Application of rapid biochemical methods for detecting avocado sunblotch disease

The method of Palukaitis & Symons (1980) for extracting low molecular weight ribonucleic acids from plant tissue was improved by CF-11-cellulose chromatography and further simplified for use in routine biochemical indexing for avocado sunblotch viroid (ASBV). Extracts were prepared routinely at 10 g dry weight equivalents (DWE) of tissue per ml; more concentrated than previously possible with many avocado cultivars. Conditions for assaying extracts of ASBV were standardised and the lower limits for detection determined as 80–230 ng ASBV/g DWE of tissue for polyacrylamide gel electrophoresis (PAGE) and 1 ng/g DWE of tissue for complementary DNA (cDNA) probe assays. The concentration of ASBV in a single infected tree varied from 5 to 5000 ng/g DWE between branches, but only to a minor degree between mature leaves and young blossoms within branches. Six independent sources of sunblotch disease were examined and all proved positive for ASBV by PAGE. The ASBV extracted from five of these sources hybridised with cDNA prepared from the sixth or standard source (Hass/SB-1), with hybridisation values ranging from 43% to 89%. In a survey of 76 trees intended for propagation in Australia, all of 17 trees previously accepted as healthy on the basis of graft transmission tests were negative for ASBV by PAGE and had cDNA hybridisation values ranging from 1.8% to 12.1%. Amongst 59 trees apparently free of sunblotch symptoms but not previously indexed, only one tree was positive for ASBV by both PAGE and cDNA probe assay. The other 58 trees were negative by PAGE but had hybridisation values ranging from 1.0% to 42.8%. Forty-nine trees had values consistent with known healthy trees (<12% hybridisation), while the results of the remaining nine trees will require confirmation by additional tests before a conclusion about ASBV is made. The cDNA probe assay successfully detected ASBV in avocado seedlings graft inoculated with Hass/SB-1, 1–2 months before symptoms were displayed but not until 6 months after inoculation. Methods for improving the cDNA probe assay still further are discussed.