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In vitro differentiation of myeloid suppressor cells (MDSC-like) from an immature myelomonocytic precursor THP-1

免疫分型 髓源性抑制细胞 人口 免疫学 生物 免疫系统 髓样 THP1细胞系 癌症研究 细胞生物学 流式细胞术 化学 细胞培养 抑制器 医学 癌症 遗传学 环境卫生
作者
Vanessa Araújo Varela,Letícia Borges da Silva Heinen,Luciana Cavalheiro Marti,Victória Bulcão Caraciolo,Tarcila Santos Datoguia,Mariane Tami Amano,Welbert Oliveira Pereira
出处
期刊:Journal of Immunological Methods [Elsevier BV]
卷期号:515: 113441-113441 被引量:4
标识
DOI:10.1016/j.jim.2023.113441
摘要

Myeloid-derived suppressor cells (MDSCs) are a heterogeneous population with a potent suppressor profile that regulates immune responses. These cells are one of the main components of the microenvironment of several diseases, including solid and hematologic tumors, autoimmunities, and chronic inflammation. However, their wide use in studies is limited due to they comprehend a rare population, which is difficult to isolate, expand, differentiate, and maintain in culture. Additionally, this population has a complex phenotypic and functional characterization. To develop a protocol for the in vitro production of MDSC-like population from the differentiation of the immature myeloid cell line THP-1. We stimulated THP-1 with G-CSF (100 ng/mL) and IL-4 (20 ng/mL) for seven days to differentiate into the MDSC-like profile. At the end of the protocol, we characterized these cells phenotypically and functionally by immunophenotyping, gene expression analysis, cytokine release dosage, lymphocyte proliferation, and NK-mediated killing essays. We differentiate THP-1 cells in an MDSC-like population, named THP1-MDSC-like, which presented immunophenotyping and gene expression profiles compatible with that described in the literature. Furthermore, we verified that this phenotypic and functional differentiation did not deviate to a macrophage profile of M1 or M2. These THP1-MDSC-like cells secreted several immunoregulatory cytokines into the microenvironment, consistent with the suppressor profile related to MDSC. In addition, the supernatant of these cells decreased the proliferation of activated lymphocytes and impaired the apoptosis of leukemic cells induced by NK cells. We developed an effective protocol for MDSC in vitro production from the differentiation of the immature myeloid cell line THP-1 induced by G-CSF and IL-4. Furthermore, we demonstrated that THP1-MDSC-like suppressor cells contribute to the immune escape of AML cells. Potentially, these THP1-MDSC-like cells can be applied on a large-scale platform, thus being able to impact the course of several studies and models such as cancer, immunodeficiencies, autoimmunity, and chronic inflammation.
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