Nuffield Department of Medicine, University of Oxford, Oxford, United Kingdom.
Nuffield Department of Medicine, Target Discovery Institute, University of Oxford, Oxford, United Kingdom.
Front Immunol. 2018 Apr 27;9:912. doi: 10.3389/fimmu.2018.00912. eCollection 2018.
Elucidation of novel peptides presented by human leukocyte antigen (HLA) class I alleles by immunopeptidomics constitutes a powerful approach that can inform the rational design of CD8 T cell inducing vaccines to control infection with pathogens such as human immunodeficiency virus type 1 (HIV-1) or to combat tumors. Recent advances in the sensitivity of liquid chromatography tandem mass spectrometry instrumentation have facilitated the discovery of thousands of natural HLA-restricted peptides in a single measurement. However, the extent of contamination of class I-bound peptides identified using HLA immunoprecipitation (IP)-based immunopeptidomics approaches with peptides from other sources has not previously been evaluated in depth. Here, we investigated the specificity of the IP-based immunopeptidomics methodology using HLA class I- or II-deficient cell lines and membrane protein-specific antibody IPs. We demonstrate that the 721.221 B lymphoblastoid cell line, widely regarded to be HLA class Ia-deficient, actually expresses and presents peptides on HLA-C*01:02. Using this cell line and the C8166 (HLA class I- and II-expressing) cell line, we show that some HLA class II-bound peptides were co-purified non-specifically during HLA class I and membrane protein IPs. Furthermore, IPs of "irrelevant" membrane proteins from HIV-1-infected HLA class I- and/or II-expressing cells revealed that unusually long HIV-1-derived peptides previously reported by us and other immunopeptidomics studies as potentially novel CD8 T cell epitopes were non-specifically co-isolated, and so constitute a source of contamination in HLA class I IPs. For example, a 16-mer (FLGKIWPSYKGRPGNF), which was detected in all samples studied represents the full p1 segment of the abundant intracellular or virion-associated proteolytically-processed HIV-1 Gag protein. This result is of importance, as these long co-purified HIV-1 Gag peptides may not elicit CD8 T cell responses when incorporated into candidate vaccines. These results have wider implications for HLA epitope discovery from abundant or membrane-associated antigens by immunopeptidomics in the context of infectious diseases, cancer, and autoimmunity.
通过免疫肽组学阐明人类白细胞抗原 (HLA) Ⅰ类等位基因呈递的新型肽,是一种强有力的方法,可以为理性设计诱导 CD8 T 细胞的疫苗提供信息,以控制人类免疫缺陷病毒 1 (HIV-1) 等病原体的感染或对抗肿瘤。液相色谱串联质谱仪器灵敏度的最新进展促进了在单次测量中发现数千种天然 HLA 限制肽。然而,以前尚未深入评估使用 HLA 免疫沉淀 (IP)-基于免疫肽组学方法鉴定的 I 类结合肽与其他来源肽的污染程度。在这里,我们使用 HLA I 类或 II 类缺陷细胞系和膜蛋白特异性抗体 IP 研究了基于 IP 的免疫肽组学方法的特异性。我们证明,广泛认为 HLA 类 Ia 缺陷的 721.221 B 淋巴母细胞系实际上表达并呈递 HLA-C*01:02 上的肽。使用该细胞系和 C8166(表达 HLA I 类和 II 类)细胞系,我们表明在 HLA I 类和膜蛋白 IP 期间,一些 HLA II 类结合肽被非特异性共纯化。此外,来自 HIV-1 感染的 HLA I 类和/或 II 类表达细胞的“无关”膜蛋白的 IP 表明,我们和其他免疫肽组学研究先前报道的异常长的 HIV-1 衍生肽作为潜在的新型 CD8 T 细胞表位被非特异性共分离,因此是 HLA I IP 中的污染来源。例如,在所有研究的样本中都检测到的 16 聚体(FLGKIWPSYKGRPGNF)代表丰富的细胞内或病毒相关的蛋白水解加工的 HIV-1 Gag 蛋白的完整 p1 片段。这个结果很重要,因为当这些长的共纯化的 HIV-1 Gag 肽被纳入候选疫苗时,它们可能不会引发 CD8 T 细胞反应。这些结果对于在传染病、癌症和自身免疫的情况下,通过免疫肽组学从丰富或膜相关抗原中发现 HLA 表位具有更广泛的意义。
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