@article{XuFahmyGarciaWesdorpetal.2023,
  author    = {Xu, Jietao and Fahmy-Garcia, Shorouk and Wesdorp, Marinus A. and Kops, Nicole and Forte, Lucia and De Luca, Claudio and Misciagna, Massimiliano Maraglino and Dolcini, Laura and Filardo, Giuseppe and Labbert{\´e}, Margot and Vanc{\´i}kov{\´a}, Karin and Kok, Joeri and van Rietbergen, Bert and Nickel, Joachim and Farrell, Eric and Brama, Pieter A. J. and van Osch, Gerjo J. V. M.},
  title     = {Effectiveness of BMP-2 and PDGF-BB adsorption onto a collagen/collagen-magnesium-hydroxyapatite scaffold in weight-bearing and non-weight-bearing osteochondral defect bone repair: in vitro, ex vivo and in vivo evaluation},
  series = {Journal of Functional Biomaterials},
  volume    = {14},
  journal   = {Journal of Functional Biomaterials},
  number    = {2},
  issn      = {2079-4983},
  doi       = {10.3390/jfb14020111},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-304019},
  year      = {2023},
  abstract  = {Despite promising clinical results in osteochondral defect repair, a recently developed bi-layered collagen/collagen-magnesium-hydroxyapatite scaffold has demonstrated less optimal subchondral bone repair. This study aimed to improve the bone repair potential of this scaffold by adsorbing bone morphogenetic protein 2 (BMP-2) and/or platelet-derived growth factor-BB (PDGF-BB) onto said scaffold. The in vitro release kinetics of BMP-2/PDGF-BB demonstrated that PDGF-BB was burst released from the collagen-only layer, whereas BMP-2 was largely retained in both layers. Cell ingrowth was enhanced by BMP-2/PDFG-BB in a bovine osteochondral defect ex vivo model. In an in vivo semi-orthotopic athymic mouse model, adding BMP-2 or PDGF-BB increased tissue repair after four weeks. After eight weeks, most defects were filled with bone tissue. To further investigate the promising effect of BMP-2, a caprine bilateral stifle osteochondral defect model was used where defects were created in weight-bearing femoral condyle and non-weight-bearing trochlear groove locations. After six months, the adsorption of BMP-2 resulted in significantly less bone repair compared with scaffold-only in the femoral condyle defects and a trend to more bone repair in the trochlear groove. Overall, the adsorption of BMP-2 onto a Col/Col-Mg-HAp scaffold reduced bone formation in weight-bearing osteochondral defects, but not in non-weight-bearing osteochondral defects.},
  language  = {en}
}
@phdthesis{Wenzel2010,
  author    = {Wenzel, Sonja},
  title     = {Etablierung eines dynamischen Kultursystems auf Calciumphosphat-Scaffolds unter Verwendung zweier verschiedener Zelllinien},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-48766},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2010},
  abstract  = {Der Ersatz von Knochengewebe durch die Methode des Tissue Engineerings stellt eine viel versprechende Alternative zu konventionellen Therapieformen dar. Jedoch m{\"u}ssen die bisherigen Kulturbedingungen verbessert werden, um das Differenzierungsverhalten von Zellen optimal steuern zu k{\"o}nnen. Dabei spielt nicht nur die Wahl eines geeigneten Scaffolds und der zu verwendenden Zellen, sondern auch die des Kultursystems eine entscheidende Rolle. In einem dynamischen Kultursystem zirkuliert Medium und bietet gegen{\"u}ber einem statischen Kultursystem ver{\"a}nderte Bedingungen bez{\"u}glich N{\"a}hrstoffversorgung und Stimulation durch Fl{\"u}ssigkeitsscherstress. Um die Einfl{\"u}sse der ver{\"a}nderten Bedingungen zu analysieren, wird in dieser Arbeit ein dynamisches Kultursystem etabliert. Dazu werden Calciumphosphat(CaP)-Scaffolds mit dem 3D Powder Printing System gedruckt und mit Zellen der Osteosarkomzelllinie MG63 oder der Fibroblastenzelllinie L-929 besiedelt. In 17 Versuchsreihen werden die zellbesiedelten Scaffolds bei unterschiedlichen Fließgeschwindigkeiten und {\"u}ber unterschiedliche Kultivierungszeitr{\"a}ume kontinuierlich perfundiert. Anhand der Wachstumsparameter Zellzahl und Zellviabilt{\"a}t, sowie der Morphologie und r{\"a}umlichen Verteilung der Zellen werden die Qualit{\"a}ten der Kultursysteme untersucht und mit statischen Kultursystemen verglichen. Die mit dem 3D Powder Printing System