Poliovirus cis-acting replication element-dependent VPg Uridylylation lowers the Km of the initiating nucleoside triphosphate for viral RNA replication

Initiation of RNA synthesis by RNA-dependent RNA polymerases occurs when a phosphodiester bond is formed between the first two nucleotides in the 5′ terminus of product RNA. The concentration of initiating nucleoside triphosphates (NTPi) required for RNA synthesis is typically greater than the concentration of NTPs required for elongation. VPg, a small viral protein, is covalently attached to the 5′ end of picornavirus negative- and positive-strand RNAs. A cis-acting replication element (CRE) within picornavirus RNAs serves as a template for the uridylylation of VPg, resulting in the synthesis of VPgpUpU_OH. Mutations within the CRE RNA structure prevent VPg uridylylation. While the tyrosine hydroxyl of VPg can prime negative-strand RNA synthesis in a CRE- and VPgpUpU_OH-independent manner, CRE-dependent VPgpUpU_OH synthesis is absolutely required for positive-strand RNA synthesis. As reported herein, low concentrations of UTP did not support negative-strand RNA synthesis when CRE-disrupting mutations prevented VPg uridylylation, whereas correspondingly low concentrations of CTP or GTP had no negative effects on the magnitude of CRE-independent negative-strand RNA synthesis. The experimental data indicate that CRE-dependent VPg uridylylation lowers the K_m of UTP required for viral RNA replication and that CRE-dependent VPgpUpU_OH synthesis was required for efficient negative-strand RNA synthesis, especially when UTP concentrations were limiting. By lowering the concentration of UTP needed for the initiation of RNA replication, CRE-dependent VPg uridylylation provides a mechanism for a more robust initiation of RNA replication.     

Replication of RNA viruses: structure of a 6 s RNA synthesized by the Q RNA polymerase

The in vitro synthesis of RNA catalyzed by the Qβ RNA polymerase has been studied using a single-stranded 6 s RNA template. Whereas Qβ RNA replication results in the synthesis predominantly of single-stranded Qβ RNA, the predominant reaction product of 6 s RNA replication was found to be double stranded. When treated with formaldehyde to dissociate complementary base pairs, 6 s RNA exhibited a decrease in molecular weight as indicated by its slower sedimentation rate and faster electrophoretic mobility. 6 s RNA also exhibited a hyperchromic thermal transition indicative of double-stranded RNA and differing markedly from that of single-stranded RNA. The T_m of this transition increased linearly with the logarithm of ionic strength. Renaturation of 6 s RNA below the T_m occurred slowly and was also dependent upon ionic strength.     

Replication of IPN virus: a cytochemical and biochemical study in SWT cells.

Although IPN virus failed to multiply at 30 degrees, it replicated at 16 degrees and 22 degrees in SWT cells. At 22 degrees the viral eclipse period lasted nearly 6 hr with maximal virion titers attained by 24 hr, whereas replication at 16 degrees was much slower. The replication of the virion was inhibited by 0.05 mug/ml of AD which did not interfere with the production of reovirus. Biochemical studies revealed that cellular DNA synthesis was markedly reduced (greater than 50%) soon after infection whereas total RNA synthesis was enhanced. The period of rapid increase in RNA synthesis paralleled the exponential production of infectious virus. Viral inclusion bodies, revealed by acridine orange-staining of virus-infected cells (SWT and RGG-2) late in the infectious cycle, were found to contain single-stranded RNA on the basis of their staining characteristics and sensitivity to RNase.     

