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    High-throughput sequencing of the paired human immunoglobulin heavy and light chain repertoire.

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    Varadarajan_2014_HighthroughputsequencingAM.pdf (295.5Kb)
    Date
    2014-02
    Author
    DeKosky, Brandon J.
    Ippolito, Gregory C.
    Deschner, Ryan P.
    Lavinder, Jason J.
    Wine, Yariv
    Rawlings, Brandon M.
    Varadarajan, Navin
    Giesecke, Claudia
    Dörner, Thomas
    Andrews, Sarah F.
    Wilson, Patrick C.
    Hunicke-Smith, Scott P.
    Willson,Grant C.
    Ellington, Andrew D.
    Georgiou, George
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    Abstract
    Each B-cell receptor consists of a pair of heavy and light chains. High-throughput sequencing can identify large numbers of heavy- and light-chain variable regions (VH and VL) in a given B-cell repertoire, but information about endogenous pairing of heavy and light chains is lost after bulk lysis of B-cell populations. Here we describe a way to retain this pairing information. In our approach, single B cells (>5 × 104 capacity per experiment) are deposited in a high-density microwell plate (125 pl/well) and lysed in situ. mRNA is then captured on magnetic beads, reverse transcribed and amplified by emulsion VH:VL linkage PCR. The linked transcripts are analyzed by Illumina high-throughput sequencing. We validated the fidelity of VH:VL pairs identified by this approach and used the method to sequence the repertoire of three human cell subsets-peripheral blood IgG+ B cells, peripheral plasmablasts isolated after tetanus toxoid immunization and memory B cells isolated after seasonal influenza vaccination
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    https://hdl.handle.net/10657/6195
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