Preparation of Distinct Ubiquitin Chain Reagents of High Purity and Yield

被引:63
作者
Dong, Ken C. [1 ]
Helgason, Elizabeth [2 ]
Yu, Christine [1 ]
Phu, Lilian [3 ]
Arnott, David P. [3 ]
Bosanac, Ivan [1 ]
Compaan, Deanne M. [1 ]
Huang, Oscar W. [2 ]
Fedorova, Anna V. [2 ]
Kirkpatrick, Donald S. [3 ]
Hymowitz, Sarah G. [1 ]
Dueber, Erin C. [2 ]
机构
[1] Genentech Inc, Dept Biol Struct, San Francisco, CA 94080 USA
[2] Genentech Inc, Dept Early Discovery Biochem, San Francisco, CA 94080 USA
[3] Genentech Inc, Dept Prot Chem, San Francisco, CA 94080 USA
关键词
ANAPHASE-PROMOTING COMPLEX; 63-LINKED POLYUBIQUITIN CHAINS; KAPPA-B ACTIVATION; 26 S PROTEASOME; STRUCTURAL BASIS; K11-LINKED POLYUBIQUITINATION; MULTIUBIQUITIN CHAIN; CONJUGATING ENZYME; RECOGNITION; PROTEIN;
D O I
10.1016/j.str.2011.06.010
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The complexity of protein ubiquitination signals derives largely from the variety of polyubiquitin linkage types that can modify a target protein, each imparting distinct functional consequences. Free ubiquitin chains of uniform linkages and length are important tools in understanding how ubiquitin-binding proteins specifically recognize these different polyubiquitin modifications. While some free ubiquitin chain species are commercially available, mutational analyses and labeling schemes are limited to select, marketed stocks. Furthermore, the multimilligram quantities of material required for detailed biophysical and/or structural studies often makes these reagents cost prohibitive. To address these limitations, we have optimized known methods for the synthesis and purification of linear, K11-, K48-, and K63-linked ubiquitin dimers, trimers, and tetramers on a preparative scale. The high purity and relatively high yield of these proteins readily enables material-intensive experiments and provides flexibility for engineering specialized ubiquitin chain reagents, such as fluorescently labeled chains of discrete lengths.
引用
收藏
页码:1053 / 1063
页数:11
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