Fungi (LSU) in soils from the South Shetland island, Antarctic Peninsula island, and Union Glacier

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Como citar

Pesquisadores deveriam citar esta obra da seguinte maneira:

Baeza M, Barahona S, Alcaino J, Cifuentes V (2018): Fungi (LSU) in soils from the South Shetland island, Antarctic Peninsula island, and Union Glacier. v1.3. SCAR - Microbial Antarctic Resource System. Dataset/Metadata. https://ipt.biodiversity.aq/resource?r=fungi_soils_s_shetland_and_antarctica&v=1.3

Direitos

Pesquisadores devem respeitar a seguinte declaração de direitos:

O editor e o detentor dos direitos deste trabalho é SCAR - Microbial Antarctic Resource System. This work is licensed under a Creative Commons Attribution (CC-BY 4.0) License.

GBIF Registration

Este recurso foi registrado no GBIF e atribuído ao seguinte GBIF UUID: 11c8e968-361d-4cea-abae-67450fa03fe8. SCAR - Microbial Antarctic Resource System publica este recurso, e está registrado no GBIF como um publicador de dados aprovado por Scientific Committee on Antarctic Research.

Palavras-chave

Metadata

Contatos

Marcelo Baeza

Originador ●
Ponto De Contato

Universidad de Chile

Santiago

CL

Salvador Barahona

Originador

Universidad de Chile

Santiago

CL

Jennifer Alcaino

Originador

Universidad de Chile

Santiago

CL

Victor Cifuentes

Originador

Universidad de Chile

Santiago

CL

Maxime Sweetlove

Provedor Dos Metadados

Research assistent

Royal Belgian Institute for Natural Sciences

Rue Vautier 29

1000 Brussels

BE

msweetlove@naturalsciences.be

Cobertura Geográfica

South Shetland Islands, Union Glacier (Antarctica)

Coordenadas delimitadoras	Sul Oeste [-79,82, -83,31], Norte Leste [-62,1, -58,1]

Cobertura Taxonômica

LSU marker gene for microbial soil Fungi

Filo	Fungi (Fungi)

Cobertura Temporal

Data Inicial / Data final	2010-01-01 / 2015-01-01

Dados Sobre o Projeto

Nenhuma descrição disponível

Título	FONDECYT grant 1130333
Financiamento	This work was supported by Comisión Nacional de Investigación Científica y Tecnológica (No. FONDECYT grant 1130333).

O pessoal envolvido no projeto:

Marcelo Baeza

Salvador Barahona

Jennifer Alcaino

Victor Cifuentes

Métodos de Amostragem

Samples were collected in sterile 50 ml plastic tubes, which were sealed and shipped at -20°C to the Genetics Laboratory of the Faculty of Science at the Universidad de Chile. Once samples arrived at the laboratory, they were maintained at -80°C until processing.

Área de Estudo	Soil samples were gathered during several expeditions to Antarctica, including Union Glacier, Lagotellerie island, King George, Deception, Snow, Dee, Livingstone, Greenwich, Robert, Nelson and Litchfield islands.

Descrição dos passos do método:

A PowerSoil DNA Isolation Kit (MO BIO Laboratories Inc., Carlsbad, CA, United States) was used for direct DNA extraction from soil samples. The manufacturers’ instructions were followed, with only one modification, the disruption step, was performed using a Mini Beadbeater-16 cell disrupter (BioSpec Bartlesville, United States) instead of vortex agitation, as no PCR-amplicons were obtained in reactions using samples obtained through vortex agitation.
The PCR reactions were performed using 1 μl of DNA sample (direct or 1/10 dilution), 5 units of Taq DNA polymerase, dNTP mix at 0.4 mM each, forward and reverse primers at 1 mM final each, PCR buffer and MgCl2 2 mM. Amplification was performed using a 2720 (Applied Biosystems) thermal cycler using the following protocol: initial denaturation at 94°C for 3 min; 35 cycles of denaturation at 94°C for 30 s, annealing at 50°C for 3 min, and extension at 72°C for 3 min; and a final extension step at 72°C for 10 min. The universal primers F63 (5′-GCA TAT CAA TAA GCG GAG GAA AAG-3′) and LR3 (5′-GGT CCG TGT TTC AAG ACG G-3′) were used; these primers have been described as specific for amplifying the fungal D1/D2 region of the large subunit ribosomal gene (LSU). In all PCR reactions, the same forward primer (F63) was used, but the reverse primer (LR3) was specific for each soil sample as a 454 adapter, a specific barcode and a linker sequence were added.
Sequencing was performed at OMICS Solutions (Santiago, Chile) using the Ion 314TM Chip Kit v2 (Thermo Fisher) and Ion Torrent personal genome machine (PGM), according to the manufacturer’s instructions (Rothberg et al., 2011). Three independent runs were performed: (i) samples from King George Island; (ii) samples from Deception, Snow, Dee, Livingstone, Greenwich, Robert, Nelson and Litchfield islands; and iii) samples from Lagotellerie and Union Glacier.

Citações bibliográficas

Baeza, M., Barahona, S., Alcaíno, J., & Cifuentes, V. (2017). Amplicon-Metagenomic Analysis of Fungi from Antarctic Terrestrial Habitats. Frontiers in microbiology, 8, 2235.
Carrasco, M., Rozas, J. M., Barahona, S., Alcaíno, J., Cifuentes, V., & Baeza, M. (2012). Diversity and extracellular enzymatic activities of yeasts isolated from King George Island, the sub-Antarctic region. BMC microbiology, 12(1), 251.
Troncoso, E., Barahona, S., Carrasco, M., Villarreal, P., Alcaíno, J., Cifuentes, V., & Baeza, M. (2017). Identification and characterization of yeasts isolated from the South Shetland Islands and the Antarctic Peninsula. Polar Biology, 40(3), 649-658.
Barahona, S., Yuivar, Y., Socias, G., Alcaíno, J., Cifuentes, V., & Baeza, M. (2016). Identification and characterization of yeasts isolated from sedimentary rocks of Union Glacier at the Antarctica. Extremophiles, 20(4), 479-491.

Metadados Adicionais

Identificadores alternativos	11c8e968-361d-4cea-abae-67450fa03fe8
	https://ipt.biodiversity.aq/resource?r=fungi_soils_s_shetland_and_antarctica