Facilitated folding and subunit assembly in Escherichia coli and in vitro of nucleoside diphosphate kinase from extremely halophilic archaeon conferred by amino-terminal extension containing hexa-His-tag

FEBS Letters
Matsujiro IshibashiMasao Tokunaga

Abstract

We have previously reported that nucleoside diphosphate kinase (HsNDK) from extremely halophilic archaeon Halobacterium salinarum was expressed in Escherichia coli as a soluble, but inactive form and required high salt concentrations for in vitro folding and activation. Here, we found that fusion of extra sequence containing hexa-His-tag at amino-terminus of HsNDK (His-HsNDK) facilitated folding and activation of HsNDK in E. coli. This is a first observation of active folding of halophilic enzyme from extremely halophilic archaeon in E. coli. The in vitro refolding rate of His-HsNDK after heat denaturation was greatly increased over the native HsNDK. Folded His-HsNDK isolated from E. coli formed a hexamer in both 0.2 M and 3.8 M NaCl at 30 degrees C, while the native HsNDK purified from H. salinarum dissociated to dimer in 0.2 M NaCl. The observed hexameric structure in 0.2 M NaCl indicates that amino-terminal extension also enhances dimer to hexamer assembly and stabilizes the structure in low salt. These results suggest that positive charges in fused amino-terminal extension are effective in suppressing the negative charge repulsion of halophilic enzyme and thus, facilitate folding and assembly of HsNDK.

References

Nov 1, 1974·Canadian Journal of Biochemistry·D Keradjopoulos, K Wulff
May 11, 2000·Extremophiles : Life Under Extreme Conditions·D MadernG Zaccai
Feb 17, 2001·Current Opinion in Structural Biology·R J Ellis
Sep 19, 2003·Journal of Protein Chemistry·Matsujiro IshibashiMasao Tokunaga
Dec 20, 2003·Protein and Peptide Letters·Matsujiro IshibashiMasao Tokunaga

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