Structural-Functional Correlations between Unique N-terminal Region and C-terminal Conserved Motif in Short-chain cis-Prenyltransferase from Tomato

被引:0
|
作者
Imaizumi, Riki [1 ]
Matsuura, Hiroaki [2 ]
Yanai, Taro [1 ]
Takeshita, Kohei [2 ]
Misawa, Shuto [1 ]
Yamaguchi, Haruhiko [3 ]
Sakai, Naoki [2 ]
Miyagi-Inoue, Yukino [3 ]
Suenaga-Hiromori, Miki [4 ]
Waki, Toshiyuki [4 ]
Kataoka, Kunishige [1 ]
Nakayama, Toru [4 ]
Yamamoto, Masaki [2 ]
Takahashi, Seiji [4 ]
Yamashita, Satoshi [1 ]
机构
[1] Kanazawa Univ, Grad Sch Nat Sci & Technol, Dept Mat Chem, Kanazawa 9201192, Japan
[2] RIKEN, SPring 8 Ctr, Sayo, Hyogo 6795148, Japan
[3] Sumitomo Rubber Ind Ltd, Kobe, Japan
[4] Tohoku Univ, Grad Sch Engn, Sendai, Miyagi 9808579, Japan
关键词
cis-prenyltransferase; isoprenoid; neryl diphosphate; disulfide bond; UNDECAPRENYL-PYROPHOSPHATE SYNTHASE; CRYSTAL-STRUCTURE; RXG MOTIF; DIPHOSPHATE; BIOSYNTHESIS; MECHANISM; RECEPTOR; SUBUNIT;
D O I
10.1002/cbic.202300796
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Neryl diphosphate (C-10) synthase (NDPS1), a homodimeric soluble cis-prenyltransferase from tomato, contains four disulfide bonds, including two inter-subunit S-S bonds in the N-terminal region. Mutagenesis studies demonstrated that the S-S bond formation affects not only the stability of the dimer but also the catalytic efficiency of NDPS1. Structural polymorphs in the crystal structures of NDPS1 complexed with its substrate and substrate analog were identified by employing massive data collections and hierarchical clustering analysis. Heterogeneity of the C-terminal region, including the conserved RXG motifs, was observed in addition to the polymorphs of the binding mode of the ligands. One of the RXG motifs covers the active site with an elongated random coil when the ligands are well-ordered. Conversely, the other RXG motif was located away from the active site with a helical structure. The heterogeneous C-terminal regions suggest alternating structural transitions of the RXG motifs that result in closed and open states of the active sites. Site-directed mutagenesis studies demonstrated that the conserved glycine residue cannot be replaced. We propose that the putative structural transitions of the order/disorder of N-terminal regions and the closed/open states of C-terminal regions may cooperate and be important for the catalytic mechanism of NDPS1.
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