Abstract

The mutans family of oral streptococci possesses antigens cross- reactive with human cardiac and skeletal muscle. This requires both caution in the development of anti-caries vaccines and intensive investigations of the immunochemistry of the cell surfaces of these microorganisms. There presently exists some confusion as to the exact nature of heart cross-reactive antigens (HRA); most reports link this property to wall-associated proteins (Spa A or P1), while others contest these findings. Recent work, however, pinpoints a 62,000 dalton (62KD) membrane-bound moiety possessing the properties of HRA. Attempts will be made to clone the 62KD membrane antigen into Escherichia coli in order to prepare purified protein and to obtain plasmids containing the relevant genetic material. Purified 62KD antigen will be analyzed as to its N-terminal amino acid sequence and its amino acid content. Because this antigen is reactive with monoclonal antibodies (mAbs) to Streptococcus pyogenes that also react with human myosin, the recombinant plasmid will be analyzed to determine the nucleotide sequence of inserted DNA in order to search for regions of homology with this eukaryotic protein. Also, cDNA probes for large regions of the myosin heavy chain will be employed in hybridization studies. If homology with myosin is found, synthetic peptides spanning these regions will be prepared as potential inhibitors in serologic assays and as immunogens to induce cross-reactive antibodies in rabbits. Inserts from the recombinant plasmid will be labeled to serve as DNA probes for the presence of this gene in chromosomal DNA for other streptococci. Simultaneously, the gene for P1 (S. mutans Ingbritt) will be cloned into E. coli to allow preparation of large amounts of purified protein. Anti-P1 immunoglobulins, affinity purified to remove other antibodies, will be used in inhibition assays to confirm the biologic role(s) of the protein in either potentiating adherence or allowing sucrose-induced cellular aggregation. The functional domains on P1 responsible for each activity will be determined either by BAL 31 exonuclease digestion of the P1 gene to obtain progressively shorter DNA inserts capable upon subcloning of yielding P1 fragments or direct cleavage of P1 by enzymes and/or cyanogen bromide. Reactive P1 fragments will be purified for N- terminal sequencing or, in the case of subclones, nucleotide sequencing would determine the relevant genetic message. Anti-P1 immunoglobulins against both cloned and native antigens will be reacted with detergent and aqueous extracts of human heart or with tissue sections by the immunogold technique. Rheumatoid factor will be removed by appropriate affinity purification. P1 also will be tested for direct binding to human heart homogenates or tissues. If positive reactions are obtained, reactive P1 epitopes (or binding sites) will be characterized as described above for functional domains. cDNA probes to detect genetic determinants for functional domains and/or epitopes will be synthesized for hybridization with DNA from streptococci.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Dental & Craniofacial Research (NIDCR)
Type
Method to Extend Research in Time (MERIT) Award (R37)
Project #
5R37DE008007-07
Application #
3482841
Study Section
Oral Biology and Medicine Subcommittee 1 (OBM)
Project Start
1986-03-01
Project End
1993-02-28
Budget Start
1992-03-01
Budget End
1993-02-28
Support Year
7
Fiscal Year
1992
Total Cost
Indirect Cost

  Institution

Name
University of Florida
Department
Type
Schools of Dentistry
DUNS #
073130411
City
Gainesville
State
FL
Country
United States
Zip Code
32611

  Publications

Sullan, Ruby May A; Li, James K; Crowley, Paula J et al. (2015) Binding forces of Streptococcus mutans P1 adhesin. ACS Nano 9:1448-60
Liao, Sumei; Klein, Marlise I; Heim, Kyle P et al. (2014) Streptococcus mutans extracellular DNA is upregulated during growth in biofilms, actively released via membrane vesicles, and influenced by components of the protein secretion machinery. J Bacteriol 196:2355-66
Funes, Soledad; Hasona, Adnan; Bauerschmitt, Heike et al. (2009) Independent gene duplications of the YidC/Oxa/Alb3 family enabled a specialized cotranslational function. Proc Natl Acad Sci U S A 106:6656-61
Ahn, Sug-Joon; Ahn, Sang-Joon; Wen, Zezhang T et al. (2008) Characteristics of biofilm formation by Streptococcus mutans in the presence of saliva. Infect Immun 76:4259-68
Dong, Yuxia; Palmer, Sara R; Hasona, Adnan et al. (2008) Functional overlap but lack of complete cross-complementation of Streptococcus mutans and Escherichia coli YidC orthologs. J Bacteriol 190:2458-69
Crowley, Paula J; Seifert, Trevor B; Isoda, Ryutaro et al. (2008) Requirements for surface expression and function of adhesin P1 from Streptococcus mutans. Infect Immun 76:2456-68
Nobbs, Angela H; Vajna, Reka M; Johnson, Jeremy R et al. (2007) Consequences of a sortase A mutation in Streptococcus gordonii. Microbiology 153:4088-97
Oli, Monika W; McArthur, William P; Brady, L Jeannine (2006) A whole cell BIAcore assay to evaluate P1-mediated adherence of Streptococcus mutans to human salivary agglutinin and inhibition by specific antibodies. J Microbiol Methods 65:503-11
Brady, L Jeannine (2005) Antibody-mediated immunomodulation: a strategy to improve host responses against microbial antigens. Infect Immun 73:671-8
Zuobi-Hasona, Kheir; Crowley, Paula J; Hasona, Adnan et al. (2005) Solubilization of cellular membrane proteins from Streptococcus mutans for two-dimensional gel electrophoresis. Electrophoresis 26:1200-5

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