Identification of a Novel Function of the AlphavirusCapping Apparatus

Vasiljeva, Lidia; Merits, Andres; Auvinen, Petri; Kääriäinen, Leevi

doi:10.1074/jbc.m910340199

Cited by 173 publications

(166 citation statements)

References 59 publications

(50 reference statements)

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“…1A, lanes 1-5), whereas P12 ∧ 3 ∧ 4 yielded nsP1 and P234 (lanes 6 -10). In these experiments nsP1 was seen as a double band, due to aberrant initiation at a downstream methionine ( [11][12][13][14][15]. Interestingly, polyproteins containing the noncleavable 1/2 site were not processed at the 2/3 site either (Fig.…”

Section: In Vitro Synthesis Of Polyproteins Mutated At the Cleavagementioning

confidence: 99%

Regulation of the Sequential Processing of Semliki Forest Virus Replicase Polyprotein

Vasiljeva

Merits

Golubtsov

et al. 2003

Journal of Biological Chemistry

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113

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The replication of most positive-strand RNA viruses and retroviruses is regulated by proteolytic processing. Alphavirus replicase proteins are synthesized as a polyprotein, called P1234, which is cleaved into nsP1, nsP2, nsP3, and nsP4 by the carboxyl-terminal protease domain of nsP2. The cleavage intermediate P123؉nsP4 synthesizes minus-strand copies of the viral RNA genome, whereas the completely processed complex is required for plus-strand synthesis. To understand the mechanisms responsible for this sequential proteolysis, we analyzed in vitro translated Semliki Forest virus polyproteins containing noncleavable processing sites or various deletions. Processing of each of the three sites in vitro required a different type of activity. Site 3/4 was cleaved in trans by nsP2, its carboxyl-terminal fragment Pro39, and by all polyprotein proteases. Site 1/2 was cleaved in cis with a half-life of about 20 -30 min. Site 2/3 was cleaved rapidly in trans but only after release of nsP1 from the polyprotein exposing an "activator" sequence present in the amino terminus of nsP2. Deletion of amino-terminal amino acids of nsP2 or addition of extra amino acid residues to its amino terminus specifically inhibited the protease activity that processes the 2/3 site. This sequence of delayed processing of P1234 would explain the accumulation of P123 plus nsP4, the early short-lived minus-strand replicase. The polyprotein stage would allow correct assembly and membrane association of the RNA-polymerase complex. Late in infection free nsP2 would cleave at site 2/3 yielding P12 and P34, the products of which, nsP1-4, are distributed to the plasma membrane, nucleus, cytoplasmic aggregates, and proteasomes, respectively.

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Section: In Vitro Synthesis Of Polyproteins Mutated At the Cleavagementioning

confidence: 99%

Regulation of the Sequential Processing of Semliki Forest Virus Replicase Polyprotein

Vasiljeva

Merits

Golubtsov

et al. 2003

Journal of Biological Chemistry

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113

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“…Protein Expression and Purification-Recombinant proteins were expressed in E. coli BL21(DE3) (Stratagene) and purified using Ni 2ϩ -affinity chromatography as described previously (16,15). Protein purification was monitored by 10 -17% SDS-PAGE (25), and protein concentration was determined with the Bradford assay (26) using Bio-Rad reagents.…”

Section: Methodsmentioning

confidence: 99%

“…nsP2 Expression Plasmids-Full-length nsP2 of SFV was produced and purified as described previously (15). To obtain a set of nsP2 mutants, containing progressive amino-terminal truncations, nine separate PCR amplifications were carried out using Pfu Turbo DNA polymerase (Stratagene), SFV infectious cDNA as a template and 3Ј-Mut (Table I) as common 3Ј primer.…”

Section: Methodsmentioning

confidence: 99%

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Site-specific Protease Activity of the Carboxyl-terminal Domain of Semliki Forest Virus Replicase Protein nsP2