Conversion of VPg into VPgpUpUOH before and during Poliovirus Negative-Strand RNA Synthesis

There are two protein primers involved in picornavirus RNA replication, VPg, the viral protein of the genome, and VPgpUpU_OH. A cis-acting replication element (CRE) within the open reading frame of poliovirus (PV) RNA allows the viral RNA-dependent RNA polymerase 3D^Pol to catalyze the conversion of VPg into VPgpUpU_OH. In this study, we used preinitiation RNA replication complexes (PIRCs) to determine when CRE-dependent VPg uridylylation occurs relative to the sequential synthesis of negative- and positive-strand RNA. Guanidine HCl (2 mM), a reversible inhibitor of PV 2C^ATPase, prevented CRE-dependent VPgpUpU_OH synthesis and the initiation of negative-strand RNA synthesis. VPgpUpU_OH and nascent negative-strand RNA molecules were synthesized coincident in time following the removal of guanidine, consistent with PV RNA functioning simultaneously as a template for CRE-dependent VPgpUpU_OH synthesis and negative-strand RNA synthesis. The amounts of [³²P]UMP incorporated into VPgpUpU_OH and negative-strand RNA products indicated that 100 to 400 VPgpUpU_OH molecules were made coincident in time with each negative-strand RNA. 3′-dCTP inhibited the elongation of nascent negative-strand RNAs without affecting CRE-dependent VPg uridylylation. A 3′ nontranslated region mutation which inhibited negative-strand RNA synthesis did not inhibit CRE-dependent VPg uridylylation. Together, the data implicate 2C^ATPase in the mechanisms whereby PV RNA functions as a template for reiterative CRE-dependent VPg uridylylation before and during negative-strand RNA synthesis.A common feature of positive-strand RNA viruses is the asymmetric replication of viral RNA. Poliovirus (PV) RNA replication has been studied extensively; however, it remains to be determined exactly how the synthesis of negative-strand RNA and that of positive-strand RNA are mechanistically distinct, culminating in the synthesis of greater amounts of positive-strand than negative-strand RNA (2). A cis-acting replication element (CRE) within the 2C open reading frame of PV RNA functions as a template for the conversion of the viral protein of the genome (VPg) into VPgpUpU_OH (24, 26, 37). 3D polymerase (3D^Pol), in concert with other viral proteins, catalyzes the conversion of VPg into VPgpUpU_OH on CRE RNA templates (22). It remains to be determined whether the tyrosine hydroxyl of VPg (14, 20, 21), the 3′ hydroxyl of VPgpUpU_OH (22, 23, 43), or both (38) are used to prime negative-strand RNA synthesis. It would be informative to know whether VPg is converted into VPgpUpU_OH before, during, and/or after the initiation of viral negative-strand RNA synthesis. Conversion of VPg into VPgpUpU_OH before the initiation of negative-strand RNA synthesis would be consistent with the possibility that it primes the initiation of negative-strand RNA synthesis. Conversely, if VPg were not converted into VPgpUpU_OH until after the initiation of negative-strand RNA synthesis, VPgpUpU_OH could not possibly participate in the initiation of negative-strand RNA synthesis. Also, because multiple copies of VPgpUpU_OH are necessary to prime reiterative initiation of positive-strand RNA synthesis (35), VPg is most likely converted into abundant amounts of VPgpUpU_OH before the initiation of positive-strand RNA synthesis.PV preinitiation RNA replication complexes (PIRCs) were used in this study to examine when VPg is converted into VPgpUpU_OH. PIRCs assemble and accumulate when PV mRNA is translated in reaction mixtures containing cytoplasmic extracts from uninfected HeLa cells and 2 mM guanidine HCl, a reversible inhibitor of viral RNA replication (5). The viral replication proteins expressed from the viral mRNA interact with lipid membranes in the cytoplasmic extracts to form RNA replication complexes (RCs) similar to those in infected cells (12). PIRCs convert VPg into VPgpUpU_OH and initiate viral RNA replication when they are isolated from reaction mixtures containing guanidine and resuspended in reaction mixtures lacking guanidine (6, 19). Guanidine HCl functions as a reversible inhibitor of PV RNA replication, both in cells (11) and in cell-free translation-replication reactions (6). In cells, PV RNA RCs fail to immediately initiate RNA replication following the removal of guanidine HCl (11). Rather, PV RCs formed in the presence of guanidine in cells appear to be translocated to a region of the cytoplasm where the RCs and their contents may be recycled and/or destroyed (11), possibly by autophagic vesicles (17). Recycling and/or destruction of RCs by autophagic vesicles would preclude their function upon the removal of guanidine. PIRCs, which form in the presence of guanidine during the translation of PV mRNA in cytoplasmic extracts of HeLa cells, immediately initiate both negative-strand RNA synthesis and CRE-dependent VPg uridylylation upon the removal of guanidine (6, 19). Viral RNA replication and VPgpUpU_OH synthesis are monitored by the incorporation of radiolabeled UTP (19-21). It is important to note that RNA replication in the context of PIRCs is artificial in that the PIRCs are stalled with guanidine and purified and then the guanidine block is removed. Despite this artificiality, the mechanisms of RNA replication within PIRCs appear to reliably represent the mechanisms of RNA replication in cells. There are several advantageous features of the PIRC experimental system: viral RNA replication is synchronous and sequential, with negative-strand RNA being made before positive-strand RNA (6); viral RNA replication is asymmetric, with an excess of positive-strand RNA being made from each negative-strand template; VPg is converted into VPgpUpU_OH in a CRE-dependent manner (20, 21); and the reaction conditions, including nucleoside triphosphate concentrations, are easily manipulated (38). Importantly, PIRCs contain all of the viral proteins associated with RNA replication and RNA replication by PIRCs faithfully mimics the asymmetric replication of PV RNA observed in cells.PV protein 2C, the target of guanidine HCl (30), is a critical but poorly understood component of PIRCs and RNA RCs in cells. PV protein 2C has an NH-terminal amphipathic helix which interacts with cellular membranes (40), a central ATPase domain where guanidine-resistant and guanidine-dependent mutations arise (31, 32), a cysteine-rich zinc binding motif (29), and a COOH-terminal RNA binding domain (34) which appears to work in concert with amino acid residues at the NH terminus to bind RNA. 2C^ATPase can oligomerize (1, 41), anchoring viral replication proteins and RNA templates within membranous RCs (4). The ability of guanidine HCl to reversibly inhibit both CRE-dependent VPg uridylylation and negative-strand RNA synthesis implicates 2C^ATPase in the mechanisms by which PV RNA functions coordinately as a template for both RNA replication and CRE-dependent VPgpUpU_OH synthesis (19, 21).In this study, we found that VPg was converted into VPgpUpU_OH before and during negative-strand RNA synthesis and that 2C^ATPase activity, in the context of membranous PIRCs, allowed PV RNA to function simultaneously as a template for CRE-dependent VPg uridylylation and as a template for negative-strand RNA synthesis. We discuss how picornaviruses coordinate the synthesis of nucleotidylylated protein primers with other steps of viral RNA replication.     

