Dextranases from oral bacteria: inhibition of water-insoluble glucan production and adherence to smooth surfaces by Streptococcus mutans

Schachtele, C F; Staat, Robert H.; Harlander, Susan K.

doi:10.1128/iai.12.2.309-317.1975

Cited by 113 publications

(46 citation statements)

References 39 publications

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“…mutans, radiolabeled as described above, were suspended to an optical density of 2.0 at 540 nm in PBS containing 0.2 mM sucrose. Two-ral portions were added to glass vials and incubated at 3?°C for intervals up to 6 h. Such incubation of S. mutans with sucrose fosters attachment of bacteria through glucan formation by the etizyme glucosyltransferase (13). Following aspiration, washing, and drying as described above, the glass vials were assayed lor radioactivity and the number of S. mutaru cells adhering was estimated.…”

Section: In Vitro Test For Enzyme-mediated Attachmentmentioning

confidence: 99%

Effects of bactericidal treatments on bacterial adherence and dental plaque formation

Ørstavik

Ruangsri

1979

European J Oral Sciences

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abstract— in vivo plaque formation was significantly reduced when tooth surfaces were subjected to topical applications of iodine (0.2% I2 in 2.0% KI) twice daily for 3 d. Similarly, in vivo plaque formation was significantly reduced on enamel surfaces that were subjected to ultraviolet irradiation. Control experiments indicated that neither ultraviolet irradiation nor iodine treatment interfered with mechanisms for bacterial apposition to dental plaque. The results are interpreted to suggest that plaque grows in mass primarily by the division and multiplication in situ by plaque bacteria, not by a continued apposition of salivary microbes.

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Section: In Vitro Test For Enzyme-mediated Attachmentmentioning

confidence: 99%

Effects of bactericidal treatments on bacterial adherence and dental plaque formation

Ørstavik

Ruangsri

1979

European J Oral Sciences

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“…sobrinus are predominant producers of the enzyme dextranase (Dex) which cleaves a-1,6-linkages of glucans (Walker et al 1981;Igarashi et al 1992;Wanda and Curtis 1994). The Dex is thought to be responsible both for the control of the amount and content of extracellular glucans and for the metabolic utilization of extracellular glucans (Schachtele et al 1975;Germaine et al 1977;Walker et al 1981;Felgenhauer and Trautner 1983;Colby et al 1995). From these results, the Dex has been thought to be an important determinant of virulence.…”

Section: Introductionmentioning

confidence: 99%

Analysis of a dextran-binding domain of the dextranase of Streptococcus mutans

Morisaki

Igarashi

Yamamoto

et al. 2002

Lett Appl Microbiol

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Aims: To examine the dextran‐binding domain of the dextranase (Dex) of Streptococcus mutans.  Methods and Results: Deletion mutants of the Dex gene of Strep. mutans were prepared by polymerase chain reaction and expressed in Escherichia coli cells. Binding of the truncated Dexs to dextran was measured with a Sephadex G‐150 gel. Although the Dexs which lacked the N‐terminal variable region lost enzyme activity, they still retained dextran‐binding ability. In addition, further deletion into the conserved region from the N‐terminal did not influence the dextran‐binding ability. However, the Dex which carried a deletion in the C‐terminus still possessed both enzyme activity and dextran‐binding ability. Further deletion into the conserved region from the C‐terminal resulted in complete disappearance of both enzyme and dextran‐binding activities.  Conclusions: Deletion analysis of the Dex gene of Strep. mutans showed that the C‐terminal side (about 120 amino acid residues) of the conserved region of the Dex was essential for dextran‐binding ability.  Significance and Impact of the Study: The dextran‐binding domain was present in a different area from the catalytic site in the conserved region of the Dex molecule. The amino acid sequence of the dextran‐binding domain of the Dex differed from those of glucan‐binding regions of other glucan‐binding proteins reported.

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“…Dex also possesses an N-terminal signal peptide and a C-terminal sorting signal in VRs (15,18,35). In addition, Dex is thought to be responsible both for controling the amount and nature of extracellular glucans and for utilizing extracellular glucans as a carbohydrate source (5,21,25,28,34). Consequently, Dex is thought to be one of the virulent factors in mutans streptococci.In this paper we sequenced and characterized the dex gene of S. rattus ATCC19645 and compared the Dex molecule of S. rattus with that of S. mutans, S. sobrinus, Streptococcus downei, and Streptococcus salivarius.…”

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confidence: 99%

Molecular Characterization of Dextranase from Streptococcus rattus

Igarashi

Morisaki

Goto

2004

Microbiology and Immunology

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Streptococcus rattus is a cariogenic bacterium classified under mutans streptococci (36). This organism is usually isolated from the oral cavities of rats and occasionally of humans. As most studies concerning cariogenic properties of mutans streptococci have focused on Streptococcus mutans and Streptococcus sobrinus, which are frequently isolated from the human oral cavity, little is known about those of S. rattus. Before now many factors associated with cariogenicity of S. mutans and S. sobrinus have been determined (4,8,20); for example, one of them is a dextranase (Dex) that hydrolyzes α-1, 6-linkage in a glucan molecule produced from sucrose by mutans streptococci (3,7,8,13,34). Although a wide range of bacterial species associated with dental plaque is shown to produce Dex (19), oral streptococci, in particular mutans streptococci, are known to be a major producer of Dex (30,34). So far, the Dexs of S. mutans and S. sobrinus have been well characterized by biological and genetic studies (2, 12-15, 23, 35). Previous genetic studies showed structural features and the physiological role of Dex. It has been shown that the Dex molecule is composed of two variable regions (VRs) and a conserved region (CR) (15,18), and that catalytic and glucan-binding sites exist in the CR of the Dex molecule (12, 23). Dex also possesses an N-terminal signal peptide and a C-terminal sorting signal in VRs (15,18,35). In addition, Dex is thought to be responsible both for controling the amount and nature of extracellular glucans and for utilizing extracellular glucans as a carbohydrate source (5,21,25,28,34). Consequently, Dex is thought to be one of the virulent factors in mutans streptococci.In this paper we sequenced and characterized the dex gene of S. rattus ATCC19645 and compared the Dex molecule of S. rattus with that of S. mutans, S. sobrinus, Streptococcus downei, and Streptococcus salivarius. Materials and MethodsBacterial strains and plasmid. Streptococcus rattus ATCC19645, which was isolated from a caries lesion in rat, was grown in Todd Hewitt broth (Difco Laboratories, Detroit, Mich., U.S.A.). Escherichia coli JM109 was cultured in Luria-Bertani broth. Plasmid vector pT7Blue T (Novagen, Madison, Wisc., U.S.A.) was used for gene cloning and sequencing (14). GST gene fusion vector, pGEX-4T-2 (Pharmacia Biotech, Uppsala, Sweden), Molecular Characterization of Dextranase from

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Dextranases from oral bacteria: inhibition of water-insoluble glucan production and adherence to smooth surfaces by Streptococcus mutans

Cited by 113 publications

References 39 publications

Effects of bactericidal treatments on bacterial adherence and dental plaque formation

Effects of bactericidal treatments on bacterial adherence and dental plaque formation

Analysis of a dextran-binding domain of the dextranase of Streptococcus mutans

Molecular Characterization of Dextranase from Streptococcus rattus

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