundles , c . b ., are seen to be formed of many fine threadlike collage fibrils c . f ., ( b ) a meshwork of collagen bundles forms the bulk of the tissue , yet smaller fibers not associated with larger collagen bundles form a fine mesh - like fibrous component , f . c ., of the tissue . the fibrous nature of the matrix with interwoven bundles of collagen ( c . b .) ( fig1 ). the fine filamentous non - collagenous content of the cem is also clear ( f . c . ), forming a fine weave between the collagen bundles , c . b . surface mucosal foldings , m . f ., are evident in fig1 ( a ) , on this low magnification image raising the mucosal into numerous ridges . ( b ) a large mass in the centre of this image , possibly a cellular extension , c . e ., is seen in association with many fine fibers , passing over and around the extension . the laminated structure of the small intestine is evident in fig2 ( a ) as well as the course fibrous nature of the submucosa s . m ., the external muscle layers , m . e ., serosa , se , and epithelium of the mucosa , e . c ., are all evident . a large longitudinal fold occupies the centre of this image . ( b ) the submucosal - mucosal border is evident , the submucosa recognisable by its highly fibrous nature , while the mucosa appears as a tightly packed dense array of cells . fig2 ( a ) is a low powered micrograph of collagen orientation within the small intestine submucosa . the collagen bundles , c . b ., are orientated in parallel arrays and have adopted a corrugated conformation . these bundles are seen to form branching networks of fibers , b . f ., within this connective tissue . several erythrocytes can be seen adhering to these fibers , e . ( b ). as can be seen in fig2 ( a ) a fibroblast is present in the centre of the image . the cell has an elongated appearance , yet cellular extensions are not visible . large amounts of nuclear euchromatin indicate cells to be active , however the machinery of synthesis such as golgi apparatus and rough endoplasmic reticulum are not evident . surrounding the cell large amounts of collagen are evident in longitudinal , transverse and oblique orientation . ( b ) a collagen bundle in cross section , c . c ., reveals the individual collagen fibrils . collagen can also been seen in longitudinal section , c . l ., dark areas of elastin deposits are also present , e . d . in fig2 ( a ) extension from an active fibroblast , f . e ., are prominent on the left side of this image , being easily recognisable by their high content of rough endoplasmic reticulum and golgi apparatus . the cell nucleus is barely visible at the extreme left of the image . the extensions pass around a large bundle of collagen in cross section , c . c ., and seem to abut on a nearby cell probably another fibroblast , f . b ., ( b ) a section of the muscularis mucosae is seen to remain following delamination of the cholecyst . the outer longitudinal , o . l ., and inner circular , i . c ., muscle are indicated . the nuclei of a extra cellular matrix , s . m ., fibroblast is also evident at the extreme top right of the image . cell numbers were larger almost by a factor of two in the isolated small intestine submucosa . here cell numbers averaged 44 . 2 per cm 2 cell numbers in the cholecyst extracellular matrix averaged at 22 . 35 cells per cm 2 large discrepancies in cell numbers were observed between different regions of a sample , as well as between different sections . both tissues exhibited a relatively large standard deviation in mean cell numbers . in vitro studies of mtgase monitored the activity of 3t3 fibroblasts cultured in various concentrations of mtgase after periods ranging between 24 and 72 hours . table 1 summarises the effect of mtgase on the number of viable cells at 24 and 72 hours using the trypan blue exclusion method . after 24 hours , there was a significant decrease ( p & lt ; 0 . 05 ) in the number of viable cells in all concentrations of mtgase when compared to the control ( medium and cells ). at 72 hours , there was a significant decrease in viable cell number ( p & lt ; 0 . 05 ) observed between the highest concentration ( 0 . 05 %) of mtgase and the control , indicating cytotoxicity . table 2 demonstrates the effect of exposure to similar concentrations of mtgase on the cell proliferation after 24 and 72 hours . results after 24 hours showed a significant decrease ( p & lt ; 0 . 05 ) in the activity of cells in the presence of 0 . 05 % and 0 . 005 % mtgase , with 0 . 05 % mtgase showing the lowest level of cell proliferation . after 72 hours , a significant decrease ( p & lt ; 0 . 05 ) was noted in cell proliferation levels , where exposed to 0 . 05 % mtgase . no significant difference ( p & lt ; 0 . 05 ) was detected between low levels of mtgase ( 0 . 