High-Throughput Sorting of the Highest Producing Cell via a Transiently Protein-Anchored System
Author(s) -
KuoHsiang Chuang,
Yuan-Chin Hsieh,
I-Shiuan Chiang,
Chih-Hung Chuang,
Chien-Han Kao,
Ta-Chun Cheng,
YengTseng Wang,
Wen-Wei Lin,
BingMae Chen,
Steve R. Roffler,
Ming-Yii Huang,
TianLu Cheng
Publication year - 2014
Publication title -
plos one
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.99
H-Index - 332
ISSN - 1932-6203
DOI - 10.1371/journal.pone.0102569
Subject(s) - furin , cell sorting , microbiology and biotechnology , cleavage (geology) , membrane protein , transmembrane protein , secretion , chemistry , cell culture , cell , biology , biochemistry , membrane , receptor , enzyme , genetics , paleontology , fracture (geology)
Developing a high-throughput method for the effecient selection of the highest producing cell is very important for the production of recombinant protein drugs. Here, we developed a novel transiently protein-anchored system coupled with fluorescence activated cell sorting (FACS) for the efficient selection of the highest producing cell. A furin cleavage peptide (RAKR) was used to join a human anti-epithelial growth factor antibody (αEGFR Ab) and the extracellular-transmembrane-cytosolic domains of the mouse B7-1 antigen (B7). The furin inhibitor can transiently switch secreted αEGFR Ab into a membrane-anchored form. After cell sorting, the level of membrane αEGFR Ab-RAKR-B7 is proportional to the amount of secreted αEGFR Ab in the medium. We further selected 23 αEGFR Ab expressing cells and demonstrated a high correlation (R 2 = 0.9165) between the secretion level and surface expression levels of αEGFR Ab. These results suggested that the novel transiently protein-anchored system can easily and efficiently select the highest producing cells, reducing the cost for the production of biopharmaceuticals.
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