Recombinant renewable polyclonal antibodies

被引:14
|
作者
Ferrara, Fortunato [1 ]
D'Angelo, Sara [1 ]
Gaiotto, Tiziano [1 ]
Naranjo, Leslie [2 ]
Tian, Hongzhao [2 ]
Graeslund, Susanne [3 ]
Dobrovetsky, Elena [3 ]
Hraber, Peter [2 ]
Lund-Johansen, Fridtjof [4 ]
Saragozza, Silvia [5 ]
Sblattero, Daniele [5 ]
Kiss, Csaba [2 ]
Bradbury, Andrew R. M. [2 ]
机构
[1] New Mexico Consortium, Los Alamos, NM USA
[2] Los Alamos Natl Lab, Los Alamos, NM 87545 USA
[3] Univ Toronto, Struct Genom Consortium, Toronto, ON, Canada
[4] Univ Oslo, Oslo, Norway
[5] Univ Piemonte Orientale, Novara, Italy
基金
加拿大创新基金会; 美国国家卫生研究院; 英国惠康基金;
关键词
polyclonal recombinant antibodies; yeast display; phage display; antibody validation; CTBP; C-terminal binding protein; ELISA; enzyme linked immunosorbant assay; HCDR3; Heavy chain complementarity determining region 3; HPA; Human Protein Atlas; scFv; single chain Fv; PrESTs; Protein epitope signature tag; rrpAbs; recombinant renewable polyclonal antibodies; SDS-PAGE; sodium dodecyl sulfate polyacrylamide gel electrophoresis; TEV; tobacco etch virus; SINGLE-CHAIN ANTIBODIES; COMMERCIAL ANTIBODIES; PHYLOGENIES; GENERATION; FRAGMENTS; EVOLUTION; SELECTION; RECEPTOR;
D O I
10.4161/19420862.2015.989047
中图分类号
R-3 [医学研究方法]; R3 [基础医学];
学科分类号
1001 ;
摘要
Only a small fraction of the antibodies in a traditional polyclonal antibody mixture recognize the target of interest, frequently resulting in undesirable polyreactivity. Here, we show that high-quality recombinant polyclonals, in which hundreds of different antibodies are all directed toward a target of interest, can be easily generated in vitro by combining phage and yeast display. We show that, unlike traditional polyclonals, which are limited resources, recombinant polyclonal antibodies can be amplified over one hundred million-fold without losing representation or functionality. Our protocol was tested on 9 different targets to demonstrate how the strategy allows the selective amplification of antibodies directed toward desirable target specific epitopes, such as those found in one protein but not a closely related one, and the elimination of antibodies recognizing common epitopes, without significant loss of diversity. These recombinant renewable polyclonal antibodies are usable in different assays, and can be generated in high throughput. This approach could potentially be used to develop highly specific recombinant renewable antibodies against all human gene products.
引用
收藏
页码:32 / 41
页数:10
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