Roles of conserved active site residues in the IscS cysteine desulfurase reaction

Yilin Pang; Jing Wang; Xueping Gao; Mengyao Jiang; Lifei Zhu; Feng Liang; Mengxiang Liang; Xiaolin Wu; Xianxian Xu; Xiaojun Ren; Ting Xie; Wu Wang; Qianqian Sun; Xiaojun Xiong; Jianxin Lyu; Jianghui Li; Guoqiang Tan

doi:10.3389/fmicb.2023.1084205

Roles of conserved active site residues in the IscS cysteine desulfurase reaction

Front Microbiol. 2023 Feb 16:14:1084205. doi: 10.3389/fmicb.2023.1084205. eCollection 2023.

Authors

Yilin Pang^{1

2}, Jing Wang¹, Xueping Gao¹, Mengyao Jiang¹, Lifei Zhu¹, Feng Liang^{1

3}, Mengxiang Liang¹, Xiaolin Wu¹, Xianxian Xu¹, Xiaojun Ren^{1

4}, Ting Xie¹, Wu Wang¹, Qianqian Sun¹, Xiaojun Xiong², Jianxin Lyu^{1

4}, Jianghui Li¹, Guoqiang Tan¹

Affiliations

¹ Zhejiang Provincial Key Laboratory of Medical Genetics, Key Laboratory of Laboratory Medicine, Ministry of Education, School of Laboratory Medicine and Life Sciences, Wenzhou Medical University, Wenzhou, Zhejiang, China.
² Hunan Animal Pharmaceutical Company, Hunan Agricultural Group Company, Hunan Agricultural Development & Investment Group Company, Wangcheng Economic and Technological Development Zone, Changsha, Hunan, China.
³ Department of Laboratory Medicine, The First Affiliated Hospital of Wenzhou Medical University, Wenzhou, China.
⁴ People's Hospital of Hangzhou Medical College, Hangzhou, China.

Abstract

Escherichia coli cysteine desulfurase (CD), IscS, modifies basal metabolism by transferring sulphur (S) from L-cysteine to numerous cellular pathways, whereas NFS1, a human CD, is active only in the formation of the [Acp]₂:[ISD11]₂:[NFS1]₂ complex. Despite the accumulation of red-coloured IscS in E. coli cells as a result of the deficiency of accessible iron, as revealed in our previous studies, the mechanism of the potential enzymatic reaction remains unclear. In this study, the N-terminus of IscS was fused with the C-terminus of NFS1, which was reported to be almost fully active as IscS and exhibits a pyridoxal 5'-phosphate (PLP) absorption peak at 395 nm. Moreover, SUMO-EH-IscS exhibited significant growth recovery and NADH-dehydrogenase I activity in the iscS mutant cells. Furthermore, through in vitro and in vivo experiments combined with high-performance liquid chromatography and ultra-performance liquid chromatography-tandem mass spectrometry, it was shown that the new absorption peaks of the IscS H104Q, IscS Q183E, IscS K206A, and IscS K206A&C328S variants at 340 and 350 nm may correspond to the enzyme reaction intermediates, Cys-ketimine and Cys-aldimine, respectively. However, after mutation of the conserved active-site residues, additional absorption peaks at 420 and 430 nm were associated with PLP migration in the active-site pocket. Additionally, the corresponding absorption peaks of Cys-quinonoid, Ala-ketimine, and Ala-aldimine intermediates in IscS were 510, 325, and 345 nm, respectively, as determined by site-directed mutagenesis and substrate/product-binding analyses during the CD reaction process. Notably, red IscS formed in vitro by incubating IscS variants (Q183E and K206A) with excess L-alanine and sulphide under aerobic conditions produced an absorption peak similar to the wild-type IscS, at 510 nm. Interestingly, site-directed mutation of IscS with hydrogen bonds to PLP at Asp180 and Gln183 resulted in a loss of enzymatic activity followed by an absorption peak consistent with NFS1 (420 nm). Furthermore, mutations at Asp180 or Lys206 inhibited the reaction of IscS in vitro with L-cysteine (substrate) and L-alanine (product). These results suggest that the conserved active site residues (His104, Asp180, and Gln183) and their hydrogen bond with PLP in the N-terminus of IscS play a key role in determining whether the L-cysteine substrate can enter the active-site pocket and regulate the enzymatic reaction process. Therefore, our findings provide a framework for evaluating the roles of conserved active-site residues, motifs, and domains in CDs.

Keywords: Cys-aldimine; Cys-ketimine; active site residues; antimicrobial resistance; cysteine desulfurase; pyridoxal 5′-phosphate.