Yee Cheun Chan scite author profile

The complete nonstructural NS5 gene of dengue type 1 virus, Singapore strain S275/90 (D1-S275/90) was expressed in Escherichia coli as a glutathione S-transferase (GST) fusion protein (126 kDa). The GST-NS5 fusion protein was purified and the recombinant NS5 protein released from the fusion protein by thrombin cleavage. The recombinant NS5 had a predicted molecular weight of 100 kDa and reacted with antiserum against D1-S275/90 virus in Western blot analysis. The purified recombinant NS5 protein possessed RNA-dependent RNA polymerase activity which was inhibited (>99%) by antibodies against the recombinant NS5 protein. The polymerase product was shown to be a negative-stranded RNA molecule, of template size, which forms a double-stranded complex with the template RNA.

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Dengue haemorrhagic fever outbreak in Karachi, Pakistan, 1994

Chan

Salahuddin

Khan

et al. 1995

Transactions of the Royal Society of Tropical Medicine and Hygi

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Combined Doppler and B-mode sonography in carpal tunnel syndrome

Vijayan

Therimadasamy

Chan

et al. 2011

Journal of the Neurological Sciences

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Recombinant Dengue Virus Type 1 NS3 Protein Exhibits Specific Viral RNA Binding and NTPase Activity Regulated by the NS5 Protein

et al. 1998

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The full-length dengue virus NS3 protein has been successfully expressed as a 94-kDa GST fusion protein in Escherichia coli. Treatment of the purified fusion protein with thrombin released a 68-kDa protein which is the expected molecular mass for the DEN1 NS3 protein. The identity of this protein was confirmed by Western blotting using dengue virus antisera. Two related activities of the recombinant NS3 protein were characterized, which were the binding of the protein to the 3'-noncoding region of the dengue virus RNA genome and NTPase activity. We demonstrated using a band shift assay that the DEN1 NS3 protein could form a complex with the stem-loop structure in the 3'-noncoding region (3'-NCR), although sites outside the stem-loop may also participate in binding. Using various unlabeled homopolymeric and heteropolymeric RNAs as competitors for binding, it was further shown that the DEN1 NS3 protein exhibits preferential binding to a 94-nt RNA transcript from the 3'-NCR of the dengue virus. The NTPase activity of the recombinant DEN1 NS3 protein was characterized using a thin-layer chromatography assay. We found that the DEN1 NS3 protein possesses some aspects of NTPase activity, which are distinct from those found in other flaviviruses. Although the NS3 protein was able to utilize all four ribonucleoside triphosphates as its substrates, the NS3 protein showed a distinct preference for purine triphosphates (i.e., ATP and GTP). The addition of poly(U) did not stimulate NTPase activity in DEN1 NS3 protein, which contrasts with the reports for other flaviviral NS3 proteins. However, NTPase activity was specifically stimulated by the viral NS5 protein, which was manifested by a more than twofold increase in the rate of ATP hydrolysis and a 25% increase in the yield of ADP at the end of a 120-min reaction. These data suggest that the NTPase activity of the NS3 protein may be regulated by the viral NS5 protein during virus replication.

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Rapid, single-step RT-PCR typing of dengue viruses using five NS3 gene primers

Seah

Chow

Tan

et al. 1995

Journal of Virological Methods

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Inducible isopentenyl transferase as a high-efficiency marker for plant transformation

et al. 1999

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Overexpression of the isopentenyltransferase gene (ipt) from the Ti-plasmid of Agrobacterium tumefaciens increases cytokinin levels, leading to generation of shoots from transformed plant cells. When combined with a dexamethasone-inducible system for controlling expression, ipt expression can be used to select for transgenic regenerants without using an antibiotic-resistance marker. The combined system allows efficient cointroduction of multiple genes (in addition to ipt) and produces transgenic plants without morphological or developmental defects.

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Full-length cDNA sequence of dengue type 1 virus (Singapore strain S275/90)

Tan

Yap

et al. 1992

Virology

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Electroencephalographic changes and seizures in familial hemiplegic migraine patients with the CACNA1A gene S218L mutation

Chan

Burgunder

Wilder-Smith

et al. 2008

Journal of Clinical Neuroscience

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Yee Cheun Chan

Recombinant Dengue Type 1 Virus NS5 Protein Expressed inEscherichia coliExhibits RNA-Dependent RNA Polymerase Activity

Dengue haemorrhagic fever outbreak in Karachi, Pakistan, 1994

Combined Doppler and B-mode sonography in carpal tunnel syndrome

Recombinant Dengue Virus Type 1 NS3 Protein Exhibits Specific Viral RNA Binding and NTPase Activity Regulated by the NS5 Protein

Rapid, single-step RT-PCR typing of dengue viruses using five NS3 gene primers

Inducible isopentenyl transferase as a high-efficiency marker for plant transformation

Full-length cDNA sequence of dengue type 1 virus (Singapore strain S275/90)

Electroencephalographic changes and seizures in familial hemiplegic migraine patients with the CACNA1A gene S218L mutation

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