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A reproducible method for the enumeration of functional (cytokine producing) versus non-functional peptide-specific cytotoxic T lymphocytes in human peripheral blood

机译:枚举人类外周血中功能性(细胞因子产生)与非功能性肽特异性细胞毒性T淋巴细胞的可复制方法

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摘要

One of the most difficult laboratory challenges in the field of therapeutic cancer vaccines has been the development of uncomplicated/reproducible methods for the quantification of vaccine immunization efficacy in peripheral blood of cancer patients. Existing methods are limited by lack of functional information (tetramers), difficulties with standardization/reproducibility [enzyme-linked immunosorbent spot (ELISPOT)] and reliance on endogenous (sample-specific) antigen presentation (cytokine flow cytometry). Herein we present a reproducible method utilizing an artificial antigen-presenting cell platform for flow cytometry-based quantification of the frequency and activation status of peptide-specific cytotoxic T lymphocytes. The methodology [currently presented for cytomegalovirus human leucocyte antigen (HLA)-A2 cognant peptide antigens] allows simultaneous ex vivo quantification of activated (cytokine-producing) and inactive tetramer-positive T cells following HLA class I/peptide/CD28 stimulation independent of endogenous antigen presentation. The simplicity and reliability of the assay provide for high-throughput applications and automation. The utility and application of this method are discussed.
机译:治疗性癌症疫苗领域最困难的实验室挑战之一是开发用于量化癌症患者外周血中疫苗免疫效力的简单/可重复方法。现有方法受限于功能信息(四聚体)的缺乏,标准化/可重复性[酶联免疫吸附点(ELISPOT)]的困难以及对内源性(样品特异性)抗原呈递的依赖(细胞因子流式细胞仪)。本文中,我们提出了一种可重复使用的方法,该方法利用人工抗原呈递细胞平台基于流式细胞仪对肽特异性细胞毒性T淋巴细胞的频率和激活状态进行定量。该方法[当前针对巨细胞病毒人白细胞抗原(HLA)-A2同源肽抗原提出的方法]允许在HLA I类/肽/ CD28刺激后独立于内源性同时对活化的(产生细胞因子的)和失活的四聚体阳性T细胞进行离体定量。抗原呈递。测定的简单性和可靠性为高通量应用和自动化提供了条件。讨论了该方法的实用性和应用。

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