The paratenon contributes to scleraxis-expressing cells during patellar tendon healing.
The origin of cells that contribute to tendon healing, specifically extrinsic epitenon/paratenon cells vs. internal tendon fibroblasts, is still debated. The purpose of this study is to determine the location and phenotype of cells that contribute to healing of a central patellar tendon defect injur...
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doaj-e7ee9db427ec41adbb5c22a56b29983b2020-11-25T01:49:56ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-0183e5994410.1371/journal.pone.0059944The paratenon contributes to scleraxis-expressing cells during patellar tendon healing.Nathaniel A DymentChia-Feng LiuNamdar KazemiLindsey E Aschbacher-SmithKeith KenterAndrew P BreidenbachJason T ShearnChristopher WylieDavid W RoweDavid L ButlerThe origin of cells that contribute to tendon healing, specifically extrinsic epitenon/paratenon cells vs. internal tendon fibroblasts, is still debated. The purpose of this study is to determine the location and phenotype of cells that contribute to healing of a central patellar tendon defect injury in the mouse. Normal adult patellar tendon consists of scleraxis-expressing (Scx) tendon fibroblasts situated among aligned collagen fibrils. The tendon body is surrounded by paratenon, which consists of a thin layer of cells that do not express Scx and collagen fibers oriented circumferentially around the tendon. At 3 days following injury, the paratenon thickens as cells within the paratenon proliferate and begin producing tenascin-C and fibromodulin. These cells migrate toward the defect site and express scleraxis and smooth muscle actin alpha by day 7. The thickened paratenon tissue eventually bridges the tendon defect by day 14. Similarly, cells within the periphery of the adjacent tendon struts express these markers and become disorganized. Cells within the defect region show increased expression of fibrillar collagens (Col1a1 and Col3a1) but decreased expression of tenogenic transcription factors (scleraxis and mohawk homeobox) and collagen assembly genes (fibromodulin and decorin). By contrast, early growth response 1 and 2 are upregulated in these tissues along with tenascin-C. These results suggest that paratenon cells, which normally do not express Scx, respond to injury by turning on Scx and assembling matrix to bridge the defect. Future studies are needed to determine the signaling pathways that drive these cells and whether they are capable of producing a functional tendon matrix. Understanding this process may guide tissue engineering strategies in the future by stimulating these cells to improve tendon repair.http://europepmc.org/articles/PMC3608582?pdf=render |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Nathaniel A Dyment Chia-Feng Liu Namdar Kazemi Lindsey E Aschbacher-Smith Keith Kenter Andrew P Breidenbach Jason T Shearn Christopher Wylie David W Rowe David L Butler |
spellingShingle |
Nathaniel A Dyment Chia-Feng Liu Namdar Kazemi Lindsey E Aschbacher-Smith Keith Kenter Andrew P Breidenbach Jason T Shearn Christopher Wylie David W Rowe David L Butler The paratenon contributes to scleraxis-expressing cells during patellar tendon healing. PLoS ONE |
author_facet |
Nathaniel A Dyment Chia-Feng Liu Namdar Kazemi Lindsey E Aschbacher-Smith Keith Kenter Andrew P Breidenbach Jason T Shearn Christopher Wylie David W Rowe David L Butler |
author_sort |
Nathaniel A Dyment |
title |
The paratenon contributes to scleraxis-expressing cells during patellar tendon healing. |
title_short |
The paratenon contributes to scleraxis-expressing cells during patellar tendon healing. |
title_full |
The paratenon contributes to scleraxis-expressing cells during patellar tendon healing. |
title_fullStr |
The paratenon contributes to scleraxis-expressing cells during patellar tendon healing. |
title_full_unstemmed |
The paratenon contributes to scleraxis-expressing cells during patellar tendon healing. |
title_sort |
paratenon contributes to scleraxis-expressing cells during patellar tendon healing. |
publisher |
Public Library of Science (PLoS) |
series |
PLoS ONE |
issn |
1932-6203 |
publishDate |
2013-01-01 |
description |
The origin of cells that contribute to tendon healing, specifically extrinsic epitenon/paratenon cells vs. internal tendon fibroblasts, is still debated. The purpose of this study is to determine the location and phenotype of cells that contribute to healing of a central patellar tendon defect injury in the mouse. Normal adult patellar tendon consists of scleraxis-expressing (Scx) tendon fibroblasts situated among aligned collagen fibrils. The tendon body is surrounded by paratenon, which consists of a thin layer of cells that do not express Scx and collagen fibers oriented circumferentially around the tendon. At 3 days following injury, the paratenon thickens as cells within the paratenon proliferate and begin producing tenascin-C and fibromodulin. These cells migrate toward the defect site and express scleraxis and smooth muscle actin alpha by day 7. The thickened paratenon tissue eventually bridges the tendon defect by day 14. Similarly, cells within the periphery of the adjacent tendon struts express these markers and become disorganized. Cells within the defect region show increased expression of fibrillar collagens (Col1a1 and Col3a1) but decreased expression of tenogenic transcription factors (scleraxis and mohawk homeobox) and collagen assembly genes (fibromodulin and decorin). By contrast, early growth response 1 and 2 are upregulated in these tissues along with tenascin-C. These results suggest that paratenon cells, which normally do not express Scx, respond to injury by turning on Scx and assembling matrix to bridge the defect. Future studies are needed to determine the signaling pathways that drive these cells and whether they are capable of producing a functional tendon matrix. Understanding this process may guide tissue engineering strategies in the future by stimulating these cells to improve tendon repair. |
url |
http://europepmc.org/articles/PMC3608582?pdf=render |
work_keys_str_mv |
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