In vitro establishment of Bambusa oldhamii Munro from field-grown matrices and molecular identification of endophytic bactéria

Pasqualini, Ana Paula de Azevedo; Schneider, Gabriela Xavier; Fraga, Hugo Pacheco de Freitas; Biasi, Luiz Antonio; Quoirin, Marguerite

doi:10.1590/1983-40632019v4953673

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Special Supplement: Bamboo • Pesqui. Agropecu. Trop. 49 • 2019 • https://doi.org/10.1590/1983-40632019v4953673 copy

In vitro establishment of Bambusa oldhamii Munro from field-grown matrices and molecular identification of endophytic bactéria

Estabelecimento in vitro de Bambusa oldhamii Munro a partir de matrizes cultivadas a campo e identificação molecular de bactéria endofítica

Authorship SCIMAGO INSTITUTIONS RANKINGS

ABSTRACT

In plant micropropagation, the establishment stage is difficult, due to the presence of microorganisms in tissues from field-grown matrices, especially for bamboo. This study aimed to establish an efficient asepsis protocol for Bambusa oldhamii explants from field plants, as well as to carry out the molecular identification of a possible endophytic bacterial isolate. The explants were exposed to 70 % alcohol, 1 % sodium hypochlorite (NaOCl), 0.1 % mercuric chloride (HgCl₂), thiophanate-methyl (Cercobin^®) and chlorhexidine digluconate (2 % Riohex^®) in different combinations, and introduced into Murashige and Skoog culture medium (solid or liquid), supplemented or not with 4 mL L^-1 of Plant Preservative Mixture (PPM^TM), totaling seven treatments. The asepsis and immersion of the explants in the liquid culture medium containing 4 mL L^-1 of PPM^TM visually inhibited the bacterial and fungal growth, allowed the development of shoots with a mean length of 2.2 cm and posterior subcultures, being the best treatment used for the in vitro establishment of B. oldhamii. The molecular identification of an endophytic bacterium performed by 16S rDNA sequencing allowed to identify the bacterial isolate as Ralstonia sp., with 100 % of similarity, and the phylogenetic analysis grouped it with Ralstonia pickettii. In addition, the bacterial isolate showed to be sensitive to 4 mL L^-1 of PPM^TM by the minimum inhibitory concentration test.

KEYWORDS:
Ralstonia; bamboo; micropropagation

Treatments	Bacterial growth (%)		Fungal growth (%)		Total microbial growth (%)		Length of new shoots (cm)
T1	17	A	46	B	63	BC	1.4	AB
T2	8	A	4	A	12	A	0.8	B
T3	8	A	25	AB	33	AB	1.4	AB
T4	58	B	0	A	58	BC	1.1	B
T5	0	A	13	A	13	A	2.3	A
T6	4	A	0	A	4	A	2.2	A
T7	75	B	8	A	83	C	1.4	AB
CV (%)	6.72		6.73		6.83		8.69

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[TFN1] * T1: immersion in 70 % alcohol for 30 s and 1 % NaOCl for 10 min; T2: immersion in 70 % alcohol for 30 s and 0.1 % HgCl₂ for 10 min; T3: immersion in 70 % alcohol for 30 s, 0.1 % HgCl₂ for 10 min and 1 % NaOCl for 10 min; T4, T5 and T6: immersion in 2 g L^-1 of thiophanate methyl for 24 h, 70 % alcohol for 30 s, 0.1 % HgCl₂ for 10 min and 1 % NaOCl for 10 min; T7: immersion in 1 % chlorhexidine digluconate for 2 h, 2 g L^-1 of thiophanate methyl for 24 h, 70 % alcohol for 30 s, 0.1 % HgCl₂ for 10 min and 1 % NaOCl for 10 min. The treatments T1, T2, T3, T4 and T7 were established in Murashige and Skoog medium (MS); T5 and T6 in MS plus 4 mL L^-1 of PPM^TM; T6 in liquid MS; and the others were semisolid.

[TFN2] ** Means followed by the same letter do not differ by the Tukey test at 5 % of probability.