Your search keyword '"Poulsen LK"' showing total 19 results

1. New unstable variants of green fluorescent protein for studies of transient gene expression in bacteria.

Author

Andersen JB, Sternberg C, Poulsen LK, Bjorn SP, Givskov M, and Molin S

Subjects

Amino Acid Sequence, Animals, Base Sequence, DNA Primers genetics, Gene Expression, Genes, Reporter, Green Fluorescent Proteins, Half-Life, Luminescent Proteins metabolism, Molecular Sequence Data, Recombinant Proteins genetics, Recombinant Proteins metabolism, Scyphozoa genetics, Escherichia coli genetics, Genetic Variation, Luminescent Proteins genetics, Pseudomonas putida genetics

Abstract

Use of the green fluorescent protein (Gfp) from the jellyfish Aequorea victoria is a powerful method for nondestructive in situ monitoring, since expression of green fluorescence does not require any substrate addition. To expand the use of Gfp as a reporter protein, new variants have been constructed by the addition of short peptide sequences to the C-terminal end of intact Gfp. This rendered the Gfp susceptible to the action of indigenous housekeeping proteases, resulting in protein variants with half-lives ranging from 40 min to a few hours when synthesized in Escherichia coli and Pseudomonas putida. The new Gfp variants should be useful for in situ studies of temporal gene expression.

Published

1998

2. Simultaneous determination of gene expression and bacterial identity in single cells in defined mixtures of pure cultures.

Author

Poulsen LK, Dalton HM, Angles ML, Marshall KC, Molin S, and Goodman AE

Subjects

Bacteria cytology, Escherichia coli cytology, Escherichia coli enzymology, Escherichia coli genetics, In Situ Hybridization, Fluorescence, Moraxella cytology, Moraxella enzymology, Moraxella genetics, Oligonucleotide Probes, beta-Galactosidase metabolism, Bacteria enzymology, Bacteria genetics, Bacteriological Techniques, Gene Expression

Abstract

A protocol was developed to achieve the simultaneous determination of gene expression and bacterial identity at the level of single cells; a chromogenic beta-galactosidase activity assay was combined with in situ hybridization of fluorescently labelled oligonucleotide probes to rRNA. The method allows monitoring of gene expression and quantification of beta-galactosidase activity in single cells.

Published

1997

3. Whole-cell hybridization of Methanosarcina cells with two new oligonucleotide probes.

Author

Sørensen AH, Torsvik VL, Torsvik T, Poulsen LK, and Ahring BK

Subjects

Anaerobiosis, Biomass, Bioreactors, Fluorescein, Fluoresceins, In Situ Hybridization adverse effects, Methanosarcina growth & development, Rhodamines, Sensitivity and Specificity, In Situ Hybridization methods, Methanosarcina genetics, Oligonucleotide Probes genetics, RNA, Ribosomal, 16S genetics

Abstract

Two new oligonucleotide probes targeting the 16S rRNA of the methanogenic genus Methanosarcina were developed. The probes have the following sequences (Escherichia coli numbering): probe SARCI551, 5'-GAC CCAATAATCACGATCAC-3', and probe SARCI645, 5'-TCCCGGTTCCAAGTCTGGC-3'. In situ hybridization with the fluorescently labelled probes required several modifications of standard procedures. Cells of Methanosarcina mazeii S-6 were found to lyse during the hybridization step if fixed in 3% formaldehyde and stored in 50% ethanol. Lysis was, however, not observed with cells fixed and stored in 1.6% formaldehyde-0.85% NaCl. Extensive autofluorescence of the cells was found upon hybridization in the presence of 5 mM EDTA, but successful hybridization could be obtained without addition of this compound. The mounting agent Citifluor AF1, often used in conjugation with the fluorochrome fluorescein, was found to wash the labelled probes out of the cells. Stable labelling could be obtained with rhodamine-labelled probes when the specimen was mounted in immersion oil, and high hybridization intensities of the Methanosarcina cells were found even in the presence of biomass from an anaerobic reactor. The inherent high autofluorescence of the biomass could be lowered by use of a highly specific narrow-band filter. The probes were found to be specific for Methanosarcina and useful for detection of this genus in samples from anaerobic reactors.

