Competence for genetic transformation in encapsulated strains of Streptococcus pneumoniae: two allelic variants of the peptide pheromone

Pozzi, Gianni; Masala, Laura; Iannelli, Francesco; Manganelli, Riccardo; Håvarstein, Leiv Sigve; Piccoli, Luca; Simon, Daniel; Morrison, Donald A.

doi:10.1128/jb.178.20.6087-6090.1996

Cited by 254 publications

(265 citation statements)

References 24 publications

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“…The resulting plasmid pJY4164-ply was transformed into S. pneumoniae strain WU2 by using competencestimulating peptide 2 (as described in ref. 35; synthesized by the Biopolymer Facility at Harvard University) at a concentration of 100 ng͞ml by using protocols as described (36). Colonies that were resistant to erythromycin (0.3 g͞ml) were screened for pneumolysin production by measuring the hemolytic activity of supernatants from overnight cultures in Todd-Hewitt medium supplemented with 0.5% yeast extract.…”

Section: Methodsmentioning

confidence: 99%

Recognition of pneumolysin by Toll-like receptor 4 confers resistance to pneumococcal infection

Malley

Henneke

Morse

et al. 2003

Proc. Natl. Acad. Sci. U.S.A.

629

583

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Streptococcus pneumoniae is one of the leading causes of invasive bacterial disease worldwide. Fragments of the cell wall and the cytolytic toxin pneumolysin have been shown to contribute substantially to inflammatory damage, although the interactions between pneumococcal components and host-cell structures have not been elucidated completely. Results of a previous study indicated that cell-wall components of pneumococci are recognized by Toll-like receptor (TLR)2 but suggested that pneumolysin induces inflammatory events independently of this receptor. In this study we tested the hypothesis that pneumolysin interacts with surface proteins of the TLR family other than TLR2. We found that pneumolysin stimulates tumor necrosis factor-␣ and IL-6 release in wild-type macrophages but not in macrophages from mice with a targeted deletion of the cytoplasmic TLR-adapter molecule myeloid differentiation factor 88, suggesting the involvement of the TLRs in pneumolysin recognition. Purified pneumolysin synergistically activated macrophage responses together with preparations of pneumococcal cell walls or staphylococcal peptidoglycan, which are known to activate TLR2. Furthermore, when compared with wild-type macrophages, macrophages from mice that carry a spontaneous mutation in TLR4 (P712H) were hyporesponsive to both pneumolysin alone and the combination of pneumolysin with pneumococcal cell walls. Finally, these TLR4-mutant mice were significantly more susceptible to lethal infection after intranasal colonization with pneumolysin-positive pneumococci than were control mice. We conclude that the interaction of pneumolysin with TLR4 is critically involved in the innate immune response to pneumococcus.

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Section: Methodsmentioning

confidence: 99%

Recognition of pneumolysin by Toll-like receptor 4 confers resistance to pneumococcal infection

Malley

Henneke

Morse

et al. 2003

Proc. Natl. Acad. Sci. U.S.A.

629

583

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“…The capsular variants of otherwise isogenic strains were constructed in three different genetic backgrounds-TIGR4 (originally of serotype 4) and 603 and 618 (both originally of serotype 6B)-by using a previously described method (48). In short, the parent strain was rendered unencapsulated by insertion of a cassette into the capsule locus using the transformation protocol published by Pozzi et al (37) and the bicistronic Janus cassette constructed by Sung et al (46). Encapsulated mutants were generated by replacing the cassettes with a cps locus from a donor strain.…”

