Persulfidation maintains cytosolic G6PDs activity through changing tetrameric structure and competing cysteine sulfur oxidation under salt stress in Arabidopsis and tomato

拟南芥 胞浆 生物化学 化学 拟南芥 氧化应激 四聚体 半胱氨酸 生物物理学 氧化磷酸化 细胞生物学 突变体 生物 基因
作者
Xiaofeng Wang,Cong Shi,Yanfeng Hu,Ying Ma,Yuying Yi,Honglei Jia,Fali Li,Haotian Sun,Li Tian,Xiuyu Wang,Tianjinhong Li,Jisheng Li
出处
期刊:New Phytologist [Wiley]
卷期号:240 (2): 626-643 被引量:12
标识
DOI:10.1111/nph.19188
摘要

Summary Glucose‐6‐phosphate dehydrogenases (G6PDs) are essential regulators of cellular redox. Hydrogen sulfide (H 2 S) is a small gasotransmitter that improves plant adaptation to stress; however, its role in regulating G6PD oligomerization to resist oxidative stress remains unknown in plants. Persulfidation of cytosolic G6PDs was analyzed by mass spectrometry (MS). The structural change model of AtG6PD6 homooligomer was built by chemical cross‐linking coupled with mass spectrometry (CXMS). We isolated AtG6PD6 C159A and SlG6PDC C155A transgenic lines to confirm the in vivo function of persulfidated sites with the g6pd5 , 6 background. Persulfidation occurs at Arabidopsis G6PD6 Cystine (Cys)159 and tomato G6PDC Cys155, leading to alterations of spatial distance between lysine (K)491‐K475 from 42.0 Å to 10.3 Å within the G6PD tetramer. The structural alteration occurs in the structural NADP + binding domain, which governs the stability of G6PD homooligomer. Persulfidation enhances G6PD oligomerization, thereby increasing substrate affinity. Under high salt stress, cytosolic G6PDs activity was inhibited due to oxidative modifications. Persulfidation protects these specific sites and prevents oxidative damage. In summary, H 2 S‐mediated persulfidation promotes cytosolic G6PD activity by altering homotetrameric structure. The cytosolic G6PD adaptive regulation with two kinds of protein modifications at the atomic and molecular levels is critical for the cellular stress response.
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