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Longitudinal Analysis of the Human B Cell Response to Ebola Virus Infection.

Cell. 2019-05; 
DavisCarl W,JacksonKatherine J L,McElroyAnita K,HalfmannPeter,HuangJessica,ChennareddyChakravarthy,PiperAshley E,LeungYvonne,Albari?oCésar G,CrozierIan,EllebedyAli H,SidneyJohn,SetteAlessandro,YuTianwei,NielsenSandra C A,GoffArthur J,SpiropoulouChristina F,SaphireErica Ollman,CavetGuy,KawaokaYoshihiro,MehtaAneesh K,GlassPamela J,BoydScott D,Ahmed
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Codon Optimization Codon optimization and DNA synthesis were performed by GenScript and Gen9. mAb-containing supernatants from transfected expi293 cells were clarified by centrifugation and then incubated with protein A agarose resin (GenScript) in batch format overnight, followed by washing, elution, and buffer exchange into DPBS as described (Smith et al., 2009). Get A Quote

摘要

Ebola virus (EBOV) remains a public health threat. We performed a longitudinal study of B cell responses to EBOV in four survivors of the 2014 West African outbreak. Infection induced lasting EBOV-specific immunoglobulin G (IgG) antibodies, but their subclass composition changed over time, with IgG1 persisting, IgG3 rapidly declining, and IgG4 appearing late. Striking changes occurred in the immunoglobulin repertoire, with massive recruitment of naive B cells that subsequently underwent hypermutation. We characterized a large panel of EBOV glycoprotein-specific monoclonal antibodies (mAbs). Only a small subset of mAbs that bound glycoprotein by ELISA recognized cell-surface glycoprotein. However, th... More

關鍵詞

B cell repertoire,Ebola,IgG subclass,antibody evolution,public clono
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