Lidocaine inhibits migration of tenocytes by downregulating focal adhesion kinase and paxillin phosphorylation

Author:

Chang Hsiang‐Ning1,Chen Chih‐Kuang2,Yu Tung‐Yang1ORCID,Pang Jong‐Hwei S.13,Hsu Chih‐Chin4ORCID,Lin Li‐Ping23ORCID,Tsai Wen‐Chung256

Affiliation:

1. Department of Physical Medicine and Rehabilitation Chang Gung Memorial Hospital at Linkou Taoyuan City Taiwan

2. Department of Physical Medicine and Rehabilitation Chang Gung Memorial Hospital at Taoyuan Taoyuan City Taiwan

3. Graduate Institute of Clinical Medical Sciences Chang Gung University Taoyuan City Taiwan

4. Department of Physical Medicine and Rehabilitation Chang Gung Memorial Hospital at Keelung Keelung City Taiwan

5. School of Medicine Chang Gung University Taoyuan City Taiwan

6. Center of Comprehensive Sports Medicine Chang Gung Memorial Hospital at Taoyuan Taoyuan City Taiwan

Abstract

AbstractLidocaine is the most frequently applied local infiltration anesthetic agent for treating tendinopathies. However, studies have discovered lidocaine to negatively affect tendon healing. In the current study, the molecular mechanisms and effects of lidocaine on tenocyte migration were evaluated. We treated tenocytes intrinsic to the Achilles tendons of Sprague–Dawley rats with lidocaine. The migration ability of cells was analyzed using electric cell‐substrate impedance sensing (ECIS) and scratch wound assay. We then used a microscope to evaluate the cell spread. We assessed filamentous actin (F‐actin) cytoskeleton formation through immunofluorescence staining. In addition, we used Western blot analysis to analyze the expression of phospho‐focal adhesion kinase (FAK), FAK, phospho‐paxillin, paxillin, and F‐actin. We discovered that lidocaine had an inhibitory effect on the migration of tenocytes in the scratch wound assay and on the ECIS chip. Lidocaine treatment suppressed cell spreading and changed the cell morphology and F‐actin distribution. Lidocaine reduced F‐actin formation in the tenocyte during cell spreading; furthermore, it inhibited phospho‐FAK, F‐actin, and phospho‐paxillin expression in the tenocytes. Our study revealed that lidocaine inhibits the spread and migration of tenocytes. The molecular mechanism potentially underlying this effect is downregulation of F‐actin, phospho‐FAK, and phospho‐paxillin expression when cells are treated with lidocaine.

Funder

Chang Gung Memorial Hospital, Linkou

Publisher

Wiley

Subject

Orthopedics and Sports Medicine

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