gedruckten Scaffolds erweisen sich als geeignet: Nach 6-t{\"a}giger Kultur k{\"o}nnen unter dem Rasterelektronenmikroskop auf den CaP-Scaffolds eine reichliche Zellbesiedelung mit morphologisch gesunden Zellen, die in das Porensystem hineinwachsen, beobachtet werden. Bei beiden Zelllinien nehmen in beiden Kultursystemen die Wachstumsparameter {\"u}ber einen 6-t{\"a}gigen Kultivierungszeitraum stetig zu und eine Langzeitkultur {\"u}ber 30 Tage kann in beiden Kultursystemen am Leben erhalten werden. Die kontinuierliche Perfusion in einem dynamischen Kultursystem wirkt sich auf das Zellwachstum g{\"u}nstig aus. Im Vergleich von dynamischen zu statischem Kultursystem {\"u}ber einen 6-t{\"a}gigen Kultivierungszeitraum wachsen beide Zelllinien im dynamischen Kultursystem besser. Dabei spielt die Fließgeschwindigkeit im dynamischen Kultursystem auf die verbesserte N{\"a}hrstoffversorgung und Stimulation durch Fl{\"u}ssigkeitsscherstress eine Rolle. Außerdem ist zu beachten, dass der Einfluss der Fließgeschwindigkeit des Mediums auf die einzelnen Scaffolds innerhalb des Kulturcontainers unterschiedlich ist. Dies h{\"a}ngt vom Str{\"o}mungsprofil im Container ab und macht sich durch eine erh{\"o}hte Standardabweichung der Messwerte gegen{\"u}ber der statischen Kultur bemerkbar.},
  subject      = {Zellkultur},
  language  = {de}
}
@article{WaxmanStrzalkowskaWangetal.2023,
  author    = {Waxman, Susannah and Strzalkowska, Alicja and Wang, Chao and Loewen, Ralitsa and Dang, Yalong and Loewen, Nils A.},
  title     = {Tissue-engineered anterior segment eye cultures demonstrate hallmarks of conventional organ culture},
  series = {Graefe's Archive for Clinical and Experimental Ophthalmology},
  volume    = {261},
  journal   = {Graefe's Archive for Clinical and Experimental Ophthalmology},
  number    = {5},
  doi       = {10.1007/s00417-022-05915-z},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-323845},
  pages     = {1359-1368},
  year      = {2023},
  abstract  = {Background Glaucoma is a blinding disease largely caused by dysregulation of outflow through the trabecular meshwork (TM), resulting in elevated intraocular pressure (IOP). We hypothesized that transplanting TM cells into a decellularized, tissue-engineered anterior segment eye culture could restore the outflow structure and function. Methods Porcine eyes were decellularized with freeze-thaw cycles and perfusion of surfactant. We seeded control scaffolds with CrFK cells transduced with lentiviral vectors to stably express eGFP and compared them to scaffolds seeded with primary TM cells as well as to normal, unaltered eyes. We tracked the repopulation behavior, performed IOP maintenance challenges, and analyzed the histology. Results Transplanted cells localized to the TM and progressively infiltrated the extracellular matrix, reaching a distribution comparable to normal, unaltered eyes. After a perfusion rate challenge to mimic a glaucomatous pressure elevation, transplanted and normal eyes reestablished a normal intraocular pressure (transplanted = 16.5 ± 0.9 mmHg, normal = 16.9 ± 0.9). However, eyes reseeded with eGFP-expressing CrFK cells could not regulate IOP, remaining high and unstable (27.0 ± 6.2 mmHg) instead. Conclusion Tissue-engineered anterior segment scaffolds can serve as readily available, scalable ocular perfusion cultures. This could reduce dependency on scarce donor globes in outflow research and may allow engineering perfusion cultures with specific geno- and phenotypes.},
  language  = {en}
}
@article{WagenbrennerPokerHeinzetal.2022,
  author    = {Wagenbrenner, Mike and Poker, Konrad and Heinz, Tizian and Herrmann, Marietta and Horas, Konstantin and Ebert, Regina and Mayer-Wagner, Susanne and Holzapfel, Boris M. and Rudert, Maximilian and Steinert, Andre F. and Weißenberger, Manuel},
  title     = {Mesenchymal stromal cells (MSCs) isolated from various tissues of the human arthritic knee joint possess similar multipotent differentiation potential},
  series = {Applied Sciences},
  volume    = {12},
  journal   = {Applied Sciences},
  number    = {4},
  issn      = {2076-3417},
  doi       = {10.3390/app12042239},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-262334},
