2016
DOI: 10.1128/jb.00353-16
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A Type I Signal Peptidase Is Required for Pilus Assembly in the Gram-Positive, Biofilm-Forming Bacterium Actinomyces oris

Abstract: The Gram-positive bacterium Actinomyces oris, a key colonizer in the development of oral biofilms, contains 18 LPXTG motifcontaining proteins, including fimbrillins that constitute two fimbrial types critical for adherence, biofilm formation, and polymicrobial interactions. Export of these protein precursors, which harbor a signal peptide, is thought to be mediated by the Sec machine and require cleavage of the signal peptide by type I signal peptidases (SPases). Like many Gram-positive bacteria, A. oris expre… Show more

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Cited by 18 publications
(40 citation statements)
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“…S1A). To explore if overexpression of CafA in the ΔgspA/ΔsrtA double mutant rescues its coaggregation defect, we introduced into this strain a multicopy plasmid-expressing CafA under the control of a constitutive promoter (pCafA) (29), and coaggregation was quantitatively determined as described before (37). Compared to the MG1 strain, which coaggregation efficiency was normalized to 1, overexpression of CafA could not rescue the coaggregation defect of the ΔgspA/ΔsrtA mutant (SI Appendix, Fig.…”
Section: A Critical Positional Role Of the Pilus Tip In Interspecies mentioning
confidence: 99%
“…S1A). To explore if overexpression of CafA in the ΔgspA/ΔsrtA double mutant rescues its coaggregation defect, we introduced into this strain a multicopy plasmid-expressing CafA under the control of a constitutive promoter (pCafA) (29), and coaggregation was quantitatively determined as described before (37). Compared to the MG1 strain, which coaggregation efficiency was normalized to 1, overexpression of CafA could not rescue the coaggregation defect of the ΔgspA/ΔsrtA mutant (SI Appendix, Fig.…”
Section: A Critical Positional Role Of the Pilus Tip In Interspecies mentioning
confidence: 99%
“…Both PCR products were used as templates for overlapping PCR with primers VKOR-HindIII-F and HA-NdeI-R. The PCR product generated was gel purified and digested with HindIII and NdeI (New England BioLabs [NEB]) and subsequently ligated into pCWU10 (36). The resulting plasmid was introduced into DH5␣, and plasmid DNA was purified for sequencing using primer pVKORseq (see Table S1) to confirm the insertion sequence.…”
Section: Methodsmentioning
confidence: 99%
“…Cell fractionation was performed as previously described (36). Briefly, log-phase cell cultures of various strains were obtained and normalized to an OD 600 of 1.0 (36). Cells were fractionated into culture medium (S), cell wall (W), membrane (M), and cytoplasmic (C) fractions; proteins were precipitated using trichloroacetic acid (TCA) and washed with acetone.…”
Section: Methodsmentioning
confidence: 99%
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