Mechanism of bacitracin resistance in gram-negative bacteria that synthesize exopolysaccharides

Pollock, Thomas J.; Thorne, Linda; Yamazaki, Motohide; Mikolajczak, Marcia; Armentrout, Richard W.

doi:10.1128/jb.176.20.6229-6237.1994

Cited by 70 publications

(59 citation statements)

References 36 publications

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“…The order of assembly prior to polymerization is glucose, glucose, mannose, glucuronic acid, and finally mannose (24). Our genetic complementation tests also showed that the wild-type gumD gene of X. campestris could restore synthesis of sphingans in analogous Bac r Sps Ϫ (sphingan polysaccharide-negative) mutants of Sphingomonas strains (45). Since there are two glucose residues in the backbone of each of the sphingans, we reasoned that the Bac r Sps Ϫ mutants were probably also blocked in the transfer of glucose-P to IP.…”

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confidence: 57%

“…Most of the gum genes required by this bacterium for synthesis and secretion of xanthan gum have been described (3,6,19,20,58). Previously we learned from genetic complementation tests that a special class of mutations in X. campestris which are simultaneously xanthan gum negative (Gum Ϫ ) and resistant to bacitracin (Bac r ) are in the gumD gene (45). This gene is required to transfer glucose-P from UDP-Glc to a carrier isoprenylphosphate (IP) to give glucoseisoprenylpyrophosphate (Glc-PPI) and is the first dedicated step in synthesis of xanthan gum (59).…”

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confidence: 99%

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Linkage of genes essential for synthesis of a polysaccharide capsule in Sphingomonas strain S88

Yamazaki¹,

Thorne²,

Mikolajczak³

et al. 1996

J Bacteriol

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Several structurally related capsular polysaccharides that are secreted by members of the genus Sphingomonas are being developed as aqueous rheological control agents for diverse industrial and food applications. They include gellan (S-60), welan (S-130), rhamsan (S-194), S-657, S-88, S-198, S-7, and NW-11. We refer to these polysaccharides as sphingans, after the genus name. This paper characterizes the first gene cluster isolated from a Sphingomonas species (S88) that is required for capsule synthesis. Overlapping DNA segments which spanned about 50 kbp of S88 DNA restored the synthesis of sphingan S-88 in capsule-negative mutants. The mutations were mapped into functional complementation groups, and the contiguous nucleotide sequence for the 29-kbp cluster was determined. The genetic complementation map and the DNA sequences were interpreted as an extended multicistronic locus containing genes essential for the assembly and secretion of polysaccharide S-88. Many of the deduced amino acid sequences were similar to gene products from other polysaccharide-secreting bacteria such as Rhizobium meliloti (succinoglycan), Xanthomonas campestris (xanthan gum), and Salmonella enterica (O antigen). The S88 locus contained a four-gene operon for the biosynthesis of dTDP-L-rhamnose, an essential precursor for the sphingans. Unexpectedly, there were also two genes for secretion of a lytic or toxin-like protein nested within the polysaccharide cluster. The conservation and linkage of genes that code for a defensive capsule and genes for secretion of an offensive lysin or toxin suggest a heretofore unknown pathogenic life history for Sphingomonas strain S88.The ''sphingans'' are capsular polysaccharides that have similar but not identical structures and are secreted by members of the genus Sphingomonas (44). The group includes S-88, S-60 (gellan), S-130 (welan), S-194 (rhamsan), heteropolysaccharide 7,41,43). As diagrammed in Fig. 1, the sphingans have different side groups, and either L-rhamnose or L-mannose is found at one position in the backbone. L-Mannose itself is exceedingly rare in nature. Aqueous solutions of the polymers have unique and useful rheological properties (41). Gellan is currently produced by large-scale aerobic fermentation for use as a gelling agent in foods and microbiological culture media, and welan is marketed for control of aqueous viscosity. It is not clear how the structural variations in the polymers give rise to distinct rheological properties.Sphingomonas strains have been isolated from diverse environments and with a wide range of metabolic activities. The sphingan-secreting strains were isolated from plant tissue, water, and soil. Chemoheterotrophic strains with the ability to metabolize toluene, naphthalene, cresol, and other aromatic compounds were recently isolated from deep terrestrial subsurface sediments (12). And other strains have been studied for their ability to degrade lignin (38). Sphingomonas bacteria have also been isolated from human clinical specimens and from hospital wate...

