Development and Analysis of Anaerobic Biofilms Onto Hydrophobic and Hydrophilic Surfaces

Fluorescent in situ hybridization (FISH) with domain and group specific probes that target intracellular 16S rRNA were used to investigate microbial composition of anaerobic biofilms developed on polypropylene (hydrophobic) and glass (hydrophilic) surfaces fitted inside a Modified Robbins Device (MR...

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Bibliographic Details
Published in:Environmental technology 2004-07, Vol.25 (7), p.809-817
Main Authors: Araujo, J.C., Mortara, R., Campos, J.R., Vazoller, R.F.
Format: Article
Language:English
Subjects:
"IN SITU" HYBRIDIZATION
ANAEROBIC BIOFILMS
Applied sciences
Archaea
Bacteria, Anaerobic - genetics
Bacteria, Anaerobic - growth & development
Biofilms - growth & development
Bioreactors
DNA, Bacterial - analysis
Equipment Design
Exact sciences and technology
Glass
HYDROPHOBIC AND HYDROPHILIC SURFACES
In Situ Hybridization, Fluorescence
Methanobacteriaceae
MODIFIED ROBBINS DEVICE
OLIGONUCLEOTIDE PROBE
Pollution
Polypropylenes
RNA, Ribosomal, 16S - analysis
Waste Disposal, Fluid - methods
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Summary:Fluorescent in situ hybridization (FISH) with domain and group specific probes that target intracellular 16S rRNA were used to investigate microbial composition of anaerobic biofilms developed on polypropylene (hydrophobic) and glass (hydrophilic) surfaces fitted inside a Modified Robbins Device (MRD). Crushed anaerobic granular sludge was used as inoculum for biofilm development in the MRD. The inoculum and biofilms formed showed nearly the same microbial composition, both were dominated by hydrogenotrophic methanogenic Archaea related to the Methanobacteriaceae as detected by the specific probe (MB1174). This group accounted for 44 to 90% of the DAPI-stained cells. Cells which hybridized to the Bacteria specific probe (EUB338) accounted for 3-18% of the DAPI-stained cells. After the first day of the biofilm formation experiment, a larger number of cells, 4.6× 10 4 cells mm -2 , could be seen colonizing the polypropylene coupon compared to the glass, 8.2 × 10 3 cells mm -2 . However, after 9 days these numbers were very similar, i.e. 6.3 × 10 5 cells mm -2 and 7.2 × 10 5 cells mm -2 , for the glass and polypropylene coupons, respectively. Our data suggest that the hydrophobicity of the support material did not influence the initial development and the microbial composition of anaerobic biofilms developed in the MRD.
ISSN:0959-3330
1479-487X
DOI:10.1080/09593330.2004.9619372