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不同的研究人员在两种体外细胞因子检测方法中均观察到 TGN1412 类似物的水相和固相形式能够引起阳性反应。

Different players generate positive responses in two in vitro cytokine assay formats with aqueous and immobilized TGN1412 analog.

机构信息

Research Division, Chugai Pharmaceutical Co., Ltd., 1-135 Komakado, Gotemba, Shizuoka, 412-8513, Japan.

Research Division, Chugai Pharmaceutical Co., Ltd., 1-135 Komakado, Gotemba, Shizuoka, 412-8513, Japan.

出版信息

Biochem Biophys Res Commun. 2018 Jul 7;502(1):91-97. doi: 10.1016/j.bbrc.2018.05.125. Epub 2018 May 24.

DOI:10.1016/j.bbrc.2018.05.125
PMID:29787754
Abstract

To detect potential risk of severe cytokine release syndrome, in vitro assay formats with human cells have been developed. The two major testing platforms are a combination of whole blood with aqueous-phase test articles (whole blood cytokine assay, WBCA) and peripheral blood mononuclear cells with solid-phase articles (PBMC assay). Significant induction of cytokines was seen in both assays after treatment with a widely used control agent, TGN1412 or its analog CD28SA, but the WBCA cytokine profile differed from what was expected from clinical experience. In the WBCA, potential risk of CD28SA was detected by elevation of IL-8 whereas IL-2, a key cytokine after stimulation of CD28, was not induced in approximately 40% of donor samples. Therefore, further mechanistic understanding of the different responses in the in vitro assay was needed. In this study of donor samples treated with CD28SA, we compared the induction of cytokines and identified the cytokine-producing cells in the two assays. IL-2 was markedly elevated in all the donors in the PBMC assay but only in 1 of 3 donors in the WBCA. IL-8, the most sensitive biomarker in the WBCA, was produced by monocytes and granulocytes. T cells, the most relevant player in the PBMC assay with CD28SA, did not contribute to the positive response seen in two donors in the WBCA, which suggests that different players caused the positive cytokine responses to CD28SA in the two assays.

摘要

为了检测潜在的严重细胞因子释放综合征风险,已经开发出了使用人类细胞的体外检测方法。主要的两个检测平台是全血与水相测试物的组合(全血细胞因子检测,WBCA)和外周血单核细胞与固相测试物的组合(PBMC 检测)。在使用广泛使用的对照剂 TGN1412 或其类似物 CD28SA 进行处理后,这两种检测都显著诱导了细胞因子的产生,但 WBCA 的细胞因子谱与临床经验预期的不同。在 WBCA 中,通过升高 IL-8 检测到 CD28SA 的潜在风险,而在大约 40%的供体样本中,刺激 CD28 后关键细胞因子 IL-2 并未被诱导。因此,需要进一步深入了解体外检测中不同的反应机制。在这项针对 CD28SA 处理的供体样本的研究中,我们比较了两种检测中细胞因子的诱导,并鉴定了产生细胞因子的细胞。在 PBMC 检测中,所有供体的 IL-2 都显著升高,但在 WBCA 中只有 3 个供体中的 1 个升高。在 WBCA 中作为最敏感的生物标志物的 IL-8 是由单核细胞和粒细胞产生的。在 PBMC 检测中与 CD28SA 最相关的 T 细胞并没有导致 WBCA 中 2 个供体的阳性反应,这表明在两种检测中,不同的细胞因子导致了对 CD28SA 的阳性细胞因子反应。

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