{"title":"Inducing and regulating human naive CD4<sup>+</sup> t cell proliferation by different antigen presenting cells.","authors":"Fabienne Mazerolles, Frédéric Rieux-Laucat","doi":"10.1016/j.jim.2024.113775","DOIUrl":null,"url":null,"abstract":"<p><p>We have shown in previous studies that naive CD4<sup>+</sup> T cells isolated from human peripheral blood are induced to proliferate by CD4<sup>neg</sup>CD11c<sup>+</sup>CD14<sup>neg</sup>CD16<sup>neg</sup> dendritic cells presenting the superantigen SEE. Since this population is very poorly expressed in blood, we tried to find other antigen presenting cells (APCs) to induce this proliferation. The aim of the previous studies was to investigate the regulation of T cell proliferation in pediatric monogenic autoimmune diseases and the regulation of this proliferation by regulatory T cells (TREGs). Since the blood samples from pediatric patients were very small, it was important to study other APCs that are more commonly present in the blood. In this study we tested different APCs isolated from controls, CD19<sup>+</sup> B cells, CD11c<sup>+</sup>CD14<sup>+</sup> and CD11c<sup>+</sup>CD14<sup>neg</sup> monocytes, CD11c<sup>+</sup>CD14<sup>neg</sup>CD16<sup>+</sup> and CD16<sup>neg</sup> dendritic cells. The different T cell populations, naive effector T cells and regulatory T cells were separated simultaneously from the same sample. We show in these studies that CD19<sup>+</sup> B cells, CD14<sup>neg</sup> and more specifically CD14<sup>neg</sup>CD16<sup>+</sup>, are also able to induce T cell proliferation as previously described with CD14<sup>neg</sup>CD16<sup>neg</sup> DCs, but under different conditions. No proliferation was induced with CD14<sup>+</sup> monocytes. However, these three APCs are less potent than CD16<sup>neg</sup> and inhibition by TREG is more difficult to detect. In addition, when we test the role of CTLA-4 in the regulation of TEFF proliferation, we observe that for some APCs, the inhibition by CTLA-4 was quite different. No inhibition was observed with CD19<sup>+</sup> B cells in contrast to CD11c<sup>+</sup>CD14<sup>neg</sup>CD16<sup>+</sup> and CD11c<sup>+</sup>CD14<sup>neg</sup>CD16<sup>neg</sup> .</p>","PeriodicalId":16000,"journal":{"name":"Journal of immunological methods","volume":" ","pages":"113775"},"PeriodicalIF":1.6000,"publicationDate":"2024-11-13","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Journal of immunological methods","FirstCategoryId":"3","ListUrlMain":"https://doi.org/10.1016/j.jim.2024.113775","RegionNum":4,"RegionCategory":"医学","ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q4","JCRName":"BIOCHEMICAL RESEARCH METHODS","Score":null,"Total":0}
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Abstract
We have shown in previous studies that naive CD4+ T cells isolated from human peripheral blood are induced to proliferate by CD4negCD11c+CD14negCD16neg dendritic cells presenting the superantigen SEE. Since this population is very poorly expressed in blood, we tried to find other antigen presenting cells (APCs) to induce this proliferation. The aim of the previous studies was to investigate the regulation of T cell proliferation in pediatric monogenic autoimmune diseases and the regulation of this proliferation by regulatory T cells (TREGs). Since the blood samples from pediatric patients were very small, it was important to study other APCs that are more commonly present in the blood. In this study we tested different APCs isolated from controls, CD19+ B cells, CD11c+CD14+ and CD11c+CD14neg monocytes, CD11c+CD14negCD16+ and CD16neg dendritic cells. The different T cell populations, naive effector T cells and regulatory T cells were separated simultaneously from the same sample. We show in these studies that CD19+ B cells, CD14neg and more specifically CD14negCD16+, are also able to induce T cell proliferation as previously described with CD14negCD16neg DCs, but under different conditions. No proliferation was induced with CD14+ monocytes. However, these three APCs are less potent than CD16neg and inhibition by TREG is more difficult to detect. In addition, when we test the role of CTLA-4 in the regulation of TEFF proliferation, we observe that for some APCs, the inhibition by CTLA-4 was quite different. No inhibition was observed with CD19+ B cells in contrast to CD11c+CD14negCD16+ and CD11c+CD14negCD16neg .
我们在以前的研究中已经证明,从人类外周血中分离出来的幼稚 CD4+ T 细胞会被呈现超抗原 SEE 的 CD4negCD11c+CD14negCD16neg 树突状细胞诱导增殖。由于这一群体在血液中的表达量很低,我们试图寻找其他抗原呈递细胞(APC)来诱导这种增殖。之前研究的目的是调查小儿单基因自身免疫性疾病对 T 细胞增殖的调控以及调节性 T 细胞(TREGs)对这种增殖的调控。由于儿科患者的血液样本非常少,因此研究血液中更常见的其他 APCs 非常重要。在这项研究中,我们测试了从对照组、CD19+ B 细胞、CD11c+CD14+ 和 CD11c+CD14neg 单核细胞、CD11c+CD14negCD16+ 和 CD16neg 树突状细胞中分离出来的不同 APC。不同的 T 细胞群、幼稚效应 T 细胞和调节性 T 细胞同时从同一样本中分离出来。我们在这些研究中发现,CD19+ B 细胞、CD14neg,更具体地说是 CD14negCD16+,也能诱导 T 细胞增殖,就像之前用 CD14negCD16neg DCs 所描述的那样,但条件不同。CD14+ 单核细胞不能诱导 T 细胞增殖。不过,这三种 APC 的作用不如 CD16neg 强,而且 TREG 的抑制作用更难检测到。此外,当我们检测 CTLA-4 在 TEFF 增殖调控中的作用时,我们发现 CTLA-4 对某些 APC 的抑制作用大不相同。与 CD11c+CD14negCD16+ 和 CD11c+CD14negCD16neg 相反,CD19+ B 细胞没有抑制作用。
期刊介绍:
The Journal of Immunological Methods is devoted to covering techniques for: (1) Quantitating and detecting antibodies and/or antigens. (2) Purifying immunoglobulins, lymphokines and other molecules of the immune system. (3) Isolating antigens and other substances important in immunological processes. (4) Labelling antigens and antibodies. (5) Localizing antigens and/or antibodies in tissues and cells. (6) Detecting, and fractionating immunocompetent cells. (7) Assaying for cellular immunity. (8) Documenting cell-cell interactions. (9) Initiating immunity and unresponsiveness. (10) Transplanting tissues. (11) Studying items closely related to immunity such as complement, reticuloendothelial system and others. (12) Molecular techniques for studying immune cells and their receptors. (13) Imaging of the immune system. (14) Methods for production or their fragments in eukaryotic and prokaryotic cells.
In addition the journal will publish articles on novel methods for analysing the organization, structure and expression of genes for immunologically important molecules such as immunoglobulins, T cell receptors and accessory molecules involved in antigen recognition, processing and presentation. Submitted full length manuscripts should describe new methods of broad applicability to immunology and not simply the application of an established method to a particular substance - although papers describing such applications may be considered for publication as a short Technical Note. Review articles will also be published by the Journal of Immunological Methods. In general these manuscripts are by solicitation however anyone interested in submitting a review can contact the Reviews Editor and provide an outline of the proposed review.
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