Proteomic Analysis and Identification of
            <i>Streptococcus pyogenes</i>
            Surface-Associated Proteins

Severin, Anatoly; Nickbarg, Elliott; Wooters, Joseph; Quazi, Shakey A.; Matsuka, Yury V.; Murphy, Ellen; Moutsatsos, Ioannis K.; Zagursky, Robert J.; Olmsted, Stephen B.

doi:10.1128/jb.01132-06

Cited by 142 publications

(158 citation statements)

References 63 publications

Supporting

Mentioning

142

Contrasting

Unclassified

Order By: Relevance

“…Conjecture exists in the scientific literature regarding the biological relevance and certitude of surface expression of anchorless proteins in GAS [5,30]. To validate our findings and to test protective vaccine efficacy of the selected anchorless surface proteins, full-length M1 protein, ADI, TF and FBA were adjuvanted with Complete Freund's Adjuvant (CFA) and used to subcutaneously immunize BALB/c mice and the survival recorded following lethal intraperitoneal M1 GAS challenge.…”

Section: Anchorless Proteins Elicit Protective Immunitymentioning

confidence: 82%

“…These authors also demonstrated considerable cross-protection of the 30-valent vaccine against non-vaccine M serotypes [4]. Recently, a series of independent studies have documented a class of GAS cell wall-associated or secreted metabolic enzymes that contain neither N-terminal leader sequences nor C-terminal cell wall anchors [5][6][7][8][9]. Perhaps because these molecules do not fit common categories of bacterial vaccine antigen, e.g.…”

mentioning

confidence: 99%

See 1 more Smart Citation

Conserved anchorless surface proteins as group A streptococcal vaccine candidates

et al. 2012

View full text Add to dashboard Cite

Section: Anchorless Proteins Elicit Protective Immunitymentioning

confidence: 82%

mentioning

confidence: 99%

Conserved anchorless surface proteins as group A streptococcal vaccine candidates

et al. 2012

View full text Add to dashboard Cite

“…In total, taking into account the membrane protein fraction and the envelope-associated soluble protein fraction, one of the most remarkable findings of this work was the large amount of ribosomal proteins detected: 41 out of the 52 ribosomal proteins annotated in the B. longum NCC 2705 genome were identified. Ribosomal proteins are very often found associated with the cell surface in bacteria, and although they are thought to have a certain affinity for the inner leaflet of the membrane, they have also been detected on the bacterial surface exposed to the external medium (Severin et al, 2007;Tjalsma et al, 2008). In some cases it has even been demonstrated that ribosomal proteins are immunomodulatory for humans (Spence & Clark, 2000).…”

Section: Discussionmentioning

confidence: 99%

“…In relation to this, with the aim of determining the protein profile of the B. longum envelope, and as a first approach to undertaking deeper functional studies, we analysed different subcellular fractions. The application of gel-based and gel-free technologies, combined with high-throughput techniques, allowed us to identify 218 proteins; about 70 % of them were predicted to be, or were previously described as being, in the cell envelope of Gram-positive bacteria (Antikainen et al, 2007;Candela et al, 2007;Eymann et al, 2004;Granato et al, 2004;Jang & Hanash 2003;Kelly et al, 2005b;Nandakumar et al, 2005;Rivera-Amill et al, 2001;Rodríguez-Ortega et al, 2006;Schaumburg et al, 2004;Severin et al, 2007;Silveira et al, 2004;Tjalsma et al, 2008;Wolff et al, 2007). Furthermore, 48 of them are predicted to be integral membrane proteins (contain hypothetical transmembrane segments) and 30 of them have different extracytoplasmic sorting signals.…”

Section: Discussionmentioning

confidence: 99%

The cell-envelope proteome of Bifidobacterium longum in an in vitro bile environment

et al. 2009

View full text Add to dashboard Cite

Host-bacteria interactions are often mediated via surface-associated proteins. The identification of these proteins is an important goal of bacterial proteomics. To address how bile can influence the cell-envelope proteome of Bifidobacterium longum biotype longum NCIMB 8809, we analysed its membrane protein fraction using stable isotope labelling of amino acids in cell culture (SILAC). We were able to identify 141 proteins in the membrane fraction, including a large percentage of the theoretical transporters of this species. Moreover, the envelope-associated soluble fraction was analysed using different subfractionation techniques and differential in-gel fluorescence electrophoresis (DIGE). This approach identified 128 different proteins. Some of them were well-known cell wall proteins, but others were highly conserved cytoplasmic proteins probably displaying a 'moonlighting' function. We were able to identify 11 proteins in the membrane fraction and 6 proteins in the envelope-associated soluble fraction whose concentration varied in the presence of bile. Bile promoted changes in the levels of proteins with important biological functions, such as some ribosomal proteins and enolase. Also, oligopeptide-binding proteins were accumulated on the cell surface, which was reflected in a different tripeptide transport rate in the cells grown with bile. The data reported here will provide the first cell-envelope proteome map for B. longum, and may contribute to understanding the bile tolerance of these bacteria

show abstract

“…For intracellular proteome preparation (Malmström et al, 2012a), the bacterial cells were lysed using a bead-beater and centrifuged, and the supernatant was prepared for MS analysis, as subsequently described. For surface proteome preparation (Severin et al, 2007;Solis et al, 2010), surface-associated proteins were released by trypsination of the bacterial cells in a hypotonic solution. The trypsinated bacteria were gently centrifuged and the supernatant was prepared for MS analysis, as subsequently described.…”

Section: Introductionmentioning

confidence: 99%

Surface proteins of group G Streptococcus in different phases of growth: patterns of production and implications for the host–bacteria relationship

et al. 2014

View full text Add to dashboard Cite

Group G Streptococcus (GGS) is a human bacterial pathogen expressing surface proteins FOG and protein G (PG) which interact with several host defence systems, including the complement and contact systems. Selected reaction monitoring mass spectrometry, electron microscopy and protein binding assays were used to track the amounts of FOG and PG intracellularly and on the bacterial surface during different phases of growth. Large and increasing amounts of PG were present on the surface in the stationary growth phase, and this was due to de novo production. In contrast, the amount of FOG did not change substantially during this phase. Apart from PG, a number of housekeeping proteins also increased in abundance in the stationary phase. These results show that GGS protein production is active during the stationary phase and that the bacteria actively remodel their surface and enter a less pro-inflammatory state in this phase.

show abstract

Proteomic Analysis and Identification of Streptococcus pyogenes Surface-Associated Proteins

Cited by 142 publications

References 63 publications

Conserved anchorless surface proteins as group A streptococcal vaccine candidates

Conserved anchorless surface proteins as group A streptococcal vaccine candidates

The cell-envelope proteome of Bifidobacterium longum in an in vitro bile environment

Surface proteins of group G Streptococcus in different phases of growth: patterns of production and implications for the host–bacteria relationship

Contact Info

Product

Resources

About