TY - JOUR
T1 - Harnessing the synergy of perfusable muscle flap matrix and adipose-derived stem cells for prevascularization and macrophage polarization to reconstruct volumetric muscle loss
AU - Zhang, Qixu
AU - Chiu, Yulun
AU - Chen, Youbai
AU - Wu, Yewen
AU - Dunne, Lina W.
AU - Largo, Rene D.
AU - Chang, Edward I.
AU - Adelman, David M.
AU - Schaverien, Mark V.
AU - Butler, Charles E.
N1 - Funding Information:
This work was supported by a grant from The Plastic Surgery Foundation (PSF312406, to Q. Zhang) and by the Kyte Fund through MD Anderson's Department of Plastic Surgery. This research was also supported by the NIH through MD Anderson's Cancer Center Support Grant (P30CA016672) and used MD Anderson's High Resolution Electron Microscopy Facility, Flow Cytometry and Cellular Imaging Core Facility, and Proteomics and Metabolomics Core Facility. We thank Joseph Munch and Madison Semro in MD Anderson's Research Medical Library for editing the manuscript; Zhenbo Han in MD Anderson's Department of Molecular & Cellular Oncology for help with multiphoton immunofluorescence imaging; Jared Burks in MD Anderson's Department of Leukemia for help with immunostaining imaging; David Hawkes in MD Anderson's Proteomics and Metabolomics Core Facility for help with mass spectrometry; Kenneth Dunner, Jr. in MD Anderson's High Resolution Electron Microscopy Facility for assistance with SEM imaging; Michael Gallagher in MD Anderson's Department of Medical Graphics & Photography for editing the graphical abstract; and Nathan Poling for editing the videos.
Funding Information:
This work was supported by a grant from The Plastic Surgery Foundation ( PSF312406 , to Q. Zhang) and by the Kyte Fund through MD Anderson's Department of Plastic Surgery. This research was also supported by the NIH through MD Anderson's Cancer Center Support Grant ( P30CA016672 ) and used MD Anderson's High Resolution Electron Microscopy Facility, Flow Cytometry and Cellular Imaging Core Facility, and Proteomics and Metabolomics Core Facility. We thank Joseph Munch and Madison Semro in MD Anderson's Research Medical Library for editing the manuscript; Zhenbo Han in MD Anderson's Department of Molecular & Cellular Oncology for help with multiphoton immunofluorescence imaging; Jared Burks in MD Anderson's Department of Leukemia for help with immunostaining imaging; David Hawkes in MD Anderson's Proteomics and Metabolomics Core Facility for help with mass spectrometry; Kenneth Dunner, Jr., in MD Anderson's High Resolution Electron Microscopy Facility for assistance with SEM imaging; Michael Gallagher in MD Anderson's Department of Medical Graphics & Photography for editing the graphical abstract; and Nathan Poling for editing the videos.
Publisher Copyright:
© 2022 The Authors
PY - 2023/4
Y1 - 2023/4
N2 - Muscle flaps must have a strong vascular network to support a large tissue volume and ensure successful engraftment. We developed porcine stomach musculofascial flap matrix (PDSF) comprising extracellular matrix (ECM) and intact vasculature. PDSF had a dominant vascular pedicle, microcirculatory vessels, a nerve network, well-retained 3-dimensional (3D) nanofibrous ECM structures, and no allo- or xenoantigenicity. In-depth proteomic analysis demonstrated that PDSF was composed of core matrisome proteins (e.g., collagens, glycoproteins, proteoglycans, and ECM regulators) that, as shown by Gene Ontology term enrichment analysis, are functionally related to musculofascial biological processes. Moreover, PDSF−human adipose-derived stem cell (hASC) synergy not only induced monocytes towards IL-10−producing M2 macrophage polarization through the enhancement of hASCs' paracrine effect but also promoted the proliferation and interconnection of both human skeletal muscle myoblasts (HSMMs) and human umbilical vein endothelial cells (HUVECs) in static triculture conditions. Furthermore, PDSF was successfully prevascularized through a dynamic perfusion coculture of hASCs and HUVECs, which integrated with PDSF and induced the maturation of vascular networks in vitro. In a xenotransplantation model, PDSF demonstrated myoconductive and immunomodulatory properties associated with the predominance of M2 macrophages and regulatory T cells. In a volumetric muscle loss (VML) model, prevascularized PDSF augmented neovascularization and constructive remodeling, which was characterized by the predominant infiltration of M2 macrophages and significant musculofascial tissue formation. These results indicate that hASCs' integration with PDSF enhances the cells’ dual function in immunomodulation and angiogenesis. Owing in part to this PDSF-hASC synergy, our platform shows promise for vascularized muscle flap engineering for VML reconstruction.
AB - Muscle flaps must have a strong vascular network to support a large tissue volume and ensure successful engraftment. We developed porcine stomach musculofascial flap matrix (PDSF) comprising extracellular matrix (ECM) and intact vasculature. PDSF had a dominant vascular pedicle, microcirculatory vessels, a nerve network, well-retained 3-dimensional (3D) nanofibrous ECM structures, and no allo- or xenoantigenicity. In-depth proteomic analysis demonstrated that PDSF was composed of core matrisome proteins (e.g., collagens, glycoproteins, proteoglycans, and ECM regulators) that, as shown by Gene Ontology term enrichment analysis, are functionally related to musculofascial biological processes. Moreover, PDSF−human adipose-derived stem cell (hASC) synergy not only induced monocytes towards IL-10−producing M2 macrophage polarization through the enhancement of hASCs' paracrine effect but also promoted the proliferation and interconnection of both human skeletal muscle myoblasts (HSMMs) and human umbilical vein endothelial cells (HUVECs) in static triculture conditions. Furthermore, PDSF was successfully prevascularized through a dynamic perfusion coculture of hASCs and HUVECs, which integrated with PDSF and induced the maturation of vascular networks in vitro. In a xenotransplantation model, PDSF demonstrated myoconductive and immunomodulatory properties associated with the predominance of M2 macrophages and regulatory T cells. In a volumetric muscle loss (VML) model, prevascularized PDSF augmented neovascularization and constructive remodeling, which was characterized by the predominant infiltration of M2 macrophages and significant musculofascial tissue formation. These results indicate that hASCs' integration with PDSF enhances the cells’ dual function in immunomodulation and angiogenesis. Owing in part to this PDSF-hASC synergy, our platform shows promise for vascularized muscle flap engineering for VML reconstruction.
KW - Decellularization
KW - Extracellular matrix
KW - Macrophage polarization
KW - Muscle flap fabrication
KW - Vascularization
KW - Volumetric muscle loss
UR - http://www.scopus.com/inward/record.url?scp=85141310361&partnerID=8YFLogxK
UR - http://www.scopus.com/inward/citedby.url?scp=85141310361&partnerID=8YFLogxK
U2 - 10.1016/j.bioactmat.2022.10.023
DO - 10.1016/j.bioactmat.2022.10.023
M3 - Article
AN - SCOPUS:85141310361
VL - 22
SP - 588
EP - 614
JO - Bioactive Materials
JF - Bioactive Materials
SN - 2452-199X
ER -