Calcium-Regulated Type III Secretion of Yop Proteins by an Escherichia coli hha Mutant Carrying a Yersinia pestis pCD1 Virulence Plasmid

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Infection and Immunity, February 2006, p. 1381-1386, Vol. 74, No. 2
0019-9567/06/$08.00+0 doi:10.1128/IAI.74.2.1381-1386.2006
Copyright © 2006, American Society for Microbiology. All Rights Reserved.

Calcium-Regulated Type III Secretion of Yop Proteins by an Escherichia coli hha Mutant Carrying a Yersinia pestis pCD1 Virulence Plasmid

Sara Schesser Bartra, Michael W. Jackson, Julia A. Ross, and Gregory V. Plano^*

Department of Microbiology and Immunology, University of Miami Miller School of Medicine, P.O. Box 016960 (R-138), Miami, Florida 33101

Received 8 August 2005/ Returned for modification 14 September 2005/ Accepted 19 October 2005

ABSTRACT

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A series of four large deletions that removed a total of ca.36 kb of DNA from the ca. 70-kb Yersinia pestis pCD1 virulenceplasmid were constructed using lambda Red-mediated recombination.Escherichia coli hha deletion mutants carrying the virulenceplasmid with the deletions expressed a functional calcium-regulatedtype III secretion system. The E. coli hha/pCD1 system shouldfacilitate molecular studies of the type III secretion process.

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Yersinia pestis is the etiologic agent of plague, an often fataldisease of both animals and humans (6). The pathogenicty ofY. pestis results largely from its ability to evade the defensesof its mammalian hosts. This ability is dependent upon the presenceof a 70-kb plasmid designated pCD1 in Y. pestis KIM (18, 28).Plasmid pCD1 and related plasmids (2) in the enteropathogenicyersiniae (Yersinia enterocolitica and Yersinia pseudotuberculosis)encode a set of secreted antihost proteins termed Yersinia outerproteins (Yops) and a unique delivery system, classified asa type III secretion system (T3SS) (13). The type III secretionapparatus, or "injectisome" as it is sometimes called, spansthe bacterial cell envelope and allows extracellular yersiniaeto inject Yops directly into host phagocytic cells (15, 29,32). Injected Yops prevent bacterial engulfment and block productionof proinflammatory cytokines (26, 27, 34).

The type III secretion process is activated by contact betweena bacterium and the surface of a eukaryotic cell (33). Followingcell contact, effector Yops are injected into the eukaryoticcell and are not found in substantial amounts in the extracellularenvironment, indicating that the type III secretion processis activated only at the point of contact between the two cells.In vitro, Yop secretion is blocked in the presence of millimolaramounts of extracellular calcium and is activated during growthat 37°C in the absence of calcium (23, 35). Secretion ofYops in vitro is accompanied by cessation of bacterial growth,an event termed growth restriction (3).

To determine the minimum number of pCD1 genes required to expressa functional calcium-regulated T3SS, we created four large deletionsin plasmid pCD1 that together removed more than one-half ofthe genetic material carried on the plasmid (Fig. 1A). The fourdeletions eliminated pCD1 sequences at positions 41,640 to 52,022( ${Delta}$ 1), 3,740 to 15,602 ( ${Delta}$ 2), 61,430 to 70,331 ( ${Delta}$ 3), and 55,568 to60,495 ( ${Delta}$ 4). In general, the deletions were designed to removethe genes encoding the six effector Yops (yopE, yopH, yopJ,yopM, yopT, and ypkA), two chaperones (sycE and sycT), ylpA,yopK, yadA, all uncharacterized open reading frames, and essentiallyall transposable elements. The four deletions did not disruptthe low-calcium response (Lcr) region (positions 15,801 to 41,540),the origin of replication, the partitioning region, or the sycHgene.

