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Use of randomly mutagenized genomic cDNA banks of Potato spindle tuber viroid to screen for viable versions of the viroid genome

Więsyk, Aneta and Candresse, Thierry and Zagórski-Ostoja, Włodzimierz and Góra-Sochacka, Anna (2011) Use of randomly mutagenized genomic cDNA banks of Potato spindle tuber viroid to screen for viable versions of the viroid genome. Journal of general virology, 92 (2). pp. 457-466. ISSN 0022-1317

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Official URL: http://vir.sgmjournals.org/

Abstract

In an effort to study sequence space allowing the recovery of viable Potato spindle tuber viroid (PSTVd) variants we have developed an in vivo selection (Selex) method to produce and bulk-inoculate by agroinfiltration large PSTVd cDNA banks in which a short stretch of the genome is mutagenized to saturation. This technique was applied to two highly conserved six nucleotide-long regions of the PSTVd genome, the left terminal loop (TL bank) and part of the polypurine stretch in the upper strand of pre-melting loop 1 (PM1 bank). In each case, PSTVd accumulation was observed in a large fraction of bank-inoculated tomato plants. Characterization of the progeny molecules showed the recovery of the parental PSTVd sequence in 89% (TL bank) and 18% (PM1 bank) of the analyzed plants. In addition, viable and genetically stable PSTVd variants with mutations outside of the known natural variability of PSTVd were recovered in both cases, although at different rates. In the case of the TL region, mutations were recovered at five of the six mutagenized positions (357, 358, 359, 1 and 3 of the genome) while for the PM1 regions mutations were recovered at all six targeted positions (50-55), providing significant new insight on the plasticity of the PSTVd genome.

Item Type:Article
Uncontrolled Keywords:Viroid, PSTVd; terminal hairpin; polypurine; pre-melting loop 1; Selex
Subjects:Q Science > QR Microbiology > QR355 Virology
Divisions:Department of Protein Biosynthesis
ID Code:28
Deposited By: dr Anna Gora-Sochacka
Deposited On:21 Mar 2011 06:07
Last Modified:01 Oct 2015 08:18

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