005 % and 0 . 0005 %) and the control . tables 3 and 4 quantify the results obtained from the trypan blue exclusion and the alamarblue ™ assays , respectively , where cells were seeded on gelatin film substrates cross - linked with various concentrations of mtgase . table 3 shows the number of viable cells on each substrate after 24 , 48 and 72 hours . there was a significant decrease p & lt ; 0 . 05 ) in cell viability on mtgase cross - linked gelatin films after 24 hours compared to the control . a similar trend was seen after 48 hours cultivation , but at 72 hours , only cell growth on 0 . 03 % mtgase - cross - linked gelatin was significantly different ( p & lt ; 0 . 05 ) from the control . table 4 displays no significant difference in cell proliferation levels for each substrate up to a period of 48 hours . after 72 hours however , proliferation levels of cells seeded on 0 . 02 % mtgase - cross - linked gelatin were significantly lower ( p & lt ; 0 . 05 ) than the control . in vitro studies examined independently the cell behaviour when exposed to mtgase and mtgase - cross - linked gelatin . in order to develop a wide ranging toxicity profile of the enzyme , 3t3 fibroblasts were cultured in 6 - well tissue culture plates containing 0 . 05 %, 0 . 005 % and 0 . 0005 % mtgase . cell viability and cell proliferation of 3t3 fibroblasts were quantitatively measured by the trypan blue exclusion and ( calorimetric method ) alamarblue ™ assays . after 72 hours cultivation in medium with added mtgase , it was evident from both assays that mtgase at a concentration of 0 . 05 % displayed toxic effects ( table 2 and 3 ). lower concentrations of mtgase did not elicit such toxic responses as no statistically significant difference ( p & lt ; 0 . 05 ) was noted between the test wells and the control wells ( medium and cells ). subsequently , all other tests , including mechanical , were carried out using mtgase concentrations ranging from 0 . 01 % to 0 . 03 %. concentrations less than 0 . 01 % were deemed to have no effect on the mechanical properties ( results not included ). the cytocompatibility of gelatin cross - linked with mtgase was examined by similar methods mentioned above , trypan blue exclusion and alamarblue ™ assay . although significant differences ( p & lt ; 0 . 05 ) were detected in cell viability and cell proliferation between the control substrate ( tissue culture grade polystyrene ) and gelatin films cross - linked with mtgase , the overall trend discerned in the results of these tests indicate no evidence of toxicity , since cells reached confluency after 72 hours . cem was isolated by a mechanical procedure , cleaned with ethanol and stored in strepto - penicillin . the isolation involved careful peeling of mucosal and serosal layers , and scrapping off the remaining muscularis layer . the isolated cem was treated with 70 % ethanol for 2 - 4 hrs , for cleaning . then it was washed thoroughly with distilled water for 24 - 48 h and preserved in 1 % penicillin - streptomycin solution at 4 ° c . decellularisation : extraction with sds ( 32 ) and trypsin digestion ( 33 ) are known for decellularisation of pulmonary heart valves and for producing a novel scaffold from aorta ( 34 ). procedure : treat the extracted tissue with 1 % sodium dodecyl sulphate ( in 10 mm tris buffer ) for 1 - 4 days . rinse with tris buffer , ph 8 and treat with trypsin - edta ( 0 . 05 % trypsin in 10 mm tris buffer and 0 . 1 % edta , ph 8 , overnight ( 18 h ) at 37 ° c . glutaraldehyde treatment — scaffolds can be immersed in 100 ml of a 0 . 01m hepes buffered ( ph 7 . 4 ) solution containing 0 . 2 wt % glutaraldehyde ( ga ) ( from a 25 % solution , merck ). the reaction is allowed to proceed for 24 h at 20 ° c ., after which the scaffolds can be stored in a 0 . 01m hepes buffered solution containing 0 . 2 wt % ga . carbodiimide treatment : if cross linking is desired , use 20 mm edc ( 1 - ethy - 3 - 3 - dimethylaminoprpyl carbodiimide - hcl ) and 10 mm n - hydroxysuccinimide in hepes buffer , ph 6 . 5 and the duration of treatment is 72 h at room temperature . rinse with 100 mm na2hpo4 to quench and neutralize residual edc ( vanwachem et al 2001 ). ether based : scaffolds can be immersed in 100 ml of a 2 - morpholinoethane sulfonic acid ( mes buffer , ph 4 . 5 )] buffered solution containing 4 g of 1 , 4 - butanediol diglycidyl ether ( 4 wt %). crosslinking was allowed to proceed for 144 h at 20 ° c ., after which the scaffolds are washed 5 times 30 min with normal saline . the scaffolds can then be stored in 0 . 