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Elimination of Grapevine leafroll associated virus-3, Grapevine rupestris stem pitting associated virus and Grapevine virus A from a Tunisian Cultivar by Somatic Embryogenesis and Characterization of the Somaclones Using Ampelographic Descriptors

  • Bouamama-Gzara, Badra (Center of Biotechnology of Borj-Cedria. Laboratory of Plant Molecular Physiology) ;
  • Selmi, Ilhem (Institut National de Recherche Agronomique de Tunisie, Laboratoire de Protection des Vegetaux) ;
  • Chebil, Samir (Center of Biotechnology of Borj-Cedria. Laboratory of Plant Molecular Physiology) ;
  • Melki, Imene (Center of Biotechnology of Borj-Cedria. Laboratory of Plant Molecular Physiology) ;
  • Mliki, Ahmed (Center of Biotechnology of Borj-Cedria. Laboratory of Plant Molecular Physiology) ;
  • Ghorbel, Abdelwahed (Center of Biotechnology of Borj-Cedria. Laboratory of Plant Molecular Physiology) ;
  • Carra, Angela (Consiglio Nazionale delle Ricerche UOS di Palermo, Instituto di Bioscienze e BioRisorse) ;
  • Carimi, Francesco (Consiglio Nazionale delle Ricerche UOS di Palermo, Instituto di Bioscienze e BioRisorse) ;
  • Mahfoudhi, Naima (Institut National de Recherche Agronomique de Tunisie, Laboratoire de Protection des Vegetaux)
  • Received : 2017.06.13
  • Accepted : 2017.08.29
  • Published : 2017.12.01

Abstract

Prospecting of local grapevine (Vitis vinifera L.) germplasm revealed that Tunisia possesses a rich patrimony which presents diversified organoleptic characteristics. However, viral diseases seriously affect all local grapevine cultivars which risk a complete extinction. Sanitation programs need to be established to preserve and exploit, as a gene pool, the Tunisian vineyards areas. The presence of the Grapevine leafroll associated virus-3 (GLRaV-3), Grapevine stem pitting associated virus (GRSPaV) and Grapevine virus A (GVA), were confirmed in a Tunisian grapevine cultivar using serological and molecular analyses. The association between GRSPaV and GVA viruses induces more rugose wood symptoms and damages. For this reason the cleansing of the infected cultivar is highly advisable. Direct and recurrent somatic embryos of cv. 'Hencha' were successfully induced from filament, when cultured on $Ch{\acute{e}}e$and Pool (1987). based-medium, enriched with $2mg1^{-1}$ of 2,4-dichlorophenoxyacetic acid and $2.5mg1^{-1}$ of Thidiazuron, after 36 weeks of culture. After six months of acclimatization, RT-PCR carried on 50 somaplants confirmed the absence of GVA, GRSPaV as well as GLRaV-3 viruses in all somaplants. Ampelographic analysis, based on eight OIV descriptors, was carried out on two years acclimated somaplants, compared to the mother plant. Results demonstrated that the shape and contours of 46 somaclones leaves are identical to mother plant leaves and four phenotypically off-type plants were observed. The healthy state of 100% 'Hencha' somaclones and the high percentage of phenotypically true-to-type plants demonstrate that somatic embryogenesis is a promising technique to adopt for grapevine viruses elimination.

Keywords

References

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