Meios de cultura para detectar e critérios para avaliar e divulgar atividade de enzimas extracelulares produzidas por fungos fitopatogênicos

Ferreira, Ana Beatriz Monteiro; Fischer, Ivan Herman; Leite, Luís Garrigós; Padovani, Carlos Roberto; Bueno, César Júnior

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Sumário

SCIENTIFIC ARTICLE, PLANT PATOLOGY • Arq. Inst. Biol. 86 • 2019 • https://doi.org/10.1590/1808-1657000592017 copiar

Meios de cultura para detectar e critérios para avaliar e divulgar atividade de enzimas extracelulares produzidas por fungos fitopatogênicos

Autoria SCIMAGO INSTITUTIONS RANKINGS

RESUMO:

As enzimas extracelulares estão envolvidas na patogênese de fungos em plantas. Atualmente, não há uma padronização de meios de cultura, formas de analisar e divulgar os dados de enzimas extracelulares produzidas em condições in vitro. Assim, o presente trabalho objetivou comparar os meios de cultura específicos relatados na literatura (normal) com o meio de batata-dextrose-ágar mais adição do substrato específico para produção de enzimas extracelulares por três diferentes fungos fitopatogênicos habitantes de solo (Fusarium solani f. sp. passiflorae, Sclerotium rolfsii e Rhizoctonia solani AG-4 HGI), bem como avaliar os dados das enzimas por cinco critérios diferentes. O delineamento experimental adotado foi o inteiramente ao acaso, em esquema de três fatores (meios, isolados e enzimas), com seis repetições. As enzimas investigadas foram amilase, carboximetilcelulase, lipase, lacase, catalase e gelatinase. Os meios normais detectaram mais enzimas, e essa detecção foi mais precisa em comparação com os meios de batata-dextrose-ágar mais o substrato específico. Os critérios que calcularam a área da coroa circular para as enzimas amilase, carboximetilcelulase, lipase e lacase e adotaram a escala de notas para medir a intensidade (0=ausência até 4=intensa) de catalase e gelatinase foram os melhores para avaliar e divulgar os resultados das enzimas. Assim, sugere-se padronizar os meios normais para estudos de produção de enzimas, bem como os critérios citados para avaliar e divulgar os dados das atividades das referidas enzimas.