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FIG. 1. Construction of plasmid pCD1- ${Delta}$ 1234. (A) Map of the whole pCD1 plasmid of Y. pestis KIM5. The outer circle shows the positions of identified pCD1 genes and open reading frames (open boxes). Genes located on the outside of the circle are transcribed in a clockwise direction, whereas genes located on the inside of the circle are transcribed in a counterclockwise direction. Transposable elements are indicated by solid boxes. The pCD1 sequences removed by deletions ${Delta}$ 1, ${Delta}$ 2, ${Delta}$ ,3 and ${Delta}$ 4 are indicated by the labeled lines. Reprinted from reference 28 with permission of the publisher. (B) Agarose gel electrophoretogram of plasmid pCD1 and derivatives of this plasmid. Plasmid DNA was isolated from Y. pestis KIM8, KIM8 ${Delta}$ 1, KIM8 ${Delta}$ 2, KIM8 ${Delta}$ 3, KIM8 ${Delta}$ 4, KIM8 ${Delta}$ 12, KIM8 ${Delta}$ 123, and KIM8 ${Delta}$ 1234 by the procedure of Kado and Liu (21), separated on 0.7% agarose gels, and stained with ethidium bromide. CD, chromosomal DNA.

Lambda Red-mediated recombination was used to delete each specifiedregion of pCD1 and to simultaneously insert an FLP recognitiontarget-flanked kanamycin resistance (kan) cassette or a dhfrcassette essentially as described by Datsenko and Wanner (8).PCR products used to construct the gene replacements were generatedusing plasmid pKD4 (kan) or dhfr (EZ::TN<DHFR>; Epicentre,Madison, WI) as a template for PCR. The oligonucleotide primersused in this study are listed in Table 1. Deletions were confirmedby PCR analysis. Each individual deletion was initially constructedin plasmid pCD1 of Y. pestis KIM8 (pMT1⁺, pCD1⁺, and pPCP1^–),which generated kanamycin-resistant (Km^r) strains KIM8 ${Delta}$ 1, KIM8 ${Delta}$ 2, and KIM8 ${Delta}$ 3, as well as trimethoprim-resistant (Tm^r) strainKIM8 ${Delta}$ 4. Plasmid pCP20, which encodes the FLP recombinase (8),was electroporated into KIM8 ${Delta}$ 1 to facilitate removal of theFLP recognition target-flanked kan cassette, generating strainKIM8 ${Delta}$ 1s. Plasmids pKD46 and pCP20, which carry temperature-sensitiveorigins of replication, were cured from the kanamycin-sensitivestrain by overnight growth at 39°C (8). The presence ofthe deletions and the absence of pKD46 and pCP20 were confirmedby PCR analysis and by agarose gel electrophoresis of plasmidsisolated by the method of Kado and Liu (21).

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TABLE 1. Oligonucleotides used for lambda Red-mediated recombination

To construct a pCD1 variant that had all four deletions, weused lambda Red-mediated recombination (8) to sequentially deletethree additional regions ( ${Delta}$ 2, ${Delta}$ 3, and ${Delta}$ 4) from pCD1 of KIM8 ${Delta}$ 1s.PCR products used to construct the sequential gene replacementswere generated using pKD4 (kan), pKD3 (cat), or dhfr as thetemplate for PCR. The ${Delta}$ 2::kan, ${Delta}$ 3::cat, and ${Delta}$ 4::dhfr insertionaldeletions were confirmed by PCR analysis and by agarose gelelectrophoresis of plasmids isolated by the method of Kado andLiu (21). The resultant multiple-deletion pCD1 plasmids pCD1- ${Delta}$ 12(kan), pCD1- ${Delta}$ 123 (kan₂ cat₃), and pCD1- ${Delta}$ 1234 (kan₂ cat₃ dhfr₄),as well as the original single-deletion plasmids pCD1- ${Delta}$ 1 (kan),pCD1- ${Delta}$ 2 (kan), pCD1- ${Delta}$ 3 (kan), and pCD1- ${Delta}$ 4 (dhfr), were isolatedand electroporated into Y. pestis KIM10 (pMT1⁺, pCD1^–,pPCP1^–), generating Y. pestis KIM8 ${Delta}$ 1 (Km^r), KIM8 ${Delta}$ 2 (Km^r),KIM8 ${Delta}$ 3 (Km^r), KIM8 ${Delta}$ 4 (Tm^r), KIM8 ${Delta}$ 12 (Km^r), KIM8 ${Delta}$ 123 (Km^r Cm^r),and KIM8 ${Delta}$ 1234 (Km^r Cm^r Tm^r) in a clean genetic background (Fig.1B). The resultant strains were used in all subsequent studies.