  year      = {2022},
  abstract  = {(1) Background: The mesenchymal stromal cells (MSCs) of different tissue origins are applied in cell-based chondrogenic regeneration. However, there is a lack of comparability determining the most suitable cell source for the tissue engineering (TE) of cartilage. The purpose of this study was to compare the in vitro chondrogenic potential of MSC-like cells from different tissue sources (bone marrow, meniscus, anterior cruciate ligament, synovial membrane, and the infrapatellar fat pad removed during total knee arthroplasty (TKA)) and define which cell source is best suited for cartilage regeneration. (2) Methods: MSC-like cells were isolated from five donors and expanded using adherent monolayer cultures. Differentiation was induced by culture media containing specific growth factors. Transforming growth factor (TGF)-ß1 was used as the growth factor for chondrogenic differentiation. Osteogenesis and adipogenesis were induced in monolayer cultures for 27 days, while pellet cell cultures were used for chondrogenesis for 21 days. Control cultures were maintained under the same conditions. After, the differentiation period samples were analyzed, using histological and immunohistochemical staining, as well as molecularbiological analysis by RT-PCR, to assess the expression of specific marker genes. (3) Results: Plastic-adherent growth and in vitro trilineage differentiation capacity of all isolated cells were proven. Flow cytometry revealed the clear co-expression of surface markers CD44, CD73, CD90, and CD105 on all isolated cells. Adipogenesis was validated through the formation of lipid droplets, while osteogenesis was proven by the formation of calcium deposits within differentiated cell cultures. The formation of proteoglycans was observed during chondrogenesis in pellet cultures, with immunohistochemical staining revealing an increased relative gene expression of collagen type II. RT-PCR proved an elevated expression of specific marker genes after successful differentiation, with no significant differences regarding different cell source of native tissue. (4) Conclusions: Irrespective of the cell source of native tissue, all MSC-like cells showed multipotent differentiation potential in vitro. The multipotent differentiation capacity did not differ significantly, and chondrogenic differentiation was proven in all pellet cultures. Therefore, cell suitability for cell-based cartilage therapies and tissue engineering is given for various tissue origins that are routinely removed during total knee arthroplasty (TKA). This study might provide essential information for the clinical tool of cell harvesting, leading to more flexibility in cell availability.},
  language  = {en}
}
@article{WagenbrennerMayerWagnerRudertetal.2021,
  author    = {Wagenbrenner, Mike and Mayer-Wagner, Susanne and Rudert, Maximilian and Holzapfel, Boris Michael and Weissenberger, Manuel},
  title     = {Combinations of hydrogels and mesenchymal stromal cells (MSCs) for cartilage tissue engineering — a review of the literature},
  series = {Gels},
  volume    = {7},
  journal   = {Gels},
  number    = {4},
  issn      = {2310-2861},
  doi       = {10.3390/gels7040217},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-250177},
  year      = {2021},
  abstract  = {Cartilage offers limited regenerative capacity. Cell-based approaches have emerged as a promising alternative in the treatment of cartilage defects and osteoarthritis. Due to their easy accessibility, abundancy, and chondrogenic potential mesenchymal stromal cells (MSCs) offer an attractive cell source. MSCs are often combined with natural or synthetic hydrogels providing tunable biocompatibility, biodegradability, and enhanced cell functionality. In this review, we focused on the different advantages and disadvantages of various natural, synthetic, and modified hydrogels. We examined the different combinations of MSC-subpopulations and hydrogels used for cartilage engineering in preclinical and clinical studies and reviewed the effects of added growth factors or gene transfer on chondrogenesis in MSC-laden hydrogels. The aim of this review is to add to the understanding of the disadvantages and advantages of various combinations of MSC-subpopulations, growth factors, gene transfers, and hydrogels in cartilage engineering.},