Published

1997

4. Activity and three-dimensional distribution of toluene-degrading Pseudomonas putida in a multispecies biofilm assessed by quantitative in situ hybridization and scanning confocal laser microscopy.

Author

Møller S, Pedersen AR, Poulsen LK, Arvin E, and Molin S

Subjects

Base Sequence, Microscopy, Confocal, Molecular Sequence Data, Oligonucleotide Probes, Biofilms, In Situ Hybridization, Pseudomonas putida metabolism, Toluene metabolism

Abstract

As a representative member of the toluene-degrading population in a biofilter for waste gas treatment, Pseudomonas putida was investigated with a 16S rRNA targeting probe. The three-dimensional distribution of P. putida was visualized in the biofilm matrix by scanning confocal laser microscopy, demonstrating that P. putida was present throughout the biofilm. Acridine orange staining revealed a very heterogeneous structure of the fully hydrated biofilm, with cell-free channels extending from the surface into the biofilm. This indicated that toluene may penetrate to deeper layers of the biofilm, and consequently P. putida may be actively degrading toluene in all regions of the biofilm. Furthermore, measurements of growth rate-related parameters for P. putida showed reduced rRNA content and cell size (relative to that in a batch culture), indicating that the P. putida population was not degrading toluene at a maximal rate in the biofilm environment. Assuming that the rRNA content reflected the cellular activity, a lower toluene degradation rate for P. putida present in the biofilm could be estimated. This calculation indicated that P. putida was responsible for a significant part (65%) of the toluene degraded by the entire community.

Published

1996

5. Role of lipopolysaccharide in colonization of the mouse intestine by Salmonella typhimurium studied by in situ hybridization.

Author

Licht TR, Krogfelt KA, Cohen PS, Poulsen LK, Urbance J, and Molin S

Subjects

Animals, Base Sequence, DNA Probes chemistry, Female, In Situ Hybridization, Intestinal Mucosa microbiology, Mice, Molecular Sequence Data, RNA, Ribosomal, 16S analysis, Salmonella typhimurium immunology, Time Factors, Bacterial Adhesion, Cecum microbiology, Colon microbiology, Lipopolysaccharides immunology, Salmonella typhimurium pathogenicity

Abstract

An avirulent, streptomycin-resistant Salmonella typhimurium strain, SL5319, and its lipopolysaccharide (LPS)-deficient mutant strain, SL5325, differ in their ability to colonize the large intestines of streptomycin-treated mice. When fed to mice independently, the strains colonize equally well, but when fed together, the LPS-deficient mutant is outcompeted by the wild-type strain during establishment in the gut (J.J. Nevola, B.A.D. Stocker, D.C. Laux, and P.S. Cohen, Infect. Immun. 50:152-159, 1985). In the present study, the spatial distribution in the intestinal mucosal layer of the two strains was visualized by specific hybridization to bacterial rRNA in histological sections of mouse colon and cecum. The first day after infection, 9.8% of the smooth SL5319 cells observed in mucus were found to be associated with the mouse epithelial cells, but three days after infection, the corresponding fraction of adhering bacteria was reduced to 2.1%. The LPS-deficient S. typhimurium strain was confined to the part of the mucosal layer closest to the colonic lumen and was not observed to adhere to the epithelium either at day 1 or 3 after infection. Quantitative determinations of the distance from the S. typhimurium cells to the epithelial wall confirmed that the average distance for the rough S. typhimurium SL5325 was much larger than for its smooth counterpart, S. typhimurium SL5319. Quantification of the hybridization signal from bacteria isolated from the cecal mucus revealed that the two strains had the same ribosome concentration, indicating that they have the same potential for growth in the intestinal environment. On the basis of these observations, we suggest that the better colonization ability of the strain carrying wild-type LPS is due to the better abilities to penetrate the intestinal mucosal layer and to subsequently bind to the epithelial cells in vivo.

