In vitro evaluation of a novel non-mulberry silk scaffold for use in tendon regeneration

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dc.contributor.author Musson, David en
dc.contributor.author Naot, Dorit en
dc.contributor.author Chhana, Ashika en
dc.contributor.author Matthews, Brya en
dc.contributor.author McIntosh, Julie en
dc.contributor.author Lin, Sandy en
dc.contributor.author Choi, AJ en
dc.contributor.author Callon, Karen en
dc.contributor.author Coleman, B en
dc.contributor.author Cornish, Jillian en
dc.coverage.spatial Queenstown, New Zealand en
dc.date.accessioned 2018-10-18T00:02:38Z en
dc.date.issued 2015-05-01 en
dc.identifier.citation 2014 en
dc.identifier.issn 1937-3341 en
dc.identifier.uri http://hdl.handle.net/2292/42757 en
dc.description.abstract Tearing of the rotator cuff tendon in the shoulder is a significant clinical problem, with large/full-thickness tears present in ∼22% of the general population and recurrent tear rates postarthroscopic repair being quoted as high as 94%. Tissue-engineered biomaterials are increasingly being investigated as a means to augment rotator cuff repairs, with the aim of inducing host cell responses to increase tendon tissue regeneration. Silk-derived materials are of particular interest due to the high availability, mechanical strength, and biocompatibility of silks. In this study, Spidrex®, a novel knitted, non-mulberry silk fibroin scaffold was evaluated in vitro for its potential to improve tendon regeneration. Spidrex was compared with a knitted Bombyx mori silk scaffold, a 3D collagen gel and Fiberwire® suture material. Primary human and rat tenocytes successfully adhered to Spidrex and significantly increased in number over a 14 day period (p<0.05), as demonstrated by fluorescent calcein-AM staining and alamarBlue® assays. A similar growth pattern was observed with human tenocytes cultured on the B. mori scaffold. Morphologically, human tenocytes elongated along the silk fibers of Spidrex, assuming a tenocytic cell shape, and were less circular with a higher aspect ratio compared with human tenocytes cultured on the B. mori silk scaffold and within the collagen gel (p<0.05). Gene expression analysis by real-time PCR showed that rat tenocytes cultured on Spidrex had increased expression of tenocyte-related genes such as fibromodullin, scleraxis, and tenomodulin (p<0.05). Expression of genes that indicate transdifferentiation toward a chondrocytic or osteoblastic lineage were significantly lower in tenocytes cultured on Spidrex in comparison to the collagen gel (p<0.05). Immunogenicity assessment by the maturation of and cytokine release from primary human dendritic cells demonstrated that Spidrex enhanced dendritic cell maturation in a similar manner to the clinically used suture material Fiberwire, and significantly upregulated the release of proinflammatory cytokines (p<0.05). This suggests that Spidrex may induce an early immune response postimplantation. While further work is required to determine what effect this immune response has on the tendon healing process, our in vitro data suggests that Spidrex may have the cytocompatibility and bioactivity required to support tendon regeneration in vivo. en
dc.publisher Mary Ann Liebert en
dc.relation.ispartofseries Tissue Engineering Part A: Tissue Engineering en
dc.rights Items in ResearchSpace are protected by copyright, with all rights reserved, unless otherwise indicated. Previously published items are made available in accordance with the copyright policy of the publisher. en
dc.rights.uri https://researchspace.auckland.ac.nz/docs/uoa-docs/rights.htm en
dc.title In vitro evaluation of a novel non-mulberry silk scaffold for use in tendon regeneration en
dc.type Journal Article en
dc.identifier.doi 10.1089/ten.tea.2014.0128 en
pubs.issue 9-10 en
pubs.begin-page 1539 en
pubs.volume 21 en
dc.identifier.pmid 25604072 en
pubs.author-url http://online.liebertpub.com/doi/10.1089/ten.tea.2014.0128 en
pubs.end-page 1551 en
dc.rights.accessrights http://purl.org/eprint/accessRights/RestrictedAccess en
pubs.subtype Article en
pubs.elements-id 461779 en
pubs.org-id Medical and Health Sciences en
pubs.org-id Medical Sciences en
pubs.org-id Anatomy and Medical Imaging en
pubs.org-id Molecular Medicine en
pubs.org-id School of Medicine en
pubs.org-id Medicine Department en
pubs.org-id School of Graduate Studies en
pubs.org-id Science en
pubs.org-id Biological Sciences en
pubs.org-id Science Research en
pubs.org-id Maurice Wilkins Centre (2010-2014) en
dc.identifier.eissn 1937-335X en
pubs.record-created-at-source-date 2014-11-18 en
pubs.dimensions-id 25604072 en


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