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Streptococcus pneumoniae is a commensal of the human upper respiratory tract and moreover, the
causative agent of several life-threatening diseases including pneumonia, sepsis, otitis media, and
meningitis. Due to the worldwide rise of resistance to antibiotics in pneumococci the understanding
of its physiology is of increasing importance. In this context, the analysis of the pneumococcal
proteome is helpful as comprehensive data on protein abundances in S. pneumoniae may provide
an extensive source of information to facilitate the development of new vaccines and drug
treatments.
It is known that protein phosphorylation on serine, threonine and tyrosine residues is a major
regulatory post-translational modification in pathogenic bacteria. This reversible post-translational
modification enables the translation of extracellular signals into cellular responses and therewith
adaptation to a steadily changing environment. Consequently, it is of particular interest to gather
precise information about the phosphoproteome of pneumococci. S. pneumoniae encodes a single
Serine/Threonine kinase-phosphatase couple known as StkP-PhpP.
To address the global impact and physiological importance of StkP and PhpP which are closely
linked to the regulation of cell morphology, growth and cell division in S. pneumoniae, proteomics
with an emphasis on phosphorylation and dephosphorylation events on Ser and Thr residues was
applied. Thus, the non-encapsulated pneumococcal D39Δcps strain (WT), a kinase (ΔstkP) and
phosphatase mutant (ΔphpP) were analyzed in in a mass spectrometry based label-free
quantification experiment. The global proteome analysis of the mutants deficient for stkP or phpP
already proved the essential role of StkP-PhpP in the protein regulation of the pneumococcus.
Proteins with significantly altered abundances were detected in diverse functional groups in both
mutants. Noticeable changes in the proteome of the stkP deletion mutant were observed in
metabolic processes such as “Amino acid metabolism” and also in pathways regulating genetic
and environmental information processing like “Transcription” and “Signal transduction”.
Prominent changes in the metabolism of DNA, nucleotides, carbohydrates, cofactors and vitamins
as well as in the categories “Transport and binding proteins” and “Glycan biosynthesis and
metabolism” have been additionally detected in the proteome of the phosphatase mutant. Still, the
quantitative comparison of WT and mutants revealed more significantly altered proteins in ΔphpP
than in ΔstkP. Moreover, the results indicated that the loss of function of PhpP causes an increased
abundance of proteins in the pneumococcal phosphate uptake system Pst. Furthermore, the
obtained quantitative proteomic data revealed an influence of StkP and PhpP on the twocomponent
systems ComDE, LiaRS, CiaRH, and VicRK.
Recent studies of the pneumococcal StkP/PhpP couple demonstrated that both proteins play an
essential role in cell growth, cell division and separation. Growth analyses and the phenotypic
characterization of the mutants by electron-microscopy performed within this work pointed out
that ΔphpP and ΔstkP had different growth characteristics and abnormal cell division and cell
separation. Nevertheless, the morphological effects could not be explained by changes in protein
abundances on a global scale. So, the in-depth analysis of the phosphoproteome was mandatory
to deliver further information of PhpP and StkP and their influence in cell division and
peptidoglycan synthesis by modulating proteins involved in this mechanisms.
For more detailed insights into the activity, targets and target sites of PhpP and StkP the advantages
of phosphopeptide enrichment using titanium dioxide and spectral library based data evaluation
were combined. Indeed, the application of an adapted workflow for phosphoproteome analyses
and the use of a recently constructed broad spectral library, including a large number of
phosphopeptides (504) highly enhanced the reliable and reproducible identification of
phosphorylated proteins in this work.
Finally, already known targets and target sites of StkP and PhpP, detected and described in other
studies using different experimental procedures, have been identified as a proof of principle
applying the mass spectrometry based phosphoproteome approach presented in this work.
Referring to the role of StkP in cell division and cell separation a number of proteins participating
in cell wall synthesis and cell division that are apparently phosphorylated by StkP was identified.
In comparison to StkP, the physiological function and role of the co-expressed phosphatase PhpP
is poorly understood. But, especially the list of previously unknown putative target substrates of
PhpP has been extended remarkably in this work. Among others, five proteins with direct
involvement in cell division (DivIVA, GpsB) and peptidoglycan biosynthesis (MltG, MreC, MacP)
can be found under the new putative targets of PhpP.
All in all, this work provides a complex and comprehensive protein repository of high proteome
coverage of S. pneumoniae D39 including identification of yet unknown serine/threonine/tyrosine
phosphorylation, which might contribute to support various research interests within the scientific
community and will facilitate further investigations of this important human pathogen.
