Bartonella: new explanations for old diseases

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Bartonella: new explanations for old diseases

GILBERT GREUB and DIDIER RAOULT

Unité des Rickettsies, Faculté de Médecine, Université de la Méditerranée, Marseille, France

Corresponding author: Professor D. Raoult (e-mail: didier.raoult{at}medecine.univ-mrs.fr, gilbert.greub@medecine.univ-mrs.fr).

Received 24 May 2002; accepted 4 June 2002.

Introduction

TOP
Introduction
The red blood cell
Conclusions
References

Until recently, there were only two recognised human diseasescaused by Bartonella spp.: trench fever due to B. quintana andCarrion's disease due to B. bacilliformis. Since then, Bartonellaspp. have been recognised as causative agents of further humandiseases, including bacillary angiomatosis, cat-scratch disease,chronic bacteraemia, chronic lymphadenopathy, meningoencephalitis,stellar retinitis, myelitis, granulomatous hepatitis, endocarditis,osteomyelitis and peliosis hepatitis [1] (Table 1). In parallel,the genus Bartonella, which until 1993 contained only one species(B. bacilliformis), was broadly extended by reclassifying withinit the genera Rochalimea [2] and Grahamella [3], and by thedescription of new Bartonella species (Fig. 1). Based on phylogeneticanalysis of the 16S rRNA sequences, the relatedness of Bartonellaspp. to other alpha-2 Proteobacteria including Brucella spp.,Afipia spp., Agrobacterium tumefaciens, Bradyrhizobium spp.and Bosea spp. has been demonstrated [2, 3]. Active researchon the pathogenesis of Bartonella infections has been triggeredby the increased number of species of Bartonella, the re-emergenceof older disease due to Bartonella, such as the modern formof trench fever that affects alcoholics and homeless people[4], the recognition of the role of Bartonella in AIDS-relateddiseases and the description of new clinical entities due toBartonella spp. As a facultative intracellular bacterium, Bartonellainteracts closely with its host cells. The study of these interactionsgave an insight into some of the underlying virulence factorsand pathogenic mechanisms, which may be common or specific tothe host cell or to the Bartonella species studied, or both.Interactions of Bartonella spp. with (i) red blood cells and(ii) endothelial cells have been studied for several years,but (iii) bone marrow progenitor cells may also play a centralrole as a sanctuary site in the pathogenesis of Bartonella (Fig. 2).

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Table 1. Bartonella infections in man and related clinical entities

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Fig. 1. Neighbour-joining tree resulting from comparison of sequences of groEL encoding genes of most Bartonella spp. identified to date. The values at each node represent the percentage of times each branch was found in 100 bootstrap replicates.

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Fig. 2. Interactions of Bartonella spp. with red blood cells, endothelial cells and a putative sanctuary site located in the bone marrow. Bartonella and Bartonella-associated factors are represented in pink, host cell-associated factors are represented in green.

The red blood cell

TOP
Introduction
The red blood cell
Conclusions
References

Infection of the red blood cell: a persistence and dissemination strategy

Bartonella infections are vector-borne diseases characterisedby a natural cycle, vectors and reservoir hosts [5]. Human pathogenicityis either related to natural infection (B. quintana and B. bacilliformis)or to incidental infections (for other Bartonella spp.), acquiredthrough contact with naturally infected mammals. Many Bartonellaspp. have been shown to multiply and persist in red blood cells,sharing common persistence and dissemination strategies. Thus,B. henselae was found to infect cat red blood cells [6–8]and B. tribochorum those of rats [9], whereas B. quintana [10]and B. bacilliformis [11] were shown to invade human red bloodcells. Bacteraemias were described even in healthy mammals,thus being one established exception to one of Koch's basicstatements: ‘Bacteria do not occur in the blood or tissuesof healthy animals or humans’ [12]. It was shown in thered blood cells of rats that the bacterial replication of B.tribocorum was regulated and stopped at a maximum of eight bacteria/cell[9]. The mechanism of regulation is unknown, but it preventshaemolysis and allows the persistence of Bartonella spp. withinred blood cells. Disregulation of this mechanism, with uninterruptedmultiplication of B. bacilliformis within red blood cells, mightexplain the rare acute haemolytic form of Carrion's disease(Oroya fever). However, as treatment of Bartonella with proteinaseK has been shown to reduce the haemolytic activity of B. bacilliformisby 25%, a bacterial protein may also be involved in Oroya fever-associatedhaemolysis [13]. The ability of Bartonella to persist in erythrocytesfor long periods may have been driven by evolutionary constraints,as it increases its transmissibility by blood-sucking arthropods.This persistence, which explains the prolonged bacteraemia insymptomatic and asymptomatic subjects, and the occurrence ofdisseminated disease in the homeless (chronic bacteraemia) orAIDS patients (bacillary angiomatosis), may also be favouredby the intra-erythrocytic localisation which partially protectsBartonella from the immune system.

