2011
DOI: 10.1128/jb.05170-11
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Peptide-Regulated Gene Depletion System Developed for Use in Streptococcus pneumoniae

Abstract: To facilitate the study of pneumococcal genes that are essential for viability or normal cell growth, we sought to develop a tightly regulated, titratable gene depletion system that interferes minimally with normal cellular functions. A possible candidate for such a system is the recently discovered signal transduction pathway regulating competence for natural transformation in Streptococcus thermophilus. This pathway, which is unrelated to the ComCDE pathway used for competence regulation in Streptococcus pne… Show more

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Cited by 33 publications
(44 citation statements)
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“…These two fragments were fused in an overlap extension PCR with the flanking primers ds95 and ds98 resulting in a lytF-CHAP pcsB chimera. LytF-CHAP PcsB was expressed in S. pneumoniae by using the ComRS system described by Berg et al 30 The 5 0 and 3 0 regions of the Janus cassette in strain SPH131 (see above) were amplified by the primer pairs khb31/khb36 and khb33/khb34, respectively, and then fused to the 5 0 and 3 0 ends of the lytF-CHAP pcsB fragment by overlap extension PCR using the primers khb31 and khb34. The resulting fragment was transformed into strain SPH131, replacing the Janus cassette and giving rise to strain SPH252.…”
Section: Methodsmentioning
confidence: 99%
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“…These two fragments were fused in an overlap extension PCR with the flanking primers ds95 and ds98 resulting in a lytF-CHAP pcsB chimera. LytF-CHAP PcsB was expressed in S. pneumoniae by using the ComRS system described by Berg et al 30 The 5 0 and 3 0 regions of the Janus cassette in strain SPH131 (see above) were amplified by the primer pairs khb31/khb36 and khb33/khb34, respectively, and then fused to the 5 0 and 3 0 ends of the lytF-CHAP pcsB fragment by overlap extension PCR using the primers khb31 and khb34. The resulting fragment was transformed into strain SPH131, replacing the Janus cassette and giving rise to strain SPH252.…”
Section: Methodsmentioning
confidence: 99%
“…As pcsB is an essential gene in S. pneumoniae R6, an extra copy of the wild-type gene had to be expressed ectopically before the native pcsB gene could be removed and replaced by a Janus cassette 42 . For ectopic expression of pcsB, we employed the R6 derivative SPH131, which has the ComRS expression/depletion system integrated in its genome 30 . First, the pcsB gene was amplified with the primers 35 and 36 and DNA from strain RH1 as template.…”
Section: Methodsmentioning
confidence: 99%
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“…To protect themselves against their own fratricins, S. pneumoniae cells produce an immunity protein termed ComM (Berg et al, 2011). In S. mutans the two genes murN (SMU.716) and murM (SMU.717) show homology to ComM but they were not upregulated.…”
Section: Cultivation Mediummentioning
confidence: 99%
“…After incubation at 37 uC for 120 min, cells were spread on Todd-Hewitt (TH) agar plates supplemented with kanamycin (400 mg ml 21 ), streptomycin (200 mg ml 21 ) or spectinomycin (200 mg ml 21 ) to select for transformants. When required, the inducer peptide ComS* (NH 2 -LPYFAGCL-COOH) was added to the medium during transformation and selection on agar plates to induce ectopic gene expression from the P comX promoter (Berg et al, 2011.…”
Section: Methodsmentioning
confidence: 99%