Published

1996

6. Phylogenetic position of the spirochetal genus Cristispira.

Author

Paster BJ, Pelletier DA, Dewhirst FE, Weisburg WG, Fussing V, Poulsen LK, Dannenberg S, and Schroeder I

Subjects

In Situ Hybridization, Molecular Sequence Data, Polymerase Chain Reaction, RNA, Ribosomal, 16S genetics, Spirochaetales genetics, Phylogeny, Spirochaetales classification

Abstract

Comparative sequence analysis of 16S rRNA genes was used to determine the phylogenetic relationship of the genus Cristispira to other spirochetes. Since Cristispira organisms cannot presently be grown in vitro, 16S rRNA genes were amplified directly from bacterial DNA isolated from Cristispira cell-laden crystalline styles of the oyster Crassostrea virginica. The amplified products were then cloned into Escherichia coli plasmids. Sequence comparisons of the gene coding for 16S rRNA (rDNA) insert of one clone, designated CP1, indicated that it was spirochetal. The sequence of the 16S rDNA insert of another clone was mycoplasmal. The CP1 sequence possessed most of the individual base signatures that are unique to 16S rRNA (or rDNA) sequences of known spirochetes. CP1 branched deeply among other spirochetal genera within the family Spirochaetaceae, and accordingly, it represents a separate genus within this family. A fluorescently labeled DNA probe designed from the CP1 sequence was used for in situ hybridization experiments to verify that the sequence obtained was derived from the observed Cristispira cells.

Published

1996

7. Phylogeny of not-yet-cultured spirochetes from termite guts.

Author

Paster BJ, Dewhirst FE, Cooke SM, Fussing V, Poulsen LK, and Breznak JA

Subjects

Animals, Base Sequence, DNA Probes genetics, DNA, Bacterial genetics, DNA, Ribosomal genetics, Microscopy, Electron, Molecular Sequence Data, RNA, Bacterial genetics, RNA, Ribosomal, 16S genetics, Spirochaeta classification, Spirochaeta genetics, Spirochaeta isolation & purification, Spirochaetaceae classification, Spirochaetaceae isolation & purification, Treponema classification, Treponema genetics, Treponema isolation & purification, Insecta microbiology, Phylogeny, Spirochaetaceae genetics

Abstract

Comparisons of 16S rDNA sequences were used to determine the phylogeny of not-yet-cultured spirochetes from hindguts of the African higher termite, Nasutitermes lujae (Wasmann). The 16S rRNA genes were amplified directly from spirochete-rich hindguts by using universal primers, and the amplified products were cloned into Escherichia coli. Clones were screened with a spirochete-specific DNA probe. Analysis of 1,410 base positions of the 16S rDNA insert from one spirochete clone, designated NL1, supported its assignment to the genus Treponema, with average interspecies similarities of ca. 85%. The sequence of NL1 was most closely related (ca. 87 to 88% similarity) to sequences of Spirochaeta stenostrepta and Spirochaeta caldaria and to a previously published sequence (ca. 87% similarity) of spirochetal clone MDS1 from the Australian lower termite, Mastotermes darwiniensis (Froggatt). On the basis of 16S rRNA sequence comparisons and individual base signatures, clones NL1 and MDS1 clearly represent two novel species of Treponema, although specific epithets have not yet been proposed. The gross morphology of NL1 was determined from in situ hybridization experiments with an NL1-specific, fluorescently labeled oligonucleotide probe. Cells were approximately 0.3 to 0.4 by 30 microns in size, with a wavelength and amplitude of about 10 microns and 0.8 to 1.6 micron, respectively. Moreover, electron microscopy of various undulate cells present in gut contents confirmed that they possessed ultrastructural features typical of spirochetes, i.e., a wavy protoplasmic cylinder, periplasmic flagella, and an outer sheath. The sequence data suggest that termite gut spirochetes may represent a separate line of descent from other treponemes and that they constitute a significant reservoir of previously unrecognized spirochetal biodiversity.

