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Appl Environ Microbiol, February 1998, p. 721-732, Vol. 64, No. 2
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
In Situ Gene Expression in Mixed-Culture Biofilms:
Evidence of Metabolic Interactions between Community Members
Søren
Møller,1
Claus
Sternberg,1
Jens Bo
Andersen,1
Bjarke Bak
Christensen,1
Juan Luis
Ramos,2
Michael
Givskov,1 and
Søren
Molin1,*
Department of Microbiology, The Technical
University of Denmark, DK-2800 Lyngby, Denmark,1
and
Department of Biochemistry and Molecular and Cellular
Biology of Plants, Estación Experimental del
Zaidín, Consejo Superior de Investagaciones
Científicas, Granada, Spain2
Received 21 April 1997/Accepted 3 November 1997
Microbial communities growing in laboratory-based flow chambers
were investigated in order to study compartmentalization of specific
gene expression. Among the community members studied, the focus was in
particular on Pseudomonas putida and a strain of an
Acinetobacter sp., and the genes studied are involved in the biodegradation of toluene and related aromatic compounds. The
upper-pathway promoter (Pu) and the
meta-pathway promoter (Pm) from the TOL plasmid
were fused independently to the gene coding for the green fluorescent
protein (GFP), and expression from these promoters was studied in
P. putida, which was a dominant community member. Biofilms
were cultured in flow chambers, which in combination with scanning
confocal laser microscopy allowed direct monitoring of promoter
activity with single-cell spatial resolution. Expression from the
Pu promoter was homogeneously induced by benzyl alcohol in
both community and pure-culture biofilms, while the Pm
promoter was induced in the mixed community but not in a pure-culture
biofilm. By sequentially adding community members, induction of
Pm was shown to be a consequence of direct metabolic interactions between an Acinetobacter species and P. putida. Furthermore, in fixed biofilm samples organism identity
was determined and gene expression was visualized at the same time by
combining GFP expression with in situ hybridization with
fluorescence-labeled 16S rRNA targeting probes. This combination of
techniques is a powerful approach for investigating structure-function
relationships in microbial communities.
*
Corresponding author. Mailing address: Department of
Microbiology, Building 301, The Technical University of Denmark,
DK-2800 Lyngby, Denmark. Phone: 45 45 25 25 13. Fax: 45 45 88 73 28. E-mail: sm{at}im.dtu.dk.
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