01m hepes containing 20 % isopropyl alcohol . the experiment was conducted in a tissue culture laboratory . two types of cells were used : hela cells ( epithelial cells ) and 3t3 cells ( mouse fibroblast like cells ). these cells were seeded in 6 - well culture plates with routine media ( dmem with streptopencillin ). the density of seeding , composition of the culture medium and culture conditions were selected in accordance with routine conditions followed in our research laboratories ( ncbes ). the scaffold was incubated with the tissue culture system for 4 - 5 days . the experiment was set up in triplicates . therefore , at least 15 wells were prepared for each cell type and an equal number of control wells were also set . the control was simply cells seeded on to the culture plates . everyday , cell - viability ( by trypan blue dye exclusion test ) was determined in 3 test - wells and 3 control - wells . there was no difference in cell - viability between test and control groups . the test essentially demonstrated the viability of cells when grown along with the scaffold thereby indicating its no - cytotoxic nature . scaffolds used for the above cell - viability test were used . after incubation for 4 - 5 days , the scaffold was fixed in 10 % neutral buffered formaldehyde , paraffin blocks were made and routine histology slides were made . the histology slides were examined for light microscopic morphology . cells were found sticking on the scaffold thereby indicating that cells can grow on the scaffold . both epithelial cells and 3t3 cells survived on the scaffold surface after 4 days of incubation . high resolution photomicrographs were captured allowing accurate measurements of the mucosal and serosal surfaces of the cem ( fig2 ). mean fiber diameter was 74 ± 4 nm and 80 ± 5 nm on the mucosal and serosal sides respectively and measurements ranged from 29 nm to 155 nm and 37 nm to 219 nm respectively . mean pore diameter was 216 ± 24 nm and 264 ± 48 nm on the mucosal and serosal sides respectively and measurements ranged from 13 nm to 617 nm and 26 nm to 846 nm respectively . for these two feature types no statistical difference was found between sizes on the serosal and mucosal sides ( p & lt ; 0 . 05 ) ( table 5 ). using stereo pair photomicrographs , a stereoscope and the formula outlined above mean elevation heights calculated on the mucosal and serosal sides of cem were 316 ± 46 nm and 295 ± 38 nm respectively . measurements taken ranged from 67 nm to 1003 nm and 902 nm to 67 nm on the mucosal and serosal sides respectively and no statistical difference was found between features on the two sides ( p & lt ; 0 . 05 ) ( table 5 ). polarised light microscopy and image analysis techniques were used to generate and analyse photomicrographs thereby elucidating the orientation of collagen fibers in cem and the preferred collagen fiber orientation . cem is a thin translucent material thus allowing high quality polarised light microscopy results . due to the semi - quantitative nature of the technique results were output in terms of percentage area covered with fibers in particular angle ranges . angle ranges were taken in 10 ° increments and were all measured relative to the fundus - to - neck axis of the cholecyst . 13 % of the area of cem is covered with collagen fibers oriented between 50 ° and 60 ° while only 1 . 8 % of the area is covered with fibers oriented between 160 ° and 170 ° ( fig2 ). the preferred collagen fiber orientation was defined as the most frequently occurring orientation of collagen fibers ; statistical analysis identified this orientation as 55 °. cem biaxial tests biaxial tests were preformed along the 55 ° axis , i . e . parallel to the elucidated preferred collagen fiber ordination and along the 145 ° axis , perpendicular to collagen fiber orientation . using microsoft excel ® ( microsoft inc ., washington , usa ) and minitab ™ ( minitab inc . coventry , uk ) data generated from the biaxial tests was analysed and a stress - strain curve was created calculating average curves for each sample tested ( fig2 ). mechanical response of the material was consistent with the fiber architecture ; stiffness was higher in the direction of preferred fiber orientation than in the perpendicular direction . the stress - strain curve , in both cases , represented the classic non - linear biological response ; low stresses were experienced in the toe region of the curve and beyond a strain of ˜ 10 % stiffness of the material increased . young &# 39 ; s modulus of cem along both axes was measured in the high stiffness region of the stress - strain curves and found to be 1 kpa and 10 kpa in the parallel and perpendicular to the preferred collagen fiber orientation curves respectively . the cem samples used in this aspect of the study were isolated from the central region of the cholecyst as it is envisaged that it is from this area that templates for tissue engineering scaffolds could most suitably be created . the techniques used to examine