Published

1996

8. Physiological state of Escherichia coli BJ4 growing in the large intestines of streptomycin-treated mice.

Author

Poulsen LK, Licht TR, Rang C, Krogfelt KA, and Molin S

Subjects

Animals, Base Sequence, Cecum microbiology, Cell Division, Escherichia coli drug effects, Feces microbiology, Female, Mice, Microscopy, Fluorescence, Molecular Sequence Data, Mucus microbiology, Nucleic Acid Hybridization, RNA, Ribosomal, 23S analysis, Time Factors, Escherichia coli growth & development, Escherichia coli Infections microbiology, Intestine, Large microbiology, Streptomycin pharmacology

Abstract

Growth rates of Escherichia coli BJ4 colonizing the large intestine of streptomycin-treated mice were estimated by quantitative hybridization with rRNA target probes and by epifluorescence microscopy. The ribosomal contents in bacteria isolated from the cecal mucus, cecal contents, and feces were measured and correlated with the ribosomal contents of bacteria growing in vitro at defined rates. The data suggest that E. coli BJ4 grows at an overall high rate in the intestine. However, when taking into account the total intestinal volume and numbers of bacteria present in cecal mucus, cecal contents, and feces, we suggest that E. coli BJ4 in the intestine consists of two populations, one in the mucus which has an apparent generation time of 40 to 80 min and one in the luminal contents which is static.

Published

1995

9. Bacterial growth on surfaces: automated image analysis for quantification of growth rate-related parameters.

Author

Moller S, Kristensen CS, Poulsen LK, Carstensen JM, and Molin S

Abstract

A fast routine method for estimating bacterial cell growth rates by using the metachromatic dye acridine orange is described. The method allows simultaneous estimates of cellular RNA and DNA contents of single cells. Acridine orange staining can be used as a nonspecific supplement to quantitative species-specific hybridizations with fluorescence-labelled ribosomal probes to estimate the single-cell concentration of RNA. By automated analysis of digitized images of stained cells, we determined four independent growth rate-related parameters: cellular RNA and DNA contents, cell volume, and the frequency of dividing cells in a cell population. These parameters were used to compare physiological states of liquid-suspended and surface-growing Pseudomonas putida KT2442 in chemostat cultures. The major finding is that the correlation between substrate availability and cellular growth rate found for the free-living cells was not observed for the surface-bound cells; in contrast, the data indicate an almost constant growth rate for attached cells which was independent of the dilution rate in the chemostat.

Published

1995

10. Substratum-induced morphological changes in a marine bacterium and their relevance to biofilm structure.

Author

Dalton HM, Poulsen LK, Halasz P, Angles ML, Goodman AE, and Marshall KC

Subjects

Bacteria cytology, Bacteria genetics, Microscopy, Confocal, Microscopy, Fluorescence, Microscopy, Video, Plasmids genetics, Surface Properties, Biofilms growth & development, Marine Biology, Water Microbiology

Abstract

The effects of surfaces on the physiology of bacteria adhering to surfaces or immobilized within biofilms are receiving more interest. A study of the effects of hydrophobic and hydrophilic substrata on the colonization behavior of a marine bacterium, SW5, revealed major differences in the morphology of SW5 on these surfaces. Using epifluorescence, scanning confocal laser, and on-line visualization (time-lapse video) microscopy, the organisms at hydrophobic surfaces were characterized by the formation of tightly packed biofilms, consisting of single and paired cells, whereas those at hydrophilic surfaces exhibited sparse colonization and the formation of chains more than 100 microns long, anchored at the surface by the terminal (colonizing) cell. The results are discussed in terms of the possible factors inducing the observed morphological differences and the significance of these differences in terms of biofilm structure and plasmid transfer when SW5 is the recipient organism.

Published

1994

11. Spatial distribution of Escherichia coli in the mouse large intestine inferred from rRNA in situ hybridization.

Author

Poulsen LK, Lan F, Kristensen CS, Hobolth P, Molin S, and Krogfelt KA

Subjects

Animals, Base Sequence, In Situ Hybridization, Intestine, Small microbiology, Mice, Molecular Sequence Data, Oligonucleotide Probes chemistry, RNA, Ribosomal, 23S metabolism, Escherichia coli growth & development, Intestine, Large microbiology

Abstract

Fluorescent oligonucleotide probes targeting rRNA were used to develop an in situ hybridization technique by which the spatial distribution of Escherichia coli in the large intestines of streptomycin-treated mice was determined. Single E. coli cells were identified in thin frozen sections from the large intestines by the use of a probe specific for E. coli 23S rRNA. Furthermore, the total bacterial population was visualized with an rRNA probe targeting the domain Bacteria. By this technique, all E. coli cells were seen embedded in the mucosal material overlying the epithelial cells of the large intestine, and no direct attachment to the epithelium was observed.