Flock House Virus RNA Polymerase Initiates RNA Synthesis De Novo and Possesses a Terminal Nucleotidyl Transferase Activity

Flock House virus (FHV) is a positive-stranded RNA virus with a bipartite genome of RNAs, RNA1 and RNA2, and belongs to the family Nodaviridae. As the most extensively studied nodavirus, FHV has become a well-recognized model for studying various aspects of RNA virology, particularly viral RNA replication and antiviral innate immunity. FHV RNA1 encodes protein A, which is an RNA-dependent RNA polymerase (RdRP) and functions as the sole viral replicase protein responsible for RNA replication. Although the RNA replication of FHV has been studied in considerable detail, the mechanism employed by FHV protein A to initiate RNA synthesis has not been determined. In this study, we characterized the RdRP activity of FHV protein A in detail and revealed that it can initiate RNA synthesis via a de novo (primer-independent) mechanism. Moreover, we found that FHV protein A also possesses a terminal nucleotidyl transferase (TNTase) activity, which was able to restore the nucleotide loss at the 3′-end initiation site of RNA template to rescue RNA synthesis initiation in vitro, and may function as a rescue and protection mechanism to protect the 3′ initiation site, and ensure the efficiency and accuracy of viral RNA synthesis. Altogether, our study establishes the de novo initiation mechanism of RdRP and the terminal rescue mechanism of TNTase for FHV protein A, and represents an important advance toward understanding FHV RNA replication.