Full-Length Immune Repertoire Reconstruction and Profiling at the Transcriptome Level Using Long-Read Sequencing

被引:0
|
作者
Luo, Xuanmei [1 ,2 ]
Zhang, Lili [1 ]
Li, Yifei [1 ]
Li, Chang [1 ]
Sun, Gaoyuan [1 ]
Zhang, Chunli [3 ]
Fu, Yu [4 ]
Lv, Haozhen [5 ]
Liu, Ming [5 ]
Cui, Hongyuan [6 ]
Cai, Dali [7 ]
Zou, Lihui [2 ]
Ma, Jie [8 ]
Xiao, Fei [1 ,2 ]
机构
[1] Chinese Acad Med Sci, Beijing Hosp, Natl Ctr Gerontol, Natl Hlth Commiss,Inst Geriatr Med,Clin Biobank, Beijing, Peoples R China
[2] Chinese Acad Med Sci, Beijing Hosp, Key Lab Geriatr, Inst Geriatr Med,Beijing Inst Geriatr,Natl Ctr Ge, Beijing, Peoples R China
[3] Chinese Acad Med Sci, Beijing Hosp, Dept Hematol, Natl Ctr Gerontol,Natl Hlth Commiss,Inst Geriatr M, Beijing, Peoples R China
[4] Chinese Acad Med Sci, Beijing Hosp, Dept Dermatol, Natl Ctr Gerontol,Natl Hlth Commiss,Inst Geriatr M, Beijing, Peoples R China
[5] Chinese Acad Med Sci, Beijing Hosp, Dept Urol, Natl Ctr Gerontol,Natl Hlth Commiss,Inst Geriatr M, Beijing, Peoples R China
[6] Chinese Acad Med Sci, Beijing Hosp, Dept Gen Surg, Natl Ctr Gerontol,Inst Geriatr Med, Beijing, Peoples R China
[7] China Med Univ, Hosp 1, Dept Hematol, Shenyang, Liaoning, Peoples R China
[8] Chinese Acad Med Sci, Beijing Hosp, Ctr Biotherapy, Natl Ctr Gerontol,Inst Geriatr Med, Beijing, Peoples R China
关键词
D O I
10.1093/clinchem/hvae138
中图分类号
R446 [实验室诊断]; R-33 [实验医学、医学实验];
学科分类号
1001 ;
摘要
Background: Due to the diversity of the immune repertoire (IR), reconstructing full-length IR using traditional short-read sequencing has proven challenging. Methods: A full-length IR sequencing (FLIRseq) work flow was developed with linear rolling circle amplification and nanopore sequencing. Its accuracy and quantification ability were verified by plasmid mixtures and commercial B-cell receptor/T-cell receptor sequencing (BCR/TCR-seq) based on short reads. IRs in tissues and the peripheral blood from 8 patients with acute lymphoblastic leukemia, 3 patients with allergic diseases, 4 patients with psoriasis, and 5 patients with prostate cancer were analyzed using FLIRseq. Results: FLIRseq reads had lower mismatch rates and gap rates, and higher identify rates than nanopore reads (all P < 2.2 x -16). The relative quantification of components by FLIRseq was consistent with the actual quantification (P > 0.05). FLIRseq had superiority over BCR/TCR-seq, providing the long complementarity-determining region 3, B-cell isotype, and the rarely used V gene sequence. FLIRseq observed an increase in clonotype diversity (P < 0.05) and a decrease in the percentage of abnormal BCRs/TCRs in patients with leukemia in remission. For patients with allergic diseases or psoriasis, FLIRseq provided direct insights into V(D)J recombination and specific immunoglobulin classes. Compared with that in prostate cancer tissues, the full-length V segment of the biased T-cell receptor beta chain from lymphocytes in psoriatic tissues showed a more consistent AlphaFold2-predicted protein structure (P < 0.05). Conclusions: FLIRseq enables unbiased and comprehensive analyses of direct V(D)J recombination and immunoglobulin classes, thereby contributing to characterizing pathogenic mechanisms, monitoring minimal residual disease, and customizing adoptive cell therapy.
引用
收藏
页码:274 / 285
页数:12
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