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Open AccessJournal ArticleDOI

Hyphal Anastomosis Reactions, rDNA-Internal Transcribed Spacer Sequences, and Virulence Levels Among Subsets of Rhizoctonia solani Anastomosis Group-2 (AG-2) and AG-BI.

Donald E. Carling, +2 more
- 01 Jan 2002 - 
- Vol. 92, Iss: 1, pp 43-50
TLDR
Comparing anastomosis reactions, rDNA-internal transcribed spacer (ITS) sequences, and virulence of isolates representing Rhizoctonia solani AG-BI and six subsets of anastsomosis group (AG)-2 found grouping based on virulence does not conform to established grouping patterns within AG-2 and does not seem useful as a group-defining criterion.
Abstract
Hyphal anastomosis reactions, rDNA-internal transcribed spacer (ITS) sequences, and virulence of isolates representing Rhizoctonia solani AG-BI and six subsets of anastomosis group (AG)-2 (-2-1, -2-2 IIIB, -2-2 IV, -2-2 LP, -2-3, and -2-4) were compared. AG-2-4 is a subset described for the first time in this report. Anastomosis reactions within AG-BI and the listed subsets of AG-2 were generally strong but, between subsets, ranged from strong to a very weak "bridging" -type reaction. Anastomosis reaction alone generally did not provide adequate evidence for placement of an isolate into a subset of AG-2. Anastomosis reactions between AG-BI and the original subsets of AG-2 (-2-1 and -2-2) are very strong; for this reason, we propose that it be included as a subset of AG-2 (designation AG-2 BI). Subsets -2-3 and -2-4 show very weak bridging-type anastomosis reactions with all other subsets of AG-2 and thus may be candidates for independent AG status. Grouping within AG-2 based on rDNA-ITS sequences was consistent with the abovementioned subsets. However, grouping based on virulence as measured herein does not conform to established grouping patterns within AG-2 and does not seem useful as a group-defining criterion. A broad range of damage was observed among members of the most virulent subsets (-2-1, -2-2 IIIB, -2-2 IV, and -2-4), whereas other subsets (-2 BI, -2-2 LP, and -2-3) were similar to one another in causing a minimal level of damage. Group-specific primer pairs for each of the seven subsets of AG-2 were designed based on the abovementioned rDNA-ITS sequences. Primer pairs proved dependable and subset specific in polymerase chain reaction amplifications of purified genomic DNA from 109 isolates of R. solani and two isolates of binucleate Rhizoctonia. These primers will provide a simple and useful method for subset-specific characterization within AG-2 if further critical evaluations confirm their specificity.

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Disease Suppressive Soils: New Insights from the Soil Microbiome.

TL;DR: A number of hypotheses about the nature and ecology of microbial populations and communities of suppressive soils are proposed and the potential and limitations of new molecular techniques that can provide novel ways of testing these hypotheses are outlined.
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Characterization of AG-13, a Newly Reported Anastomosis Group of Rhizoctonia solani

TL;DR: Length and sequence of the internal transcribed spacer (ITS) regions of rDNA from isolates of AG-13 were unique among AGs of R. solani.
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Review. Biology and systematics of the form genus Rhizoctonia

TL;DR: This review focuses on the knowledge of several aspects of the species of Rhizcotonia s.
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Classification of Rhizoctonia spp. using rDNA-ITS sequence analysis supports the genetic basis of the classical anastomosis grouping

TL;DR: Comprehensive interrelationships among all the currently available MNR, BNR, and UNR groups and subgroups in GenBank were analyzed, showing the genetic relatedness among the different groups and indicating possible bridging groups between M NR, B NR, andUNR.
Journal ArticleDOI

The advancing identification and classification of Rhizoctonia spp. using molecular and biotechnological methods compared with the classical anastomosis grouping

TL;DR: Currently, the rDNA-internal transcribed spacer (ITS) sequence analysis seems to be the most appropriate method for classification of Rhizoctonia spp.
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