Adherence to red blood cells

B. bacilliformis possess polar flagella (Fig. 3) that have beenshown to mediate erythrocyte adhesion [14]. This flagella-associatedadhesion was supported by the poor adherence of non-motile variants[11] and has been confirmed by the reduction of the erythrocyte-bindingability of B. bacilliformis by 40–50% with antiflagellinantibodies [15] and by the 75% reduction in binding abilityof a flagellin-minus mutant [16]. Importantly, erythrocyte adhesionwas not fully restored by complementation of the minus-mutant[16]. As the other Bartonella spp. (except B. clarridgeiae)do not possess polar flagella and as the B. bacilliformis flagellin-minusmutant retained some adhesive ability, other important mechanismsare involved in adherence to red blood cells. One of these maybe the bundle-forming pili expressed at the surface of low-passagedB. henselae and B. bacilliformis cells, which have been implicatedin the auto-agglutination propensity of Bartonella spp. [17].Proteins exposed at the bacterial surface may also play a rolein adhesion to erythrocytes, although no proteins able to interactwith red blood cells have been identified yet. As adherenceof B. bacilliformis to red blood cells is inhibited when thebacteria are pre-treated with N-ethyl maleimide, but is notinhibited when the erythrocytes are pre-treated with the samereagent [14], the red blood cell seems to play only a passiverole in adherence. Membrane erythrocyte proteins, which bindB. bacilliformis passively, include spectrin and glycophorinsA/B [18]. Enhanced binding of Bartonella to these proteins aftertreatment of erythrocytes with trypsin or neuraminidase hassuggested a possible masking of binding site [18]. The factthat glycophorin A/B is the major receptor on human erythrocytesfor Plasmodium falciparum merozoites [19] suggests that thisprotein is also utilised by Bartonella to bind to erythrocytes.

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Fig. 3. B. bacilliformis and its polar flagella, within human erythrocytes, as seen by confocal microscopy. (Courtesy of J. M. Rolain, Marseille.)

Invasion of red blood cells

It has been speculated that the binding of Bartonella to spectrinmay be a first step necessary to alter the erythrocyte membranefor internalisation of Bartonella cells [18]. This hypothesisis supported by the role of spectrin in the maintenance of erythrocyteshape and membrane integrity and deformability [18] and by thefact that proteases from P. falciparum were shown to cleaveerythrocyte cytoskeletal components and spectrin [20]. A bacterialprotein named deformin also appeared to be involved, at leastfor B. bacilliformis, in the formation of pits and trenchesin the red cell membranes [11, 21], that may favour both colonisationand entry into the cell [17]. This molecule, initially thoughtto be a protein, seems to be a small hydrophobic molecule withaffinity for albumin, although the effector mechanism remainsto be elucidated [22]. The presence of a homologue of the deforminof B. bacilliformis that also led to the invagination of redblood cells, although less pronounced, has been identified inB. henselae culture supernate [23], suggesting that the deformin-mediatedinvasion mechanism might be shared between several Bartonellaspecies.

