Hairpin RNA-Mediated Silencing of Plum pox virus P1 and HC-Pro Genes for Efficient and Predictable Resistance to the Virus

Nicola-Negri, E. Di; Brunetti, Angela; Tavazza, Mario; Ilardi, Vincenza

doi:10.1007/s11248-005-1773-y

Cited by 101 publications

(71 citation statements)

References 30 publications

(28 reference statements)

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“…Numerous studies have indicated that IR constructs of transgenes can effectively induce RNA silencing to trigger knockout of specific gene expressions (Ali et al, 2010;Allen et al, 2004;Gavilano et al, 2006;Johansen and Carrington, 2001;Kusaba et al, 2003;Liu et al, 2002;Meli et al, 2010;Pandolfini et al, 2003;Segal et al, 2003;Smith et al, 2000;Xiong et al, 2005). In addition, a number of studies showed that IR constructs of transgenes containing virus-derived sequences transformed to plants can effectively protect plants from challenging viruses (Abhary et al 2006;Bucher et al 2006;Chen et al, 2004;Di Nicola-Negri et al 2005;Hammond et al 2006;Lennefors et al 2006;Pooggin et al 2003;Simón-Mateo and García, 2011;Tenllado et al 2003;Tenllado et al, 2004;Vanitharani et al, 2003;Wang et al, 2000). In particular, transient expression of a hpRNA homologous to sequences of Pepper mild mottle virus (PMMoV) caused inhibition of PMMoV accumulation (Tenllado et al, 2003).…”

Section: Discussionmentioning

confidence: 99%

“…RNA 1 encodes proteins involved in genome replication and expression, and RNA2 encodes the movement protein and the two CPs (Lisa and Boccardo, 1996). RNA silencing has been efficiently used to generate resistance against plant viruses in many ornamental plants (Bucher et al, 2006;Hammond et al, 2006;Tenllado et al, 2004) and in different host systems to obtain resistance against several other viruses (Abhary et al, 2006;Di Nicola-Negri et al, 2005;Lennefors et al, 2006;Pooggin et al, 2003;Tenllado et al, 2003;Vanitharani et al, 2003). Particularly, transgenic expression of pathogen-derived sequences encoding hpRNAs that undergo to an efficient RNA silencing is a new and agricultural sustainable strategy to obtain virus-resistant plants (Smith et al, 2000).…”

Section: Introductionmentioning

confidence: 99%

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Transient Expression of Homologous Hairpin RNA Interferes with Broad bean wilt virus 2 Infection in Nicotiana benthamiana

Yoon¹,

Ryu²,

Choi³

et al. 2012

Research in Plant Disease

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Broad bean wilt virus 2 (BBWV2), genus Fabavirus, subfamily Comovirinae, family Secoviridae, causes damage in many economically important horticultural and ornamental crops. Sequence alignments showed several conserved sequences in 5' non-coding regions (5' NCRs) of RNA 1 and RNA 2 in all BBWV2 strains characterized so far. Based on this observation, we generated a hpRNA construct (pIR-BBWV2) harboring an inverted repeat containing a 210 bp cDNA fragment homologous to 5' NCR portion of BBWV2 RNA 1 to investigate the silencing potential for its ability to interfere with a rapidly replicating BBWV2. Agrobacteriummediated transient expression of the IR-BBWV2 had a detrimental effect on BBWV2 infection, showing no distinct symptoms in non-inoculated leaves of the agroinfiltrated Nicotiana benthamiana plants. BBWV2 genomic RNAs were not detected by RT-PCR from tissues of both the inoculated leaves and upper leaves of the agroinfiltrated plants. Accumulation of virus-derived small interfering RNAs was detected in the inoculated leaf tissues of N. benthamiana plants elicited by transient expression of IR-BBWV2 indicating that RNA silencing is responsible for the resistance to BBWV2.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Transient Expression of Homologous Hairpin RNA Interferes with Broad bean wilt virus 2 Infection in Nicotiana benthamiana

Yoon¹,

Ryu²,

Choi³

et al. 2012

Research in Plant Disease

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show abstract

“…In 1998, Anandalakshmi and collaborators and Brigneti and collaborators shown that HC-Pro protein of TEV and 2b of CMV could have this role. A classic paper demonstrated that the inhibition system of the 5' end corresponding to proteins P1 and Hc-Pro was efficient to obtain plants resistant to Plum pox virus (PPV) in tobacco (Di Nicola-Negri et al, 2005). In this same study were tested four regions of the virus genome: (i) nucleotide (nt) 1-733 of the protein corresponding to P1; (ii) nt 954-1603 corresponding to the end of the protein P1 and protein portion of Hc-Pro; (iii) nt 1680-2386 corresponding to the central part of Hc-Pro/P3 and, (iv) nt 1935 to 2613 corresponding to the end of Hc-Pro protein and part of P3.…”

Section: Application Of Rnai To Obtain Transgenic Maize Lines Toleranmentioning

confidence: 99%

Maize Transformation to Obtain Plants Tolerant to Viruses by RNAi Technology

Carneiro¹,

Carneiro²

2011

Genetic Transformation

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“…This has led to the outcome that RNA silencing mechanism can be exploited to generate resistance against viral pathogens. Pathogen derived resistance (PDR) (Sanford and Johnston 1985) strategies based on RNA silencing mechanism have been utilized to develop resistance against RNA or DNA viruses (Chen et al 2004;Di Nicola-Negri et al 2005, Bonfim et al 2007Ramesh et al 2007;Zrachya et al 2007;Vanderschuren et al 2009;Patil et al 2011). Recently, RNAi-based resistance to mixed infection of three different viruses has been reported in soybean plants expressing separate short hairpins from a single transgene (Zhang et al 2011).…”

Section: Introductionmentioning

confidence: 99%

Identification of siRNA generating hot spots in multiple viral suppressors to generate broad-spectrum antiviral resistance in plants

Sharma

Kushwaha

Basu

et al. 2014

Physiol Mol Biol Plants

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Viruses are one of the most devastating plant pathogens causing severe economic losses worldwide. RNA silencing is a robust technology to knock down the expression of specific genes. This mechanism can be exploited to generate virus resistant plants through expression of the viral derived sequences. Viruses in turn have evolved to encode suppressors of RNA silencing to combat host defense. Mixed infection of plants is of common occurrence in nature and simultaneous targeting of suppressor(s) of multiple viruses offers an effective strategy. In this study, we have in silico designed siRNAs against suppressors of the two most devastating viruses of tomato, leaf curl causing tomato begomoviruses and Cucumber mosaic virus. Three different siRNA prediction programs were used to evaluate siRNAs generating capability of each sequence and common putative candidate siRNAs were selected fulfilling the stringent parameters. Our results indicated that in the case of each suppressor a particular region of 100-150 base pairs could be source of potent siRNAs referred as hotspots. Expression of these viral hot spots as a single construct in the plants would facilitate development of transgenic plants with a high degree of broad spectrum resistance against multiple viruses.

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Hairpin RNA-Mediated Silencing of Plum pox virus P1 and HC-Pro Genes for Efficient and Predictable Resistance to the Virus

Cited by 101 publications

References 30 publications

Transient Expression of Homologous Hairpin RNA Interferes with Broad bean wilt virus 2 Infection in Nicotiana benthamiana

Transient Expression of Homologous Hairpin RNA Interferes with Broad bean wilt virus 2 Infection in Nicotiana benthamiana

Maize Transformation to Obtain Plants Tolerant to Viruses by RNAi Technology

Identification of siRNA generating hot spots in multiple viral suppressors to generate broad-spectrum antiviral resistance in plants

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