HCV RNA‐dependent RNA polymerase replicates <i>in vitro</i> the 3′ terminal region of the minus‐strand viral RNA more efficiently than the 3′ terminal region of the plus RNA

Reigadas, Sandrine; Ventura, Michel; Sarih-Cottin, Leila; Castroviejo, Michel; Litvak, Simón; Astier-Gin, T.

doi:10.1046/j.0014-2956.2001.02532.x

Cited by 69 publications

(97 citation statements)

References 37 publications

(85 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…This result suggests that Cterminal region of NS5B might play a role in the initiation of RNA synthesis from 3'-end of HCV genome. To date, HCV NS5B polymerase has been shown to initiate RNA synthesis by snap-back or de novo mechanisms using a natural HCV RNA template (Behrens et al, 1996;Lohmann et al, 1997;Yamashita et al, 1998;Ishii et al, 1999;Oh et al, 2000;Sun et al, 2000;Ranjith-Kumar et al, 2001;Reigadas et al, 2001;Kashiwagi et al, 2002;Kim et al, 2002;Pellerin et al, 2002). Our results shown with several HCV RNA templates using TNTase-free NS5B are in agreement with the previous result obtained with E. coli-expressed NS5B (Oh et al, 1999), indicating that HCV NS5B proteins initiate RNA synthesis in a primer-independent manner.…”

Section: Discussionsupporting

confidence: 83%

“…In addition, the (-) 3'-UTR was found to serve as a better template for NS5B, supporting the observation that more plus-strand HCV genome accumulates in the infected cells than the minus-strand HCV RNA (Lohmann et al, 1999). Similar result has also been obtained with C-terminal 21 amino acid truncated NS5B (Reigadas et al, 2001), but the NS5B produced a longer than template sized product using X-RNA as a template. This result suggests that Cterminal region of NS5B might play a role in the initiation of RNA synthesis from 3'-end of HCV genome.…”

Section: Discussionsupporting

confidence: 74%

“…Even though the C-terminal 21 hydrophobic amino acids are involved in membrane anchorage of the HCV NS5B in vivo (Ivashkina et al, 2002), HCV RNA synthesis initiation seems to be influenced in vitro by this hydrophobic C-terminal domain of HCV NS5B. E. coli-expressed C-terminal 21 amino acid truncated NS5B generated a longer-than-template sized product with X-RNA (Reigadas et al, 2001). Another TNTase-free HCV NS5B with deletion of the 21 C-terminal hydrophobic amino acids copied HCV X-RNA inefficiently by internal initiation (Kashiwagi et al, 2002).…”

Section: Introductionmentioning

confidence: 99%

“…Their secondary structures have been determined (Blight and Rice, 1997;Schuster et al, 2002). The promoter in the minus-strand HCV RNA has been shown to be stronger than the promoter in the 3'-UTR of plus-strand HCV genome (Reigadas et al, 2001).…”

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Biochemical properties of full-length hepatitis C virus RNA-dependent RNA polymerase expressed in insect cells

Choi

Kim

Oh³

2003

Exp Mol Med

View full text Add to dashboard Cite

A bstractThe hepatitis C virus (HCV) RNA-dependent RNA polym erase, NS5B protein, is the key viral enzym e responsible for replication of the HCV viral RNA genom e. Although several full-length and truncated form s of the HCV NS5B proteins have been expressed previously in insect cells, contam ination of host term inal transferase (TNTase) has ham pered analysis of the RNA synthesis initiation m echanism using natural HCV RNA tem plates. W e have expressed the HCV NS5B protein in insect cells using a recom binant baculovirus and purified it to near hom ogeneity w ithout contam inated TNTase. The highly purified recom binant HCV NS5B w as capable of copying 9.6-kb full-length HCV RNA tem plate, and m ini-HCV RNA carrying both 5'-and 3'-untranslated regions (UTRs) of the HCV genom e. In the absence of a prim er, and other cellular and viral factors, the NS5B could elongate over HCV RNA tem plates, but the synthesized products were prim arily in the double stranded form , indicating that no cyclic replication occurred with NS5B alone. RNA synthesis using RNA tem plates representing the 3'-end region of HCV m inus-strand RNA and the X-RNA at the 3'-end of HCV RNA genom e w as also initiated de novo. N o form ation of dim er-size self-prim ed RNA products resulting from extension of the 3'-end hydroxyl group w as observed. Despite the internal de novo initiation from the X-RNA, the NS5B could not initiate RNA synthesis from the internal region of oligouridylic acid (U)20, suggesting that HCV RNA polym erase initiates RNA synthesis from the selected region in the 3'-UTR of HCV genom e.

show abstract

Section: Discussionsupporting

confidence: 83%

Section: Discussionsupporting

confidence: 74%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Biochemical properties of full-length hepatitis C virus RNA-dependent RNA polymerase expressed in insect cells