Published

1994

12. Analysis of fluorescent pseudomonads based on 23S ribosomal DNA sequences.

Author

Christensen H, Boye M, Poulsen LK, and Rasmussen OF

Subjects

Base Sequence, Genetic Variation, Molecular Sequence Data, Pseudomonas fluorescens chemistry, Pseudomonas putida chemistry, RNA, Ribosomal, 23S genetics, Sequence Homology, Nucleic Acid, Species Specificity, DNA, Bacterial genetics, DNA, Ribosomal genetics, Pseudomonas fluorescens genetics, Pseudomonas putida genetics

Abstract

The regions from positions 1391 to 1545 and 1620 to 1865 (Escherichia coli numbers) of the 23S ribosomal DNA sequences have been analyzed for a number of Pseudomonas fluorescens and P. putida isolates. Variability was observed only in three smaller regions from positions 1484 to 1508, 1531 to 1542, and 1714 to 1748, corresponding to helices 58, 59, and 63, respectively, where up to 53% dissimilarity was found. Sequence analysis did not allow clear distinctions among P. fluorescens biovars, P. chlororaphis, and P. putida biovar B.

Published

1994

13. Quantification of methanogenic groups in anaerobic biological reactors by oligonucleotide probe hybridization.

Author

Raskin L, Poulsen LK, Noguera DR, Rittmann BE, and Stahl DA

Subjects

Anaerobiosis, Bacteriological Techniques instrumentation, Euryarchaeota classification, Euryarchaeota genetics, Euryarchaeota growth & development, Euryarchaeota metabolism, Population Dynamics, DNA, Bacterial analysis, DNA, Ribosomal analysis, Euryarchaeota isolation & purification, Nucleic Acid Hybridization, Oligonucleotide Probes, RNA, Bacterial genetics, RNA, Ribosomal, 16S genetics, Refuse Disposal instrumentation, Sewage analysis

Abstract

The microbial community structure of anaerobic biological reactors was evaluated by using oligonucleotide probes complementary to conserved tracts of the 16S rRNAs of phylogenetically defined groups of methanogens. Phylogenetically defined groups of methanogens were quantified and visualized, respectively, by hybridization of 32P- and fluorescent-dye-labeled probes to the 16S rRNAs from samples taken from laboratory acetate-fed chemostats, laboratory municipal solid waste digestors, and full-scale sewage sludge digestors. Methanosarcina species, members of the order Methanobacteriales, and Methanosaeta species were the most abundant methanogens present in the chemostats, the solid-waste digestors, and the sewage sludge digestors, respectively.

Published

1994

14. Responses to nutrient starvation in Pseudomonas putida KT2442: analysis of general cross-protection, cell shape, and macromolecular content.

Author

Givskov M, Eberl L, Møller S, Poulsen LK, and Molin S

Subjects

Bacterial Proteins biosynthesis, Carbon metabolism, Cell Division, DNA, Bacterial analysis, Drug Tolerance, Ethanol pharmacology, Nitrogen deficiency, Osmotic Pressure, Oxidation-Reduction, Phosphates deficiency, Pseudomonas putida chemistry, Pseudomonas putida cytology, Pseudomonas putida drug effects, Ribosomes metabolism, Sulfates metabolism, Adaptation, Physiological, Glucose deficiency, Pseudomonas putida physiology

Abstract

The physiology of Pseudomonas putida KT2442 with respect to growth and carbon starvation was studied. During the transition from growth to nongrowth, the cell shape changes from cylindrical to spheric, a change which is accompanied by reductions in cell size, DNA and ribosome content, and the rate of total protein synthesis. In addition, a pattern of general cross-protection develops, which enables the cells to survive environmental stresses such as high and low temperatures, elevated osmolarity, solvents, and oxidative agents. Cultures are almost fully viable during 1 month of carbon, nitrogen, and multiple-nutrient starvation and are considered to be in an active nondormant state. In contrast, strain KT2442 does not survive well under conditions of sulfate and phosphate starvation.