Vasiljeva

Valmu

Kääriäinen

et al. 2001

Journal of Biological Chemistry

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118

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The virus-specific components (nsP1-nsP4) of Semliki Forest virus RNA polymerase are synthesized as a large polyprotein (P1234), which is cleaved by a virus-encoded protease. Based on mutagenesis studies, nsP2 has been implicated as the protease moiety of P1234. Here, we show that purified nsP2 (799 amino acids) and its C-terminal domain Pro39 (amino acids 459 -799) specifically process P1234 and its cleavage intermediates. Analysis of cleavage products of in vitro synthesized P12, P23, and P34 revealed cleavages at sites 1/2, 2/3, and 3/4. The cleavage regions of P1/2, P2/3, and P3/4 were expressed as thioredoxin fusion proteins (Trx12, Trx23, and Trx34), containing ϳ20 amino acids on each side of the cleavage sites. After exposure of these purified fusion proteins to nsP2 or Pro39, the reaction products were analyzed by SDS-polyacrylamide gel electrophoresis, mass spectrometry, and amino-terminal sequencing. The expected amino termini of nsP2, nsP3, and nsP4 were detected. The cleavage at 3/4 site was most efficient, whereas cleavage at 1/2 site required 5000-fold more of Pro39, and 2/3 site was almost resistant to cleavage. The activity of Pro39 was inhibited by N-ethylmaleimide, Zn 2؉ , and Cu 2؉ , but not by EDTA, phenylmethylsulfonyl fluoride, or pepstatin, in accordance with the thiol proteinase nature of nsP2.

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“…Viruses achieve this by encoding their own capping enzyme apparatus such as the vaccinia virus (VACV) D1/D12 subunit, baculovirus LEF-4 and reovirus l2 protein (Gross & Shuman, 1998a;Luongo et al, 2000;Shuman, 1990). In viruses such as reovirus and baculovirus, the same enzyme (l2 and LEF-4, respectively) catalyses both RTPase and mRNA GT activities, whereas VACV, West Nile virus and alpha virus encode separate RTPases (Benzaghou et al, 2006;Myette & Niles, 1996;Vasiljeva et al, 2000).…”

Section: Introductionmentioning

confidence: 99%

RNA triphosphatase and guanylyl transferase activities are associated with the RNA polymerase protein L of rinderpest virus

Gopinath

Shaila

2009

Journal of General Virology

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Rinderpest virus (RPV) large (L) protein is an integral part of the ribonucleoprotein (RNP) complex of the virus that is responsible for transcription and replication of the genome. Previously, we have shown that recombinant L protein coexpressed along with P protein (as the L-P complex) catalyses the synthesis of all viral mRNAs in vitro and the abundance of mRNAs follows a gradient of polarity, similar to the occurrence in vivo. In the present work, we demonstrate that the viral mRNAs synthesized in vitro by the recombinant L or purified RNP are capped and methylated at the N 7 guanine position. RNP from the purified virions, as well as recombinant L protein, shows RNA triphosphatase (RTPase) and guanylyl transferase (GT) activities. L protein present in the RNP complex catalyses the removal of c-phosphate from triphosphate-ended 25 nt RNA generated in vitro representing the viral N-terminal mRNA 59 sequence. The L protein forms a covalent enzyme-guanylate intermediate with the GMP moiety of GTP, whose formation is inhibited by the addition of pyrophosphate; thus, it exhibits characteristics of cellular GTs. The covalent bond between the enzyme and nucleotide is acid labile and alkali stable, indicating the presence of phosphoamide linkage. The C-terminal region (aa 1717-2183) of RPV L protein alone exhibits the first step of GT activity needed to form a covalent complex with GMP, though it lacks the ability to transfer GMP to substrate RNA. Here, we describe the biochemical characterization of the newly found RTPase/GT activity of L protein.

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Identification of a Novel Function of the AlphavirusCapping Apparatus

Cited by 173 publications

References 59 publications

Regulation of the Sequential Processing of Semliki Forest Virus Replicase Polyprotein

Regulation of the Sequential Processing of Semliki Forest Virus Replicase Polyprotein

Site-specific Protease Activity of the Carboxyl-terminal Domain of Semliki Forest Virus Replicase Protein nsP2

RNA triphosphatase and guanylyl transferase activities are associated with the RNA polymerase protein L of rinderpest virus

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