PALAVRAS-CHAVE:
enzimas; fungos fitopatogênicos habitantes de solo; metodologia

Fungi	Average	Extracellular enzynes
		Note scales
		Catalase		Gelatinase
Fusarium solani f. sp. passiflorae	Normal	2.0 (2.0; 2.0)¹ a A α 2.0 (2.0; 2.0) a A α		2.0 (2.0; 2.0) b A α 1.0 (1.0; 2.0) b B α
Fusarium solani f. sp. passiflorae	PDA	2.0 (2.0; 2.0)¹ a A α 2.0 (2.0; 2.0) a A α		2.0 (2.0; 2.0) b A α 1.0 (1.0; 2.0) b B α
Sclerotium rolfsii	Normal	2.0 (2.0; 2.0) a A α 2.0 (2.0; 2.0) a A α		1.0 (1.0; 1.0) c A β 1.0 (1.0; 2.0) b A β
Sclerotium rolfsii	PDA	2.0 (2.0; 2.0) a A α 2.0 (2.0; 2.0) a A α		1.0 (1.0; 1.0) c A β 1.0 (1.0; 2.0) b A β
Rhizoctonia solani AG-4 HGI	Normal	2.0 (2.0; 2.0) a A β 2.0 (2.0; 2.0) a A β		4.0 (3.0; 4.0) a A α 4.0 (4.0; 4.0) a A α
Rhizoctonia solani AG-4 HGI	PDA	2.0 (2.0; 2.0) a A β 2.0 (2.0; 2.0) a A β		4.0 (3.0; 4.0) a A α 4.0 (4.0; 4.0) a A α
Control	Normal	1.0 (1.0; 1.0) b A α 1.0 (1.0; 1.0) b A α		1.0 (1.0; 1.0) c A α 1.0 (1.0; 1.0) b A α
Control	PDA	1.0 (1.0; 1.0) b A α 1.0 (1.0; 1.0) b A α		1.0 (1.0; 1.0) c A α 1.0 (1.0; 1.0) b A α
Fungi	Average	Extracellular enzynes
		Enzyme activity area (mm²)
		Amylase	Carboxymethylcellulase	Lipase	Laccase
Fusarium solani f. sp. passiflorae	Normal	0.0 (0.0; 0.0) a A Ω 0.0 (0.0; 0.0) a A β	290.4 (230.8; 452.2) a A β 297.1 (58.1; 429.9) a A α	638.8 (533.2; 784.2) a B β 0.0 (0.0; 0.0) a B β	0.0 (0.0; 0.0) b A Ω 0.0 (0.0; 0.0) b A β
Fusarium solani f. sp. passiflorae	PDA	0.0 (0.0; 0.0) a A Ω 0.0 (0.0; 0.0) a A β	290.4 (230.8; 452.2) a A β 297.1 (58.1; 429.9) a A α	638.8 (533.2; 784.2) a B β 0.0 (0.0; 0.0) a B β	0.0 (0.0; 0.0) b A Ω 0.0 (0.0; 0.0) b A β
Sclerotium rolfsii	Normal	0.0 (0.0; 0.0) a A β 0.0 (0.0; 0.0) a A β	0.0 (0.0; 0.0) b A β 0.0 (0.0; 0.0) b A β	0.0 (0.0; 0.0) c A β 0.0 (0.0; 0.0) a A β	388.6 (0.0; 637.4) a A α 377.5 (0.0; 450.4) a A α
Sclerotium rolfsii	PDA	0.0 (0.0; 0.0) a A β 0.0 (0.0; 0.0) a A β	0.0 (0.0; 0.0) b A β 0.0 (0.0; 0.0) b A β	0.0 (0.0; 0.0) c A β 0.0 (0.0; 0.0) a A β	388.6 (0.0; 637.4) a A α 377.5 (0.0; 450.4) a A α
Rhizoctonia solani AG-4 HGI	Normal	0.0 (0.0; 0.0) a A β 0.0 (0.0; 0.0) a A β	0.0 (0.0; 0.0) b A β 0.0 (0.0; 0.0) b A β	372.0 (337.6; 472.0) b A α 0.0 (0.0; 0.0) a B β	240.1 (155.4; 364.8) a A α 417.4 (417.4; 615.4) a A α
Rhizoctonia solani AG-4 HGI	PDA	0.0 (0.0; 0.0) a A β 0.0 (0.0; 0.0) a A β	0.0 (0.0; 0.0) b A β 0.0 (0.0; 0.0) b A β	372.0 (337.6; 472.0) b A α 0.0 (0.0; 0.0) a B β	240.1 (155.4; 364.8) a A α 417.4 (417.4; 615.4) a A α
Control	Normal	0.0 (0.0; 0.0) a A α 0.0 (0.0; 0.0) a A α	0.0 (0.0; 0.0) b A α 0.0 (0.0; 0.0) b A α	0.0 (0.0; 0.0) c A α 0.0 (0.0; 0.0) a A α	0.0 (0.0; 0.0) b A α 0.0 (0.0; 0.0) b A α
Control	PDA	0.0 (0.0; 0.0) a A α 0.0 (0.0; 0.0) a A α	0.0 (0.0; 0.0) b A α 0.0 (0.0; 0.0) b A α	0.0 (0.0; 0.0) c A α 0.0 (0.0; 0.0) a A α	0.0 (0.0; 0.0) b A α 0.0 (0.0; 0.0) b A α

