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      In vitro bacterial plaque suppression and recolonization by S. mutans and S. sobrinus Translated title: Supressão e recolonização de placa bacteriana por S. mutans e S. sobrinus in vitro

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          Abstract

          The in vitro study of the interactions between S. mutans and S. sobrinus is important to determine the role of these microorganisms in the formation of biofilms on dental structures and their potential to induce carious lesions. The objective of this research was to study the suppression of bacterial plaque formation and its recolonization by rifampycin-resistant S.mutans and streptomycin-resistant S. sobrinus. To study the competitive relationship between these species, previously standardized strains were incubated in media containing different fermentable carbohydrates. At determined time intervals, samples were collected from mixed cultures of S. mutans and S. sobrinus, diluted and plated on BHI-agar containing rifampycin or streptomycin to determine the number of viable cells of each species by counting colony-forming units. In order to study the bacterial colonization process and in vitro recolonization of bacterial plaque, three experiments were performed: I - co-cultivation of S. mutans and S. sobrinus; II - inoculation of bacterial plaque pre formed by S. sobrinus with S. mutans; and III - bacterial plaque pre formed by S. mutans dispersed and plated on BHI- agar containing streptomycin or rifampicin to determine the number of viable cells for each species. The results indicated a predominance of S. mutans in relation to S. sobrinus, demonstrating the capacity of S. mutans to inhibit plaque formation by S. sobrinus and recolonize the surfaces.

          Translated abstract

          O estudo in vitro das interações entre S. mutans e S. sobrinus pode ser importante na determinação do papel desses microrganismos na formação de biofilmes nas estruturas dentais e seu potencial em induzir lesões cariosas. O objetivo da presente pesquisa foi estudar a supressão da formação da placa dental e sua recolonização por S. mutans rifampicina-resistentes e S. sobrinus estreptomicina-resistentes in vitro. Para avaliar as relações de competitividade entre essas espécies, cepas que foram previamente padronizadas foram incubadas em meio de cultura contendo diferentes carboidratos fermentáveis. Em intervalos de tempo determinados, amostras de S. mutans e S. sobrinus foram coletadas a partir de culturas mistas, diluídas e semeadas em placas com meio BHI-ágar contendo rifampicina ou estreptomicina para determinação do número de células viáveis de cada espécie por contagem de unidades formadoras de colônia. Para a avaliação da colonização bacteriana e recolonização da placa bacteriana in vitro, três experimentos foram realizados: I - co-cultivo de S. mutans e S. sobrinus; II - inoculação de S. mutans em placa bacteriana pré-formada por S. sobrinus; e III - placa bacteriana pré-formada por S. mutans dispersada e plaqueada em meio BHI-ágar contendo estreptomicina ou rifampicina para determinação do número de células viáveis para cada espécie. Os resultados indicaram uma predominância de S. mutans em relação ao S. sobrinus, demonstrando a capacidade do S. mutans em inibir a formação de placa por S. sobrinus e recolonizar a superfície dentária.

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          Simple and rapid detection of Streptococcus mutans and Streptococcus sobrinus in human saliva by polymerase chain reaction.

          M Kushiyama, T Oho, Tomoaki Koga (2000)
          Streptococcus mutans and Streptococcus sobrinus are major pathogens causing dental caries in humans. A simple and rapid method to detect these species in human saliva simultaneously was developed using the polymerase chain reaction (PCR). Chromosomal DNA was extracted by boiling bacterial cells in lysis solution containing 1% Triton X-100. Oligonucleotide primers specific for portions of the glucosyltransferase genes (gtfB of S. mutans and gtfI of S. sobrinus) were designed. After PCR using two sets of these primers, S. mutans and S. sobrinus were specifically identified. The method was capable of amplifying DNA fragments specific for these species from chromosomal DNA extracted from 1 x 10(3) cells, or from 10 microliters of clinical saliva samples containing 1 x 10(3) colony-forming units of either streptococcal species. A second PCR, using the first PCR product as a template with newly designed internal primers, made it possible to detect 1 x 10(2) colony-forming units of either streptococcal species in 10 microliters of saliva samples. These results indicate that the PCR method developed in this study is useful for detecting S. mutans and S. sobrinus in saliva and that it can be used in epidemiological studies to evaluate the prevalence level of these organisms.
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            Longitudinal study of transmission, diversity, and stability of Streptococcus mutans and Streptococcus sobrinus genotypes in Brazilian nursery children.

