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Yersinia pestis TonB: Role in Iron, Heme, and Hemoprotein Utilization

Robert D. Perry,^* Jessica Shah, Scott W. Bearden, Jan M. Thompson, and Jacqueline D. Fetherston

Department of Microbiology, Immunology, and Molecular Genetics, University of Kentucky, Lexington, Kentucky

Received 13 January 2003/ Returned for modification 11 March 2003/ Accepted 16 April 2003

	ABSTRACT

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In Yersinia pestis, the siderophore-dependent yersiniabactin (Ybt) iron transport system and heme transport system (Hmu) have putative TonB-dependent outer membrane receptors. Here we demonstrate that hemin uptake and iron utilization from Ybt are TonB dependent. However, the Yfe iron and manganese transport system does not require TonB.

	TEXT

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Although outer membrane (OM) receptors serve to bind selected substrates in gram-negative bacteria, the substrate must still be translocated across the OM into the periplasm. For some OM receptors, TonB functions in concert with ExbB and ExbD to transmit the energy needed for this process (12, 17). To examine the role of TonB in the various iron and heme transport systems of Yersinia pestis, we have cloned and mutated the tonB gene. As expected, our results indicate that TonB is absolutely required for the utilization of the siderophore, yersiniabactin (Ybt), as well as hemin and all tested hemoproteins. TonB does not play a role in iron transport by either the Yfe system or a putative iron transport system which functions at 26°C. A second tonB-like gene was identified in the Y. pestis genome and designated hasB due to an association with the Y. pestis has locus (18). HasB does not appear to play a role in accumulation of iron, hemin, or hemoproteins.

Sequence analysis of tonB, exbB, and exbD. The tonB gene of Y. pestis KIM10+ (4) is predicted to encode a 252-residue, 27.5-kDa protein with a pI of 5.98. SignalP analysis (15a) suggested the presence of a signal sequence; as with Escherichia coli, the Y. pestis TonB may not be cleaved (17). A BLAST homology search indicates that the Y. pestis TonB protein is 80.8% identical and 85.6% similar to TonB from Yersinia enterocolitica (14). Y. pestis TonB possesses motifs common to other TonB proteins (13), including an N-terminal hydrophobic domain, a central region with EP repeats separated from a region with KP repeats, and a C-terminal domain with an amphiphilic ß-strand. As with E. coli, the Y. pestis tonB gene appears to be monocistronic and is surrounded by similar sequences with the exception of an IS285 element inserted downstream of tonB in Y. pestis KIM10+. Y. pestis TonB has four perfectly conserved amino acids (SHLS, residues 19, 23, 30, and 34) in the N-terminal hydrophobic domain that are predicted to form an -helix (14). Visual inspection of the tonB promoter region revealed typical -10 and -35 regions and a strong putative ribosome binding site. Two potential Fur binding sites were identified; however, both of them are located well upstream of the putative promoter region.

Similarity searches identified a putative exbBD operon that is not closely linked to tonB. The Y. pestis KIM10+ exbB gene is predicted to encode a 251-residue, 26.8-kDa protein with a pI of 9.83. The exbD gene encodes a 143-residue, 15.6-kDa protein with a pI of 4.40. These proteins show a high level of similarity to ExbB (66.5% identity) and ExbD (67.8% identity) from E. coli. Contiguous genes encoding TolQ (228 residues, 25.4 kDa, pI of 6.17), TolR (142 residues, 15.5 kDa, pI of 5.55), and TolA (393 residues, 41 kDa, pI of 9.43), which are required by TolA-dependent OM receptors (15), were identified. No additional exbB- or exbD-like genes were detected.

Role of TonB in acquisition of inorganic iron by the Ybt-dependent transport system. KIM6-2073+ possesses all of the iron and heme transport systems identified in Y. pestis but contains a kanamycin gene cassette inserted into tonB. Compared to the parent strain, KIM6+, KIM6-2073+ exhibited growth defects in a defined, iron-deficient medium (PMH) that are very similar to the defects seen with KIM6-2045.1 (Fig. 1), a Y. pestis strain carrying a deletion of the OM receptor (Psn) for Ybt (7). When surplus iron is present, the growth of all three strains is nearly identical (Fig. 1). Growth of KIM6-2073+ cells was inhibited on deferrated, solidified media (PMH-S). In addition, the TonB^- mutant was unable to use Ybt produced by KIM6+. However, this mutant supports the growth of a Ybt-biosynthesis mutant (KIM6-2046.1) on PMH-S plates at 37°C. Similar growth-stimulation results were obtained using cell supernatants. These studies indicate that KIM6-2073+ still synthesizes and secretes Ybt, but it is unable to transport the Fe-Ybt complex back into the cell. KIM6-2073+ cells containing a plasmid encoding Y. pestis TonB (pYptonB) were able to grow on PMH-S plates, indicating that the observed growth defects were the result of the tonB mutation.

View larger version (22K): [in this window] [in a new window]   FIG. 1. Growth of Y. pestis strains KIM6+ (Ybt+ TonB+), KIM6-2045.1 (Psn- TonB+), and KIM2073+ (Ybt+ TonB-) at 37°C in deferrated PMH with (+Fe) and without (-Fe) FeCl3 supplementation to 10 µM was performed as previously described (8, 19).

