Fungal communities (ITS) in Antarctic brines.

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Luigimaria B, Sannino C, Selbmann L, Battitel D, Zucconi L, Azzaro M, Turchetti B, Buzzini P, Gugliemin M (2019): Fungal communities (ITS) in Antarctic brines.. v1.1. SCAR - Microbial Antarctic Resource System. Dataset/Metadata. https://ipt.biodiversity.aq/resource?r=fungal_its_communities_in_antarctic_brines&v=1.1

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L’éditeur et détenteur des droits de cette ressource est SCAR - Microbial Antarctic Resource System. Ce travail est sous licence Creative Commons Attribution (CC-BY) 4.0.

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Cette ressource a été enregistrée sur le portail GBIF, et possède l'UUID GBIF suivante : 50dc522a-3200-454c-b0ed-240b0e247923. SCAR - Microbial Antarctic Resource System publie cette ressource, et est enregistré dans le GBIF comme éditeur de données avec l'approbation du Scientific Committee on Antarctic Research.

Mots-clé

Metadata

Contacts

Borruso Luigimaria

Créateur ●
Personne De Contact

University of Bozen-Bolzano

Bozen-Bolzano

IT

Ciro Sannino

Créateur

University of Perugia

Perugia

IT

Laura Selbmann

Créateur

University of Tuscia

Viterbo

IT

Dario Battitel

Créateur

University Ca’ Foscari

Venice

IT

Laura Zucconi

Créateur

University of Tuscia

Viterbo

IT

Maurizio Azzaro

Créateur

National Research Council

Messina

IT

Benedetta Turchetti

Créateur

University of Perugia

Perugia

IT

Pietro Buzzini

Créateur ●
Personne De Contact

University of Perugia

Perugia

IT

Mauro Gugliemin

Créateur

Insubria University

Varese

IT

Maxime Sweetlove

Fournisseur Des Métadonnées

Research assistent

Royal Belgian Istitute for Natural Sciences

Rue Vautier 29

1000 Brussels

BE

msweetlove@naturalsciences.be

Couverture géographique

Flat Tarn Area, McMurdo Dry Valleys, Victoria land Antarctica

Enveloppe géographique	Sud Ouest [-75,667, 162,5], Nord Est [-75,667, 162,5]

Couverture taxonomique

Fungi, ITS2 marker gene

Phylum	Fungi (Fungi)

Couverture temporelle

Date de début	2014-01-01

Données sur le projet

Pas de description disponible

Titre	Fungal communities (ITS) in Antarctic brines.
Financement	This research was supported by grants from the National Antarctic Research Program (PNRA), Italian Ministry of Education and Research (Research Project PNRA AZ/1.05) and from the National Antarctic Museum (MNA).

Les personnes impliquées dans le projet:

Borruso Luigimaria

Méthodes d'échantillonnage

In the studied lake (280 m long and 100 m wide, maximum depth around 6 m) the brines were located only within a deep trough in correspondence of which a pingo like feature (PLF) occurs. PLF is a frost mound that intruded the lake ice surface reaching a maximum height of 45 cm and extending within an area of approximately of 500 m2. Below that mound, brines have been preliminarily identified using GPR data; they were then reached and sampled through a 51 mm diameter borehole that was drilled in the center of the frost mound using a semi-portable core auger. In particular, the first pocket of liquid brine (TF1) was found between 3.78 m, and 3.98 m. TF1 was separated by the second pocket of liquid brine (TF2) (0.84 m thick) by only a 12 cm layer of ice (containing some organic material inclusions). Below TF2 additional frozen sediments rich in organic content occurred between 4.94 m and the bottom of the borehole (5.68 m). Both brines were collected in sterile Pyrex bottles using a peristaltic pump and sterile tubing. After collections, the brines were stored at −20 °C in the dark at Mario Zucchelli Station (MZS) prior to their delivery to laboratories for chemical and microbiological analyses.

Etendue de l'étude	Three replicate samples were taken from two separate brine layers in a lake in Tarn Flat area (75°4′S 162°30′E), an ice-free area (ca. 100 km2) in the north to the McMurdo Dry Valley in Victoria Land.

Description des étapes de la méthode:

Total DNA from brines samples was aseptically extracted using Power Water DNA Isolation Kit (Qiagen, Germany) following the operating instructions. Prior to DNA extraction, the brines were thawed at 4 °C and aseptically filtered in order to collect the biomass present in each brine on sterile cellulose acetate filter (cutoff = pore size 0.2 µm Sartorius Stedim, Biotech, Germany). The quality and quantity of DNA extracted was determined by using QuBit 2.0 Fluorometer Assay (Life Technologies Corporation) and by NanoDrop 2000 c spectrophotometer (Thermo Fisher Scientific, Waltham, MA, USA). Three replicates for each brine were run on Illumina MiSeq.
Fungal internal transcribed spacer region 2 (ITS2) was amplified using IlluAdp_ITS31_NeXTf 5′-CATCGATGAAGAACGCAG-3′ and IlluAdp_ITS4_NeXTr5′-TCCTCCGCTTATTGATATGC-3′60. The PCR products were sequenced using the Illumina MiSeq platforms, following the standard protocols of the company STAB Vida Lda. (Caparica, Portugal).

Citations bibliographiques

Forte, E., Dalle Fratte, M., Azzaro, M., & Guglielmin, M. (2016). Pressurized brines in continental Antarctica as a possible analogue of Mars. Scientific reports, 6, 33158.
Borruso, L., Sannino, C., Selbmann, L., Battistel, D., Zucconi, L., Azzaro, M., ... & Guglielmin, M. (2018). A thin ice layer segregates two distinct fungal communities in Antarctic brines from Tarn Flat (Northern Victoria Land). Scientific reports, 8.

Métadonnées additionnelles

Identifiants alternatifs	50dc522a-3200-454c-b0ed-240b0e247923
	https://ipt.biodiversity.aq/resource?r=fungal_its_communities_in_antarctic_brines