Exploring heterotrophic bacterial diversity of Antarctic samples through cultivation

The microbial diversity on Antarctica is largely under-explored. As part of the AMBIO-project that aims to explore the factors affecting bacterial distribution patterns in Antarctica, nine samples from different regions were investigated. They include two samples from the Belgian Base site at Utstei...

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Bibliographic Details
Main Authors: Peeters, Karolien, Verleyen, Elie, Ertz, Damien, Hodgson, Dominique, Willems, Anne
Format: Conference Object
Language:English
Published: Universiteit Gent. Faculteit Wetenschappen 2009
Subjects:
Biology and Life Sciences
cultivation
heterotrophic bacterial diversity
Antarctica
Antarctic
Shackleton
Pourquoi Pas
Pourquoi-Pas
Pourquoi-Pas?
Ongul
Ongul Island
Langhovde
Lützow-Holm Bay
Frozen Lake
Pensacola Mountains
Utsteinen
Pourquoi Pas Island
Forlidas Pond
Antarc*
Online Access:https://biblio.ugent.be/publication/936624
http://hdl.handle.net/1854/LU-936624
Description
Summary:The microbial diversity on Antarctica is largely under-explored. As part of the AMBIO-project that aims to explore the factors affecting bacterial distribution patterns in Antarctica, nine samples from different regions were investigated. They include two samples from the Belgian Base site at Utsteinen: BB50 from a green microbial/algal mat on gravel from the nunatak and BB115 from a black mat on gravel and rock debris from a frozen lake on the south side of the nunatak Utsteinen; two samples from the Trans-Antarctic Mountains: TM2 from a cyanobacterial mat at the bottom of Forlidas Pond (Pensacola Mountains) and TM4 from Lundström Lake (Shackleton Mountains); a littoral sample PQ1 from Pourquoi-Pas Lake (Pourquoi-Pas Island); samples LA3 (Langhovde Peninsula), SK5 (Skarvsness Peninsula) and WO10 (West Ongul Island) from three lakes at Lützow-Holm Bay, Syowa and sample SO6 from the Schirmacher Oasis. Samples were investigated with a culture-dependent approach. Dilution series were plated on four media (MA, R2A, R2A/10 and PYGV) and incubated at three temperatures (4, 15 and 20ºC). Different types of colonies were picked up for all conditions. As a fast way of screening the isolates, the genotypic typing method rep-PCR fingerprinting was used. Cluster analysis of fingerprint patterns using Bionumerics software revealed a number of clusters (cut-off level 80%) of similar strains and a number of separate isolates. Representatives of each rep-cluster and the separate isolates were used in partial 16S rDNA sequencing to obtain a first approximate identification. For the different samples, between 338 (BB115) and 669 (WO10) isolates were obtained and purified. Rep-PCR fingerprinting analysis resulted in 33 (LA3) to 101 (BB50) clusters and 54 (BB115) to 151 (PQ1) separate isolates (excluding samples WO10 and SO6 for which the analysis is not finished yet). The preliminary results of the 16S rDNA sequencing show a large diversity, distributed over the major phylogenetic groups. The BB samples and TM4 are dominated by ...

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