Distinct 3D Architecture and Dynamics of the Human HtrA2(Omi) Protease and Its Mutated Variants

被引:10
|
作者
Gieldon, Artur [1 ]
Zurawa-Janicka, Dorota [2 ]
Jarzab, Miroslaw [2 ]
Wenta, Tomasz [2 ]
Golik, Przemyslaw [3 ]
Dubin, Grzegorz [3 ,4 ]
Lipinska, Barbara [2 ]
Ciarkowski, Jerzy [1 ]
机构
[1] Univ Gdansk, Fac Chem, Wita Stwosza 63, PL-80308 Gdansk, Poland
[2] Univ Gdansk, Dept Biochem, Fac Biol, PL-80308 Gdansk, Poland
[3] Jagiellonian Univ, Fac Biochem Biophys & Biotechnol, Gronostajowa 7, PL-30387 Krakow, Poland
[4] Malopolska Ctr Biotechnol, Ul Gronostajowa 7A, PL-30387 Krakow, Poland
来源
PLOS ONE | 2016年 / 11卷 / 08期
关键词
MITOCHONDRIAL QUALITY-CONTROL; SERINE-PROTEASE; CRYSTAL-STRUCTURE; HTRA-FAMILY; PARKINSONS-DISEASE; MOLECULAR-DYNAMICS; STRUCTURAL BASIS; STRESS SENSOR; ACTIVATION; DOMAIN;
D O I
10.1371/journal.pone.0161526
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
HtrA2(Omi) protease controls protein quality in mitochondria and plays a major role in apoptosis. Its HtrA2(S306A) mutant (with the catalytic serine routinely disabled for an X-ray study to avoid self-degradation) is a homotrimer whose subunits contain the serine protease domain (PD) and the regulatory PDZ domain. In the inactive state, a tight inter-domain interface limits penetration of both PDZ-activating ligands and PD substrates into their respective target sites. We successfully crystalized HtrA2(V226K/S306A), whose active counterpart HtrA2(V226K) has had higher proteolytic activity, suggesting higher propensity to opening the PD-PDZ interface than that of the wild type HtrA2. Yet, the crystal structure revealed the HtrA2(V226K/S306A) architecture typical of the inactive protein. To get a consistent interpretation of crystallographic data in the light of kinetic results, we employed molecular dynamics (MD). V325D inactivating mutant was used as a reference. Our simulations demonstrated that upon binding of a specific peptide ligand NH2-GWTMFWV-COOH, the PDZ domains open more dynamically in the wild type protease compared to the V226K mutant, whereas the movement is not observed in the V325D mutant. The movement relies on a PDZ vs. PD rotation which opens the PD-PDZ interface in a lid-like (budding flower-like in trimer) fashion. The noncovalent hinges A and B are provided by two clusters of interfacing residues, harboring V325D and V226K in the C- and N-terminal PD barrels, respectively. The opening of the subunit interfaces progresses in a sequential manner during the 50 ns MD simulation. In the systems without the ligand only minor PDZ shifts relative to PD are observed, but the interface does not open. Further activation-associated events, e.g. PDZ-L3 positional swap seen in any active HtrA protein (vs. HtrA2), were not observed. In summary, this study provides hints on the mechanism of activation of wtHtrA2, the dynamics of the inactive HtrA2(V325D), but does not allow to explain an increased activity of HtrA2(V226K).
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页数:19
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