The influence of regulatory proteins on the physiology and virulence of Streptococcus pneumoniae
(2015)
In conclusion, this work identifies the regulator ArgR2 as activator of the S. pneumoniae TIGR4 arginine deiminase system and arginine-ornithine transporter ArcD, which is needed for uptake of the essential amino acid arginine. Although ArgR2 activates ArcD expression and uptake of arginine is required to maintain pneumococcal fitness, the deficiency of ArgR2 increases TIGR4 virulence under in vivo conditions, suggesting that other factors regulated by ArgR2 counterbalance the reduced uptake of arginine by ArcD. Thus this works illustrates that the physiological homeostasis of pneumococci is complex and that ArgR2 plays a key role in maintaining bacterial fitness. Moreover, Rex was identified as a regulator of housekeeping genes including genes encoding glycolytic enzymes. In vitro studies and gene expression analyses suggested that the regulator Rex does not have an influence on the physiology of S. pneumoniae. However, a co-infection experiment demonstrated that Rex is involved in maintaining pneumococcal fitness and robustness under in vivo conditions.
Streptococcus pneumoniae (pneumococci) are lancet-shaped, Gram-positive, alpha-hemolytic, facultative anaerobic human specific commensals of the upper and lower respiratory tract. Pneumococci may convert to pathogenic bacteria and spread to the lungs and blood. In different population groups, such as children, the elderly and immunocompromised individuals, pneumococci can cause local infections such as bronchitis, rhinitis, acute sinusitis, and otitis media as well as life-threatening invasive diseases such as community-acquired pneumonia, sepsis and meningitis. Pneumococci are surrounded by a rigid and complex exoskeleton, the peptidoglycan, also referred to as murein sacculus. The peptidoglycan (PNG) protects the cells from rupture by osmotic pressure and maintains their characteristic shape. The PNG is a heteropolymer made up of glycan strands that are cross-linked by short peptides and during growth the existing murein is continuously hydrolyzed by specific lytic enzymes to enable the insertion of new peptidoglycan. Bacterial cell-wall hydrolases are essential for peptidoglycan turnover and crucial to preserve cell shape. The D,D-carboxypeptidase DacA and L,D-carboxypeptidase DacB of Streptococcus pneumoniae function in a sequential manner. This study determined the crystal structure of the surface-exposed lipoprotein DacB, which differs considerably from the DacA structure. DacB contains a Zn2+ ion in its catalytic center located in the middle of a fully exposed, large groove. Two different conformations with differently arranged active site topology were identified. In addition the critical residues for catalysis and substrate specificity were identified. Deficiency in DacA or DacB resulted in a modified peptidoglycan peptide composition and led to an altered cell shape of the dac-mutants. In contrast, lgt-mutant lacking lipoprotein diacylglyceryl transferase activity required for proper lipoprotein maturation retained L,D-carboxypeptidase activity and showed an intact murein sacculus. Furthermore, this study demonstrated the pathophysiological effects of disordered DacA or DacB activities. Real-time bioimaging of intranasally infected mice indicated a substantially attenuated virulence of dacB- and dacAdacB-mutants pneumococci, while loss of function of DacA had no significant effect. In addition, uptake of these mutants by professional phagocytes was enhanced, while their adherence to lung epithelial cells was decreased. The second part of this study focused on the functional and structure determination of the soluble dimeric pneumococcal lipoprotein PccL. Because of its calycin fold and structural homology with the lipocalin YxeF from Bacillus subtilis, PccL was introduced as the first member of the lipocalin protein family in pneumococci and named “PccL” (Pneumococcal calycin fold containing Lipoprotein). Similar to other lipocalins, the distinct beta-barrel, which is open at one end, is significantly conserved in PccL. Moreover, the application of the in vivo acute pneumonia mouse infection model and the in vitro phagocytosis as well as adherence invasion studies revealed considerable differences in colonization and invasive infection between the wild-type D39 and the pccL-mutant. In conclusion, this study characterized the crucial role of pneumococcal carboxypeptidases DacA and DacB for PGN architecture, bacterial shape and pathogenesis. By applying in vivo and in vitro approaches, a close relationship between PGN metabolism and pathophysiological effects was discovered. In addition, the high resolution structure of DacB has been solved and analyzed and a structure model with a resolution of 2.0 Å is provided. Furthermore, analysis of the PGN composition was applied to indicate the impact of an impaired lipoprotein biogenesis pathway on localization and activity of DacB. The major impact of carboxypeptidases on cell shape and virulence proposes DacB as a promising target for the development of novel drugs or due to its surface exposition also as a promising vaccine candidate. PccL is the first pneumococcal lipocalin-like protein and this study indicated its contribution to pneumococcal virulence. However, the mechanism and the mode of action of PccL are still unknown and have to be deciphered in further studies.
