Quantification of rhizomania virus by automated RNA isolation and PCR based methods in sugar beet

Claudia Chiodi; Giuseppe Concheri; Andrea Squartini; Samathmika Ravi; Chiara Broccanello; Matteo Moro; Piergiorgio Stevanato

doi:10.1007/s13337-021-00674-7

Quantification of rhizomania virus by automated RNA isolation and PCR based methods in sugar beet

Virusdisease. 2021 Mar;32(1):161-166. doi: 10.1007/s13337-021-00674-7. Epub 2021 Mar 19.

Authors

Claudia Chiodi¹, Giuseppe Concheri¹, Andrea Squartini¹, Samathmika Ravi¹, Chiara Broccanello¹, Matteo Moro¹, Piergiorgio Stevanato¹

Affiliation

¹ DAFNAE, Dipartimento di Agronomia Animali Alimenti Risorse Naturali e Ambiente, Università Degli Studi Di Padova, Viale dell'Università 16, 35020 Legnaro, PD Italy.

Abstract

Rhizomania is a grave disease affecting sugar beet (Beta vulgaris L.). It is caused by the Beet Necrotic Yellow Vein Virus (BNYVV), an RNA virus transmitted by the plasmodiophorid vector Polymyxa betae. Genetic resistance to the virus has been accomplished mostly using phenotype-genotype association studies. As yet, the most convenient method to ascertain plant resistance has been the quantification of viral titer in roots through the ELISA test. This method is particularly time-consuming and clashes with the necessities of modern plant breeding. Here, we propose an alternative and successful phenotyping method based on the automatic extraction of the viral RNA from sugar beet roots and its relative and absolute quantification by quantitative real-time PCR (qRT-PCR) and digital PCR (dPCR), respectively. Such a method enables an improved standardization of the study, as well as an accurate quantification of the virus also in those samples presenting low virus titer, with respect to the ELISA test.

Supplementary information: The online version contains supplementary material available at 10.1007/s13337-021-00674-7.

Keywords: Digital PCR; High-throughput phenotyping; Quantitative real-time PCR; Rhizomania virus; Sugar beet.