Enzymes	F. solani	Control	F. solani	Control	F. solani	Control	F. solani	Control	F. solani	Control
	Criteria to evaluate extracellular enzymes
	1 - Note scale and Area (mm²)		2 - EI		3 - Pz		4 - RA		5 - Symbols and Halo (mm) + Note scale
Catalase	2.0² a B (2.0; 2.0)	1.0 a A (1.0; 1.0)	*		*		*		+	-
Gelatinase	2.0 a B (2.0; 2.0)	1.0 a A (1.0; 1.0)	*		*		*		+	-
Amylase	0.0 a A (0.0; 0.0)	0.0 a A (0.0; 0.0)	1.0 b A (1.0; 1.0)	1.0 a A (1.0; 1.0)	1.0 (N)	1.0 (N)	NSEA	NSEA	0 (0)	0 (0)
CMCase¹	290.4 b B (230.8; 452.2)	0.0 a A (0.0; 0.0)	0.92 b A (0.88; 0.94)	1.0 a A (1.0; 1.0)	0.92 (P)	1.0 (N)	NSEA	NSEA	4 (1)	0 (0)
Lipase	638.8 c B (533.2; 784.2)	0.0 a A (0.0; 0.0)	0.87 a A (0.85; 0.89)	1.0 a B (1.0; 1.0)	0.87 (P)	1.0 (N)	NSEA	NSEA	8 (2)	0 (0)
Laccase	0.0 a A (0.0; 0.0)	0.0 a A (0.0; 0.0)	1.0 b A (1.0; 1.0)	1.0 a A (1.0; 1.0)	1.00 (N)	1.0 (N)	NSEA	NSEA	0 (0)	0 (0)
Enzymes	S. rolfsii	Control	S. rolfsii	Control	S. rolfsii	Control	S. rolfsii	Control	S. rolfsii	Control
	Criteria to evaluate extracellular enzymes
	1 - Note scale and Area (mm²)		2 - EI		3 - Pz		4 - RA		5 - Symbols and Halo (mm) + Note scale
Catalase	2.0 a B (2.0; 2.0)	1.0 a A (1.0; 1.0)	*		*		*		+	-
Gelatinase	1.0 b A (1.0; 1.0)	1.0 a A (1.0; 1.0)	*		*		*		-	-
Amylase	0.0 a A (0.0; 0.0)	0.0 a A (0.0; 0.0)	1.0 a A (1.0; 1.0)	1.0 a A (1.0; 1.0)	1.0 (N)	1.0 (N)	NSEA	NSEA	0 (0)	0 (0)
CMCase¹	0.0 a A (0.0; 0.0)	0.0 a A (0.0; 0.0)	1.0 a A (1.0; 1.0)	1.0 a A (1.0; 1.0)	1.0 (N)	1.0 (N)	NSEA	NSEA	0 (0)	0 (0)
Lipase	0.0 a A (0.0; 0.0)	0.0 a A (0.0; 0.0)	1.0 a A (1.0; 1.0)	1.0 a A (1.0; 1.0)	1.0 (N)	1.0 (N)	NSEA	NSEA	0 (0)	0 (0)
Laccase	388.6 b A (0.0; 637.4)	0.0 a B (0.0; 0.0)	0.92 a A (0.89; 1.0)	1.0 a A (1.0; 1.0)	0.93 (P)	1.0 (N)	NSEA	NSEA	4 (1)	0 (0)
Enzymes	R. solani	Control	R. solani	Control	R. solani	Control	R. solani	Control	R. solani	Control
	Criteria to evaluate extracellular enzymes
	1 - Note scale and Area (mm²)		2 - EI		3 - Pz		4 - RA		5 - Symbols and Halo (mm) + Note scale
Catalase	2.0 b B (2.0; 2.0)	1.0 a A (1.0; 1.0)	*		*		*		+	-
Gelatinase	4.0 a B (3.0; 4.0)	1.0 a A (1.0; 1.0)	*		*		*		+++	-
Amylase	0.0 a A (0.0; 0.0)	0.0 a A (0.0; 0.0)	1.0 b A (1.0; 1.0)	1.0 a A (1.0; 1.0)	1.0 (N)	1.0 (N)	NSEA	NSEA	0 (0)	0 (0)
CMCase¹	0.0 a A (0.0; 0.0)	0.0 a A (0.0; 0.0)	1.0 b A (1.0; 1.0)	1.0 a A (1.0; 1.0)	1.0 (N)	1.0 (N)	NSEA	NSEA	0 (0)	0 (0)
Lipase	372.0 c A (337.6; 472.0)	0.0 a B (0.0; 0.0)	0.89 a B (0.87; 0.91)	1.0 a A (1.0; 1.0)	0.89 (P)	1.0 (N)	NSEA	NSEA	5 (1)	0 (0)
Laccase	240.1 b A (155.4; 364.8)	0.0 a B (0.0; 0.0)	0.89 a B (0.83; 0.91)	1.0 a A (1.0; 1.0)	0.87 (P)	1.0 (N)	NSEA	NSEA	5 (1)	0 (0)

