First Report of Rhizoctonia solani AG2-1 on roots of wheat in Kazakhstan

Göksel Özer; İmren Mustafa; Tugba Bozoglu; Abdelfattah A Dababat

doi:10.1094/PDIS-04-21-0786-PDN

First Report of Rhizoctonia solani AG2-1 on roots of wheat in Kazakhstan

Plant Dis. 2021 May 25. doi: 10.1094/PDIS-04-21-0786-PDN. Online ahead of print.

Authors

Göksel Özer¹, İmren Mustafa², Tugba Bozoglu³, Abdelfattah A Dababat⁴

Affiliations

¹ Abant Izzet Baysal Universitesi, 52942, Plant Pathology, Abant Izzet Baysal University, Agriculture and Natural Sciences, Golkoy Campus, Bolu, Turkey, 14280; gokozer@gmail.com.
² , University of Abant Izzet Baysal Faculty of Agriculture and Natural Sciences , Department of Plant Protection, Gölköy Campus, Bolu, Turkey, 14280; m.imren37@gmail.com.
³ Department of Plant Protection, Faculty of Agriculture, Bolu Abant Izzet Baysal University, Bolu 14030, Turkey, Bolu, Turkey; bzglu.tugba24@gmail.com.
⁴ CIMMYT Turkey, CIMMYT Uluslararası Buğday ve Mısır Geliştirme Merkezi, Şehit Cem Ersever Caddesi No : 9/11, Tarla Bitkileri Araştırma Enstitüsü Kampüsü içi, Ankara, Ankara, Turkey, 06170; a.dababat@cgiar.org.

PMID: 34032487
DOI: 10.1094/PDIS-04-21-0786-PDN

Abstract

In June 2019, approximately 20 tillers of wheat (Triticum aestivum L.) were sampled at the ripening stage (Feekes scale 11) from four different fields in Almaty, Kazakhstan. Brown lesions (3-5 mm in length) were present on the roots of sampled plants, with 20% incidence. To determine the causal agent, diseased roots were surface disinfected in sodium hypochlorite solution (1%) for 3 min, rinsed triple with sterile distilled water, air-dried in a laminar flow hood, and plated onto one-fifth strength potato dextrose agar (PDA) supplemented with 50 ppm chloramphenicol. After three days, the hyphal fragments that developed from the sections were transferred to fresh PDA and incubated at 23°C with 12-h photoperiod for 7 days to obtain pure cultures. Brown pigmented fungal colonies with a constriction at the base of hyphal branches, septa near the branching point, and right-angled branching resembling Rhizoctonia solani were observed. The identification anastomosis group (AG) of a representative isolate for each field was conducted by sequencing the internal transcribed spacer (ITS) region of rDNA with the universal primers ITS4 and ITS5 (White et al. 1990). The resulting sequences of 693 bp length were deposited in GenBank (accession nos. MW898143:MW898146). These sequences were 100% identical to the isolate 8Rs of R. solani AG2-1 (accession no. AF354063). To confirm the pathogenicity of the four isolates, the colonized wheat kernels method described by Demirci (1998) was used to inoculate a sterile potting mix containing peat, vermiculite, and soil (1:1:1 by v/v/v) into which wheat (cv. Seri) was planted. Control pots were inoculated with sterile wheat kernels using the same procedure. Wheat plants were left to grow for four weeks under controlled environmental conditions with a 23°C temperature regime. During the period that the plants remained in the glasshouse, the typical light regime was 16 h. Brown lesions were observed on the roots of plants in the inoculated pots whereas no symptoms were observed on plants grown in the control pots. R. solani was consistently reisolated from symptomatic plants, thereby confirming Koch's postulates. To our knowledge, this is the first report of R. solani AG2-1 on roots of wheat in Kazakhstan. R. solani AG2-1 isolates have been previously reported to be a weak pathogen to wheat (Roberts and Sivasithamparam 1986; Sturrock et al. 2015; Jaaffar et al. 2016; Özer et al. 2019). We suggest further studies are required to characterize the impact of R. solani AG2-1 in wheat. Considering crop rotation, the selection of non-host crops to this AG group is important to pathogen management, by reducing the amount of inoculum in the soil.

Keywords: Causal Agent; Epidemiology; Fungi; Pathogen detection; Subject Areas; disease development and spread.