Molecular dissection of a dahlia isolate of potato spindle tuber viroid inciting a mild symptoms in tomato

Daiki Tsushima; Taro Tsushima; Teruo Sano

doi:10.1016/j.virusres.2015.12.018

Molecular dissection of a dahlia isolate of potato spindle tuber viroid inciting a mild symptoms in tomato

Virus Res. 2016 Mar 2:214:11-8. doi: 10.1016/j.virusres.2015.12.018. Epub 2015 Dec 28.

Authors

Daiki Tsushima¹, Taro Tsushima², Teruo Sano³

Affiliations

¹ Department of Bio-resources, Faculty of Agriculture and Life Science, Hirosaki University, Hirosaki 036-8561, Japan; Union Graduate school of Agricultural Sciences, Iwate University, 3-18-8 Ueda, Morioka, Iwate 020-8550, Japan.
² Department of Bio-resources, Faculty of Agriculture and Life Science, Hirosaki University, Hirosaki 036-8561, Japan.
³ Department of Bio-resources, Faculty of Agriculture and Life Science, Hirosaki University, Hirosaki 036-8561, Japan. Electronic address: sano@cc.hirosaki-u.ac.jp.

PMID: 26732488
DOI: 10.1016/j.virusres.2015.12.018

Abstract

The dahlia isolate of potato spindle tuber viroid (PSTVd) accumulates slowly and induces mild disease symptoms in tomato (Solanum lycopersicum, cv. Rutgers) plants in contrast to the intermediate isolate (PSTVd-I). The dahlia isolate (PSTVd-D) differs from PSTVd-I in eight locations: 42 and 43 in the terminal left (TL); 64/65, 311, and 312/313 in the pathogenicity (P); 118 and 126 in the variable (V); and 201 in the terminal right (TR) domains. To investigate the molecular determinants in the PSTVd-D genome responsible for the attenuation of symptom severity and lower replication/accumulation in tomato plants, a series of mutants between PSTVd-D and PSTVd-I were constructed by focusing first on the mutations in the TL and P domains in the left-hand half of the molecule. Then, more detailed analysis was performed on the three mutations at positions 118, 126, and 201 in the V and TR domains. One of these mutations is located around the boundary of the right border of the RY-motif, a predicted recognition site of Virp1, a viroid-binding protein. Of 14 mutants (seven based on PSTVd-D and the other seven based on PSTVd-I) examined, 11 propagated stably and three lost infectivity. Mutations in the TL and P domains (42U, 43C, 310U/C, and U or UU insertion to 311/312 in PSTVd mild types) majorly influenced the expression of mild-like symptoms. In contrast, when each of the mutations at 118, 126, and 201 in the V and TR domains were exchanged independently, they minimally influenced systemic accumulation and symptom expression. Mutants based on PSTVd-D with PSTVd-I-type mutations at nucleotide positions 118, 126, and/or 201 showed mild symptoms similar to PSTVd-D, but their systemic accumulation was a little faster than PSTVd-D. In contrast, mutants based on PSTVd-I with PSTVd-D-type mutations at 118, 126, and/or 201 nucleotide positions showed severe symptoms similar to PSTVd-I, and the systemic accumulation was similar to or a little slower than PSTVd-I. The nucleotide at position 201 could be changed to U, G, or A, but C was not acceptable for replication. Because introduction of C at the position 201 can change the loop structure at the right boundary of the RY-motif's consensus sequence, the loop structure may influence recognition by Virp1.

Keywords: Accumulation; Pathogenicity; Replication; Terminal right domain; Variable domain; Viroid.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

DNA Mutational Analysis
DNA, Viral
Dahlia / virology*
Genome, Viral
Genomic Instability
Mutation
Nucleic Acid Conformation
Phenotype
Plant Diseases / virology*
Solanum lycopersicum / virology
Viroids / genetics*
Viroids / isolation & purification*

Substances

DNA, Viral