Creation of genome-wide protein expression libraries using random activation of gene expression

被引:60
作者
Harrington, JJ [1 ]
Sherf, B [1 ]
Rundlett, S [1 ]
Jackson, PD [1 ]
Perry, R [1 ]
Cain, S [1 ]
Leventhal, C [1 ]
Thornton, M [1 ]
Ramachandran, R [1 ]
Whittington, J [1 ]
Lerner, L [1 ]
Costanzo, D [1 ]
McElligott, K [1 ]
Boozer, S [1 ]
Mays, R [1 ]
Smith, E [1 ]
Veloso, N [1 ]
Klika, A [1 ]
Hess, J [1 ]
Cothren, K [1 ]
Lo, K [1 ]
Offenbacher, J [1 ]
Danzig, J [1 ]
Ducar, M [1 ]
机构
[1] Athersys Inc, Cleveland, OH 44115 USA
关键词
D O I
10.1038/88107
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Here we report the use of random activation of gene expression (RAGE) to create genome-wide protein expression libraries. RAGE libraries containing only 5 x 10(6) individual clones were found to express every gene tested, including genes that are normally silent in the parent cell line. Furthermore, endogenous genes were activated at similar frequencies and expressed at similar levels within RAGE libraries created from multiple human cell lines, demonstrating that RAGE libraries are inherently normalized. Pools of RAGE clones were used to isolate 19,547 human gene clusters, similar to 53% of which were novel when tested against public databases of expressed sequence tag (EST) and complementary DNA (cDNA). Isolation of individual clones confirmed that the activated endogenous genes can be expressed at high levels to produce biologically active proteins. The properties of RAGE libraries and RAGE expression clones are well suited for a number of biotechnological applications including gene discovery, protein characterization, drug development, and protein manufacturing.
引用
收藏
页码:440 / 445
页数:6
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