  language  = {en}
}
@phdthesis{Wagenbrenner2021,
  author    = {Wagenbrenner, Mike Helmut},
  title     = {In vitro-Charakterisierung mesenchymaler Stromazellen aus dem menschlichen H{\"u}ftgelenk},
  doi       = {10.25972/OPUS-23711},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-237110},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2021},
  abstract  = {In dieser Arbeit konnte erstmals gezeigt werden, dass plastik-adh{\"a}rent wachsende, multipotente Vorl{\"a}uferzellen, die eine f{\"u}r MSCs charakteristische Kombination von Oberfl{\"a}chenantigenen tragen, aus allen vier untersuchten Geweben des arthrotischen H{\"u}ftgelenks isoliert werden konnten. MSC-{\"a}hnliche Zellen k{\"o}nnen somit nicht nur in der Spongiosa und im Gelenkknorpel, sondern auch in der anterioren Gelenkkapsel und dem Ligamentum capitis femoris (LCF) des arthrotisch ver{\"a}nderten menschlichen H{\"u}ftgelenks nachgewiesen werden. Die FACS Analyse der Oberfl{\"a}chenantigene auf Zellen, die aus den vier unterschiedlichen Geweben eines beispielhaft gew{\"a}hlten Spenders isoliert wurden, zeigte eine deutliche Expression der Antigene CD44, CD73, CD90 und CD105. Unabh{\"a}ngig vom Nativgewebe zeigten somit alle untersuchten Zellen ein f{\"u}r MSCs charakteristisches, aber nicht spezifisches Profil an Antigenen auf ihrer Oberfl{\"a}che. Eine {\"U}bereinstimmung mit den ISCT Kriterien f{\"u}r MSCs war aufgrund der fehlenden Kontrolle h{\"a}matopoetischer Marker nicht m{\"o}glich. Die multipotente Differenzierung der isolierten Zellen erfolgte mithilfe spezifischer Differenzierungsmedien in Monolayer-Kulturen oder f{\"u}r die chondrogene Differenzierung in dreidimensionalen Pellet-Kulturen. Nach 21 Tagen konnten in allen differenzierten Kulturen histologisch und immunhistochemisch klare Zeichen der Osteo- und Adipogenese detektiert werden, w{\"a}hrend die Auswertung spezifischer Markergene eine klare Steigerung der Expression dieser im Vergleich zu den Negativkontrollen zeigte. Histologische und immunhistochemische Auswertungen best{\"a}tigten auch eine erfolgreiche chondrogene Differenzierung der Zell-Pellets aus Spongiosa, Knorpel und Kapsel. Lediglich in den chondrogen differenzierten Zell-Pellets aus dem LCF konnte immunhistochemisch keine Bildung des knorpelspezifischen Matrixproteins Col II nachgewiesen werden. Mikroskopisch zeigten vor allem die differenzierten MSC-Pellets aus Spongiosa und Knorpel morphologisch eine starke {\"A}hnlichkeit zu hyalinem Knorpelgewebe. Trotz dieser Abstufungen zeigten sich f{\"u}r die relative Expression der chondrogenen Markergene AGG, Col II und Sox-9 keine signifikanten Unterschiede zwischen den differenzierten MSC-Kulturen der vier unterschiedlichen Nativgewebe. Ein positiver Nachweis des Markers Col X wies nach 27 Tagen sowohl in differenzierten als auch in undifferenzierten Pellet-Kulturen auf eine leichte chondrogene Hypertrophie hin. Zusammenfassend zeigten sich keine signifikanten Unterschiede im Hinblick auf das osteogene und adipogene Differenzierungspotential aller untersuchten Zellen. W{\"a}hrend das chondrogene Differenzierungspotential der Zellen aus Spongiosa, Knorpel und Kapsel sich aus histologischer und immunhistochemischer Sicht {\"a}hnelte, zeigten Pellets aus dem LCF ein schw{\"a}cheres chondrogenes Differenzierungspotential in vitro. Obwohl somit erstmals MSC-{\"a}hnliche Zellen aus dem LCF und Gewebsproben, die neben dem Stratum synoviale auch das Stratum fibrosum der H{\"u}ftgelenkskapsel beinhalteten, charakterisiert wurden, sind weitere wissenschaftliche Arbeiten notwendig, um das multipotente Differenzierungspotential dieser Zellen zu optimieren.},
  subject      = {H{\"u}ftgelenk},
  language  = {de}
}
@article{VottelerCarvajalBerrioPudlasetal.2012,
  author    = {Votteler, Miriam and Carvajal Berrio, Daniel A. and Pudlas, Marieke and Walles, Heike and Schenke-Layland, Katja},
  title     = {Non-contact, Label-free Monitoring of Cells and Extracellular Matrix using Raman Spectroscopy},
  series = {Journal of Visual Expression},