Secretion of Yops by Y. pestis KIM8, KIM8 ${Delta}$ 1, KIM8 ${Delta}$ 12, KIM8 ${Delta}$ 123,and KIM8 ${Delta}$ 1234 was measured following growth of the bacteriain TMH medium for 5 h at 37°C in the presence and absenceof calcium. Concentrated culture supernatant proteins were separatedby sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis(PAGE) and stained with Coomassie blue R-250 (Fig. 2A). Allfive strains secreted Yops in the absence of calcium but notin the presence of calcium. Y. pestis KIM8 ${Delta}$ 1234, which had allfour deletions, expressed and secreted YopB, YopD, YopN, andLcrV but none of the effector Yops. In addition to the deletionsin plasmid pCD1 mentioned above, a deletion ( ${Delta}$ 5) eliminatingthe pCD1 sequence at positions 55,568 to 70,331 from pCD1 ofY. pestis KIM8 was constructed using primers ${Delta}$ 4-P1 and ${Delta}$ 3-P2.Y. pestis KIM8 carrying plasmid pCD1- ${Delta}$ 5, in which the sycH genewas deleted, expressed and secreted only low levels of Yops(data not shown), confirming that SycH is required for efficientT3SS gene expression (4). These studies confirmed that withthe exception of sycH, all of the genes required to expressa functional calcium-regulated T3SS are encoded in the Lcr regionof plasmid pCD1. Similar results were obtained by Trulzsch etal. (36), who inserted the entire Lcr region of the Y. enterocoliticapYV virulence plasmid into a cosmid vector (mini-pYV). In thiscase, the mini-pYV plasmid directed secretion and translocationof effector Yops encoded on expression plasmids provided intrans. Although the mini-pYV plasmid encoded a functional T3SS,it did not carry the sycH gene; therefore, LcrQ (YscM)-dependentregulation of T3SS gene transcription was not reconstitutedwith this construct. SycH, the chaperone for YopH and LcrQ,is required for efficient export of the negative regulatorycomponent LcrQ in the absence of calcium (4, 37). Deletion ofsycH prevents secretion of LcrQ and results in repression ofT3SS gene transcription (30, 31).

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FIG. 2. Secretion and translocation of Yops by Y. pestis strains carrying plasmid pCD1 or versions of this plasmid with deletions. (A) Y. pestis KIM8, KIM8 ${Delta}$ 1, KIM8 ${Delta}$ 12, KIM8 ${Delta}$ 123, and KIM8 ${Delta}$ 1234 were grown in TMH medium with (lanes +) or without (lanes –) 2.5 mM CaCl₂ for 5 h at 37°C. Volumes of trichloroacetic acid-precipitated culture supernatant proteins corresponding to equal numbers of bacteria were resolved by SDS-PAGE and stained with Coomassie blue. The positions of different Yops are indicated on the right, and the molecular masses (in kilodaltons) of protein standards are indicated on the left. (B) Translocation of YopE₁₂₉-ELK into HeLa cells. Y. pestis KIM8 ${Delta}$ 123, KIM8 ${Delta}$ 1234, KIM8-3002.P40 ( ${Delta}$ yopE ${Delta}$ yopJ; parent), KIM8-3002.41 ( ${Delta}$ yopE ${Delta}$ yopJ ${Delta}$ yopB), and KIM8-3002.41 complemented with pYopB2, all carrying pYopE₁₂₉-ELK, were used to infect HeLa cell monolayers at a multiplicity of infection of 30. After 3 h of incubation at 37°C, infected monolayers were solubilized with SDS-PAGE sample buffer and analyzed by SDS-PAGE and immunoblotting with anti-Elk antipeptide antibodies ( ${alpha}$ -ELK) and phosphospecific anti-Elk antipeptide antibodies ( ${alpha}$ -P-ELK). The position of YopE₁₂₉-ELK is indicated by arrowheads.