At the molecular level, the genes of the invasion-associatedlocus (ial) identified in B. bacilliformis have been shown toconfer an invasive phenotype to minimally invasive Escherichiacoli strains [24]. The ial contains two genes named ialA andialB. Immediately upstream lies a gene encoding a carboxy-terminalprotease, ctpA, and another gene encoding the filament A polypeptide(FilA) [17, 25]. Downstream lie two open reading frames thatdo not share homology with other species [17, 25]. These sixgenes are thought to constitute a pathogenicity gene cluster,as (i) both ialA and ialB genes are needed to confer the invasivephenotype to E. coli; (ii) the gene encoding for the adhesionand invasion locus (Ail) protein of Yersinia enterocolitica,which is implicated in host cell attachment and invasion, shares60% amino acid similarity with that encoded by ialB; and (iii)FilA exhibits amino acid similarity with various filamentousproteins including the M1 of Streptococcus pyogenes, involvedin adhesion and invasion [17]. Furthermore, CtpA might alsobe involved in virulence, as a C-terminal protease of Salmonellatyphimurium enhances intra-macrophage survival [26]. More importantly,several genes of this cluster have been sequenced in other Bartonellaspp., and also in other facultatively intracellular bacteria,suggesting that some of the adhesion, invasion and persistencemechanisms used by Bartonella may be common to these species.Thus, the amino acid sequence of B. bacilliformis ialA shared73% homology with that of B. clarridgeiae and 49% with thatof Brucella melitensis, another member of the Rhizobium group,while the amino acid sequence of B. bacilliformis CtpA shared81% homology with that of B. quintana and 71% with that of Br.melitensis (homology analysis performed with ClustalW) [27].Whether ialA and ialB may explain the peculiar tropism of Bartonellafor red blood cells remains to be defined. The role played byCtpA, FilA and both additional orphan open-reading frames remainsalso to be clarified. A role in quorum sensing, i.e., regulationof the intra-erythrocytic growth of Bartonella may be possible.In conclusion, it appears that specific (polar flagella) andcommon (deformin, invasion-associated locus) mechanisms havebeen developed by the different Bartonella spp. to adhere toand invade the red blood cells.

Angiogenesis

Apart from their tropism for red blood cells, a second typicalpathogenic feature of Bartonella spp. is their ability to triggerangiogenesis. Such pathological angiogenesis is observed inbacillary angiomatosis and peliosis [28–31].

An unknown protein The first experimental evidence that Bartonella-related angiogenesismay be due to a protein was afforded by Garcia et al. in 1990[32]. They demonstrated that B. bacilliformis extracts possessan activity that stimulates endothelial cell proliferation upto three times that of a control [32]. The factor, which wasfound to be specific for endothelial cells and was larger than12–14 kDa (not dialysed), was thought to be a proteinbecause it was heat sensitive and precipitated with ammoniumsulphate 45% [32]. B. bacilliformis extracts were also reportedto stimulate the production of tissue plasminogen [32]. Livebacteria were later shown to increase both parameters (angiogenesisand tissue plasminogen production) in a fashion similar to thehomogenates of B. bacilliformis [33]. In 1994, Conley demonstratedin a similar in-vitro model that B. henselae induces an angiogenicfactor, whose susceptibility to trypsin also suggests that thefactor may be a protein. More recently, it has been shown thatthis factor may be secreted by B. henselae [34], indicatingthat B. henselae may induce endothelial cell proliferation independentlyof bacterial invasion. The dramatic effect of erythromycin onthe cutaneous lesions of bacillary angiomatosis [35, 36] maybe due to inhibition of the production of the proteic angiogenicfactor(s), as erythromycin is known to inhibit protein productionat the ribosomal level. An angiogenesis-based effect would betterexplain the rapidity of its effect and its lack of a sustainedresponse than a direct microbicidal one.

Vascular endothelial growth factor (VEGF) VEGF, angiopoietins and ephrins were proved to be critical andspecific for blood vessel formation [37]. Recently, Kempf etal. demonstrated that B. henselae induce EA.hy 926 cells (permanentendothelial cell line expressing factor VIII) to produce VEGF,which in turn was able to stimulate the proliferation of endothelialcells and the growth of B. henselae [38]. In the same study,Kempf et al. showed that the administration of VEGF-neutralisingantibodies reduced endothelial proliferation by 50% [38], suggestingthat other factors are involved, such as angiopoietins, ephrinsor the yet unknown proteic factor discussed above.