cem architecture necessitated the fixation of the tissue with glutaraldehyde and , in the case of sem , the chemical drying of the tissue in hmds . effects of glutaraldehyde fixation have been examined using an x - ray microscope to compare the diameter of fixed and unfixed cells ; fixation reduced the measurement by only 15 %. in another study sem preparation by ethanol dehydration and hmds drying was proven to be the most optimal method of maintaining original morphology . biologic length scale topographic features have been shown to strongly modulate a variety of fundamental cell behavior in diverse cell types therefore the incorporation of biologic length scale features is a critical parameter in choosing a material for tissue engineering of scaffolds . recent studies on the response of epithelial cells to a ridge and groove type substratum with pitches ranging from 400 nm - 4000 nm indicated that at a pitch of 400 nm cells were aligned and elongated with the ridges , while at a pitch of 4000 nm effects of topography were lost . also , when cells were exposed to flow , those on the 400 nm pitch surfaces were more tightly adhered than those on the 4000 nm pitch surfaces . in a similar study , further highlighting the importance of topography , and in particular nano - scale topography , the influence of surface elevations ranging from 95 - 13 nm on the growth of endothelial cells was investigated ; the largest cellular response was seen on the 13 nm features . these studies indicate that nanoscale topographical features exert a significant influence on cellular behavior and therefore are a critical factor in the design of scaffolds for tissue engineering applications . our findings demonstrate that cem topography resembles the topographies of previously studied basement membrane layers , which facilitate the growth of cells in vivo ; average feature sizes are in the nano - scale range and high standard deviations indicate roughness of both the cem and basement membrane surfaces . it is therefore concluded that the topography of cem is conducive to optimal cellular growth and is similar to previously characterised extracellular topographies in vivo . previous studies on cem have demonstrated that it has a low cellular and muscle content and high collagen content . collagen is an important load bearing structural protein and its structural configuration is therefore intrinsically related to cem mechanical properties . polarised light microscopy is a non - destructive technique , which does not necessitate the staining or labelling of tissue samples and has previously been used to identify collagen fiber structural configuration in other biological tissues including bone , cartilage and skin . the system used in this study incorporated circularly polarised light , which eliminated the dependency of brightness on sample orientation , and a rotating polariser which facilitated the capture of 50 views of the same area at different angles thereby allowing the complete visualisation of the crimped collagen fibers . using a fixed polariser , only sections of the crimped collagen fiber which were not aligned with the transmission axis of either polarising filter would be visible under polarised light . although a significant proportion of the area of cem is covered with fibers oriented between 50 ° and 60 °, studies on small intestinal submucosa ( sis ),, identified more distinct preferred collagen fiber orientation angle . collagen fibers in sis are oriented parallel to the long axis of the intestine with only occasional fiber populations oriented at approximately ± 28 °. studies on bovine pericardium , an extensively studied biomaterial have revealed a lesser degree of collagen fiber orientation and substantial inter and intra specimen variability . the more extensive distribution of collagen fiber orientations in cem and bovine pericardium may be a reflection of the sac - like structure of these organs compared to the tubular structure of the small intestine ; however , our findings indicate that , unlike bovine pericardium , cem does not exhibit similar inter - and intra - sample variability . the consistent , wider range of collagen fiber orientations increases the suitability of cem as a biomaterial for multi - axial loading applications . biaxial , as opposed to uniaxial testing was carried out as it bears more resemblance to potential loading conditions in vivo . all mechanical testing parameters such as preconditioning techniques , maximum loads applied and strain rate were chosen due to their physiological relevance . the gauge length , i . e . the point at which a material transitions from compression to tension , is the point at which strain should ideally be measured from ; however due to the folded , wrinkled nature