The injection of Yops into a eukaryotic cell is essentiallya three-step process that involves (i) attachment of the bacteriumto a eukaryotic cell via specific bacterial adhesins, (ii) secretionof effector Yops across the bacterial membranes, and (iii) translocationof Yops across the eukaryotic membrane. The ability of Y. pestisKIM8 ${Delta}$ 123 and KIM8 ${Delta}$ 1234 to inject Yops into a eukaryotic cellwas evaluated using the ELK tag reporter system described previously(9). Y. pestis KIM8 ${Delta}$ 123, KIM8 ${Delta}$ 1234, KIM8-3002.P40 ( ${Delta}$ yopE ${Delta}$ yopJ),KIM8-3002.41 ( ${Delta}$ yopE ${Delta}$ yopJ ${Delta}$ yopB), and KIM8-3002.41 carrying pYopB2were transformed with plasmid pYopE₁₂₉-ELK (9). The reporterplasmid encodes a truncated YopE protein with a C-terminal ELKtag that is phosphorylated upon translocation into a eukaryoticcell. Cultured HeLa cells were infected at a multiplicity ofinfection of 30 for 3 h at 37°C, and the infected monolayerswere analyzed by SDS-PAGE and immunoblot analysis (Fig. 2B).The total YopE₁₂₉-ELK expressed during the infection was detectedwith anti-ELK antipeptide antibodies, whereas YopE₁₂₉-ELK translocatedinto the HeLa cells was phosphorylated and detected with phospho-specificantipeptide antibodies (Cell Signaling Technology).

Immunoblot analysis with anti-ELK antipeptide antibodies demonstratedthat all the strains expressed comparable amounts of the YopE₁₂₉-ELKprotein (Fig. 2B, top panel). Y. pestis KIM8-3002.P40 (parent),KIM8 ${Delta}$ 123, and KIM8 ${Delta}$ 1234 translocated approximately equal amountsof YopE₁₂₉-ELK into the HeLa cells (Fig. 2B, bottom panel).In contrast, the translocation-defective ${Delta}$ yopB strain was unableto inject the YopE₁₂₉-ELK protein into the HeLa cells. Providingcomplementing plasmid pYopB2 in trans completely restored theability of the yopB deletion mutant to translocate the YopE₁₂₉-ELKprotein. These studies confirmed that the pCD1- ${Delta}$ 1234 plasmidencodes a functional T3SS capable of injecting Yops into eukaryoticcells.

The calcium-regulated secretion of Yops by Yersinia spp. isdependent upon at least 30 different pCD1 genes; however, therole of chromosomal genes in this process is not fully understood.Recently, several chromosomal genes required for efficient expressionof the Yersinia spp. T3SS have been identified (7, 10, 19, 20);however, the gene products identified thus far do not appearto be intimately involved in the type III secretion processper se. To determine if the Y. pestis chromosome carries genesthat are essential for expression of a functional calcium-regulatedT3SS, we moved the pCD1- ${Delta}$ 1234 construct into E. coli DH5 ${alpha}$ andBL21. Only low levels of Yop expression and no Yop secretionwere observed in E. coli DH5 ${alpha}$ or BL21 carrying plasmid pCD1- ${Delta}$ 1234,indicating that pCD1 T3SS genes are not efficiently expressedin E. coli (17) (Fig. 3 and data not shown).