Published

1994

15. Identification of coccoid Escherichia coli BJ4 cells in the large intestine of streptomycin-treated mice.

Author

Krogfelt KA, Poulsen LK, and Molin S

Subjects

Animals, Cecum microbiology, Cell Differentiation, Culture Media, Escherichia coli cytology, Escherichia coli isolation & purification, Feces microbiology, Female, Intestine, Large drug effects, Mice, Models, Biological, Rats, Streptomycin pharmacology, Escherichia coli growth & development, Intestine, Large microbiology

Abstract

Escherichia coli BJ4, a rat isolate, was used to examine the growth and differentiation of the microorganism in its natural habitat, the intestine. Growth of E. coli BJ4 in the large intestine of streptomycin-treated mice was compared with its growth in laboratory media. By a number of methods, it was shown that E. coli BJ4 differentiates, during growth in the intestine, into two distinct populations, one that has the characteristics of the laboratory-grown strain and one that appears as a coccoid cell. Furthermore, it was shown that there is a natural selection for the coccoid-type cell in the intestine, while in laboratory media growth of rod-shaped E. coli BJ4 is enhanced.

Published

1993

16. Use of rRNA fluorescence in situ hybridization for measuring the activity of single cells in young and established biofilms.

Author

Poulsen LK, Ballard G, and Stahl DA

Subjects

Base Sequence, DNA Probes, DNA, Bacterial genetics, Desulfovibrio vulgaris genetics, Desulfovibrio vulgaris growth & development, Desulfovibrio vulgaris metabolism, Ecology, Escherichia coli genetics, Escherichia coli metabolism, Molecular Sequence Data, RNA, Bacterial genetics, RNA, Bacterial metabolism, RNA, Ribosomal genetics, In Situ Hybridization, Fluorescence, RNA, Ribosomal metabolism

Abstract

We describe the in situ use of rRNA-targeted fluorescent hybridization probes in combination with digital microscopy to quantify the cellular content of ribosomes in relationship to the growth rate of single cells of a specific population of sulfate-reducing bacteria in multispecies anaerobic biofilms. Using this technique, we inferred that this population was growing with an average generation time of 35 h in a young biofilm, whereas the doubling time in an established biofilm was significantly longer. Conventional chemical determinations of the RNA, DNA, and protein contents of this culture at different growth rates were also carried out, and the resulting data were compared with the rRNA fluorescence in situ hybridization data.

Published

1993

17. Leishmania donovani-reactive Th1- and Th2-like T-cell clones from individuals who have recovered from visceral leishmaniasis.

Author

Kemp M, Kurtzhals JA, Bendtzen K, Poulsen LK, Hansen MB, Koech DK, Kharazmi A, and Theander TG

Subjects

Animals, Antigens, Protozoan immunology, Antigens, Surface analysis, Clone Cells, Humans, Interferon-gamma metabolism, Interleukin-4 metabolism, Leukotrienes metabolism, Lymphocyte Activation, Leishmania donovani immunology, Leishmaniasis, Visceral immunology, T-Lymphocyte Subsets immunology, T-Lymphocytes, Helper-Inducer immunology

Abstract

Infections in humans by Leishmania donovani parasites can result in a fatal disease, visceral leishmaniasis (VL), or in a self-limiting asymptomatic infection. In murine models of the infection employing Leishmania major, the course of the disease can be directed into a VL-like syndrome by interleukin-4 (IL-4)-producing Th2 cells, or cure may result by Th1 cells secreting gamma interferon (IFN-gamma). The present study examined the potential of human T cells to generate Th1 or Th2 responses to L. donovani. The profiles of IFN-gamma, IL-4, and lymphotoxin secretion after antigen stimulation were analyzed in a panel of L. donovani-reactive CD4+ human T-cell clones generated from individuals who had recovered from VL after antimonial treatment. Two of the T-cell clones produced large amounts of IL-4 without production of IFN-gamma, seven clones produced both IFN-gamma and IL-4, and eight produced only IFN-gamma. This is the first report of a Th1- and Th2-type response in human leishmaniasis. These results suggest that in analogy with murine models, there is a dichotomy in the human T-cell response to L. donovani infections. Preferential activation of IL-4-producing Th2-like cells may be involved in the exacerbation of human VL, whereas activation of IFN-gamma-producing Th1 cells may protect the host from severe disease. Identification of leishmanial antigens activating one or the other type of T cells will be important in the development of vaccines against leishmaniasis.

