Balasubramanian Akhila, Prachar Marek, Klaproth Birgit, Copeland Victoria, Justesen Sune, Wen Yi, Siegel Robert W, Malherbe Laurent P
Lilly Research Laboratories, Eli Lilly and Company, Indianapolis, IN, United States.
Lilly Oncology, Eli Lilly and Company, Copenhagen, Denmark.
Front Immunol. 2025 Aug 8;16:1641289. doi: 10.3389/fimmu.2025.1641289. eCollection 2025.
Adeno-associated virus (AAV)-mediated gene therapy is a promising approach to treat genetic disorders, offering advantages such as high transduction efficiency, diverse tissue tropism, and an acceptable safety profile. However, the immunogenicity of AAV vectors, particularly the activation of AAV capsid-specific CD8 T cells, significantly impacts therapeutic efficacy and safety. Capsid-specific T cell responses are currently monitored in the clinic using overlapping peptides, which do not represent the naturally presented capsid immunopeptidome. Our previous work identified the naturally presented peptides of AAV capsids using MHC-associated peptide proteomics (MAPPs).
In this study, we compared overlapping and MAPPs-derived peptides of the AAV9 capsid in their capacity to trigger capsid-specific T cell responses in healthy donor PBMCs.
Both peptide groups induced measurable T cell responses in FluoroSpot assays only after an expansion phase, reflecting the low frequency of circulating capsid-specific T cells in both seropositive and seronegative donors. Surprisingly, overlapping and MAPPs-derived capsid peptides expanded largely distinct T cells that did not cross-react. The T cell response to MAPPs-derived capsid peptides was dominated by capsid-specific CD8 T cells recognizing peptides eluted from HLA Class I, allowing us to identify CD8 T cell capsid epitopes in healthy donors. By screening 13 matrix pools (comprising 41 HLA Class I MAPPs peptides of the AAV9 capsid) in 24 healthy donors using FluoroSpot assays, we identified ten epitopes eliciting IFN-γ release in at least one donor. 9 of the 10 identified epitopes were novel, varied between 9-13 amino acids in length, and displayed strong binding to their predicted HLA binding alleles. Only one of four previously reported capsid CD8 T cell epitopes elicited a response in the tested cohort of healthy donors with diverse HLAs. Remarkably, in two instances where MAPPs peptides of different lengths were presented on HLA Class I, CD8 T cell response was only observed to longer epitopes.
Our results represent the first extensive analysis of the naturally presented peptides of the AAV9 capsid. This work provides strategies to improve the detection of the capsid-specific CD8 T cell response in the clinic and reduce vector immunogenicity through the identification of novel CD8 T cell epitopes.
腺相关病毒(AAV)介导的基因治疗是一种治疗遗传疾病的有前景的方法,具有转导效率高、组织嗜性多样和安全性可接受等优点。然而,AAV载体的免疫原性,特别是AAV衣壳特异性CD8 T细胞的激活,显著影响治疗效果和安全性。目前临床上使用重叠肽监测衣壳特异性T细胞反应,而这些重叠肽并不代表天然呈现的衣壳免疫肽组。我们之前的工作利用与主要组织相容性复合体(MHC)相关的肽组学(MAPPs)鉴定了AAV衣壳的天然呈现肽。
在本研究中,我们比较了AAV9衣壳的重叠肽和MAPPs衍生肽在健康供体外周血单个核细胞(PBMC)中触发衣壳特异性T细胞反应的能力。
仅在扩增阶段后,两组肽在荧光斑点试验中均诱导出可测量的T细胞反应,这反映了血清阳性和血清阴性供体中循环衣壳特异性T细胞的低频性。令人惊讶的是,重叠肽和MAPPs衍生的衣壳肽扩增出的T细胞在很大程度上是不同的,且不发生交叉反应。对MAPPs衍生的衣壳肽的T细胞反应主要由识别从HLA I类洗脱的肽的衣壳特异性CD8 T细胞主导,这使我们能够在健康供体中鉴定出CD8 T细胞衣壳表位。通过在24名健康供体中使用荧光斑点试验筛选13个矩阵库(包含AAV9衣壳的41种HLA I类MAPPs肽),我们鉴定出至少在一名供体中引发γ干扰素释放的10个表位。所鉴定的10个表位中有9个是新的,长度在9 - 13个氨基酸之间,并与其预测的HLA结合等位基因表现出强结合。在之前报道的四个衣壳CD8 T细胞表位中,只有一个在具有不同HLA的健康供体测试队列中引发了反应。值得注意的是,在两种情况下,不同长度的MAPPs肽在HLA I类上呈现时,仅观察到对较长表位的CD8 T细胞反应。
我们的结果代表了对AAV9衣壳天然呈现肽的首次广泛分析。这项工作提供了在临床上改进衣壳特异性CD8 T细胞反应检测以及通过鉴定新的CD8 T细胞表位降低载体免疫原性的策略。