  volume    = {63},
  journal   = {Journal of Visual Expression},
  number    = {e3977},
  doi       = {10.3791/3977},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-124569},
  year      = {2012},
  abstract  = {Non-destructive, non-contact and label-free technologies to monitor cell and tissue cultures are needed in the field of biomedical research.1-5 However, currently available routine methods require processing steps and alter sample integrity. Raman spectroscopy is a fast method that enables the measurement of biological samples without the need for further processing steps. This laser-based technology detects the inelastic scattering of monochromatic light.6 As every chemical vibration is assigned to a specific Raman band (wavenumber in cm-1), each biological sample features a typical spectral pattern due to their inherent biochemical composition.7-9 Within Raman spectra, the peak intensities correlate with the amount of the present molecular bonds.1 Similarities and differences of the spectral data sets can be detected by employing a multivariate analysis (e.g. principal component analysis (PCA)).10 Here, we perform Raman spectroscopy of living cells and native tissues. Cells are either seeded on glass bottom dishes or kept in suspension under normal cell culture conditions (37 °C, 5\% CO2) before measurement. Native tissues are dissected and stored in phosphate buffered saline (PBS) at 4 °C prior measurements. Depending on our experimental set up, we then either focused on the cell nucleus or extracellular matrix (ECM) proteins such as elastin and collagen. For all studies, a minimum of 30 cells or 30 random points of interest within the ECM are measured. Data processing steps included background subtraction and normalization.},
  language  = {en}
}
@article{ThibaudeauTaubenbergerTheodoropoulosetal.2015,
  author    = {Thibaudeau, Laure and Taubenberger, Anna V. and Theodoropoulos, Christina and Holzapfel, Boris M. and Ramuz, Olivier and Straub, Melanie and Hutmacher, Dietmar W.},
  title     = {New mechanistic insights of integrin β1 in breast cancer bone colonization},
  series = {Oncotarget},
  volume    = {6},
  journal   = {Oncotarget},
  number    = {1},
  doi       = {10.18632/oncotarget.2788},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-175432},
  pages     = {332-344},
  year      = {2015},
  abstract  = {Bone metastasis is a frequent and life-threatening complication of breast cancer. The molecular mechanisms supporting the establishment of breast cancer cells in the skeleton are still not fully understood, which may be attributed to the lack of suitable models that interrogate interactions between human breast cancer cells and the bone microenvironment. Although it is well-known that integrins mediate adhesion of malignant cells to bone extracellular matrix, their role during bone colonization remains unclear. Here, the role of β1 integrins in bone colonization was investigated using tissue-engineered humanized in vitro and in vivo bone models. In vitro, bone-metastatic breast cancer cells with suppressed integrin β1 expression showed reduced attachment, spreading, and migration within human bone matrix compared to control cells. Cell proliferation in vitro was not affected by β1 integrin knockdown, yet tumor growth in vivo within humanized bone microenvironments was significantly inhibited upon β1 integrin suppression, as revealed by quantitative in/ex vivo fluorescence imaging and histological analysis. Tumor cells invaded bone marrow spaces in the humanized bone and formed osteolytic lesions; osteoclastic bone resorption was, however, not reduced by β1 integrin knockdown. Taken together, we demonstrate that β1 integrins have a pivotal role in bone colonization using unique tissue-engineered humanized bone models.},
  language  = {en}
}
@article{ThibaudeauTaubenbergerHolzapfeletal.2014,
  author    = {Thibaudeau, Laure and Taubenberger, Anna V. and Holzapfel, Boris M. and Quent, Verena M. and Fuehrmann, Tobias and Hesami, Parisa and Brown, Toby D. and Dalton, Paul D. and Power, Carl A. and Hollier, Brett G. and Hutmacher, Dietmar W.},
  title     = {A tissue-engineered humanized xenograft model of human breast cancer metastasis to bone},
