Effect of Endomorphin-1 on Maturation and Expression of TLR4 in Peripheral Blood Dendritic Cells Induced by High Glucose.

Chuan-miao Liu; Tian-hua Yang; Min Huang; Cheng Zhou; Yong-hai LI; Zheng-hong LI

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Effect of Endomorphin-1 on Maturation and Expression of TLR4 in Peripheral Blood Dendritic Cells Induced by High Glucose.

Author: Chuan-Miao LIU ¹ ; Tian-Hua YANG ² ; Min HUANG ¹ ; Cheng ZHOU ² ; Yong-Hai LI ² ; Zheng-Hong LI ³
Author Information

1. Department of Infecction, The First Affiliated Hospital of Bengbu Medical College, Bengbu 233004, Anhui Province, China.
2. Laboratory of Physiology, Bengbu Medical College, Bengbu 233030, Anhui Province, China.
3. Laboratory of Physiology, Bengbu Medical College, Bengbu 233030, Anhui Province, China. E-mail: lizhbbmc@163.com.
Publication Type:Journal Article
MeSH: Cell Differentiation; Cells, Cultured; Cytokines; Dendritic Cells; Glucose; Humans; Oligopeptides; Toll-Like Receptor 4
From: Journal of Experimental Hematology 2018;26(3):886-893
CountryChina
Language:Chinese
Abstract:
OBJECTIVETo investigate the effects of endomorphin-1 (EM-1) on the maturation phenotype, cytokine secretion, T cell proliferation and TLR4 expression in human peripheral blood dendritic cells (PBDCs) stimulated and induced by high glucose, and to explore the regulatory mechanism of EM-1 on DC immune function.
METHODSPeripheral blood mononuclear cells (PBMNCs) were induced into immature dendritic cells (imDCs). The high glucose was used as the stimulating factor, and the EM-1 was used as the interventional factor. Then, the experiments were divided into normal glucose group (NG group), high glucose group (HG group), high glucose plus EM-1 group (EM group) and high glucose plus EM-1 and naloxone group (Nal group), respectively. The PBDC's phenotype changes were detected by flow cytometry; ELISA was used to detect the changes of cytokines secreted by PBDCs co-cultured with autologous lymphocytes; CFSE was used to detect the proliferation of T lymphocytes. TLR4 expression on PBDC surface was detected by RT-PCR.
RESULTSCompared with HG group, the expression of PBDC surface molecules CD86, CCR7 and CD36 was up-regulated in EM group (P<0.01), while the change of CD83 expression was not statistically significant. However, IL-12 and IL-10 secreted by PBDCs and the proliferation index of T-lymphocytes stimulated by PBDCs were both decreased in EM group. Compared with EM group, the expression of CD86, CCR7 and CD36 was decreased in Nal group (P<0.01), while the expression of CD83 was almost unchanged (P>0.05). T-lymphocyte proliferation index was increased very significantly in Nal group (P<0.01). The gray ratio of TLR4 in HG group was higher than that in NG group, while the gray ratio in EM group's was very significantly lower than that in HG group's (P<0.01). These results indicate that the high glucose can promote the expression of PBDC TLR4, while the EM-1 inhibits the expression of TLR4.
CONCLUSIONEM-1 up-regulates the expression of PBDC surface molecules CD86, CCR7 and CD36 stimulated and induced by high glucose, but inhibites the induction of PBDC to maturity by high glucose. And the secreted inflammatory cytokines IL-12 and IL-10 inhibites the proliferation of T lymphocytes derived from PBDCs, while naloxone inhibites the effect of EM-1. EM-1 inhibites the expression of TLR4 on PBDC surface induced by high glucose.