Choi

Kim

Oh³

2003

Exp Mol Med

View full text Add to dashboard Cite

show abstract

“…The interaction of the 5Ј-TR 230nt with 3Ј-UTR 454nt containing either wild type or complementary mutant CYC motifs was necessary for activation of the DEN2 3Ј-UTR(ϩ) RNA template (40,41). On the other hand, hepatitis C virus NS5B polymerase initiates RNA synthesis from the 3Ј-TR of the (Ϫ)-strand viral RNA more efficiently than the 3Ј-TR of the (ϩ)-strand polarity (47). Therefore, we sought to examine the template efficiency of 3Ј-TR 230nt WNV RNA of (Ϫ)-strand polarity in comparison with the 3Ј-UTR 631nt RNA of (ϩ)-strand polarity.…”

Section: Rna Synthesis By Wnv Ns5 On 3ј-oh-blocked Templates-mentioning

confidence: 99%

Requirements for West Nile Virus (–)- and (+)-Strand Subgenomic RNA Synthesis in Vitro by the Viral RNA-dependent RNA Polymerase Expressed in Escherichia coli

Nomaguchi

Teramoto

et al. 2004

Journal of Biological Chemistry

View full text Add to dashboard Cite

West Nile virus (WNV), 1 a mosquito-borne member of Flaviviridae family that consists of more than 70 human pathogens, was first isolated in 1937 from the blood of a female patient in the West Nile district of Uganda (1). Since then, the virus has been isolated in humans, birds, and bird-feeding mosquitoes, Culex univittatus. Serological studies revealed a broad distribution of the virus in Africa, West Asia including India, and the Middle East, but only occasionally isolated in Europe, and is thought to be spread by migratory birds (Ref. 2, for reviews, seeRefs. 3 and 4). WNV belongs to the Japanese encephalitis serocomplex group, which includes St. Louis encephalitis, Murray Valley encephalitis, Kunjin virus, and Japanese encephalitis virus (5, 6). WNV was not previously isolated in the Western hemisphere. The first outbreak of WNV infections occurred in New York in 1999 (7-10) in which 62 people were confirmed to be infected, seven of which were fatal. Since then, transmission of WNV is spreading rapidly throughout the United States; 12 states along the eastern seaboard in 2000 to 25 states and the District of Columbia by 2001 (3).WNV, like other flaviviruses, contain a positive (ϩ)-strand RNA of ϳ11 kb in length that is capped at the 5Ј-end and nonpolyadenylated at the 3Ј-end. WNV RNA contains conserved sequence elements within the 5Ј-and 3Ј-terminal regions (TR), which include two self-complementary cyclization motifs (5Ј-CYC and 3Ј-CYC) of 9 nt in length (11). There is a highly conserved stem-loop structure within the 3Ј-terminal 96 nt of 3Ј-UTR of flaviviral RNAs and a less conserved stem-loop structure within 5Ј-UTR (12-14) (for reviews, see Refs. 4,15,and 16). In addition, there is a potential pseudoknot tertiary structure within the 3Ј-terminal stem-loop structure of WNV RNA (17). Several host proteins have been shown to bind to the 5Ј-and 3Ј-UTR although their functional role in viral RNA replication has not been clearly established (18 -21) (for a review, see Ref. 22). By mutational analysis, the 3Ј stem-loop region within the 3Ј-UTR was shown to be important for viral replication in vivo (23,24) and in vitro (25).The flaviviral RNA genome encodes a single polyprotein precursor that were processed co-translationally and posttranslationally into three structural proteins (capsid, C; precursor membrane, prM; its processed form, membrane protein, M; and the envelope, E) and at least seven nonstructural proteins, NS1, NS2A, NS2B, NS3, NS4A, NS4B, and NS5 (for reviews, see Refs. 4,15,and 16). NS3 is a multifunctional protein; the N-terminal region of NS3 contains the serine protease domain and it requires NS2B for cleavage at the junctions of 2A-2B, 2B-3, 3-4A, and 4B-5. NS3 contains conserved motifs found in RNA helicases of the DEXH family (for reviews, see Refs. 4,15,and 16). Purified NS3 was shown to possess NTPase and RNA helicase activities (26 -32) as well as 5Ј-RNA triphosphatase activity (33, 34), the first enzyme required in 5Ј-cap synthesis.NS5 is the largest of the flaviviral nonstructural pro...

show abstract

Kinetic Analysis of C-Terminally Truncated RNA-Dependent RNA Polymerase of Hepatitis C Virus

Kashiwagi

Hara

Kohara

et al. 2002

Biochemical and Biophysical Research Communications

View full text Add to dashboard Cite

HCV RNA‐dependent RNA polymerase replicates in vitro the 3′ terminal region of the minus‐strand viral RNA more efficiently than the 3′ terminal region of the plus RNA

Cited by 69 publications

References 37 publications

Biochemical properties of full-length hepatitis C virus RNA-dependent RNA polymerase expressed in insect cells

Biochemical properties of full-length hepatitis C virus RNA-dependent RNA polymerase expressed in insect cells

Requirements for West Nile Virus (–)- and (+)-Strand Subgenomic RNA Synthesis in Vitro by the Viral RNA-dependent RNA Polymerase Expressed in Escherichia coli

Kinetic Analysis of C-Terminally Truncated RNA-Dependent RNA Polymerase of Hepatitis C Virus

Contact Info

Product

Resources

About