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Role of the lactoferrin-binding protein in pathogenesis of streptococcus uberis

dc.contributor.advisorBabiuk, Lorne A.en_US
dc.contributor.committeeMemberSchryvers, Anthony B.en_US
dc.contributor.committeeMemberPotter, Andrew A.en_US
dc.contributor.committeeMemberPolley, Lyddenen_US
dc.contributor.committeeMemberPerez-Casal, Joseen_US
dc.contributor.committeeMemberGordon, John R.en_US
dc.contributor.committeeMemberDeneer, Harryen_US
dc.contributor.committeeMemberChirino-Trejo, Manuelen_US
dc.creatorMoshynskyy, Igoren_US
dc.date.accessioned2005-07-14T14:07:13Zen_US
dc.date.accessioned2013-01-04T04:44:45Z
dc.date.available2005-07-22T08:00:00Zen_US
dc.date.available2013-01-04T04:44:45Z
dc.date.created2005-06en_US
dc.date.issued2005-06-27en_US
dc.date.submittedJune 2005en_US
dc.description.abstractThe pathogenesis of the bovine environmental pathogen Streptococcus uberis has been extensively studied, but it remains incompletely understood. The organism produces a surface protein capable of binding lactoferrin (Lbp), originally identified as an M-like streptococcal protein. We hypothesized that Lbp may play a role as a virulence factor. Structural similarity and amino acid sequence homology of Lbp to Mrelated proteins of Group A streptococci suggested a possible functional similarity between Lbp and M-like proteins, which are involved in evasion of host antibacterial defenses, adhesion to host epithelial cells and intracellular invasion by the bacteria. Alternatively, high-affinity binding of the abundant iron-chelating component of the host milk (lactoferrin) suggests that Lbp of S. uberis might play role in iron acquisition by the bacterium. Finally, Lbp might serve as a receptor for signal transduction in the bacterial cell or alter host cell signalling during infection, when the bacteria with surface-bound lactoferrin adhere to or invade the host epithelial cells. In order to test the hypothesis that Lbp is a virulence factor of S. uberis, a mutant strain of S. uberis unable to express the lactoferrin-binding protein was generated and the role of the protein was studied in comparative analyses of the mutant and the parent strains. The results of our study indicated that unlike many streptococcal M-like proteins, the lactoferrin-binding protein of S. uberis did not appear to play a role in overcoming host innate and acquired immune antibacterial responses. Both S. uberis and its lbp mutant were ingested by bovine blood neutrophils and were similar in their ability to survive in fresh bovine blood regardless of the presence either of lactoferrin or of anti-Lbp antibodies. Lbp did not promote bacterial adhesion to host epithelial cells and it was not essential for the internalization of the bacteria by host epithelial cells, since both S. uberis and lbp mutant were found capable of adhering, invading, intracellular survival and intracellular growth when the bacteria were co-cultured with bovine mammary epithelial cells. No significant differences in numbers of adherent or internalized bacteria per host cell were found between wild type and lbp mutant cells. S. uberis requirements for iron were determined to be low and Lbp was not essential for iron acquisition by the organism from iron-saturated lactoferrin. To study the role of Lbp in bacterial virulence during infection of bovine mammary glands, dairy cows in the second half of their lactation periods were challenged with the wild type S. uberis and with the lbp mutant. The results of in vivo infection suggested that expression of Lbp by the bacteria was not essential for colonization of the host mammary gland and that expression of Lbp was not associated with differences in severity of mastitis or with different levels of shedding of the bacteria by infected animals. To study the role of Lbp in signal transduction, differential bacterial cellular protein phosphorylation in the presence of bovine lactoferrin was analyzed. Since no differences in protein phosphorylation profiles were detected between S. uberis and the lbp mutant, it was concluded that Lbp is probably not a part of a classical bacterial twocomponent signalling pathway. However, we demonstrated that the expression of host genes potentially involved in cell morphogenesis, motility and signal transduction was regulated depending on the expression of Lbp by S. uberis. Down-regulation of the expression of selected host genes was verified by quantitative reverse transcription PCR. Putative iron responsive elements were identified in mRNA of several of these genes. Down-regulation of these genes in the cells overloaded with ferric iron was demonstrated by RT PCR. These results indicate that Lbp of S. uberis may interfere with host cellular signalling pathways by inducing perturbations in the cell iron status. This suggests that Lbp of S. uberis may be a virulence factor, playing a role in signal transduction or in the regulation of gene expression in host cells.en_US
dc.identifier.urihttp://hdl.handle.net/10388/etd-07142005-140713en_US
dc.language.isoen_USen_US
dc.subjectstreptococcal mastitisen_US
dc.titleRole of the lactoferrin-binding protein in pathogenesis of streptococcus uberisen_US
dc.type.genreThesisen_US
dc.type.materialtexten_US
thesis.degree.departmentVeterinary Microbiologyen_US
thesis.degree.disciplineVeterinary Microbiologyen_US
thesis.degree.grantorUniversity of Saskatchewanen_US
thesis.degree.levelDoctoralen_US
thesis.degree.nameDoctor of Philosophy (Ph.D.)en_US

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