Streptococcus pneumoniae (pneumococci) are Gram-positive cocci and commensals of the human upper respiratory tract. Pneumococcal pathogenesis requires adherence to host cells and dissemination through cellular barriers and to evade host defense mechanisms. The Pneumococcal surface protein C (PspC) is an important virulence factor which has a crucial role in pneumococcal adhesion to host cells and immune evasion by manipulating the host complement system. To elucidate the pneumococcal adherence and uptake mechanism via factor H glycosaminoglycans (dermatan sulfate and heparin) were employed as competitive inhibitors in infection experiments with epithelial cells or human polymorphonuclear leukocytes (PMNs). Glycosaminoglycans significantly inhibited the FH mediated pneumococcal adherence and subsequent invasion to host epithelial cells. Furthermore, the short consensus repeats of FH which promotes the adhesion of pneumococci to host cells were identified by blocking experiments with domain mapped antibodies for specific regions of FH. Moreover, this study indicates that FH acts as adhesion molecule via cellular receptors recognized as integrin CR3 on human PMNs. Binding of Factor H loaded pneumococci to integrins CR3 was assessed by flow cytometry. Pneumococci coated with Factor H showed a significantly increased association with PMNs. This interaction was blocked by anti-CR3 antibodies and Pra1. This project further aims to study mechanisms of pneumococcal endocytosis by host cells, their intracellular fate, and the pathogen induced host cell signal transduction cascades including the calcium signaling upon pneumococcal infection of host cells via the PspC-hpIgR interaction. To assess now the role of protein tyrosine kinases (PTKs) during pneumococcal infection via PspC, cell culture infections were performed in presence of pharmacological inhibitors of PTKs and MAPKs or by employing genetic interference techniques. Blocking the function of Src or ER1/2 and JNK and genetic-knock down of Src and FAK reduced significantly internalization of pneumococci. These data indicated the importance of a coordinated signaling between Src PTKs, ERK1/2, and JNK during PspC-pIgR-mediated uptake of pneumococci by host epithelial cells. The impact of host cells intracellular calcium concentrations on pneumococcal PspC-hpIgR mediated internalization was studied. Intracellular calcium measurement of epithelial cells performed in the presence of pneumococci suggested a calcium influx in host epithelial cells and importantly this calcium influx was PspC- hpIgR specific as pspC-deficient pneumococci were unable to mediate calcium mobilization in host cells. The increase in intracellular calcium [Ca2+]i was dependent on phospholipase C as pretreatment of cells with a phospholipase C-specific inhibitor abolished the increase in [Ca2+]i. Furthermore, role of host intracellular calcium concentrations during pneumococcal internalization was demonstrated by employing specific pharmacological inhibitors and calcium chelators in epithelial cell culture infection assays. The results revealed that elevated host cells calcium concentrations diminished pneumococcal internalization while lower calcium concentration in host epithelial cells promoted pneumococcal uptake. This study further demonstrates that dynamin, clathrin and caveolin play a key role during pneumococcal endocytosis into host cells via PspC-hpIgR. The use of specific pharmacological inhibitors or genetic interference approaches against dynamin, clathrin and caveolin in epithelial cell culture infection assays significantly blocked pneumococcal uptake. Furthermore, confocal microscopy revealed that pneumococci co-localize with clathrin. At later stages of the infection the pathogen is sorted to early, late and recycling endosomes as indicated by co-localization of pneumococci with endosomal markers such as Rab5, Rab4, Rab 7, and Lamp1. In order to get further insights into PspC-hpIgR mediated uptake mechanisms, a chimeric PspC was constructed and expressed heterologously on the surface of Lactococcus lactis. Immunofluorescence staining, immunoblot and flow cytometric analysis of L. lactis confirmed the expression of PspC on the bacterial surface. Moreover the ability of recombinant lactococci expressing PspC to adhere to and to invade pIgR-expressing epithelial cells confirmed the functional activity of PspC when exposed on the lactococcal surface. PspC expressing lactococci confirmed the specificity of PspC-hpIgR mediated endocytosis in host epithelial cells as PspC deficient lactococci were not taken up by these host cells. Confocal microscopic analysis demonstrated that only PspC expressing lactococci were sorted to early, late and recycling endosomes, similar to the intracellular fate of S. pneumoniae.