The Structural Role of RPN10 in the 26S Proteasome and an RPN2-Binding Residue on RPN13 Are Functionally Important in Arabidopsis

被引:0
|
作者
Lin, Shih-Yun [1 ]
Lin, Ya-Ling [2 ]
Usharani, Raju [1 ]
Radjacommare, Ramalingam [1 ]
Fu, Hongyong [1 ]
机构
[1] Acad Sinica, Inst Plant & Microbial Biol, Taipei 115, Taiwan
[2] Natl Chung Hsing Univ, Acad Circular Econ, Program Biol & Sustainable Technol, Nantou 540, Taiwan
关键词
RPN10; RPN13; RPN2; UCH1; UCH2; ECM29; PA200; ubiquitin receptor; 26S proteasome; Arabidopsis; SUBSTRATE RECOGNITION FUNCTION; MULTIUBIQUITIN-CHAIN-BINDING; DEUBIQUITINATING ENZYME; REGULATORY PARTICLE; PROTEIN-DEGRADATION; CORE PARTICLE; SUBUNIT; ECM29; ACTIVATION; ARCHITECTURE;
D O I
10.3390/ijms252111650
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 ubiquitin receptors RPN10 and RPN13 harbor multiple activities including ubiquitin binding; however, solid evidence connecting a particular activity to specific in vivo functions is scarce. Through complementation, the ubiquitin-binding site-truncated Arabidopsis RPN10 (N215) rescued the growth defects of rpn10-2, supporting the idea that the ubiquitin-binding ability of RPN10 is dispensable and N215, which harbors a vWA domain, is fully functional. Instead, a structural role played by RPN10 in the 26S proteasomes is likely vital in vivo. A site-specific variant, RPN10-11A, that likely has a destabilized vWA domain could partially rescue the rpn10-2 growth defects and is not integrated into 26S proteasomes. Native polyacrylamide gel electrophoresis and mass spectrometry with rpn10-2 26S proteasomes showed that the loss of RPN10 reduced the abundance of double-capped proteasomes, induced the integration of specific subunit paralogues, and increased the association of ECM29, a well-known factor critical for quality checkpoints by binding and inhibiting aberrant proteasomes. Extensive Y2H and GST-pulldown analyses identified RPN2-binding residues on RPN13 that overlapped with ubiquitin-binding and UCH2-binding sites in the RPN13 C-terminus (246-254). Interestingly, an analysis of homozygous rpn10-2 segregation in a rpn13-1 background harboring RPN13 variants defective for ubiquitin binding and/or RPN2 binding supports the criticality of the RPN13-RPN2 association in vivo.
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页数:30
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