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基于体外多克隆刺激的抗原特异性人记忆 B 细胞群体分析。

Analysis of Antigen-Specific Human Memory B Cell Populations Based on In Vitro Polyclonal Stimulation.

机构信息

David H. Smith Center for Vaccine Biology and Immunology, Department of Microbiology and Immunology, University of Rochester Medical Center, Rochester, New York.

出版信息

Curr Protoc Immunol. 2020 Dec;131(1):e109. doi: 10.1002/cpim.109.

Abstract

Antigen-specific memory B cell (MBC) populations mediate the rapid, strong, and high-affinity secondary antibody responses that play a key role in combating infection and generating protective responses to vaccination. Recently, cell staining with fluorochrome-labeled antigens together with sequencing methods such as Drop-seq and CITE-seq have provided information on the specificity, phenotype, and transcriptome of single MBCs. However, characterization of MBCs at the level of antigen-reactive populations remains an important tool for assessing an individual's B cell immunity and responses to antigen exposure. This is readily performed using a long-established method based on in vitro polyclonal stimulation of MBCs to induce division and differentiation into antibody-secreting cells (ASCs). Post-stimulation antigen-specific measurement of the MBC-derived ASCs (or the secreted antibodies) indicates the size of precursor MBC populations. Additional information about the character of antigen-reactive MBC populations is provided by analysis of MBC-derived antibodies of particular specificities for binding avidity and functionality. This article outlines a simple and reliable strategy for efficient in vitro MBC stimulation and use of the ELISpot assay as a post-stimulation readout to determine the size of antigen-specific MBC populations. Other applications of the in vitro stimulation technique for MBC analysis are discussed. The following protocols are included. © 2020 Wiley Periodicals LLC Basic Protocol 1: Polyclonal stimulation of memory B cells using unfractionated PBMCs Alternate Protocol: Stimulation of small PBMC numbers using 96-well plates with U-bottom wells Basic Protocol 2: ELISpot assay for enumeration of memory B cell-derived antibody-secreting cells.

摘要

抗原特异性记忆 B 细胞(MBC)群体介导快速、强烈和高亲和力的二次抗体反应,在对抗感染和产生疫苗保护反应方面发挥着关键作用。最近,使用荧光标记抗原对细胞进行染色,结合 Drop-seq 和 CITE-seq 等测序方法,提供了关于单个 MBC 的特异性、表型和转录组的信息。然而,抗原反应性 MBC 群体的特征描述仍然是评估个体 B 细胞免疫和对抗原暴露反应的重要工具。这可以通过使用基于体外多克隆刺激 MBC 以诱导其分裂和分化为分泌抗体的细胞(ASC)的长期建立的方法来轻松完成。刺激后对 MBC 衍生的 ASC(或分泌的抗体)进行抗原特异性测量,表明前体 MBC 群体的大小。通过分析具有特定结合亲和力和功能的抗原反应性 MBC 衍生抗体,提供有关抗原反应性 MBC 群体特征的其他信息。本文概述了一种简单可靠的策略,用于有效体外 MBC 刺激,并使用 ELISpot 测定作为刺激后的读出,以确定抗原特异性 MBC 群体的大小。讨论了体外刺激技术在 MBC 分析中的其他应用。包括以下方案。 © 2020 威利父子公司基本方案 1:使用未分级的 PBMC 对记忆 B 细胞进行多克隆刺激备选方案 1:使用 96 孔板和 U 形底孔对少量 PBMC 进行刺激基本方案 2:ELISpot 测定法用于计数记忆 B 细胞衍生的抗体分泌细胞。

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