Truncated yet functional viral protein produced via RNA polymerase slippage implies underestimated coding capacity of RNA viruses

Hagiwara‐Komoda, Yuka; Choi, Sun Hee; Sato, Mitsuru; Atsumi, Go; Abe, Junya; Fukuda, Junya; Honjo, Mie N.; Nagano, Atsushi J.; Komoda, Keisuke; Nakahara, Kenji; Uyeda, Ichiro; Naito, Shuichi

doi:10.1038/srep21411

Cited by 44 publications

(46 citation statements)

References 68 publications

(111 reference statements)

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“…Previously, we reported that in the susceptible pea line PI 250438 infected with Cl-90-1 Br2 or ClNo.30, P3N-PIPO of Cl-90-1 Br2 could be detected, but the amount of P3N-PIPO of Cl-No.30 was below the level of detection when tested by using an antibody against the PIPO peptide (7). Furthermore, we showed that the amount of P3N-PIPO produced from the P3 cistron of Cl-No.30 is significantly smaller than that of Cl-RB in an in vitro translation system using MM2 dL (an extract derived from A. thaliana MM2d cells) and wheat germ extract (7,13). In this study, we showed evidence that the P3 cistron of ClNo.30 produced less P3N-PIPO protein than did Cl-RB in vivo in agroinfiltrated N. benthamiana leaves (Fig.…”

Section: Discussionmentioning

confidence: 99%

“…We previously showed that P3N-PIPO was detected in Cl-RB-infected plants but was below the level of detection in Cl-No.30-infected plants of a susceptible pea cultivar, PI 250438, indicating that the level of P3N-PIPO from Cl-No.30 is significantly lower than that of P3N-PIPO from Cl-90-1 Br2 (7). The same difference was observed when P3N-PIPO was produced from the P3 cistron of each virus by using an in vitro translation system with an A. thaliana cell-free system and wheat germ extract (7,13). In this study, we compared the accumulation of Cl-No.30 P3N-PIPO with that of Cl-RB P3N-PIPO in a transient-expression system, agroinfiltration in N. benthamiana leaf tissues.…”

Section: P3 Of CLmentioning

confidence: 94%

“…The pTA/RB-P3(PIPO:FLAG Ϫ1 ), pTA/No.30-P3(PIPO:FLAG Ϫ1 ), pTA/RB-P3N-PIPO:FLAG mk , and pTA/No.30-P3N-PIPO:FLAG mk constructs were previously described (13).…”

Section: Methodsmentioning

confidence: 99%

“…As a control experiment, we compared the protein/mRNA ratios of P3N-PIPO:FLAG mk , which has mutations that enable the production of P3N-PIPO in the zero frame but does not produce P3 frame product, between Cl-RB and Cl-No.30 ( Fig. 5A) (13). Western blot analysis indicated that there were no visible differences in protein accumulation between Cl-RB and Cl-No.30 (Fig.…”

Section: P3 Of CLmentioning

confidence: 99%

“…P3N-PIPO has an essential role in virus cell-to-cell movement (10). Three independent groups, including our own, recently showed that P3N-PIPO is produced mainly by transcriptional slippage within the P3 gene (11)(12)(13).…”

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confidence: 99%

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P3N-PIPO, a Frameshift Product from the P3 Gene, Pleiotropically Determines the Virulence of Clover Yellow Vein Virus in both Resistant and Susceptible Peas

Atsumi

Suzuki

Miyashita

et al. 2016

J Virol

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IMPORTANCEControl of plant viral disease has relied on the use of resistant cultivars; however, emerging mutant viruses have broken many types of resistance. Recently, we revealed that Cl-90-1 Br2 breaks the recessive resistance conferred by cyv1, mainly by accumulating a higher level of P3N-PIPO than that of the nonbreaking isolate Cl-No.30. Here we show that a susceptible pea line recognized the increased amount of P3N-PIPO produced by Cl-90-1 Br2 and activated the salicylic acid-mediated defense pathway, inducing lethal systemic cell death. We found a gradation of virulence among ClYVV isolates in a cyv1-carrying pea line and two susceptible pea lines. This study suggests a trade-off between breaking of recessive resistance (cyv1) and host viability; the latter is presumably regulated by the dominant Cyn1 gene, which may impose evolutionary constraints upon P3N-PIPO for overcoming resistance. We propose a working model of the host strategy to sustain the durability of resistance and control fast-evolving viruses.H ost plants protect themselves from virus infection by activating defense systems mediated by immune receptors (e.g., nucleotide-binding-site-leucine-rich-repeat [NB-LRR] proteins) (1). Plants have many NB-LRR immune receptors, each of which recognizes specific viral proteins. The activated immune response is referred to as a hypersensitive response (HR) and is often accompanied by cell death. When an HR is induced, the virus is localized in and around the infection locus. NB-LRR immune receptors are encoded by resistance genes that are genetically dominant.Another important defense against plant virus infection is genetically recessive resistance (2). The viral life cycle totally relies on host cells, and viruses require host factors in order to multiply within cells and move to neighboring cells. Therefore, the lack of a specific host-coopted factor required for the viral life cycle leads to host resistance against the virus, which would be recessively inherited. Many natural recessive resistance genes against viruses have been identified in diverse crops (2). Extensive studies have been carried out on viruses belonging to the Potyvirus genus, the major genus of the Potyviridae family, which is one of the two largest plant virus genera and is found in most climatic regions worldwide (3). These viruses infect a broad range of host plants, including both monocots and dicots. They cause considerable crop damage, resulting in severe economic losses. Most of the recessive

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Section: Discussionmentioning

confidence: 99%

Section: P3 Of CLmentioning

confidence: 94%

“…The pTA/RB-P3(PIPO:FLAG Ϫ1 ), pTA/No.30-P3(PIPO:FLAG Ϫ1 ), pTA/RB-P3N-PIPO:FLAG mk , and pTA/No.30-P3N-PIPO:FLAG mk constructs were previously described (13).…”

Section: Methodsmentioning

confidence: 99%

Section: P3 Of CLmentioning

confidence: 99%

mentioning

confidence: 99%

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P3N-PIPO, a Frameshift Product from the P3 Gene, Pleiotropically Determines the Virulence of Clover Yellow Vein Virus in both Resistant and Susceptible Peas

Atsumi

Suzuki

Miyashita

et al. 2016

J Virol

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Presenting Peptides at the Surface of Potyviruses In Planta

Sánchez

Ponz

2018

Methods in Molecular Biology

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Potyviruses are plant viruses with elongated, flexuous virions amenable to modifications in the only viral structural protein, the coat protein (CP). Out of the several theoretically possible modifications to the CP, the one most exploited for peptide presentation is the genetic fusion of the peptide-to-be-expressed, to the CP N-terminus. Successful high-level expression of the modified CP has been achieved this way. The purified recombinant viral particles incorporate most, if not all, the properties of the expressed peptides. For many purposes, the recombinant virus particles present in extracts of infected plants should be purified for further use. Procedures for carrying out the whole process, from cloning to purification are described in the chapter.

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