Gunter Dirix

Identification of different emitting species in the red fluorescent protein DsRed by means of ensemble and single-molecule spectroscopy

The photophysics and photochemistry taking place in the DsRed protein, a recently cloned red fluorescent protein from a coral of the Discosoma genus, are investigated here by means of ensemble and single-molecule time-resolved detection and spectroscopic measurements. Ensemble time-resolved data reveal that 25% of the immature green chromophores are present in tetramers containing only this immature form. They are responsible for the weak fluorescence emitted at 500 nm. The remaining 75% of the immature green chromophores are involved in a fluorescence resonance energy transfer process to the red species. The combination of time-resolved detection with spectroscopy at the single-molecule level reveals, on 543-nm excitation of individual DsRed tetramers, the existence of a photoconversion of the red chromophore emitting at 583 nm and decaying with a 3.2-ns time constant into a super red one emitting at 595 nm and for which the decay time constant ranges between 2.7 and 1.5 ns. The phenomenon is further corroborated at the ensemble level by the observation of the creation of a super red form and a blue absorbing species on irradiation with 532-nm pulsed light at high excitation power. Furthermore, single-molecule experiments suggest that a similar photoconversion process might occur in the immature green species on 488-nm excitation.

Peptide signal molecules and bacteriocins in Gram-negative bacteria: a genome-wide in silico screening for peptides containing a double-glycine leader sequence and their cognate transporters.

Quorum sensing (QS) in Gram-negative bacteria is generally assumed to be mediated by N-acyl-homoserine lactone molecules while Gram-positive bacteria make use of signaling peptides. We analyzed the occurrence in Gram-negative bacteria of peptides and transporters that are involved in quorum sensing in Gram-positive bacteria. Many class II bacteriocins and inducing factors produced by lactic acid bacteria (LAB) and competence stimulating peptides (CSPs) synthesized by streptococci are processed by their cognate ABC-transporters during their secretion. During transport, a conserved leader sequence, termed the double-glycine motif (GG-motif), is cleaved off by the N-terminal domain of the transporter, which belongs to the Peptidase C39 protein family. Several peptides containing a GG-motif were recently described in Gram-negative bacteria (Trends Microbiol 2001;9:164-8). To screen for additional putative GG-motif containing peptides, an in silico strategy based on MEME, HMMER2.2 and Wise2 was designed. Using a curated training set, a motif model of the leader peptide was built and used to screen over 120 fully sequenced bacterial genomes. The screening methodology was applied at the nucleotide level as probably many small peptide genes have not been annotated and may be absent from the non-redundant databases. It was found that 33% of the screened genomes of Gram-negative bacteria contained one or more transporters carrying a Peptidase C39 domain, compared to 44% of the genomes of Gram-positive bacteria. The transporters can be subdivided into four classes on the basis of their domain organization. Genes coding for putative peptides containing 23-142 amino acids and a GG-motif were found in close association with genes coding for Peptidase C39 domain containing proteins. These peptides show structural similarity to bacteriocins and peptide pheromones of Gram-positive bacteria. The possibility of signal transduction based on peptide signaling in Gram-negative bacteria is discussed.

Processing and export of peptide pheromones and bacteriocins in Gram-negative bacteria

Cell-density-dependent gene expression is widespread in bacteria and is mediated by extracellular communication molecules. Gram-negative bacteria often use N-acyl homoserine lactones, whereas cell-cell signaling in Gram-positive bacteria is accomplished using post-translationally processed peptide pheromones. In many Gram-positive bacteria, export of these peptides requires the activity of a dedicated ATP-binding cassette (ABC) transporter, which cleaves off a typical leader peptide termed the double-glycine leader sequence concomitant with translocation across the membrane. Inspection of bacterial genome sequences has revealed the presence of similar ABC transporters, as well as genes encoding peptides with double-glycine-type leader sequences in Gram-negative bacteria, and it is suggested that the postulated transported peptides could perform a signaling function.