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FIG. 3. Expression and secretion of Yops by an E. coli hha deletion mutant carrying pCD1- ${Delta}$ 1234. E. coli BL21 and BL21 hha with and without plasmid pCD1- ${Delta}$ 1234 were grown in TMH medium with (lanes +) or without (lanes –) 2.5 mM CaCl₂ for 5 h at 37°C. Cultures of Y. pestis KIM8 and KIM8 ${Delta}$ 1234 were grown under identical conditions. Volumes of culture supernatant (Sup.) proteins and cell pellet (Pellet) fractions corresponding to equal numbers of bacteria were analyzed by SDS-PAGE and immunoblotting with antisera specific for YopN or YopD. The locations of YopN and YopD are indicated by arrowheads.

Transcription of T3SS genes in Yersinia spp. is negatively regulatedby a small histone-like protein designated YmoA (7). E. colistrains express a protein homologous to YmoA, designated Hha(24), which functions with H-NS to thermoregulate the transcriptionof several virulence-related genes (22, 25). To examine therole of Hha in regulating the expression of pCD1- ${Delta}$ 1234 T3SS genesin E. coli DH5 ${alpha}$ and BL21, we used lambda Red-mediated recombinationto delete the hha locus and to insert a kan cassette at thesite of the deletion. The deletion of hha in both DH5 ${alpha}$ and BL21was confirmed by PCR analysis. Plasmid pKD46 was cured fromthe hha deletion mutants, and the pCD1- ${Delta}$ 1234 plasmid was electroporatedinto the pKD46-cured hha deletion strains.

Expression and secretion of YopN and YopD by Y. pestis KIM8and KIM8 ${Delta}$ 1234 and by E. coli BL21, BL21 ${Delta}$ hha, DH5 ${alpha}$ , and DH5 ${alpha}$ ${Delta}$ hhawith and without plasmid pCD1- ${Delta}$ 1234 were determined followinggrowth of the bacteria at 37°C in TMH medium in the presenceand absence of calcium (Fig. 3). The E. coli BL21 and DH5 ${alpha}$ hhadeletion strains carrying plasmid pCD1- ${Delta}$ 1234 secreted YopN andYopD in the absence of calcium but not in the presence of calcium.The amounts of YopN and YopD secreted by these strains werecomparable to or slightly less than the amounts secreted byY. pestis KIM8 or KIM8 ${Delta}$ 1234. These studies confirmed that plasmidpCD1- ${Delta}$ 1234 contains the complete complement of genes unique tothe yersiniae that are required to express a functional T3SS.Interestingly, the E. coli hha strains carrying pCD1- ${Delta}$ 1234 secretedhigh levels of Yops but did not exhibit growth restriction (datanot shown), suggesting that the physiological determinants thatlink growth and secretion are unique to the yersiniae.

E. coli DH5 ${alpha}$ and BL21 are avirulent bacteria that do not expressthe surface adhesins required for attachment to the surfaceof eukaryotic cells (5). Therefore, the E. coli strains thatexpress a functional T3SS should not be able to attach to HeLacells and inject Yops. Indeed, E. coli DH5 ${alpha}$ ${Delta}$ hha and BL21 ${Delta}$ hhacarrying pCD1- ${Delta}$ 1234 and pYopE₁₂₉-ELK expressed the YopE₁₂₉-ELKprotein but did not translocate the protein into cultured HeLacells (data not shown).