of cem in the unloaded state and the difficulty associated with balancing the load cells a preload of 10 mn was placed on each load cell prior to commencing the test . the gauge length was measured from the preload . various clamping mechanisms were considered , however a series of small hooks were chosen as the optimum mechanism as they reduced stress concentrations and permitted stretching of the sample in both directions along the edges . the stress - strain curve for cem is typical of that for any soft tissue . the uncrimping of the collagen fibers which are embedded in a compliant extracellular matrix is represented by the low stress toe region of the curve . at a strain of ˜ 10 % the response transitions from low stress to high stress and the material becomes considerably stiffer possibly due to a combination of fully extended collagen fibers and collagen fiber re - alignment as occurs in other soft tissues . cem displays a more elastic response than that of sis . at a biaxial stress of 250 kpa cem exhibits strains of 23 . 4 % and 30 . 5 % parallel to and perpendicular to the preferred collagen orientations respectively , while at the same level of stress sis strains by only 8 % along each axis . this difference in strain responses may be attributed to a more distinct collagen fiber orientation in sis compared to that of cem , different sample mounting techniques and considerable differences in thickness between the two materials ; fresh sis has a thickness of 1 mm compared to 0 . 35 mm for sis . the wide distribution of collagen fiber orientation angles in cem is also reflected by the differences in the mechanical responses of the axes parallel to and perpendicular to the preferred fiber orientation . previous studies have shown that heart valves have a particularly distinct collagen fiber orientation and exhibit a high degree of anisotropy ( 18 , 30 ); at 60n / m of tension there is a difference of 65 % strain between the responses of the circumferential and radial axes of a heart valve cusp . at the same level of tension cem exhibits only an 8 % difference . further , more detailed mechanical testing of cem , possible involving strain field analysis or investigating the possibility of layering the material may reveal more conservative levels of strain and a sharper transition from the low stress region to the high stress region . however , biaxial mechanical test findings in this study have confirmed that stiffness is higher in the preferred collagen fiber direction , i . e . 55 ° to the fundus - to - neck axis , than in that of the perpendicular direction and that the degree of anisotropy is reflected in the differences in strains between the parallel and perpendicular stress - strain curves . cem is an anisotropic biomaterial with similar topographic features to surfaces which have previously been demonstrated to support the growth of cells . findings of this study also indicate that cem has a preferred orientation of 55 °, which is an important factor when isolating tissue engineering scaffold templates . additionally , biaxial tests have confirmed the findings of the collagen orientation study and highlighted the intrinsic relationship between collagen fiber orientation and mechanical properties . architectural characteristics of a material play a signficant role in determining potential applications for the material and are critical parameters for tissue engineering scaffold design . these results demonstrate the suitability of using cem as a tissue engineering scaffold material . the cem was isolated by mechanically peeling off the mucosal and serosal layers of the cholecyst . the isolated cem or crosslinked cem ( treated with 0 . 625 % glutaraldehyde ( ga )) was either freeze - dried ( cemfd , gaxcemfd ) or vacuum - dried ( cemvd , gaxcemvd ). in vitro collagenase degradation studies were performed on 3 mg of samples in 1 ml of tris - hcl buffer ( ph 7 . 4 ) containing 30 u / ml of bacterial collagenase , 0 . 005m cacl , and 0 . 05 mg / ml sodium azide at 37 ° c . the degradations were stopped at 2 , 4 , 24 , 48 and 72 hours . cemvd and cemfd samples showed a maximum percent weight loss of 72 . 19 ± 2 . 08 and 79 . 53 ± 2 . 42 respectively , while gaxcemvd and gaxcemfd showed just 2 . 96 ± 0 . 69 and 3 . 94 ± 1 . 44 . these results indicate that crosslinking cem with ga drastically reduced its collagenase degradability ( p & lt ; 0 . 005 ). the method of drying did not show significant effect on the rate of collagenase degradation of the cem and gaxcem samples , except for cem at 2 h ( p & lt ; 0 . 