Please use this identifier to cite or link to this item: https://repository.unej.ac.id/xmlui/handle/123456789/97058
Title: Purification and Characterization of Recombinant Sugarcane Sucrose Phosphate Synthase Expressed in E. coli and Insect Sf9 Cells: An Importance of the N-terminal Domain for an Allosteric Regulatory Property
Authors: Sawitri, Widhi Dyah
Narita, Hirotaka
Ishizaka-Ikeda, Etsuko
Sugiharto, Bambang
Hase, Toshiharu
Nakagawa, Atsushi
Keywords: allosteric regulation
carbon metabolism
recombinant enzyme
sucrose phosphate synthase
sugarcane
Issue Date: 30-Jan-2016
Publisher: J. Biochem. 2016;159(6):599–607
Abstract: Sucrose phosphate synthase (SPS) catalyses the transfer of glycosyl group of uridine diphosphate glucose to fructose-6-phosphate to form sucrose-6-phosphate. Plant SPS plays a key role in photosynthetic carbon metabolisms, which activity is modulated by an allosteric activator glucose-6-phosphate (G6P). We produced recombinant sugarcane SPS using Escherichia coli and Sf9 insect cells to investigate its structure-function relationship. When expressed in E. coli, two forms of SPS with different sizes appeared; the larger was comparable in size with the authentic plant enzyme and the shorter was trimmed the N-terminal20kDa region off. In theinsectcells, only enzyme with the authentic size was produced. We purified the trimmed SPS and the full size enzyme from insect cells and found their enzymatic properties differed significantly; the full size enzyme was activated allosterically by G6P, while the trimmed one showed a high activity even without G6P. We further introduced a series of N-terminal truncations up to 171 residue and found G6P-independent activity was enhanced by the truncation. These combined results indicated that the N-terminal region of sugarcane SPS is crucial for the allosteric regulation by G6P and may function like a suppressor domain for the enzyme activity.
URI: http://repository.unej.ac.id/handle/123456789/97058
Appears in Collections:LSP-Jurnal Ilmiah Dosen

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