Published

1993

18. Monitoring the enrichment and isolation of sulfate-reducing bacteria by using oligonucleotide hybridization probes designed from environmentally derived 16S rRNA sequences.

Author

Kane MD, Poulsen LK, and Stahl DA

Subjects

Base Sequence, Desulfovibrio classification, Desulfovibrio genetics, Desulfovibrio physiology, Microscopy, Fluorescence, Microscopy, Phase-Contrast, Molecular Sequence Data, Nucleic Acid Hybridization, Phylogeny, RNA, Bacterial chemistry, Species Specificity, Desulfovibrio isolation & purification, Oligonucleotide Probes, RNA, Ribosomal, 16S chemistry

Abstract

A fluorescently labeled version of a population-specific oligonucleotide hybridization probe was used to monitor the enrichment and isolation of a sulfate-reducing bacterium from a multispecies anaerobic bioreactor. The organism was originally identified as a molecular isolate that was phylogenetically related to Desulfovibrio vulgaris by amplification and sequencing of part of its 16S rRNA sequence. The sequence, in turn, was used to design a population-specific probe. The anaerobic medium used for the organism's enrichment and isolation was based on the physiological properties of the its closest relatives as identified by sequence comparisons. Of 30 isolates examined, only 3 hybridized with the probe. Nearly complete 16S rRNA sequences determined for each of these three isolates (i) had no mismatches with the probe target site, (ii) were identical to the amplified partial sequence of about 500 nucleotides and to one another in all other positions, and (iii) were 93.9% similar to that of D. vulgaris. In addition, one isolate chosen for further study (strain PT-2) had a substrate specificity comparable to that of D. vulgaris. These results confirmed that polymerase chain reaction amplification of 16S rRNA sequences from environmental samples can be accurate and can also provide phylogenetic information from which aspects of a population's physiology can be inferred.

Published

1993

19. Inhibition of human lymphocyte proliferation and cleavage of interleukin-2 by Pseudomonas aeruginosa proteases.

Author

Theander TG, Kharazmi A, Pedersen BK, Christensen LD, Tvede N, Poulsen LK, Odum N, Svenson M, and Bendtzen K

Subjects

Binding, Competitive, Humans, Interleukin-2 antagonists & inhibitors, Interleukin-2 pharmacology, Lymphocytes metabolism, Phytohemagglutinins, Pseudomonas aeruginosa immunology, Receptors, Immunologic drug effects, Receptors, Interleukin-2, Endopeptidases pharmacology, Immunosuppressive Agents pharmacology, Interleukin-2 metabolism, Lymphocyte Activation drug effects, Pancreatic Elastase pharmacology, Pseudomonas aeruginosa enzymology, Serine Endopeptidases

Abstract

This study was undertaken to determine the effect of Pseudomonas aeruginosa alkaline protease (AP) and elastase (ELA) on human lymphocyte function. AP at 50 micrograms/ml and ELA at 12 micrograms/ml caused a 50% inhibition of phytohemagglutinin-induced proliferation. There was no difference in the effect of proteases on CD4- and CD8-positive cells. To determine the effect of proteases on interleukin-2 (IL-2)-induced cell proliferation, the proteases and IL-2 were added to the IL-2-dependent CTLL-2 cell line. AP and ELA inhibited the proliferation of these cells. When IL-2 was added in excess, the inhibition was partly reversed. ELA at 10 micrograms/ml cleaved IL-2, as judged by size chromatography of a reaction mixture containing 125I-labeled IL-2 and the proteases. The ELA-digested IL-2 exhibited a reduced binding capacity to IL-2 receptors on the lymphocytes. Furthermore, treatment of phytohemagglutinin-stimulated lymphocytes with AP and ELA resulted in inhibition of binding of intact IL-2 to IL-2 receptors on the stimulated lymphocytes. These results indicated that P. aeruginosa-derived enzymes are able to interfere with human lymphocyte function in vitro and that this effect might be due to cleavage of IL-2.

Published

1988