Importantly, VEGF not only induces endothelial proliferationbut also cell migration through several pathways that includethe activation of a small GTP-ase RhoA, which is associatedwith phosphorylation of myosin light chain [39]. This may easilyexplain why Bartonella-associated angiogenesis is also characterisedby altered spatial organisation within the monolayer and changesin cell morphology due to cytoskeleton re-organisation [40].However, the impaired migratory ability of Bartonella-infectedendothelial cells [41] was more surprising. This impaired mobilitymight result from the formation of thick robust stress fibres,probably via the activation of RhoA, as suggested by an inactivationassay [41]. Thus, the cells that effectively participate inangiogenesis are probably uninfected endothelial cells thatrespond to VEGF produced by the infected ones. B. henselae notonly promotes the formation of new permissive cells but alsoprotects the infected cells from apoptosis. Indeed, Bartonellasuppress both early and late events in apoptosis, namely caspaseactivation and DNA fragmentation [42]. This anti-apoptotic effect,found to be specific for endothelial cells [42], may be mediatedat least partially by VEGF, which is known to protect the cellsfrom apoptosis [43].

Peliosis hepatitis Peliosis hepatitis, which corresponds histologically to multipleblood-filled cystic spaces often communicating with the hepaticsinusoids, was initially thought to be induced by viruses [44].Similar lesions were later observed in mice or rats exposedto various drugs or toxins, including phalloidine and oxazepam[45, 46] and reported in patients with advanced cancer or receivinganabolic steroids. The Bartonella-associated peliosis hepatitis,associated with HIV infection, differs from that of classicalpeliosis hepatitis by the additional presence of clumps of bacteria[47]. Recently, while studying the ability of VEGF to blocktumour regression, Wong et al. observed that mice implantedwith VEGF-expressing tumours sustained high morbidity and mortalitythat were out of proportion to the tumour burden. High serumlevels of VEGF were associated with a lethal hepatic syndromecharacterised by massive sinusoidal dilatation and endothelialcell proliferation and apoptosis [48]. A striking reversal ofVEGF-induced liver pathology was achieved by surgical excisionof VEGF-secreting tumours or by systemic administration of apotent VEGF antagonist [48]. As this VEGF-induced syndrome resemblescancer and Bartonella-induced peliosis hepatitis, the bacillarypeliosis hepatitis may be directly due to the VEGF producedby the infected endothelial cells and by other infected cellsthat are known to secrete VEGF, such as erythroblasts [49].

Placenta growth factor The placenta growth factor (PIGF) is analogous to VEGF and issecreted by the placenta and erythroblasts [37, 49]. Its effecton Bartonella multiplication remains to be defined, as doesthe role played by Bartonella in its production. However, thepresence of vascular lesions in the maternal placenta of miceinfected experimentally with B. birtlesii [50], and the roleplayed by VEGF in Bartonella pathogenesis [38], suggest thatPIGF might be involved in the genesis of the reproductive disordersobserved by Boulouis et al. in infected mice.

Endothelial cells

The Bartonella–endothelial cell interaction is not restrictedto angiogenesis stimulation. Thus, (i) invasion of endothelialcells was described for B. quintana [51], B. henselae [52] andB. bacilliformis [53], and (ii) a pro-inflammatory activationof endothelial cells was postulated, which is thought to bea result of receptor-ligand interactions between the activatedendothelium and circulating neutrophils [54].

Adherence to endothelial cells The bacterial ligands that may be involved in adherence mayinclude bundle-forming pili (see above) and several outer-membraneproteins (OMPs). Of the nine proteins located in the outer membraneof B. henselae, five were shown to bind human umbilical veinendothelial cells [55]. Of these, a 43-kDa protein (Omp43),that exhibits a similar amino acid sequence to the Omp2b porinof Brucella spp., was shown to have especially high affinitywith endothelial cells, suggesting that it may play a majorrole in Bartonella pathogenesis [55, 56]. The endothelial receptorsinvolved in Bartonella adhesion may include intercellular adhesionmolecule-1 (ICAM-1), which has been shown to be enriched especiallyat the tips of the protrusions of the endothelial membrane [52].Interestingly, endothelial adhesion molecules (ICAM-1 and E-selectin)expression is upregulated via NF- ${kappa}$ B translocation, induced byB. henselae [52].

Invasion of endothelial cells Endothelial cells are invaded by two mechanisms: (i) endocytosisof bacteria, similar to that present in other intracellularclades, and (ii) the engulfment of clustered bacteria by a uniquehost cell structure called the invasome [52]. Invasion is associatedwith cytoskeletal re-arrangements, themselves induced by Bartonellavia Rho GTPase signalling [41].

