| Literature DB >> 32382019 |
Cheng Ji1, Jiahui Zhang1, Yuan Zhu2, Hui Shi1, Siqi Yin1, Fengtian Sun1, Qiongni Wang1, Leilei Zhang1, Yongmin Yan1, Xu Zhang1, Wenrong Xu3, Hui Qian4.
Abstract
Exosomes from human umbilical cord mesenchymal stem cells (hucMSC-Ex) have been suggested as novel nanomaterials for regeneEntities:
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Year: 2020 PMID: 32382019 PMCID: PMC7205986 DOI: 10.1038/s41419-020-2510-4
Source DB: PubMed Journal: Cell Death Dis Impact factor: 8.469
Fig. 1HucMSC-Ex treatment reduced renal interstitial fibrosis.
a The size of hucMSC-Ex was measured by NTA. b The morphology of hucMSC-Ex was identified by TEM. c The images of hucMSC-Ex were detected by cryo-EM. d Western blot assay for exosomal markers CD9, CD63, and Alix in hucMSC-Ex. e CM-DiR labeled hucMSC-Ex (10 mg/kg) were intravenously administrated into 14d UUO rats. The distribution of CM-DiR labeled hucMSC-Ex in the kidney detected by IVIS imaging system. f Schematic of UUO induction and exosomes treatment. UUO rats were intravenously injected with exosomes (10 mg/kg/injection) on days 6, 9, and 12. The rats were sacrificed on day 14 for subsequent experiments (n = 10). g Representative images of HE staining, Sirius red and Masson staining of kidneys in 14d UUO rats treated with hucMSC-Ex. Bar = 100 μm.
Fig. 2Sustained mechanical stress induced YAP activation and aggravated renal fibrosis.
a YAP immunohistochemistry staining of UUO 7d, 14d kidney sections. Bar = 100 μm. b Quantification of YAP-positive nuclei per field of view from the a experiment. c Double immunofluorescent staining of YAP and α-SMA in the kidneys of control and UUO (at 7 and 14 days) rats (Green: YAP; Red: α-SMA). Bar = 50 μm. d Western blot assay for YAP protein expression in the kidneys of control and UUO rats (at 7 and 14 days) rats (n = 3). e Nuclear localization of YAP in NRK-52E cells treated with different stiff gel for 48 h was detected by confocal microscopy. Bar=25 μm. f Statistical analysis the expression of YAP in cytoplasm and nuclear under mechanical pressure. **P < 0.01.
Fig. 3HucMSC-Ex attenuated tubulointerstitial fibrosis by inhibited YAP.
a YAP immunohistochemistry staining of 14d UUO kidney with hucMSC-Ex treatment. Bar=100 μm. b Quantification of YAP-positive nuclei per field of view from the a experiment. c Double immunofluorescent staining of YAP and α-SMA in the kidney of 14d UUO rats treated with hucMSC-Ex (Green: YAP; red: α-SMA). Bar = 50 μm. d Western blot analyses of YAP expression in the kidney of 14d UUO rats with hucMSC-Ex intervene (n = 3). e The co-localization of YAP and α-SMA in NRK-52E cells cultured under stiff gel condition in the presence of hucMSC-Ex was detected by double immunofluorescent staining. Bar=25 μm. f Statistical analysis the expression of YAP in cytoplasm and nuclear with hucMSC-Ex therapy. **P < 0.01.
Fig. 4HucMSC-Ex delivered CK1δ and β-TRCP to promote YAP ubiquitination and degradation.
a Western blot assay for CK1δ and β-TRCP proteins in hucMSC-Ex (n = 4). b The internalization of hucMSC-Ex (PKH67, green) in NRK-52E cells was observed by confocal microscopy. Bar = 25 μm. c The expression of CK1δ and β-TRCP in NRK-52E cells under mechanical stress. Bar = 25 μm. d The expression of CK1δ, β-TRCP, and YAP in the kidneys of 14d UUO rats with hucMSC-Ex treatment was determined by immunohistochemistry. Bar = 100 μm. e Western blot assay for CK1δ and β-TRCP proteins in the kidneys of 14d UUO rats treated with hucMSC-Ex (n = 3). f NRK-52E cells were pre-treated with MG132 (20 μm) for 5 h followed by stiff gel stimulation in the presence of hucMSC-Ex. YAP protein level was detected by western blot. g The ubiquitination of YAP protein with hucMSC-Ex treatment determined by co-IP.
Fig. 5CK1δ and β-TRCP knockdown decreased anti-fibrosis effective of hucMSC-Ex.
a Expression of CK1δ and β-TRCP in hucMSC-Ex was determined by western blot and qRT-PCR. b Representative images of HE and Masson staining in the UUO model with hucMSC-Ex, shCK1δ-Ex, and shβ-TRCP-Ex. Bar = 100 μm. c Double immunofluorescent staining of YAP and α-SMA in the kidneys of the UUO model treated with hucMSC-Ex, shCK1δ-Ex, and shβ-TRCP-Ex. Bar = 50 μm. d Western blot analyses for CK1δ and β-TRCP in NRK-52E after hucMSC-Ex treatment. e The expression of CK1δ, β-TRCP, YAP, and α-SMA in UUO14d with hucMSC-Ex, shCK1δ-Ex, and shβ-TRCP-Ex treatment was detected by western blot. f A proposed hypothesis for hucMSC-Ex attenuated tubulointerstitial fibrosis through CK1δ and β-TRCP mediated YAP ubiquitination and degradation.