Profiling immunoglobulin repertoires across multiple human tissues by RNA Sequencing

Mangul, Serghei; Mandric, Igor; Yang, Haiou; Strauli, Nicolas; Montoya, Dennis; Rotman, Jeremy; Wey, Will Van Der; Ronas, Jiem R.; Statz, Benjamin; Yao, Douglas; Zelikovsky, Alexander; Spreafico, Roberto; Shifman, Sagiv; Zaitlen, Noah; Rossetti, Maura; Ansel, K. Mark; Eskin, Eleazar

doi:10.1101/089235

Cited by 9 publications

(15 citation statements)

References 28 publications

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“…To generate the BCR-Seq dataset, we have used Immunoglobulin heavy chain (IGH) transcripts. To generate the TCR-Seq dataset, we have used T cell receptor alpha chain (TCRA) 28 . For both BCR-Seq and TCR-Seq we generated samples with read length between 50 and 100bp.…”

Section: Simulated Datasets Generationmentioning

confidence: 99%

Benchmarking of computational error-correction methods for next-generation sequencing data

Mitchell

Mandric

Martin

et al. 2019

Preprint

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Recent advancements in next-generation sequencing have rapidly improved our ability to study genomic material at an unprecedented scale. Despite substantial improvements in sequencing technologies, the errors present in the data still risk confounding downstream analysis and limiting the applicability of sequencing technologies in clinical tools. Computational error-correction promises to eliminate sequencing errors, but the relative performance of error correction algorithms remains unknown. In this paper, we evaluate the ability of error-correction algorithms to fix errors across different types of datasets that contain various level of heterogeneity. We highlight the advantages and limitations of computational error correction techniques across different domains of biology, including immunogenomics and virology. To demonstrate the efficacy of our technique, w e applied the UMI-based high-fidelity sequencing protocol to eliminate sequencing errors from both simulated data and the raw reads. We then performed a realistic evaluation of error correction methods. We find that method performance varies substantially across different types of datasets, with no single method performing best on all types of examined data. Finally, we also identified the techniques that offer a good balance between precision and sensitivity.

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Section: Simulated Datasets Generationmentioning

confidence: 99%

Benchmarking of computational error-correction methods for next-generation sequencing data

Mitchell

Mandric

Martin

et al. 2019

Preprint

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“…8A, left). The presence of ADVAX clonotypes was then explored in a second HD dataset reported by S. Mangul and colleagues, and consisting exclusively of public TCR clonotypes (41). The public clonotypes were extracted from RNA-Seq data generated by the Genotype-Tissue Expression Consortium, using samples from 544 individuals, and based on the reconstruction of approximately 200,000 TCR CDR3 sequences.…”

Section: Resultsmentioning

confidence: 99%

“…More than one third of the Gag293-specific TRAV24 clonotypes from vaccinees were present in the dataset reported by Heather et al (40), and half of those were also present in an independently obtained public clonotype dataset reported by Mangul. et al (41). Multiple Gag293-specific TRAV24 clonotypes could be detected in the healthy repertoire at frequencies above 10 −5 , which is in the high range of T cell precursor frequencies estimated for HIV-derived CD4 epitopes (39, 45, 46).…”

Section: Discussionmentioning

confidence: 98%

“…Left: % found in a dataset of 541,401 TRA clonotypes and 693,571 TRB clonotypes from healthy donors (HD) (40); Right: % found in a dataset of 4,406 TRA public clonotypes and 3,101 TRB public clonotypes from healthy donors (HD) (41); The percentage of TRAV29 (white bar), TRAV24 (black bar), and TRBV2 (grey bar) Gag293-specific clonotypes found at least once in the HD repertoires is reported.…”

Section: Figurementioning

confidence: 99%

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DNA Vaccination by Electroporation Amplifies Broadly Cross-Restricted Public TCR Clonotypes Shared with HIV Controllers

Mukhopadhyay

Galperin

Patgaonkar

et al. 2017

The Journal of Immunology

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Rare patients who spontaneously control HIV replication provide a useful model to inform HIV vaccine development. HIV controllers develop particularly efficient antiviral CD4+ T cell responses mediated by shared high-affinity TCRs. To determine whether the candidate DNA vaccine ADVAX could induce similar responses, we analyzed Gag-specific primary CD4+ T cells from healthy volunteers who received ADVAX DNA by electroporation. Vaccinated volunteers had an immunodominant response to the Gag293 epitope with a functional avidity intermediate between that of controllers and treated patients. The TCR repertoire of Gag293-specific CD4+ T cells proved highly biased, with a predominant usage of the TRBV2 gene in vaccinees as well as controllers. TRAV gene usage was more diverse, with the dominance of TRAV29 over TRAV24 genes in vaccinees, while TRAV24 predominated in controllers. Sequence analysis revealed an unexpected degree of overlap between the specific repertoires of vaccinees and controllers, with the sharing of TRAV24 and TRBV2 public motifs (>30%) and of public clonotypes characteristic of high-affinity TCRs. MHC-II tetramer binding revealed a broad HLA-DR cross-restriction, explaining how Gag293-specific public clonotypes could be selected in individuals with diverse genetic backgrounds. TRAV29 clonotypes also proved cross-restricted, but conferred responses of lower functional avidity upon TCR transfer. In conclusion, DNA vaccination by electroporation primed for TCR clonotypes that were associated with HIV control, highlighting the potential of this vaccine delivery method. This study provides the first proof-of-concept that clonotypic analysis may be used as a tool to monitor the quality of vaccine-induced responses and modulate these towards “controller-like” responses.

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“…The original protocols could only sequence unpaired single chains of these receptors; recent protocols make it possible to sequence paired chains [176,177] to give a complete picture of the receptor repertoire. New algorithms allow repertoire sequences to be extracted from DNA-seq or RNA-seq data from bulk tissue [178][179][180] or single cells [181] .…”

Section: Pathway Analysismentioning

confidence: 99%

Informatics for Cancer Immunotherapy

Hammerbacher

Charen

2017

Preprint

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Abstract:The rapid development of immunomodulatory cancer therapies has led to a concurrent increase in the application of informatics techniques to the analysis of tumors, the tumor microenvironment, and measures of systemic immunity. In this review, the use of tumors to gather genetic and expression data will first be explored. Next, techniques to assess tumor immunity are reviewed, including HLA status, predicted neoantigens, immune microenvironment deconvolution and T-cell receptor (TCR) sequencing. Attempts to integrate these data are in early stages of development and are discussed next. Finally, we review the application of these informatics strategies to therapy development, with a focus on vaccines, adoptive cell transfer, and checkpoint blockade therapies.

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Profiling immunoglobulin repertoires across multiple human tissues by RNA Sequencing

Cited by 9 publications

References 28 publications

Benchmarking of computational error-correction methods for next-generation sequencing data

Benchmarking of computational error-correction methods for next-generation sequencing data

DNA Vaccination by Electroporation Amplifies Broadly Cross-Restricted Public TCR Clonotypes Shared with HIV Controllers

Informatics for Cancer Immunotherapy

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