Cloning of the
            <i>Streptococcus mutans</i>
            Gene Encoding Glucan Binding Protein B and Analysis of Genetic Diversity and Protein Production in Clinical Isolates

Mattos-Graner, Renata O.; Jin, Shaowei; King, William F.; Chen, Tsute; Smith, Daniel J.; Duncan, Marilyn J.

doi:10.1128/iai.69.11.6931-6941.2001

Cited by 95 publications

(143 citation statements)

References 35 publications

(34 reference statements)

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“…Consistently, atypical long-chain phenotypes are found in v icK isogenic mutants obtained in S. pnemoniae , S. mutans , and S. sanguinis [90,105,106,111]. In VicR regulons, the most conserved target gene encodes PcsB (protein required for cell separation of group B Streptococcus ) that was first identified in group B streptococci [114] and orthologue GbpB (glucan-binding protein B in S. mutans ) [115,116]. Table 2 shows comparisons of VicR gene targets among streptococcal species of the oral cavity and oropharynx.…”

Section: Vicrk Regulons Of Tcss Are Diverse and Species-specificmentioning

confidence: 89%

Two-component signal transduction systems in oral bacteria

Mattos-Graner

Duncan²

2017

Journal of Oral Microbiology

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We present an overview of how members of the oral microbiota respond to their environment by regulating gene expression through two-component signal transduction systems (TCSs) to support conditions compatible with homeostasis in oral biofilms or drive the equilibrium toward dysbiosis in response to environmental changes. Using studies on the sub-gingival Gram-negative anaerobe Porphyromonas gingivalis and Gram-positive streptococci as examples, we focus on the molecular mechanisms involved in activation of TCS and species specificities of TCS regulons.

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Section: Vicrk Regulons Of Tcss Are Diverse and Species-specificmentioning

confidence: 89%

Two-component signal transduction systems in oral bacteria

Mattos-Graner

Duncan²

2017

Journal of Oral Microbiology

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“…The instability of the gbpB mutant indicates that it may be an essential protein; its homology to peptidoglycan hydrolase may mean that GbpB is essential for cell-wall cycling and synthesis (Mattos-Graner et al, 2001. Recently, it became apparent that GbpB was identical to the immunodominant glycoprotein IDG-60 and the general stress protein GSP-781 (Chia et al, 2001a,b;Mattos-Graner et al, 2001).…”

Section: Functions Of Gbpsmentioning

confidence: 99%

“…The null mutant of GbpB is unstable (Mattos-Graner et al, 2002), precluding in vitro investigation. However, the amount of GbpB produced by clinical isolates correlates with their biofilm-forming abilities (Mattos-Graner et al, 2001). The loss of GbpC in the same model system as used with GbpA results in a biofilm about twice as thick as normal (Fig.).…”

Section: Functions Of Gbpsmentioning

confidence: 99%

Glucan-binding Proteins of the Oral Streptococci

Banas

Vickerman

2003

Critical Reviews in Oral Biology & Medicine

282

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ABSTRACT:The synthesis of extracellular glucan is an integral component of the sucrose-dependent colonization of tooth surfaces by species of the mutans streptococci. In investigators' attempts to understand the mechanisms of plaque biofilm development, several glucan-binding proteins (GBPs) have been discovered. Some of these, the glucosyltransferases, catalyze the synthesis of glucan, whereas others, designated only as glucan-binding proteins, have affinities for different forms of glucan and contribute to aspects of the biology of their host organisms. The functions of these latter glucan-binding proteins include dextran-dependent aggregation, dextranase inhibition, plaque cohesion, and perhaps cell wall synthesis. In some instances, their glucan-binding domains share common features, whereas in others the mechanism for glucan binding remains unknown. Recent studies indicate that at least some of the glucan-binding proteins modulate virulence and some can act as protective immunogens within animal models. Overall, the multiplicity of GBPs and their aforementioned properties are testimonies to their importance. Future studies will greatly advance the understanding of the distribution, function, and regulation of the GBPs and place into perspective the facets of their contributions to the biology of the oral streptococci.

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“…Integrities of the genomic DNA samples were checked in samples electrophoretically resolved in 1% agarose gel (Invitrogen, Barcelona, Spain) and stained with ethidium bromide (5 μg/mL). Isolates were confirmed for species identity in PCR reactions with primers specific for gtfB, enconding glucosyltransferase B (5'-ACTACACTTTCGGGTGGCTTGG-3' and 5'-CAGTATAAGCGCCAGTTTCATC-3') (17) (Invitrogen) and specific to gbpB, enconding glucan-binding protein B (5'-CAACAGAAGCACAACCATCA-3' and 5'-TGTCCACCATTACCCCAGT-3') (18). The reactions were performed as described elsewhere (17,18) and the PCR products were analyzed by electrophoresis.…”

Section: Isolation Of S Mutans Strains and Extraction Of Genomic Dnamentioning

confidence: 99%

Genotypic diversity of S. mutans in dental biofilm formed in situ under sugar stress exposure

et al. 2007

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In situ dental biofilm composition under sugar exposure is well known, but sugar effect on the genotypic diversity of S. mutans in dental biofilm has not been explored. This study evaluated S. mutans genotypic diversity in dental biofilm formed in situ under frequent exposure to sucrose and its monosaccharide constituents (glucose and fructose). Saliva of 7 volunteers was collected for isolation of S. mutans and the same volunteers wore intraoral palatal appliances, containing enamel slabs, which were submitted to the following treatments: distilled and deionized water (negative control), 10% glucose + 10% fructose (fermentable carbohydrates) solution or 20% sucrose (fermentable and EPS inductor) solution, 8x/day. After 3, 7 and 14 days, the biofilms were colleted and S. mutans colonies were isolated. Arbitrarily primed polymerase chain reaction (AP-PCR) of S. mutans showed that salivary genotypes were also detected in almost all biofilm samples, independently of the treatment, and seemed to reflect those genotypes present at higher proportion in biofilms. In addition to the salivary genotypes, others were found in biofilms but in lower proportions and were distinct among treatment. The data suggest that the in situ model seems to be useful to evaluate genotypic diversity of S. mutans, but, under the tested conditions, it was not possible to clearly show that specific genotypes were selected in the biofilm due to the stress induced by sucrose metabolism or simple fermentation of its monosaccharides.

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Cloning of the Streptococcus mutans Gene Encoding Glucan Binding Protein B and Analysis of Genetic Diversity and Protein Production in Clinical Isolates

Cited by 95 publications

References 35 publications

Two-component signal transduction systems in oral bacteria

Two-component signal transduction systems in oral bacteria

Glucan-binding Proteins of the Oral Streptococci

Genotypic diversity of S. mutans in dental biofilm formed in situ under sugar stress exposure

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