Sawitri Widhi Dyah, Afidah Siti Nurul, Nakagawa Atsushi, Hase Toshiharu, Sugiharto Bambang
Center for Development of Advanced Science and Technology (CDAST), University of Jember, Jl. Kalimantan 37, Jember, 68121, Indonesia.
Postgraduate Program in Biotechnology, Jember University, J1. Kalimantan 37, Jember, 68121, Indonesia.
Biophys Rev. 2018 Apr;10(2):293-298. doi: 10.1007/s12551-017-0360-9. Epub 2017 Dec 8.
Sucrose phosphate synthase (SPS) is believed to be the key enzyme for controlling the biosynthesis of sucrose. SPSs consist of a functional glycosyltransferase domain that shares conserved residues with the glycosyltransferase domain of sucrose biosynthesis-related protein. The formation of sucrose-6-phosphate is catalyzed by SPS with the transfer of a glycosyl group of uridine diphosphate glucose (UDP-G) as an activated donor sugar to a fructose-6-phosphate as a sugar acceptor. However, understanding of the mechanism of catalytic and substrate binding in SPS is very limited. Based on amino acid sequence alignments with several enzymes that belong to the glycosyltransferase family, the UDP-G binding sites that might be critical for catalytic mechanism were identified. Here, we report that single point mutation of R496, D498, and V570 located in the proposed UDP-G binding site led to less active or complete loss of enzyme activity. Through structure-based site-directed mutagenesis and biochemical studies, the results indicated that these residues contribute to the catalytic activity of plant SPS. Moreover, understanding of the UDP-G binding site provides an insight into new strategies for enzyme engineering and redesigning a catalytic mechanism for UDP.
蔗糖磷酸合酶(SPS)被认为是控制蔗糖生物合成的关键酶。SPS由一个功能性糖基转移酶结构域组成,该结构域与蔗糖生物合成相关蛋白的糖基转移酶结构域具有保守的残基。蔗糖磷酸合酶催化尿苷二磷酸葡萄糖(UDP-G)的糖基作为活化供体糖转移到果糖-6-磷酸作为糖受体,从而形成蔗糖-6-磷酸。然而,对SPS催化和底物结合机制的了解非常有限。基于与属于糖基转移酶家族的几种酶的氨基酸序列比对,确定了可能对催化机制至关重要的UDP-G结合位点。在此,我们报告位于拟UDP-G结合位点的R496、D498和V570单点突变导致酶活性降低或完全丧失。通过基于结构的定点诱变和生化研究,结果表明这些残基有助于植物SPS的催化活性。此外,对UDP-G结合位点的了解为酶工程和重新设计UDP催化机制提供了新策略。