  series = {Disease Models \& Mechanisms},
  volume    = {7},
  journal   = {Disease Models \& Mechanisms},
  number    = {2},
  doi       = {10.1242/dmm.014076},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-117466},
  pages     = {299-309},
  year      = {2014},
  abstract  = {The skeleton is a preferred homing site for breast cancer metastasis. To date, treatment options for patients with bone metastases are mostly palliative and the disease is still incurable. Indeed, key mechanisms involved in breast cancer osteotropism are still only partially understood due to the lack of suitable animal models to mimic metastasis of human tumor cells to a human bone microenvironment. In the presented study, we investigate the use of a human tissue-engineered bone construct to develop a humanized xenograft model of breast cancer-induced bone metastasis in a murine host. Primary human osteoblastic cell-seeded melt electrospun scaffolds in combination with recombinant human bone morphogenetic protein 7 were implanted subcutaneously in non-obese diabetic/severe combined immunodeficient mice. The tissue-engineered constructs led to the formation of a morphologically intact 'organ' bone incorporating a high amount of mineralized tissue, live osteocytes and bone marrow spaces. The newly formed bone was largely humanized, as indicated by the incorporation of human bone cells and human-derived matrix proteins. After intracardiac injection, the dissemination of luciferase-expressing human breast cancer cell lines to the humanized bone ossicles was detected by bioluminescent imaging. Histological analysis revealed the presence of metastases with clear osteolysis in the newly formed bone. Thus, human tissue-engineered bone constructs can be applied efficiently as a target tissue for human breast cancer cells injected into the blood circulation and replicate the osteolytic phenotype associated with breast cancer-induced bone lesions. In conclusion, we have developed an appropriate model for investigation of species-specific mechanisms of human breast cancer-related bone metastasis in vivo.},
  language  = {en}
}
@article{SulimanSunPedersenetal.2016,
  author    = {Suliman, Salwa and Sun, Yang and Pedersen, Torbjorn O. and Xue, Ying and Nickel, Joachim and Waag, Thilo and Finne-Wistrand, Anna and Steinm{\"u}ller-Nethl, Doris and Krueger, Anke and Costea, Daniela E. and Mustafa, Kamal},
  title     = {In vivo host response and degradation of copolymer scaffolds functionalized with nanodiamonds and bone morphogenetic protein 2},
  series = {Advanced Healthcare Materials},
  volume    = {5},
  journal   = {Advanced Healthcare Materials},
  number    = {6},
  doi       = {10.1002/adhm.201500723},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-189764},
  pages     = {730-742},
  year      = {2016},
  abstract  = {The aim is to evaluate the effect of modifying poly[(L-lactide)-co-(epsilon-caprolactone)] scaffolds (PLCL) with nanodiamonds (nDP) or with nDP+physisorbed BMP-2 (nDP+BMP-2) on in vivo host tissue response and degradation. The scaffolds are implanted subcutaneously in Balb/c mice and retrieved after 1, 8, and 27 weeks. Molecular weight analysis shows that modified scaffolds degrade faster than the unmodified. Gene analysis at week 1 shows highest expression of proinflammatory markers around nDP scaffolds; although the presence of inflammatory cells and foreign body giant cells is more prominent around the PLCL. Tissue regeneration markers are highly expressed in the nDP+BMP-2 scaffolds at week 8. A fibrous capsule is detectable by week 8, thinnest around nDP scaffolds and at week 27 thickest around PLCL scaffolds. mRNA levels of ALP, COL1 alpha 2, and ANGPT1 are signifi cantly upregulating in the nDP+BMP-2 scaffolds at week 1 with ectopic bone seen at week 8. Even when almost 90\% of the scaffold is degraded at week 27, nDP are observable at implantation areas without adverse effects. In conclusion, modifying PLCL scaffolds with nDP does not aggravate the host response and physisorbed BMP-2 delivery attenuates infl ammation while lowering the dose of BMP-2 to a relatively safe and economical level.},
  language  = {en}
}