Criterion 1 - Calculation of the circular crown area. Formula described by GIECK (without yearGIECK, K. Manual de fórmulas técnicas. São Paulo: Hemus.). This formula was used to quantify the enzymes amylase, carboxymethylcellulase, lipase, and laccase. The catalase and gelatinase enzymes were quantified by symbols describing their intensity, which were later transformed into a note scale, with 1 = absent (or - = symbol: absent); 2 = weak (or + = symbol: weak); 3 = moderate (or ++ = symbol: moderate); 4 = intense (or +++ = symbol: intense). For catalase, the intensity refers to the size of bubble formation and for gelatinase, the liquefaction or not of the medium;
Criterion 2 - Calculation of the enzymatic index (EI). Formula described by BOCCHESE et al. (2003BOCCHESE, C.A.C.; MARTINELLI, J.A.; MATSUMURA, A.T.S.; FEDERIZZI, L.C.; PRESTES, A.M. Virulência, atividade enzimática e padrões de isoesterases de isolados de Pyrenophora chaetomioides, agente etiológico da mancha de grãos e folhas de aveia. Fitopatologia Brasileira, Brasília, v.28, n.1, p.11-16, 2003. http://doi.org/10.1590/S0100-41582003000100002
http://doi.org/10.1590/S0100-41582003000... ). This index was applied to the enzymes amylase, carboxymethylcellulase, lipase, and laccase;
Criterion 3 - Calculation of the Pz index. Formula described by HANKIN; ANAGNOSTAKIS (1975HANKIN L.; ANAGNOSTAKIS, S.L. The use of solid media for detection of enzyme production by fungi. Mycologia, New York, v.61, n.3, p.597-607, 1975. https://doi.org/10.2307/3758395
https://doi.org/10.2307/3758395... ). According to the index, enzyme activity is negative (N) when Pz = 1, positive (P) when 0.64 ≤ Pz < 1, and strongly positive (SP) when Pz < 0,64. This index was applied to the enzymes amylase, carboxymethylcellulase, lipase, and laccase;
Criterion 4 - Calculation of the RA index. Formula and criterion described by KRISHNAN et al. (2011KRISHNAN, A.; ALIAS, S.A.; WONG, C.M.V.L.; KA-LAI, P.; CONVEY, P. Extracellular hydrolase enzyme production by soil fungi from King George Island, Antarctica. Polar Biology, Berlin, v.34, p.1535-1542, 2011. https://doi.org/10.1007/s00300-011-1012-3
https://doi.org/10.1007/s00300-011-1012-... ) and other authors. If RA > 1, enzymatic activity (SEA) is significant, and if RA < 1, enzymatic activity is not significant (NSEA). This index was applied to the enzymes amylase, carboxymethylcellulase, lipase, and laccase;
Criterion 5 - Method described by BASTOS (2005BASTOS C.N. Produção de enzimas extracelulares por Crinipellis perniciosa. Fitopatologia Brasileira, Brasília, v.30, n.3, p.286-288, 2005. http://doi.org/10.1590/S0100-41582005000300011
http://doi.org/10.1590/S0100-41582005000... ). Measurement of the diameter of the halo formed around the colonies, represented by the note scale: (0), no enzyme production; (1), halo with diameter between 1-5 mm; (2), diameter between 5-10 mm; (3), diameter between 10-20 mm; (4), diameter between 20-30 mm; e (5), diameter higher than 30 mm. This method was applied to the enzymes amylase, carboxymethylcellulase, lipase, and laccase. To evaluate the enzymes catalase and gelatinase, BASTOS (2005BASTOS C.N. Produção de enzimas extracelulares por Crinipellis perniciosa. Fitopatologia Brasileira, Brasília, v.30, n.3, p.286-288, 2005. http://doi.org/10.1590/S0100-41582005000300011
http://doi.org/10.1590/S0100-41582005000... ) used symbols for a subjective estimation of enzyme production, based on the intensity of the enzymes formed in the medium: +++ intense; ++ moderate; + weak; and - absent;
^*The method does not contemplate enzyme evaluation; ¹carboxymethylcellulase; ²median and maximum and minimum values of the interquartile half-amplitude data.
Different lowercase letters indicate significance (p < 0.05) among enzymes for each fungus; different uppercase letters indicate significance of the fungus (p < 0.05) within the enzyme, according to Dunn’s multiple comparison test with the Bonferroni correction (ZAR, 2009ZAR, J.H. Biostatistical analysis. 5. ed. New Jersey: Prentice-Hall. 2009. 994p.).

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[1] *Corresponding author: cjbueno@biologico.sp.gov.br