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Bacterial diversity in closed cryoconite holes in Southern Victoria Land (Antarctica)

Versão mais recente publicado por SCAR - Microbial Antarctic Resource System em Mar 19, 2019

Amplicon sequencing dataset of that profiled Bacteria (16S ssu rRNA gene) in different closed cryoconite holes on the Diamond Glacier and Koettliz Glacier (Southern Victoria Land, Antarctica).

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Webster-Brown J, Hawes I, Jungblut A, Wood S, Christenson H (2019): Bacterial diversity in closed cryoconite holes in Southern Victoria Land (Antarctica). v1.2. SCAR - Microbial Antarctic Resource System. Dataset/Metadata. https://ipt.biodiversity.aq/resource?r=bacteria_in_closed_cryoconite_holes_antarctica&v=1.2

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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.

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Este recurso foi registrado no GBIF e atribuído ao seguinte GBIF UUID: f03a9318-a568-433a-9c5d-db0b88b7e2a4. 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.

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Contatos

Quem criou esse recurso:

Jenny Webster-Brown

University of Canterbury Christchurch NZ

Ian Hawes

University of Canterbury Christchurch NZ

Anne Jungblut

Natural History Museum London GB

Susanna Wood

University of Waikato Hamilton NZ

Hannah Christenson

University of Canterbury Christchurch NZ

Quem pode responder a perguntas sobre o recurso:

Jenny Webster-Brown

University of Canterbury Christchurch NZ

Quem preencher os metadados:

Maxime Sweetlove

Research assistent

Royal Belgian Institute of Natural Sciences Rue Vautier 29 1000 Brussels BE msweetlove@naturalsciences.be

Quem mais foi associado com o recurso:

Usuário

Cobertura Geográfica

Diamind and Koettliz Glaciers (Southern Victoria Land, Antarctica)

Coordenadas delimitadoras	Sul Oeste [-79.5, 159], Norte Leste [-78.08, 165.03]

Cobertura Taxonômica

Bacteria were profiled based on amplicon sequencing of the 16S ssu rRNA gene

Domínio	Bacteria (Bacteria)

Métodos de Amostragem

Access through the ice lid was accomplished using a 50-mm diameter Kovacs ice drill, which was cleaned between each hole with antibacterial wipes. Water samples were collected directly into three 60-mL centrifuge tubes for determination of major ions and isotopes, using a manual vacuum apparatus. A sample (1 L) was collected by vacuum into an acid-washed PVC bottle. A subsample (100 mL) filtered (Whatman GF/F) into an acid-washed polyethylene bottle and frozen for later nutrient analysis.

Área de Estudo	Cryoconite holes were sampled in the austral summer (December–January), during Antarctic field seasons between2010 and 2013 at the Koettlitz Glacier and Diamond Glacier (Southern Victoria Land, Antarctica). Only cryoconite holes with a diameter of greater than 30 cm (which were typically also greater than 35 cm deep) routinely contained liquid water, and were targeted for sampling. Selection was based on replicate N+1 being the next encountered appropriately sized closed cryoconite hole encountered in a random direction from replicate N.

Área de Estudo

Cryoconite holes were sampled in the austral summer (December–January), during Antarctic field seasons between2010 and 2013 at the Koettlitz Glacier and Diamond Glacier (Southern Victoria Land, Antarctica). Only cryoconite holes with a diameter of greater than 30 cm (which were typically also greater than 35 cm deep) routinely contained liquid water, and were targeted for sampling. Selection was based on replicate N+1 being the next encountered appropriately sized closed cryoconite hole encountered in a random direction from replicate N.

Descrição dos passos do método:

DNA was extracted from sediment using the MoBio Power Soil kit (USA). Biosystems, USA). A region of the 16S rRNA gene covering the V3 and 4 sections was ampli ed by PCR (iCycler; Biorad) using bacterial-speci c primers 515F and 806R (Caporaso et al. 2011). PCR reactions were performed in 50 μL volumes with the reaction mixture containing; 45 μL of Platinu PCR SuperMix High Fidelity (Life Technologies, USA), 10 μM of each primer, and 10–20 ng of template DNA. The reaction mix- ture was held at 94◦C for 2 min followed by 27 cycles of 94◦C for 30 s, 54◦C for 30 s, 68◦C for 45 s, with a nal extension step at 68◦C for 5 min. PCR products were puri ed (Agencour AMPur XP Kit; Beckman Coulter, USA), quanti ed (Qubit 20 Fluorometer, Life Technologies, USA), diluted to 1 ng μL−1 and submitted to New Zealand Genomics Limited (Auckland, New Zealand) for library preparation. Libraries were sequenced on a MiSeq Illumina platform (2 × 250 reads).

Citações bibliográficas

Webster-Brown, J. G., Hawes, I., Jungblut, A. D., Wood, S. A., & Christenson, H. K. (2015). The effects of entombment on water chemistry and bacterial assemblages in closed cryoconite holes on Antarctic glaciers. FEMS microbiology ecology, 91(12). https://doi.org/10.1093/femsec/fiv144

Metadados Adicionais

Identificadores alternativos	f03a9318-a568-433a-9c5d-db0b88b7e2a4
	https://ipt.biodiversity.aq/resource?r=bacteria_in_closed_cryoconite_holes_antarctica