Type IV secretion system and the VirB operon Type IV secretion systems consist of a multiprotein channelthat transports DNA or protein from bacteria to host cell. Sucha system is present in A. tumefaciens, another alpha-2 proteobacteriumthat parasitises plants. A gene cluster, the virB operon ofA. tumefaciens, plays a critical role in the formation of thechannel through which the transfer of oncogenic T-DNA occurs,resulting in tumour formation [58]. Type IV secretion systemscoded by the virB operon are also present in Br. suis and Bordetellapertussis, where they appear to be required for survival inhost macrophages and exportation of the pertussis toxin, respectively[59, 60]. Recently, Padmalayan et al. discovered that the geneencoding an immunogenic 17-kDa antigen of B. henselae was locatedwithin the virB operon of B. henselae [61]. The virB operonof B. henselae encodes 10 genes, of which eight share significanthomology to those of A. tumefaciens, suggesting that it encodesfor a type IV secretion system. Interestingly, no homologuesof the gene encoding the immunogenic 17-kDa antigen are presentoutside Bartonella spp. [61]. Its expression is stimulated byendothelial cells [62]. Although the molecule that may be transferredto the host cell remains to be defined, some have speculatedthat it may be involved in the production of VEGF by the endothelialcells.

Activation of endothelial cells A pro-inflammatory activation of endothelial cells was postulated,which is thought to be a result of receptor-ligand interactionsbetween the activated endothelium and circulating neutrophils[54]. This is supported by the recent demonstration that B.henselae itself and B. henselae-derived OMPs induce an NF- ${kappa}$ B-dependentupregulation of E-selectin and ICAM-1 in endothelial cells,which in turn results in enhanced polymorphonuclear rollingand adhesion [57].

Primary niche

In the rat model of B. tribochorum infection, the presence ofperiodic erythrocyte infection waves has been demonstrated [9],that echo the 5-day periodicity of the ‘Quintan fever'.The fact that Bartonella parasitise erythrocytes without leadingto haemolysis, with the exception of B. bacilliformis, suggeststhat the re-infection waves are due to the liberation of thebacteria from a distant sanctuary site [54]. This unknown primaryniche might be the endothelial cells, as suggested by Dehio[54]. However, a number of hints suggest that the primary nicheor sanctuary site might instead be located in the bone marrow,as follows. (i) Although, in vitro, Bartonella is able to entervarious cells, including macrophages [63], only erythrocytesand endothelial cells are permissive to Bartonella in vivo.The cells that play the role of primary niche should thus sharesome characteristics common to erythrocytes and endothelialcells. Candidates are mainly the cells that are issued by differentiationof the haemangioblast, the common precursor of both erythrocytesand endothelial cells. These include mainly angioblasts anderythroblasts. (ii) The fact that erythroblasts express VEGF[49], a factor known to enhance Bartonella replication [38].(iii) All organs involved in bacillary angiomatosis could potentiallyplay the role of sanctuary, including brain, penis, vulva, cervix,muscle and bone marrow [64–68]. However, after skin, boneis the second most frequent site, and bone lesions of bacillaryangiomatosis are characterised by well circumscribed osteolysis,that is often painful and usually affects long bones [69]. Painpattern and osteolysis echo those found in mastocytosis andmultiple myeloma, suggesting that bone marrow cells may be infectedby Bartonella. (iv) The outstanding features of trench feverare pain and tenderness in the shins and relapsing fever [70].Many subjects also present only with painful shins, which wereoften, in the absence of fever, wrongly attributed to flat feetor rheumatism due to prolonged standing in mud and water [70].This suggests that B. quintana may involve the bone marrow intrench fever patients. (v) The fact that bone marrow cells arehighly permissive to Br. melitensis, a phylogenetically closerelative of Bartonella spp. and to many other intracellularpathogens.

Conclusions

TOP
Introduction
The red blood cell
Conclusions
References

Future research should especially be aimed at defining the factors(i) determining the host specificity (especially for human-specificspecies), (ii) involved in erythrocyte and endothelial cellinfection, and (iii) controlling Bartonella-associated angiogenesis.Moreover, the location in the host of a Bartonella sanctuary,if any, which could be responsible for the observed relapsesof intra-erythrocytic infections should be identified. Bonemarrow progenitors such as erythroblasts might be a potentialcandidate but this should be investigated further.

References

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Conclusions
References

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