Fate of African Cassava Mosaic Virus Coat Protein Deletion Mutants after Agroinoculation

Head-to-tail dimeric clones of both DNA A and DNA B of potato yellow mosaic geminivirus (PYMV) were constructed. These constructs were infectious when inoculated onto Nicotiana benthamiana plants either as DNA or by agroinoculation and were also infectious for tomato plants by agroinoculation. The dimers were not infectious for potato plants following inoculation by either method. Symptom induction required both DNA A and DNA B but agroinoculation with DNA A alone resulted in virus spread in 30% of the inoculated N. benthamiana plants. Leaf disc explants of N. benthamiana, tomato and potato could all be infected by agroinoculation indicating that the method of delivery of the DNA to intact potato plants was unsuitable for successful inoculation rather than an inherent inability of the virus to replicate/spread in potato per se.

supporting

confidence: 77%

mentioning

confidence: 99%

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The infectivity of dimeric potato yellow mosaic geminivirus clones in different hosts

Buragohain

Sung²,

Coffin³

et al. 1994

“…The deleted region in the progeny DNA A was replaced by cloning vector DNA sequestered from pUC DNA surrounding the DNA A fragment in the inoculated construct. Size reversion of ACMV DNA A has been shown previously for systemic infections resulting with coat protein deletion mutants (Etessami et al, 1989;Klinkenberg et al, 1989). Klinkenberg et al (1989) showed that the size reversion observed for ACMV DNA A with the coat protein deletion mutants was produced following systemic spread, whereas in dividing callus ceils the deleted DNA A was replicated.…”

Section: Agroinoculation Of Dna a Deletion Mutantsmentioning

confidence: 97%

Mutagenesis of the AC3 open reading frame of African cassava mosaic virus DNA A reduces DNA B replication and ameliorates disease symptoms

Morris

Richardson

Eddy

et al. 1991

Small insertions were made independently at each of four unique restriction sites on African cassava mosaic virus (ACMV) DNA A to disrupt the three overlapping complementary-sense open reading frames (ORFs) herein designated AC1, AC2 and AC3. The DNA A mutants were assayed for their infectivity by agroinoculation of monomeric constructs to Nicotiana benthamiana plants containing chromosomal insertions of ACMV DNA B. Disruption of the AC30RF alone resulted in a delay and amelioration of disease symptoms which correlated with reduced replication of DNA B. Normal replication of DNA A still carrying the AC30RF mutation was found in extracts from these plants. No ACMV DNA or symptoms were observed in corresponding inoculations with either the simultaneous disruption of the overlapping AC2 and AC30RFs or disruption of the ACI ORF. Complementation by the inoculation of different mutant pairs produced a delay in disease symptoms followed by repair of mutated sites. A DNA A construct with the virus-sense AV1 (coat protein) ORF deleted was infectious producing typical ACMV disease symptoms. A similar construct with a larger deletion encompassing the complementary-sense AC30RF produced symptomless infections. The DNA recovered from plants revealed DNA A of normal size where the position of the deleted ORF was replaced with cloning vector DNA. Significantly reduced DNA B replication was observed for the AC3 deletion construct.

“…Binary vector clones were introduced into Agrobacterium tumefaciens strain GV3850 (Zambryski et al, 1983) and used to agroinoculate Nicotiana benthamiana and A. conyzoides plants as described by Saunders et al (2004). N. benthamiana leaf disks were prepared and maintained as described by Klinkenberg et al (1989) and DNA was extracted from plant tissues and analysed by Southern blot hybridization as described by Saunders et al (2004). Equal amounts of DNA were loaded in each lane.…”

Section: Methodsmentioning

confidence: 99%

Replication promiscuity of DNA-β satellites associated with monopartite begomoviruses; deletion mutagenesis of the Ageratum yellow vein virus DNA-β satellite localizes sequences involved in replication

Saunders

Briddon

Stanley

2008

102

Pseudorecombination studies in Nicotiana benthamiana demonstrate that Ageratum yellow vein virus (AYVV) and Eupatorium yellow vein virus (EpYVV) can functionally interact with DNA-β satellites associated with AYVV, EpYVV, cotton leaf curl Multan virus (CLCuMV) and honeysuckle yellow vein virus (HYVV). In contrast, CLCuMV shows some specificity in its ability to interact with distinct satellites and HYVV is able to interact only with its own satellite. Using an N. benthamiana leaf disk assay, we have demonstrated that HYVV is unable to trans-replicate other satellites. To investigate the basis of trans-replication compatibility, deletion mutagenesis of AYVV DNA-β has been used to localize the origin of replication to approximately 360 nt, encompassing the ubiquitous nonanucleotide/stem–loop structure, satellite conserved region (SCR) and part of the intergenic region immediately upstream of the SCR. Additional deletions within this intergenic region have identified a region that is essential for replication. The capacity for DNA-β satellites to functionally interact with distinct geminivirus species and its implications for disease diversification are discussed.