Previous studies have suggested that Hha and YmoA, which exhibit82% amino acid sequence identity, are interchangeable (1, 11).Our results indicate that Hha in E. coli, but not YmoA in Y.pestis, prevents essentially all pCD1 T3SS gene expression at37°C. The reason for the difference is unclear; however,we hypothesize that it could be related to the amount of YmoAor Hha present in the relevant bacterial cells at 37°C.We have demonstrated previously that YmoA is rapidly degradedby the Lon protease at 37°C in Y. pestis, a process thatis essential to trigger T3SS gene transcription in Y. pestis(20). It is possible that Hha is more resistant to Lon-mediatedproteolysis and is not rapidly degraded at 37°C in E. coli.To begin to examine this possibility, we constructed plasmidpFLAG-Hha, which encodes the Hha protein with an N-terminal14-amino-acid tag (N-MDYKDDDDKVKLLE-Hha). Plasmid pFLAG-Hhawas electroporated into E. coli DH5 ${alpha}$ and BL21, whereas plasmidpFLAG-YmoA was electroporated into Y. pestis KIM5-3001 (20).The stability of FLAG-Hha and FLAG-YmoA at 37°C was determinedby determining the amounts of these proteins after new synthesiswas blocked by addition of chloramphenicol (40 µg/ml)to the cultures, as described previously (20). Samples correspondingto equal numbers of bacteria were removed at specific timesand analyzed by SDS-PAGE and immunoblot analysis with the FLAGM2 antibody (Sigma, St. Louis, MO) (Fig. 4). As previously demonstrated,FLAG-YmoA was rapidly degraded at 37°C in Y. pestis. FLAG-Hhawas stable at 37°C in lon-deficient E. coli BL21 (14), butit was degraded in E. coli DH5 ${alpha}$ . These results suggest that Hha,like YmoA, is degraded in a Lon-dependent manner; however, thehalf-life of FLAG-YmoA in Y. pestis (19.3 min) was significantlyless than the half-life of FLAG-Hha in DH5 ${alpha}$ (40.3 min). Theseresults suggest that the degradation of Hha in E. coli and thedegradation of YmoA in Y. pestis are to some extent different,and the difference may account for the ability of Hha to suppresspCD1 gene transcription at 37°C in E. coli. Alternate explanationsare also possible, and further studies are required to determinethe mechanism by which Hha represses T3SS gene transcriptionat 37°C in E. coli.

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FIG. 4. Stability of FLAG-Hha in E. coli DH5 ${alpha}$ and BL21. E. coli DH5 ${alpha}$ and BL21, both carrying pFLAG-Hha, as well as Y. pestis KIM5-3001 carrying pFLAG-YmoA, were grown in heart infusion broth containing 2.5 mM CaCl₂ for 3 h at 37°C. Chloramphenicol (final concentration, 40 µg/ml) was added to block protein synthesis. An aliquot of each culture was removed at the times indicated at the top (15m, 15 min; 30m, 30 min). Whole-cell protein extracts from equivalent numbers of bacteria were separated by SDS-PAGE, transferred to Immobilon-P membranes, and probed with antibodies specific for the FLAG epitope tag.

The E. coli ${Delta}$ hha/pCD1- ${Delta}$ 1234 strain-plasmid combination providesa system to study the Yersinia spp. type III secretion processin a heterologous host. Previously, only the Erwinia chrysanthemiT3SS has been shown to function in a heterologous bacterialhost (16). The combination of the pCD1- ${Delta}$ 1234 virulence plasmidlacking the genes encoding all six translocated effector Yopswith an avirulent E. coli host provides a reliable and safesystem to analyze the molecular events involved in the Y. pestistype III secretion process. The procedures for preparation andmanipulation of membrane vesicles suitable for in vitro secretionstudies have been developed and fine-tuned in E. coli (12).Thus, the E. coli ${Delta}$ hha/pCD1- ${Delta}$ 1234 system should facilitate thedevelopment of in vitro secretion assays that are required todissect the molecular events involved in the type III secretionprocess.

ACKNOWLEDGMENTS

This work was supported by Public Health Service grants AI 50552and AI 39575 from the National Institutes of Health to G.V.P.

FOOTNOTES

* Corresponding author. Mailing address: Department of Microbiology and Immunology, University of Miami Miller School of Medicine, P.O. Box 016960 (R-138), Miami, FL 33101. Phone: (305) 243-6310. Fax: (305) 243-4623. E-mail: gplano{at}med.miami.edu.