View larger version (25K): [in this window] [in a new window]   FIG. 2. Uptake of 55FeCl3 by Y. pestis strains KIM6+ (Ybt+ TonB+), KIM6-2073+ (Ybt+ TonB-), and KIM6-2045.1 (Psn- TonB+) was monitored as described previously (1, 6). Where indicated (closed symbols), cells were metabolically poisoned by addition of 100 µM carbonyl cyanide m-chlorophenylhydrazone 10 min prior to addition of isotope. These data are from a single experiment but are representative of three independent assays.

Role of TonB in acquisition of inorganic iron by Ybt-independent transport systems. To assess the role of TonB in iron acquisition by the YfeABCD iron and manganese transport system (1, 2), the tonB::kan mutation was introduced into KIM6, a Y. pestis strain missing the Ybt system, and a derivative of KIM6 carrying a yfeAB mutation (KIM6-2031.1). We compared the ability of these strains to grow at 30°C on solidified-PMH plates containing a 0 to 5 µM gradient of conalbumin. KIM6-2073 (a tonB::kan KIM6 strain) was as effective as KIM6 at acquiring iron from conalbumin (Fig. 3). Loss of the Yfe system caused a significant reduction in growth across the gradient (compare KIM6 to KIM6-2031.1 in Fig. 3). KIM6-2073 does not show a similar defect. Compared to KIM6-2031.1, the growth of KIM6-2073.1 (Yfe^- TonB^-) was slightly delayed and inhibited. Iron transport assays (Fig. 4) also indicate that uptake of iron by the Yfe system does not depend upon TonB. Iron uptake by KIM6 and KIM6-2073 are nearly identical, while uptake by the Yfe^- and Yfe^- TonB^- mutants is greatly reduced. Overall, these results suggest that the Yfe system is not TonB dependent.

View larger version (22K): [in this window] [in a new window]   FIG. 3. Growth of Y. pestis KIM6 (Ybt- Yfe+ TonB+ HasB+), KIM6-2031.1 (Ybt- Yfe- TonB+ HasB+), KIM6-2073 (Ybt- Yfe+ TonB- HasB+), and KIM6-2073.1 (Ybt- Yfe- TonB- HasB+) at 30°C across PMH plates containing a gradient of the iron chelator conalbumin (0 to 5 µM) (1). Bars represent incremental growth against the concentration gradient over a 72-h period. Growth distances were recorded in millimeters from 0 (no growth) to 90 (confluent growth). The data shown are from a single growth assay but are representative of three independent experiments.

View larger version (26K): [in this window] [in a new window]   FIG. 4. Uptake of 55FeCl3 by Y. pestis KIM6 (Ybt- Yfe+ TonB+ HasB+), KIM6-2031.1 (Ybt- Yfe- TonB+ HasB+), KIM6-2073 (Ybt- Yfe+ TonB- HasB+), and KIM6-2073.1 (Ybt- Yfe- TonB- HasB+) at 37°C. Where indicated (closed symbols), cells were metabolically poisoned by addition of 100 µM carbonyl cyanide m-chlorophenylhydrazone 10 min prior to addition of isotope. These data are from a single experiment but are representative of three independent assays.

Role of TonB in heme transport. The effect of a tonB mutation on the ability of Y. pestis to utilize hemin and various hemoproteins as iron sources (10, 21) was tested on PMH plates containing 100 µM ethylenediamine-di(o-hydroxyphenyl) acetic acid (EDDA), a concentration that inhibits the growth of KIM6+. Similar to the case with strain KIM6-2060.1+ (in which hmuP'RSTUV genes have been deleted), KIM6-2073+ was unable to use hemin or any of the hemoproteins as iron sources (Table 1). KIM6-2073+ containing pYptonB was able to use hemin as an iron source. This confirms that the Hmu system is TonB dependent. TonB dependency of the highly homologous Y. enterocolitica Hem system has also been demonstrated (20).

Our results with the TonB^- mutant show that the Y. pestis HasB protein cannot substitute for TonB in the Ybt and Hmu transport systems. To determine whether HasB is required for TonB-independent inorganic iron uptake, we constructed a Y. pestis TonB^- HasB^- double mutant and tested its capacity for inorganic iron accumulation. The levels of energy-dependent iron accumulation by KIM6 (TonB⁺ HasB⁺), KIM6-2073 (TonB^- HasB⁺), KIM6-2080 (TonB⁺ HasB^-), and KIM6-2073.2 (TonB^- HasB^-) were nearly identical (data not shown), indicating that the observed iron uptake was not HasB dependent.

	ACKNOWLEDGMENTS

 
This work was supported by Public Health Service grants AI25098 and AI33481.

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Microbiology, Immunology, and Molecular Genetics, MS415 Medical Center, University of Kentucky, Lexington, KY 40536-0298. Phone: (859) 323-6341. Fax: (859) 257-8994. E-mail: rperry{at}pop.uky.edu.

Editor: J. T. Barbieri

Present address: Centers for Disease Control, Division of Vector-Borne Infectious Diseases, Bacterial Zoonoses Branch, Fort Collins, Colo.

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