Characterization of<i>Armillaria</i>isolates from tea (<i>Camellia sinensis</i>) in Kenya

Otieno, W.; Sierra, Ana Pérez; Termorshuizen, A.J.

doi:10.1080/15572536.2004.11833146

Cited by 16 publications

(9 citation statements)

References 26 publications

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“…13,14) Methods based on molecular techniques are nowadays routinely used and provided a new perspective for phylogenetic and taxonomic studies.…”

Section: )mentioning

confidence: 99%

“…11,12) Furthermore, mating pairings require fresh haploid cultures that sometimes are not available and a long period is required to obtain results. 13,14) Methods based on molecular techniques are nowadays routinely used and provided a new perspective for phylogenetic and taxonomic studies. 12,[15][16][17] PCR-RFLP analysis profiles of intergenic spacer 1 (IGS-1) have been successfully applied to the Armillaria species identification.…”

Section: 2)mentioning

confidence: 99%

“…12,[15][16][17] PCR-RFLP analysis profiles of intergenic spacer 1 (IGS-1) have been successfully applied to the Armillaria species identification. 12,13,18,19) Sequencing of the internal transcribed spacer (ITS) and intergenic spacer 1 (IGS-1) regions 14,20,21) has also been used for identification. The ITS and IGS sequences available in the GenBank and the development of efficient software have provided a valuable tool for differentiation as well as for the detection of polymorphism and heterogeneity among species.…”

Section: 2)mentioning

confidence: 99%

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Identification of Armillaria nabsnona in Gastrodia Tubers

Sekizaki

Kuninaga

Yamamoto

et al. 2008

Biological & Pharmaceutical Bulletin

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Armillaria species (Basidiomycota, Agaricales, Tricholomataceae) are well known to be the cause of root rot and death to woody plants in boreal, temperate and tropical regions worldwide.1) Generally this species has a broad variety of hosts, presenting pathogenic or symbiotic properties depending on the available substrate. 1,2)Armillaria has been identified as an associate in certain achlorophyllous taxa of Orchidaceae including Gastrodia elata BL. 3,4) and Galeola septentrionalis REICHB. 5) Although many reports refer to Armillaria mellea as the main fungus symbiont of G. elata, 3,6) 4)In eastern traditional medicine, the tubers of this orchid have been used for the treatment of many kinds of diseases including headache, rheumatism, seizure, dizziness and circulation problems. 7,8) G. elata is considered as a difficult species to cultivate due to the need for different kinds of fungi colonization to achieve its full development.6) To increase the knowledge of the cultivation process and understand its relationship with the Armillaria, it is important to first identify which Armillaria species is involved in the association.In past decades, the identification of Armillaria spp. was based on mating tests and morphological characteristics. 2,9,10) However, those methods are very limited due to the great number of biological species and similar morphological characteristics among them.11,12) Furthermore, mating pairings require fresh haploid cultures that sometimes are not available and a long period is required to obtain results. 13,14) Methods based on molecular techniques are nowadays routinely used and provided a new perspective for phylogenetic and taxonomic studies.12,15-17) PCR-RFLP analysis profiles of intergenic spacer 1 (IGS-1) have been successfully applied to the Armillaria species identification. 12,13,18,19) Sequencing of the internal transcribed spacer (ITS) and intergenic spacer 1 (IGS-1) regions 14,20,21) has also been used for identification. The ITS and IGS sequences available in the GenBank and the development of efficient software have provided a valuable tool for differentiation as well as for the detection of polymorphism and heterogeneity among species. The ITS and IGS-1 of the ribosomal DNA are known to be highly polymorphic enabling the accurate species differentiation of the Armillaria.11) In some cases, however, ITS1 region sequences were proven to be nearly uniform among the Armillaria of northern hemisphere species. 11)The aim of this study was to apply molecular biological tools to identify which Armillaria species are involved in the association with G. elata. The ITS and IGS-1 regions of rDNA were amplified and sequenced for further comparison with other Armillaria species. PCR-RFLP of the IGS-1 region was performed with three different endonucleases. Morphological characteristics and compatibility tests were also used in the analysis. MATERIALS AND METHODS Fungal Isolation and CultivationFungal samples were harvested in July 2005, found in different root parts of G. elata, which ...

