Lineage Tracing Reveals Distinctive Fates for Mesothelial Cells and Submesothelial Fibroblasts during Peritoneal Injury

Chen, Yi Ting; Chang, Yu; Pan, Szu Yu; Chou, Yu‐Hsiang; Chang, Fan‐Ren; Yeh, Pei Ying; Liu, Yuan Hung; Chiang, Wen‐Chih; Chen, Ming-Fong; Wu, Mai‐Szu; Tsai, Tun‐Jun; Duffield, Jeremy S.; Lin, Shuei‐Liong

doi:10.1681/asn.2013101079

Cited by 126 publications

(176 citation statements)

References 46 publications

(76 reference statements)

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“…CreERT2 or Col1a1 GFP mice, Chen et al 25 reported that the contribution of MCs to myofibroblasts is rare in the liver. By treating Wt1…”

Section: On the Basis Of The Labeling Efficiency Of Mcs In The Wt1mentioning

confidence: 99%

“…In addition, they reported that MCs are negative for GFP in the Col1a1 GFP mouse liver. Chen et al 25 did not analyze the body wall in these models. In our experimental condition, we labeled 12.5% and 14.5% of MCs in the body wall and liver, respectively, in the Wt1…”

Section: On the Basis Of The Labeling Efficiency Of Mcs In The Wt1mentioning

confidence: 99%

“…23e25 Sakai et al 24 reported that connective tissue growth factor (CTGF) secreted from MCs induces the proliferation and myofibroblastic conversion of fibroblasts in peritoneal fibrosis. Chen et al 25 traced liver MCs in mouse peritoneal fibrosis models and indicated that fibroblasts are the main source of myofibroblasts in liver injury. However, the origin of myofibroblasts in peritoneal fibrosis remains to be determined by rigorous cell lineage tracing.…”

mentioning

confidence: 99%

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Myofibroblastic Conversion and Regeneration of Mesothelial Cells in Peritoneal and Liver Fibrosis

Lua

Pappoe

et al. 2015

The American Journal of Pathology

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“…CreERT2 or Col1a1 GFP mice, Chen et al 25 reported that the contribution of MCs to myofibroblasts is rare in the liver. By treating Wt1…”

Section: On the Basis Of The Labeling Efficiency Of Mcs In The Wt1mentioning

confidence: 99%

Section: On the Basis Of The Labeling Efficiency Of Mcs In The Wt1mentioning

confidence: 99%

mentioning

confidence: 99%

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Myofibroblastic Conversion and Regeneration of Mesothelial Cells in Peritoneal and Liver Fibrosis

Lua

Pappoe

et al. 2015

The American Journal of Pathology

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“…Numerous studies have revealed signaling pathways of angiogenesis and fibrosis in the context of epithelial mesenchymal transition (EMT) (mesothelial cell to myofibroblast) associated with PDderived peritoneal injury (for review [67,85]). However, the primary origin of myofibroblast in PD peritoneum is argued by recent insight [86]. Otherwise, the dialysate level of connective tissue growth factor (CTGF), which inhibits bone morphogenetic protein-7 (BMP-7) and activates transforming growth factor (TGF)-β (pro-fibrosis factor), was shown be correlated to high-fast PET [87].…”

Section: Pathological Findings Of Pd Associated Infectious Peritonitismentioning

confidence: 99%

Recommendations for pathological diagnosis on biopsy samples from peritoneal dialysis patients

Kawanishi

Honda

Hamada

2017

Pleura and Peritoneum

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Peritoneal dialysis (PD) has been established as an essential renal replacement therapy for patients with end stage renal disease during the past half century. Histological evaluation of the peritoneal membrane has contributed to the pathophysiological understanding of PD-related peritoneal injury such as peritonitis, fibrosis, and encapsulating peritoneal sclerosis (EPS). Hyalinizing peritoneal sclerosis (HPS), also known as simple sclerosis, is observed in almost all of PD patients. HPS is morphologically characterized by fibrosis of the submesothelial interstitium and hyalinizing vascular wall, particularly of the post-capillary venule (PCV). Two histological factors, the thickness of submesothelial compact zone (SMC) and the lumen/vessel ratio (L/V) at the PCV, have been used for the quantitative evaluation of HPS. The measuring system on SMC thickness and L/V ratio is easy and useful for evaluating the severity of HPS. On the other hand, EPS is characterized by unique encapsulation of the intestines by an "encapsulating membrane". This newly formed membranous structure covers the visceral peritoneum of the intestines, which contains fibrin deposition, angiogenesis, and proliferation of fibroblast-like cells and other inflammatory cells. This review will cover the common understandings of PD-related peritoneal alterations and provide a basic platform for clinical applications and future studies in this field.

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“…Os miofibroblastos derivados do mesotélio seriam as responsáveis pela produção de colágeno e fibronectina resultando na fibrose peritoneal (28,36). No entanto, estudos in vivo não foram capazes de demonstrar esse fenômeno e recentemente, Chen YT e cols, demonstraram elegantemente que os miofibroblastos da camada submesotelial peritoneal se originam dos fibroblastos residentes predominantemente (37). A ativação desses fibroblastos resultaria na produção de fatores prófibróticos bem como no aumento da expressão VEGF que contribui para a neoangiogênese (38).…”

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Análise do efeito do ácido valpróico no modelo experimental de fibrose peritoneal em ratos

Costalonga¹

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Lineage Tracing Reveals Distinctive Fates for Mesothelial Cells and Submesothelial Fibroblasts during Peritoneal Injury

Cited by 126 publications

References 46 publications

Myofibroblastic Conversion and Regeneration of Mesothelial Cells in Peritoneal and Liver Fibrosis

Myofibroblastic Conversion and Regeneration of Mesothelial Cells in Peritoneal and Liver Fibrosis

Recommendations for pathological diagnosis on biopsy samples from peritoneal dialysis patients

Análise do efeito do ácido valpróico no modelo experimental de fibrose peritoneal em ratos

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