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  • Molecular cloning, expression, characterization and mutation of Plasmodium falciparum guanylate kinase.

Molecular cloning, expression, characterization and mutation of Plasmodium falciparum guanylate kinase.

Molecular and biochemical parasitology (2008-04-01)
Mahmoud Kandeel, Masayuki Nakanishi, Takayuki Ando, Kamal El-Shazly, Tarek Yosef, Yoshihito Ueno, Yukio Kitade
초록

The present work describes cloning, expression, purification, characterization, and mutation of Plasmodium falciparum guanylate kinase (PlasmoDB ID PFI1420w). Amino-acid sequence alignment revealed important differences especially in K42-V51, Y73-A77, and F100-L110, which include residues important for kinase activity, and at helix 3, which is important for domain movements. The catalytic efficiency for dGMP was 22-fold lower than that for GMP, whose value is the lowest among known guanylate kinases. dGMP was found to a competitive inhibitor for GMP with K(i)=0.148 mM and a mixed-type inhibitor with regard to ATP with measured K(i)=0.4 mM. The specificity constant (K(cat)/K(m)) of the four examined mutants varied for natural substrate GMP/dGMP, indicating the involvement of different mechanisms in substrate recognition and subsequent loop-domain movement. These results show that P. falciparum guanylate kinase is structurally and biochemically distinct from other guanylate kinases and could be a possible target in drug development.

MATERIALS
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Sigma-Aldrich
2′-Deoxyguanosine 5′-monophosphate sodium salt hydrate, ≥99% (HPLC)