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“…13,14) Methods based on molecular techniques are nowadays routinely used and provided a new perspective for phylogenetic and taxonomic studies.…”

Section: )mentioning

confidence: 99%

Section: 2)mentioning

confidence: 99%

Section: 2)mentioning

confidence: 99%

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Identification of Armillaria nabsnona in Gastrodia Tubers

Sekizaki

Kuninaga

Yamamoto

et al. 2008

Biological & Pharmaceutical Bulletin

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“…A requirement for a temperature reduction to induce primordia has been reported previously in Armillaria, in an undescribed species from Africa, where cultures colonised at 25 C required a temperature decrease to 20 C to initiate primordia development (Otieno et al 2003). Fruiting in other Armillaria species, however, does not appear to be reliant upon a temperature reduction, or perhaps the higher colonisation temperature prior to movement into cooler growth rooms provides a sufficient temperature decrease.…”

Section: Discussionmentioning

confidence: 80%

A reliable in vitro fruiting system for Armillaria mellea for evaluation of Agrobacterium tumefaciens transformation vectors

et al. 2015

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Armillaria mellea is a serious pathogen of horticultural and agricultural systems in Europe and North America. The lack of a reliable in vitro fruiting system for heterothallic A. mellea has hindered research and required dependence on intermittently available wild-collected basidiospores of endemic genotypes, necessitating the use of variable genetic material in transformation studies. Here we describe a reliable, reproducible in vitro fruiting method for heterothallic A. mellea from the western US. Isolates and growth conditions were evaluated to determine effective fruiting conditions. Following medium colonisation for 4 weeks, cultures were incubated under warm/bright conditions for 4-6 weeks before incubation in dim/cool conditions. Primordia emerged within 3-4 weeks following a temperature decrease and this was most efficient when coupled with a light reduction. Basidiocarps matured within 3-4 weeks and produced viable basidiospores. Agrobacterium tumefaciens and vectors were evaluated by transformation of in vitro-produced basidiospores and a versatile transformation vector was constructed to simplify promoter and marker gene exchange using homologous recombination in yeast. Fruiting bodies and viable basidiospores of A. mellea have been reliably produced in vitro which, coupled with the enhanced knowledge of suitable A. tumefaciens strains and vectors for transformation, will assist future genetic research into this important pathogen.

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“…Only one isolate of the type H was found in Tottori Prefecture. The A. mellea type G pattern corresponded to the pattern of A. mellea isolates from Kenya and São Thomé in the Gulf of Guinea (Otieno et al 2003). However, the Alu I digestion pattern of A. mellea isolates from Japan were different from those of European and North American A. mellea isolates (Harrington and Wingfield 1995;Kim et al 2000;Schulze and Bahnweg 1998).…”

Section: Comparisons Among Armillaria Species In the Worldmentioning

confidence: 87%

Identification of Armillaria species in Japan using PCR-RFLP analysis of rDNA intergenic spacer region and comparisons of Armillaria species in the world

Matsushita

Suzuki

2005

Journal of Forest Research

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Armillaria species from Japan were characterized using polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) of the intergenic spacer region-1 (IGS-1) of ribosomal DNA (rDNA). Eleven different digestion patterns by restriction endonuclease Alu I were found among 70 isolates of seven Armillaria species in Japan. Isolates within Armillaria nabsnona, A. ostoyae, A. cepistipes, and Japanese biological species E showed the same Alu I digestion patterns. Five Alu I patterns were detected for A. gallica, three patterns for A. mellea, and two patterns for A. tabescens. Seven Armillaria species in Japan were clearly distinguished by using the profiles obtained when PCR products were digested with Alu I, Msp I, and Hae III restriction enzymes. There was considerable variability of Alu I restriction sites within the IGS-1 between the isolates of five Armillaria species, A. gallica, A. nabsnona, A. cepistipes, A. mellea, and A. tabescens, in Japan and those of their European and North American counterparts.

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Characterization ofArmillariaisolates from tea (Camellia sinensis) in Kenya

Cited by 16 publications

References 26 publications

Identification of Armillaria nabsnona in Gastrodia Tubers

Identification of Armillaria nabsnona in Gastrodia Tubers

A reliable in vitro fruiting system for Armillaria mellea for evaluation of Agrobacterium tumefaciens transformation vectors

Identification of Armillaria species in Japan using PCR-RFLP analysis of rDNA intergenic spacer region and comparisons of Armillaria species in the world

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