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confidence: 57%

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confidence: 99%

Linkage of genes essential for synthesis of a polysaccharide capsule in Sphingomonas strain S88

Yamazaki¹,

Thorne²,

Mikolajczak³

et al. 1996

J Bacteriol

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“…BacA homologs were also identified in Streptococcus pneumoniae and Staphylococcus aureus and are important for resistance to bacitracin, presumably by increasing the synthesis of C 55 -isoprenyl phosphate (6). In some gramnegative bacteria, mutations that block the synthesis of exopolysaccharides also lead to bacitracin resistance, presumably by increasing the supply of the common C 55 -isoprenyl phosphate carrier (22).…”

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Regulation of the Bacillus subtilis bcrC Bacitracin Resistance Gene by Two Extracytoplasmic Function σ Factors

2002

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Bacitracin resistance is normally conferred by either of two major mechanisms, the BcrABC transporter, which pumps out bacitracin, or BacA, an undecaprenol kinase that provides C 55 -isoprenyl phosphate by de novo synthesis. We demonstrate that the Bacillus subtilis bcrC (ywoA) gene, encoding a putative bacitracin transport permease, is an important bacitracin resistance determinant. A bcrC mutant strain had an eightfoldhigher sensitivity to bacitracin. Expression of bcrC initiated from a single promoter site that could be recognized by either of two extracytoplasmic function (ECF) factors, X or M . Bacitracin induced expression of bcrC, and this induction was dependent on M but not on X . Under inducing conditions, expression was primarily dependent on M . As a consequence, a sigM mutant was fourfold more sensitive to bacitracin, while the sigX mutant was only slightly sensitive. A sigX sigM double mutant was similar to a bcrC mutant in sensitivity. These results support the suggestion that one function of B. subtilis ECF factors is to coordinate antibiotic stress responses.

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“…A. pullulans strain NRRL Y-2331-1, which produces high yields of a nonpigmented form of pullulan, 9 was obtained from the United States Department of Agriculture (USDA). The growth media consisted of a complex nitrogen stock solution with sucrose as the carbon source, 5 containing (per 1 L of ultrapure water): 2.0 g of yeast extract, 0.5 g of (NH 4 ) 2 SO 4 , 1.0 g of NaCl, 0.2 g of MgSO 4 , 3.0 g of K 2 HPO 4 , 0.01 g of FeSO 4 , 0.01 g of MnSO 4 , 0.01 g of ZnSO 4 , and 50 g of sucrose. All ingredients, excluding ZnSO 4 , MnSO 4 , FeSO 4 , and MgSO 4 , were mixed and autoclaved for 45 min at 121°C.…”

Section: Methodsmentioning

confidence: 99%

“…2 However, naturally occurring and mutant strains of A. pullulans exist that produce reduced levels of melanin. 5,6 A. pullulans may produce other macromolecules, depending on culture conditions. For example, cells grown on sucrose produce pullulan and an acidic glucan with uronic acid components, whereas cells cultured on maltose produce a heteropolysaccharide containing glucose, galactose, and mannose.…”

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confidence: 99%

Adhesion of Aureobasidium pullulans Is Controlled by Uronic Acid Based Polymers and Pullulan

et al. 2005

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Aureobasidium pullulans is a potentially pathogenic microfungus that produces and secretes the polysaccharide pullulan and other biomacromolecules, depending on the microbe's physiological state. The role of these macromolecules in mediating adhesion and attachment were examined. Interfacial forces and adhesion affinities of A. pullulans were probed for early-exponential phase (EEP) and late-exponential phase (LEP) cells, using atomic force microscopy (AFM). Biochemical assays showed that A. pullulans produces both pullulan and a uronic acid based polymer. The pullulan is not produced until the LEP, and it can be removed by treatment with pullulanase. Both adhesion forces between the microbe and the AFM tip (silicon nitride) and attachment of the cells to quartz sand grains were controlled by the density of the uronic acid polymer. Uronic acid polymers doubled in density between the EEP and the LEP and were unaffected by the enzyme pullulanase. Retention to quartz in a packed column was quantified using the collision efficiency (R), the fraction of collisions between the microbes, and the sand grains, that result in attachment. Adhesion forces and retention on glass were well correlated, with these values being higher for EEP cells (F adh ) 7.65 ( 4.67 nN; R ) 1.15) than LEP (F adh ) 2.94 ( 0.75; R ) 0.49) and LEP + pullulanase cells (F adh ) 2.33 ( 2.01 nN; R ) 0.43). Steric interactions alone do not describe the adhesion behavior of this fungus, but they do provide information regarding the length and density of the macromolecules studied.

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Mechanism of bacitracin resistance in gram-negative bacteria that synthesize exopolysaccharides

Cited by 70 publications

References 36 publications

Linkage of genes essential for synthesis of a polysaccharide capsule in Sphingomonas strain S88

Linkage of genes essential for synthesis of a polysaccharide capsule in Sphingomonas strain S88

Regulation of the Bacillus subtilis bcrC Bacitracin Resistance Gene by Two Extracytoplasmic Function σ Factors

Adhesion of Aureobasidium pullulans Is Controlled by Uronic Acid Based Polymers and Pullulan

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