            Flávia Flório, Claudia C. de A. Pereira, Marlise Klein (2004)
            The aim of this study was to perform a follow-up evaluation of the Streptococcus mutans and Streptococcus sobrinus colonization profile of children's oral cavities, which included the pattern of vertical transmission from mother to child, genotypic diversity, and stability of the strains. The subjects were 16 mother-child pairs, who were monitored for 20 months. Samples of saliva, tongue dorsum, alveolar ridge mucosa, and dental plaque from the children were collected bimonthly. Saliva samples from the mothers were also collected. After isolation and identification, the arbitrarily primed PCR method was performed for the genotypic characterization of S. mutans (968 isolates) and S. sobrinus (111 isolates). At the time the strains were acquired, the children harbored one to four distinct genotypes of S. mutans and only one genotype of S. sobrinus. Although S. mutans prevalence and genotypic diversity were greater than those of S. sobrinus, the presence of matching genotypes of S. mutans and S. sobrinus was similar (in 81.25 and 83.33% of mother-child pairs, respectively), suggesting vertical transmission for both species. This longitudinal study showed an increase in genotypic diversity of S. mutans in the oral cavity during the follow-up period: most of the initially acquired genotypes persisted, normally those genotypes transmitted by the mother, and some were lost during follow-up; new strains were also acquired. In conclusion, S. mutans and S. sobrinus genotypes acquired from maternal or alternative sources may show effective persistence in the oral cavity and/or transitory detection in the children's mouths, reflecting the continuous development of oral microbiota in children.
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              Mutacin production in Streptococcus mutans genotypes isolated from caries-affected and caries-free individuals.

              Luciana Gonçalves, Marcelo NAPIMOGA, Adriane Rosa (2005)
              Relationships between genetic diversity and mutacin production in Streptococcus mutans were evaluated in 319 clinical isolates from eight caries-affected and eight caries-free individuals. The isolates were submitted to mutacin typing and AP-PCR (arbitrarily primed polymerase chain reaction) assay. The mutacin production was detected for 12 Streptococcus sp. indicator strains. Results showed significant variations in the mutacin production profiles and the inhibitory spectra of both groups. A possible association was seen between mutacin activity and the distinct patterns of Streptococcus sp. colonization in the two groups. Genotyping by AP-PCR using the primers OPA-02 and OPA-13 revealed 101 distinct genotypes against 48 phenotypes identified by mutacin typing. No correlation was observed between the inhibitory spectra of mutacin and genotypic similarities based on AP-PCR analyses. According to our results, strains of the same S. mutans genotype showed different mutacin profiles, suggesting a high degree of interstrain diversity. In conclusion, mutacin production seems to be of clinical importance in the colonization of S. mutans and is highly diversified in the S. mutans species. Copyright (c) Blackwell Munksgaard, 2005
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                Author and article information

                Journal
                Journal ID (publisher-id): bjm
                Title: Brazilian Journal of Microbiology
                Abbreviated Title: Braz. J. Microbiol.
                Publisher: Sociedade Brasileira de Microbiologia (São Paulo, SP, Brazil )
                ISSN (Print): 1517-8382
                ISSN (Electronic): 1678-4405
                Publication date (Print and electronic): March 2006
                Volume: 37
                Issue: 1
                Pages: 20-25
                Affiliations
                [01] Bauru SP orgnameUniversidade Sagrado Coração orgdiv1Departamento de Biologia Oral Brasil
                [02] Três Corações MG orgnameUniversidade Vale do Rio Verde orgdiv1Área de Diagnóstico Bucal Brasil
                [03] Piracicaba SP orgnameUniversidade Estadual de Campinas orgdiv1Faculdade de Odontologia de Piracicaba orgdiv2Laboratório de Microbiologia e Imunologia Brasil
                Article
                Publisher ID: S1517-83822006000100004 Publisher ID: S1517-8382(06)03700104
                SO-VID: 576db59f-ee59-49ca-8e92-3c3ea8900b0e
                License:

                This work is licensed under a Creative Commons Attribution-NonCommercial 4.0 International License.

                History
                Date received : 27 April 2004
                Date accepted : 15 February 2006
                Date revision received : 23 August 2004
                Page count
                Figures: 0, Tables: 0, Equations: 0, References: 21, Pages: 6
                Product

                SciELO Brazil

                Categories
                Subject: Medical Microbiology

                Keywords: Streptococcus sobrinus,suppression,Streptococcus mutans,supressão,Streptococcus mutan
                Data availability:
                Keywords: Streptococcus sobrinus, suppression, Streptococcus mutans, supressão, Streptococcus mutan

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