Editor: J. B. Bliska

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27. Palmer, L. E., S. Hobbie, J. E. Galan, and J. B. Bliska. 1998. YopJ of Yersinia pseudotuberculosis is required for the inhibition of macrophage TNF-alpha production and downregulation of the MAP kinases p38 and JNK. Mol. Microbiol. 27:953-965.[CrossRef][Medline]
28. Perry, R. D., S. C. Straley, J. D. Fetherston, D. J. Rose, J. Gregor, and F. R. Blattner. 1998. DNA sequencing and analysis of the low-Ca²⁺-response plasmid pCD1 of Yersinia pestis KIM5. Infect. Immun. 66:4611-4623.[Abstract/Free Full Text]
29. Persson, C., R. Nordfelth, A. Holmstrom, S. Hakansson, R. Rosqvist, and H. Wolf-Watz. 1995. Cell-surface-bound Yersinia translocate the protein tyrosine phosphatase YopH by a polarized mechanism into the target cell. Mol. Microbiol. 18:135-150.[CrossRef][Medline]
30. Pettersson, J., R. Nordfelth, E. Dubinina, T. Bergman, M. Gustafsson, K. E. Magnusson, and H. Wolf-Watz. 1996. Modulation of virulence factor expression by pathogen target cell contact. Science 273:1231-1233.[Abstract]
31. Rimpilainen, M., A. Forsberg, and H. Wolf-Watz. 1992. A novel protein, LcrQ, involved in the low-calcium response of Yersinia pseudotuberculosis shows extensive homology to YopH. J. Bacteriol. 174:3355-3363.[Abstract/Free Full Text]
32. Rosqvist, R., A. Forsberg, and H. Wolf-Watz. 1991. Intracellular targeting of the Yersinia YopE cytotoxin in mammalian cells induces actin microfilament disruption. Infect. Immun. 59:4562-4569.[Abstract/Free Full Text]
33. Rosqvist, R., K. E. Magnusson, and H. Wolf-Watz. 1994. Target cell contact triggers expression and polarized transfer of Yersinia YopE cytotoxin into mammalian cells. EMBO J. 13:964-972.[Medline]
34. Schesser, K., A. K. Spiik, J. M. Dukuzumuremyi, M. F. Neurath, S. Pettersson, and H. Wolf-Watz. 1998. The yopJ locus is required for Yersinia-mediated inhibition of NF-kappaB activation and cytokine expression: YopJ contains a eukaryotic SH2-like domain that is essential for its repressive activity. Mol. Microbiol. 28:1067-1079.[CrossRef][Medline]
35. Straley, S. C., G. V. Plano, E. Skrzypek, P. L. Haddix, and K. A. Fields. 1993. Regulation by Ca²⁺ in the Yersinia low-Ca²⁺ response. Mol. Microbiol. 8:1005-1010.[CrossRef][Medline]
36. Trulzsch, K., A. Roggenkamp, M. Aepfelbacher, G. Wilharm, K. Ruckdeschel, and J. Heesemann. 2003. Analysis of chaperone-dependent Yop secretion/translocation and effector function using a mini-virulence plasmid of Yersinia enterocolitica. Int. J. Med. Microbiol. 293:167-177.[CrossRef][Medline]
37. Wattiau, P., B. Bernier, P. Deslee, T. Michiels, and G. R. Cornelis. 1994. Individual chaperones required for Yop secretion by Yersinia. Proc. Natl. Acad. Sci. USA 91:10493-10497.[Abstract/Free Full Text]

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Bartra, S. S., Styer, K. L., O'Bryant, D. M., Nilles, M. L., Hinnebusch, B. J., Aballay, A., Plano, G. V. (2008). Resistance of Yersinia pestis to Complement-Dependent Killing Is Mediated by the Ail Outer Membrane Protein. Infect. Immun. 76: 612-622 [Abstract] [Full Text]

