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在铁硫簇组装过程中硫从IscS转移至IscU。

Transfer of sulfur from IscS to IscU during Fe/S cluster assembly.

作者信息

Urbina H D, Silberg J J, Hoff K G, Vickery L E

机构信息

Department of Physiology, University of California, Irvine, California 92697, USA.

出版信息

J Biol Chem. 2001 Nov 30;276(48):44521-6. doi: 10.1074/jbc.M106907200. Epub 2001 Sep 27.

DOI:10.1074/jbc.M106907200
PMID:11577100
Abstract

The cysteine desulfurase enzymes NifS and IscS provide sulfur for the biosynthesis of Fe/S proteins. NifU and IscU have been proposed to serve as template or scaffold proteins in the initial Fe/S cluster assembly events, but the mechanism of sulfur transfer from NifS or IscS to NifU or IscU has not been elucidated. We have employed [(35)S]cysteine radiotracer studies to monitor sulfur transfer between IscS and IscU from Escherichia coli and have used direct binding measurements to investigate interactions between the proteins. IscS catalyzed transfer of (35)S from [(35)S]cysteine to IscU in the absence of additional thiol reagents, suggesting that transfer can occur directly and without involvement of an intermediate carrier. Surface plasmon resonance studies and isothermal titration calorimetry measurements further revealed that IscU binds to IscS with high affinity (K(d) approximately 2 microm) in support of a direct transfer mechanism. Transfer was inhibited by treatment of IscU with iodoacetamide, and (35)S was released by reducing reagents, suggesting that transfer of persulfide sulfur occurs to cysteinyl groups of IscU. A deletion mutant of IscS lacking C-terminal residues 376-413 (IscSDelta376-413) displayed cysteine desulfurase activity similar to the full-length protein but exhibited lower binding affinity for IscU, decreased ability to transfer (35)S to IscU, and reduced activity in assays of Fe/S cluster assembly on IscU. The findings with IscSDelta376-413 provide additional support for a mechanism of sulfur transfer involving a direct interaction between IscS and IscU and suggest that the C-terminal region of IscS may be important for binding IscU.

摘要

半胱氨酸脱硫酶NifS和IscS为铁硫蛋白的生物合成提供硫。有人提出NifU和IscU在最初的铁硫簇组装过程中作为模板或支架蛋白,但从NifS或IscS到NifU或IscU的硫转移机制尚未阐明。我们利用[³⁵S]半胱氨酸放射性示踪研究来监测大肠杆菌中IscS和IscU之间的硫转移,并使用直接结合测量来研究蛋白质之间的相互作用。在没有额外硫醇试剂的情况下,IscS催化[³⁵S]半胱氨酸中的³⁵S转移到IscU,这表明转移可以直接发生,无需中间载体参与。表面等离子体共振研究和等温滴定量热法测量进一步表明,IscU以高亲和力(解离常数Kd约为2微摩尔)与IscS结合,支持直接转移机制。用碘乙酰胺处理IscU可抑制转移,还原试剂可释放³⁵S,这表明过硫化物硫转移到IscU的半胱氨酰基团上。缺少C末端残基376 - 413的IscS缺失突变体(IscSDelta376 - 413)表现出与全长蛋白相似的半胱氨酸脱硫酶活性,但对IscU的结合亲和力较低,将³⁵S转移到IscU的能力降低,并且在IscU上进行铁硫簇组装测定时活性降低。IscSDelta376 - 413的研究结果为涉及IscS和IscU直接相互作用的硫转移机制提供了额外支持,并表明IscS的C末端区域可能对结合IscU很重要。

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