Two Nonredundant SecA Homologues Function in Mycobacteria

Braunstein, Miriam; Brown, Amanda; Kurtz, Sherry L.; Jacobs, William R.

doi:10.1128/jb.183.24.6979-6990.2001

Cited by 125 publications

(175 citation statements)

References 47 publications

Supporting

Mentioning

162

Contrasting

Unclassified

Order By: Relevance

“…In E. coli the 9BlaTEM-1 reporter works with both Sec and Tat signal sequences (Broome-Smith et al, 1990;Stanley et al, 2002). The Sec and Tat pathways appear essential in M. tuberculosis (Braunstein et al, 2001;Saint-Joanis et al, 2006;Sassetti et al, 2003). Therefore, to investigate the mode of export of the ssPlcB-9BlaTEM-1 fusion protein, it was tested in M. In addition to working with the Sec and Tat pathways, the 9BlaTEM-1 reporter has been used with type II and type III secretion systems of Gram-negative bacteria (Charpentier & Oswald, 2004;Sauvonnet & Pugsley, 1996).…”

Section: Discussionmentioning

confidence: 99%

“…Whole-cell lysates of M. tuberculosis strains were prepared as described previously (Braunstein et al, 2001) with the following modifications. M. tuberculosis cultures were grown in 5 ml volumes to mid-exponential phase.…”

Section: Construction Of §Blatem-1 Fusion Plasmidsmentioning

confidence: 99%

“…Mycobacteria possess two conserved pathways for exporting proteins: the general secretion (Sec) pathway and the twin-arginine translocation (Tat) pathway (Braunstein et al, 2001;Kurtz & Braunstein, 2005;McDonough et al, 2005;Owens et al, 2002;Posey et al, 2006;Saint-Joanis et al, 2006). These systems recognize precursor proteins synthesized with amino-terminal signal sequences and transport them across the cytoplasmic membrane (DeLisa et al, 2003;Mori & Ito, 2001).…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

β-Lactamase can function as a reporter of bacterial protein export during Mycobacterium tuberculosis infection of host cells

et al. 2007

Self Cite

View full text Add to dashboard Cite

Mycobacterium tuberculosis is an intracellular pathogen that is able to avoid destruction by host immune defences. Exported proteins of M. tuberculosis, which include proteins localized to the bacterial surface or secreted into the extracellular environment, are ideally situated to interact with host factors. As a result, these proteins are attractive candidates for virulence factors, drug targets and vaccine components. Here we describe a b-lactamase reporter system capable of identifying exported proteins of M. tuberculosis during growth in host cells. Because b-lactams target bacterial cell-wall synthesis, b-lactamases must be exported beyond the cytoplasm to protect against these drugs. When used in protein fusions, b-lactamase can report on the subcellular location of another protein as measured by protection from b-lactam antibiotics. Here we demonstrate that a truncated TEM-1 b-lactamase lacking a signal sequence for export (9BlaTEM-1) can be used in this manner directly in a mutant strain of M. tuberculosis lacking the major blactamase, BlaC. The 9BlaTEM-1 reporter conferred b-lactam resistance when fused to both Sec and Tat export signal sequences. We further demonstrate that b-lactamase fusion proteins report on protein export while M. tuberculosis is growing in THP-1 macrophage-like cells. This genetic system should facilitate the study of proteins exclusively exported in the host environment by intracellular M. tuberculosis.

show abstract

Section: Discussionmentioning

confidence: 99%

Section: Construction Of §Blatem-1 Fusion Plasmidsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

β-Lactamase can function as a reporter of bacterial protein export during Mycobacterium tuberculosis infection of host cells

et al. 2007

Self Cite

View full text Add to dashboard Cite

show abstract

“…Several bacterial species, including M. tuberculosis, have been shown to possess an additional SecA protein called SecA2 (7)(8)(9). The mycobacterial secA1 and secA2 genes are genetically distinct and cannot complement each other or deletion of the essential E. coli secA gene (8,10).…”

mentioning

confidence: 99%

ADP-dependent Conformational Changes Distinguish Mycobacterium tuberculosis SecA2 from SecA1

D'Lima

Teschke

2014

Journal of Biological Chemistry

View full text Add to dashboard Cite

Background: Mycobacterium tuberculosis possesses a second SecA ATPase that is required for bacterial virulence. Results: ADP binding by SecA2 causes a conformational change observable by biochemical methods. Conclusion: ADP binding closes the clamp in SecA2. This is not observed in SecA1 or E. coli SecA. Significance: Nucleotide-dependent clamp closure suggests a mechanism by which mycobacterial SecA2 is distinguished from SecA1 by the translocation machinery.

show abstract

“…The genomes of some Gram-positive bacteria harbor two secA genes: one that encodes the canonical SecA ATPase of the protein secretory pathway (23) and another that specifies a paralogue, SecA2, supporting the secretion of only one or a few select substrates (43). SecA2 was first identified in Mycobacterium tuberculosis, where it promotes the transport of proteins across the mycobacterial envelope that aid in the pathogenesis of tuberculosis (44,45). Mycobacterial SecA2 recognizes the mature domains of a few secretory precursors to assist in their secretion, suggesting its primary function may be maintenance of export competence for proteins with the propensity for rapid folding (46).…”

Section: Discussionmentioning

confidence: 99%

Bacillus anthracis SlaQ Promotes S-Layer Protein Assembly

Nguyen-Mau

Schneewind

et al. 2015

J Bacteriol

View full text Add to dashboard Cite

Bacillus anthracis vegetative forms assemble an S-layer comprised of two S-layer proteins, Sap and EA1. A hallmark of S-layer proteins are their C-terminal crystallization domains, which assemble into a crystalline lattice once these polypeptides are deposited on the bacterial surface via association between their N-terminal S-layer homology domains and the secondary cell wall polysaccharide. Here we show that slaQ, encoding a small cytoplasmic protein conserved among pathogenic bacilli elaborating S-layers, is required for the efficient secretion and assembly of Sap and EA1. S-layer protein precursors cosediment with SlaQ, and SlaQ appears to facilitate Sap assembly. Purified SlaQ polymerizes and when mixed with purified Sap promotes the in vitro formation of tubular S-layer structures. A model is discussed whereby SlaQ, in conjunction with S-layer secretion factors SecA2 and SlaP, promotes localized secretion and S-layer assembly in B. anthracis. IMPORTANCES-layer proteins are endowed with the propensity for self-assembly into crystalline arrays. Factors promoting S-layer protein assembly have heretofore not been reported. We identified Bacillus anthracis SlaQ, a small cytoplasmic protein that facilitates S-layer protein assembly in vivo and in vitro.

show abstract

Two Nonredundant SecA Homologues Function in Mycobacteria

Cited by 125 publications

References 47 publications

β-Lactamase can function as a reporter of bacterial protein export during Mycobacterium tuberculosis infection of host cells

β-Lactamase can function as a reporter of bacterial protein export during Mycobacterium tuberculosis infection of host cells

ADP-dependent Conformational Changes Distinguish Mycobacterium tuberculosis SecA2 from SecA1

Bacillus anthracis SlaQ Promotes S-Layer Protein Assembly

Contact Info

Product

Resources

About