Section: Methodsmentioning

confidence: 99%

The Capsular Serotype ofStreptococcus pneumoniaeIs More Important than the Genetic Background for Resistance to Complement

et al. 2010

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The polysaccharide capsule of Streptococcus pneumoniae inhibits phagocytic killing by innate immune mechanisms. Certain serotypes are associated with invasive disease while others with a nasopharyngeal carriage. The invasiveness of serotypes may partly be explained by ability to resist deposition of complement (C3) on the bacterial surface and consequent opsonophagocytic killing. In our previous studies, we observed that clinical isolates of serotypes 1 and 5, which are rarely detected in asymptomatic carriage, were resistant to complement deposition and opsonophagocytosis, whereas serotypes 6B and 23F, both common in carriage, were more sensitive to deposition of C3 and opsonophagocytic killing. However, presence of significant variation in C3 deposition between isolates of the same serotype indicated that factors other than the capsule also affect complement resistance. To distinguish the relative effect of the capsular serotype and other virulence factors on C3 deposition, we compared capsule-switched mutants prepared in genetic backgrounds of pneumococcal strains TIGR4, 603, and 618. Clinical isolates which had the same multilocus sequence type but expressed different serotypes were also compared. We found that the serotype had a significant impact on complement resistance and that the more resistant the strain was to complement, the higher was the concentration of polysaccharide-specific antibodies required for opsonophagocytic killing. Comparison of strains expressing the same capsular polysaccharides in the different genetic backgrounds and various capsular mutants of the same strain suggests that while the genotype affects complement resistance, the serotype is the most important determinant. Differences between serotypes were more significant than the differences between strains.

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“…Complementation of mutants VES2585-VES2587 by pDLP49, carrying an intact copy of the tts gene under the control of its own promoter (Llull et al, 2001), was performed by a similar transformation method, but adding competence-stimulating peptide 2 (CSP-2) (Pozzi et al, 1996) to the transformation mix at a final concentration of 100 ng ml 21 . CSP-2 was used instead of CSP-1 after empirical confirmation of its ability to induce competence in type 37 derivatives.…”

Section: Methodsmentioning

confidence: 99%

Immobilization-based isolation of capsule-negative mutants of Streptococcus pneumoniae

et al. 2005

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The capsular polysaccharide (CPS) is the most important identified virulence factor of Streptococcus pneumoniae, a human pathogen of the upper respiratory tract. One limitation in studies of S. pneumoniae surface virulence factors is the lack of a reliable procedure for isolation of capsule-negative mutants of clinical strains. This paper presents an approach, based on the immobilization of pneumococci in semi-liquid (0?04 % agar) medium, to easily distinguish and select for non-capsulated mutants. A clinical S. pneumoniae type 37 strain was used as a model to show that CPS production results in bacterial immobilization in semi-liquid agar medium and restricts cell sedimentation. Descendants of CPS " mutants sedimented faster under these conditions and therefore could be separated from immobilized parental cells. The CPS " phenotype of the obtained mutants was confirmed by both immunoagglutination and immunostaining experiments using specific type 37 capsular antibodies. Complementation of immobilization with the cloned tts gene, encoding type 37 CPS synthase, confirmed that faster sedimentation of mutants was specifically due to loss of the capsule. DNA sequence determination of three independent mutants revealed a point mutation, a 46 nt deletion and a heptanucleotide duplication in the tts gene. Immobilization of strains producing other CPSs (type 2, 3 and 6) also resulted in the appearance of CPS " mutants, thus showing that immobilization-based isolation is not restricted to type 37 pneumococci. Bacterial growth in semi-liquid medium proved to be a useful model system to identify the genetic consequences of immobilization. The results indicate that immobilization due to CPS may impose selective pressure against capsule production and thus contribute to capsule plasticity.

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Competence for genetic transformation in encapsulated strains of Streptococcus pneumoniae: two allelic variants of the peptide pheromone

Cited by 254 publications

References 24 publications

Recognition of pneumolysin by Toll-like receptor 4 confers resistance to pneumococcal infection

Recognition of pneumolysin by Toll-like receptor 4 confers resistance to pneumococcal infection

The Capsular Serotype ofStreptococcus pneumoniaeIs More Important than the Genetic Background for Resistance to Complement

Immobilization-based isolation of capsule-negative mutants of Streptococcus pneumoniae

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