Resonance energy transfer in a calcium concentration-dependent cameleon protein.

We report investigations of resonance energy transfer in the green fluorescent protein and calmodulin-based fluorescent indicator constructs for Ca(2+) called cameleons using steady-state and time-resolved spectroscopy of the full construct and of the component green fluorescent protein mutants, namely ECFP (donor) and EYFP (acceptor). EYFP displays a complicated photophysical behavior including protonated and deprotonated species involved in an excited-state proton transfer. When EYFP is excited in the absorption band of the protonated species, a fast nonradiative deactivation occurs involving almost 97% of the excited protonated population and leading to a low efficiency of excited-state proton transfer to the deprotonated species. ECFP displays a multiexponential fluorescence decay with a major contributing component of 3.2 ns. The time-resolved fluorescence data obtained upon excitation at 420 nm of Ca(2+)-free and Ca(2+)-bound YC3.1 cameleon constructs point to the existence of different conformations of calmodulin dependent on Ca(2+) binding. Whereas steady-state data show only an increase in the efficiency of energy transfer upon Ca(2+) binding, the time-resolved data demonstrate the existence of three distinct conformations/populations within the investigated sample. Although the mechanism of the interconversion between the different conformations and the extent of interconversion are still unclear, the time-resolved fluorescence data offer an estimation of the rate constants, of the efficiency of the energy transfer, and of the donor-acceptor distances in the Ca(2+)-free and Ca(2+)-bound YC3.1 samples.

Collective effects in individual oligomers of the red fluorescent coral protein DsRed

We report on single-molecule experiments that were performed on two biological systems, the recently cloned red fluorescent protein of a coral of the Discosoma genus (DsRed) and the enhanced green fluorescent protein, both of which were immobilized in polyvinylalcohol. Fluorescence intensity trajectories were recorded and compared to those of a reference compound, the organic dye hexaphenylbenzene perylenemonoimide. Evidence was found for the presence of DsRed as an oligomer even at subnanomolar concentrations. Both proteins show triplet blinking in the millisecond time range. Collective effects could be observed for the Dsred oligomers.

Use of Dual Marker Transposons to Identify New Symbiosis Genes in Rhizobium.

Rhizobium etli elicits nitrogen-fixing nodules on the roots of Phaseolus vulgaris. Using a composite dual-marker mini-Tn5 transposon carrying combinations of a constitutively expressed gfp gene and a promoterless gusA gene, we identified novel genes required for an efficient symbiosis. The induction of the gusA gene was used to determine the expression level of the different target genes under conditions partly mimicking the symbiotic environment ex planta. The green fluorescence was used to localize the bacteria in infection threads or inside the plant cells. Among the identified R. etli mutants, several produced a Nod− phenotype, whereas others were Fix− or displayed a reduced acetylene reduction activity during symbiosis. Partial sequence analysis of the mutated genes allowed us to classify them as nodulation genes, nitrogen fixation genes, genes possessing various enzymatic functions previously not yet associated with symbiosis, and genes displaying no similarity to any other sequence in the database. This methodology can be used to screen large numbers of mutants in the search for novel genes important for Rhizobium-legume symbiosis, and may be adapted to study other plant-bacterium interactions.

Excited state processes in individual multichromophoric systems

Multichromophoric systems play a key role in biological systems (light harvesting antenna complexes, fluorescent proteins...) and are equally important in material science applications (e.g. light emitting devices (LED) based on conjugated polymers). Our approach to get insight in the excited state processes of such systems is to make use of dendrimers labeled with photostable perylene dyes. Dendrimers synthesis indeed allows changing the number, relative position and orientation of attached chromophores in a controlled way. In the present contribution, excited state processes such as energy hopping, singlet-singlet annihilation, singlet-triplet annihilation are identified in individual tetrachromophoric dendrimers immobilized in a polymer matrix. Similar processes are then demonstrated to occur as well in immobilized tetramers of a red fluorescent protein from a coral of the Discosoma genus (DsRed).