Mycelial growth and sporulation of Apoharknessia eucalyptorum on different culture media

AUTOR(ES)

Garrett, Alexandre Techy de Almeida

FONTE

Summa phytopathol.

DATA DE PUBLICAÇÃO

14/10/2019

RESUMO

RESUMO Apoharknessia eucalyptorum foi inicialmente descrita em 2017 e identificada em folhas de Eucalyptus dunnii no Sul do Brasil. No entanto, faltam informações sobre o cultivo in-vitro para estudos complementares. No presente estudo folhas de E. dunnii foram inoculadas para demonstrar a patogenicidade de A. eucalyptorum, e o crescimento e esporulação foram avaliados em temperaturas de 15, 20 e 25°C em quatro meios de cultura: extrato de malte-ágar (MEA), batata dextrose-ágar (PDA), suco V8-ágar (V8) e feijão dextrose-ágar (BEAN), sob luz constante. Apoharknessia eucalyptorum causou manchas foliares nas folhas inoculadas. As melhores condições para o crescimento micelial foram em 25°C em PDA, BEAN e MEA. Para a esporulação as melhores condições foram a 25°C em todos os meios testados, e também a 20°C em PDA e BEAN. As características das colônias mudaram com as temperaturas, em 15°C as colônias formaram micélio cotonoso, enquanto que em 25°C o micélio cresceu espalhado pelo meio de cultura formando margens escuras limitadas por micélio branco manchado e conídios. As condições indicadas para o crescimento e esporulação in-vitro de A. eucalyptorum são os meios MEA, PDA e BEAN em 25°C.ABSTRACT Apoharknessia eucalyptorum was first described in 2017 and identified on leaves of Eucalyptus dunnii in Southern Brazil. However, information about in vitro cultivation for complementary studies is lacking. In the present study, leaves of E. dunnii were inoculated to demonstrate the pathogenicity of A. eucalyptorum, and growth and sporulation were evaluated at temperatures of 15, 20, and 25°C on four culture media: malt extract agar (MEA); potato dextrose agar (PDA); V8 juice agar (V8); and bean dextrose agar (BEAN), under constant lighting. Apoharknessia eucalyptorum caused leaf blight on the inoculated leaves. The best conditions for mycelial growth were at 25°C on PDA, BEAN and MEA. Considering sporulation, optimal conditions were 25°C for all tested media and 20°C for PDA and BEAN. Colony characteristics changed with temperature; at 15°C colonies formed a fluffy mycelium, whereas at 25°C mycelium spread across the medium forming dark margins lined by dirty-white mycelium and conidia. The conditions indicated for in vitro growth and sporulation of A. eucalyptorum are the culture media MEA, PDA and BEAN at 25°C

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