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26.	Orth, K., L. E. Palmer, Z. Q. Bao, S. Stewart, A. E. Rudolph, J. B. Bliska, and J. E. Dixon. 1999. Inhibition of the mitogen-activated protein kinase kinase superfamily by a Yersinia effector. Science 285:1920-1923.[Abstract/Free Full Text]
27.	Palmer, L. E., S. Hobbie, J. E. Galan, and J. B. Bliska. 1998. YopJ of Yersinia pseudotuberculosis is required for the inhibition of macrophage TNF-alpha production and downregulation of the MAP kinases p38 and JNK. Mol. Microbiol. 27:953-965.[CrossRef][Medline]
28.	Perry, R. D., S. C. Straley, J. D. Fetherston, D. J. Rose, J. Gregor, and F. R. Blattner. 1998. DNA sequencing and analysis of the low-Ca²⁺-response plasmid pCD1 of Yersinia pestis KIM5. Infect. Immun. 66:4611-4623.[Abstract/Free Full Text]
29.	Persson, C., R. Nordfelth, A. Holmstrom, S. Hakansson, R. Rosqvist, and H. Wolf-Watz. 1995. Cell-surface-bound Yersinia translocate the protein tyrosine phosphatase YopH by a polarized mechanism into the target cell. Mol. Microbiol. 18:135-150.[CrossRef][Medline]
30.	Pettersson, J., R. Nordfelth, E. Dubinina, T. Bergman, M. Gustafsson, K. E. Magnusson, and H. Wolf-Watz. 1996. Modulation of virulence factor expression by pathogen target cell contact. Science 273:1231-1233.[Abstract]
31.	Rimpilainen, M., A. Forsberg, and H. Wolf-Watz. 1992. A novel protein, LcrQ, involved in the low-calcium response of Yersinia pseudotuberculosis shows extensive homology to YopH. J. Bacteriol. 174:3355-3363.[Abstract/Free Full Text]
32.	Rosqvist, R., A. Forsberg, and H. Wolf-Watz. 1991. Intracellular targeting of the Yersinia YopE cytotoxin in mammalian cells induces actin microfilament disruption. Infect. Immun. 59:4562-4569.[Abstract/Free Full Text]
33.	Rosqvist, R., K. E. Magnusson, and H. Wolf-Watz. 1994. Target cell contact triggers expression and polarized transfer of Yersinia YopE cytotoxin into mammalian cells. EMBO J. 13:964-972.[Medline]
34.	Schesser, K., A. K. Spiik, J. M. Dukuzumuremyi, M. F. Neurath, S. Pettersson, and H. Wolf-Watz. 1998. The yopJ locus is required for Yersinia-mediated inhibition of NF-kappaB activation and cytokine expression: YopJ contains a eukaryotic SH2-like domain that is essential for its repressive activity. Mol. Microbiol. 28:1067-1079.[CrossRef][Medline]
35.	Straley, S. C., G. V. Plano, E. Skrzypek, P. L. Haddix, and K. A. Fields. 1993. Regulation by Ca²⁺ in the Yersinia low-Ca²⁺ response. Mol. Microbiol. 8:1005-1010.[CrossRef][Medline]
36.	Trulzsch, K., A. Roggenkamp, M. Aepfelbacher, G. Wilharm, K. Ruckdeschel, and J. Heesemann. 2003. Analysis of chaperone-dependent Yop secretion/translocation and effector function using a mini-virulence plasmid of Yersinia enterocolitica. Int. J. Med. Microbiol. 293:167-177.[CrossRef][Medline]
37.	Wattiau, P., B. Bernier, P. Deslee, T. Michiels, and G. R. Cornelis. 1994. Individual chaperones required for Yop secretion by Yersinia. Proc. Natl. Acad. Sci. USA 91:10493-10497.[Abstract/Free Full Text]