05 ). collagen is the major structural component (& gt ; 70 %) of the cholecyst - derived extracellular matrix . the present invention reveals that its susceptibility to collagenase degradation can be reduced by crosslinking with glutaraldehyde . evaluation of in vitro swelling and degradation behaviour of cholecyst derived extracellular matrix ( cem ) and in vivo tissue response elicited by cem in subcutaneous rat implant model methods : cem was isolated by carefully peeling / scraping off the mucosal and serosal layers of the cholecyst . the samples were vacuum / freeze dried . some were crosslinked with 0 . 625 % glutaraldehyde ( ga ). swelling and degradation studies were carried out in distilled water and phosphate buffer ( ph7 . 4 ). 1 × 1 cm 2 cem , ga crosslinked cem and porcine heart valves were immobilized on subcutaneous tissue with non degradable prolene suture . rats were sacrificed at 21 and 63 days to study the tissue response to cem based implants . results : freeze dried samples showed higher degree of water uptake than vacuum dried samples . ga crosslinking drastically reduced the amount of water uptake ( fig3 ). fickian diffusion was observed with all the samples ( n = 0 . 23 ± 0 . 07 ). loss of weight was observed within 24 hours in case of vacuum / freeze dried cem samples . the subcutaneously implanted samples showed integration with the extracellular matrix and native cem samples were completely absorbed by host tissue by 63 days . the number of inflammatory cells infiltrating the implant sited was higher in ga crosslinked samples , with minimal foreign body giant cell response ( fig3 a & amp ; b ). crosslinking is essential to prevent lose of bioactive components from the ecm . native cem samples showed better tissue compatibility . cem has good potential for tissue engineering and other implant applications . the burst strength and distension of preserved tissue was measured and the primary material axis was found . cem scaffolds were isolated from fresh tissue by mechanically separating the acellular layer from the inner mucosa and outer serosa . a ball burst test jig was fabricated to comply with astm ( 43 ) standards . samples were either tested immediately , or after preservation for one week ( n = 5 in all cases ). bursting force , distension to burst and thickness were recorded . results were compared by anova ( p & lt ; 0 . 05 ). in one example , five cem scaffolds mounted on a uniform elastic ring embedded with hooks every 15 °. these preparations were tested according the method of choi et al . ( 44 ) with an precision of ± 7 . 5 °. the average thickness of the cem was 0 . 15 ± 0 . 06 mm . compared to fresh tissue , no preservation method significantly changed the mechanical strength over one week . a 5 % solution of penicillin and streptomycin , did however , stiffen the matrix ( fig2 ). a principle material axis was oriented 60 °± 22 . 5 ° from the long axis . the matrix did not show a large bias in any direction and this may have increased deviation . comparing burst test results from the single - layer cem to dual - layer small intestinal submucosa ( sis ) and urinary bladder submucosa ( ubs ) ( 44 ), showed no significant differences in the burst strength . these data show that single - layer cem scaffolds exhibit high extensibility and similar strength to dual - layer scaffolds . in the following example , the burst strength and stiffness of fresh tissue samples were measured using a ball burst test jig . four cholecyst derived extracellular matrices ( cem ) were isolated from fresh tissue by mechanically separating the mostly acellular layer from the inner mucosa and outer muscularis . each layer was slowly peeled from the one below using forceps to limit the amount of mechanical damage to the collagen scaffold through extraction . specimens were placed into a phosphate buffered saline ( pbs ) solution to prevent dehydration between the time of isolation and testing , no more than 3 hours . the burst jig was fabricated to comply with the astm d3787 - 01 , using a 44 . 45 mm inner diameter ring to clamp the specimen and a 25 . 4 mm diameter ball to apply the load perpendicular to the tissue orientation with an instron ( instron corp . canton , mass .) load frame . the plunger moved at a constant speed of 5 mm / s for the duration of the test . bursting force , distension to burst , thickness , and stiffness were recorded . the average thickness of the acellular cem was 0 . 15 mm ± 0 . 06 mm , approximately half of the unprocessed thickness of 0 . 4 mm ± 0 . 04 mm . both discarded layers this multiaxial test allows a more realistic representation of tissue performance , shown below , in a pressurised space such as the thoracic or abdominal cavities than does uniaxial testing . other acellular matrices , studied by several institutions have been subjected to ball burst testing and the results are comparable to those obtained with the cem . 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