Abstract
Bartonella alsatica is a wild rabbit pathogen causing bacteremia rarely reported in humans, with only three cases published so far, including one lymphadenitis and two endocarditis cases. Here, we report the case of a 66-year-old man who suffered from acute renal failure due to a membranoproliferative glomerulonephritis. Fluorodeoxyglucose (FDG) positron emission tomography/computed tomography (PET/CT) showed diffuse FDG uptake around the aortobifemoral graft with no indication of infection. A white blood cell scan showed an accumulation of labeled neutrophils on the left femoral part of the graft. The patient underwent surgery and an abscess around the left iliac part of the graft was found intraoperatively. Intraoperative samples were all negative, but 16S rRNA gene-based PCR was positive, and the sequence was positioned among the Bartonella species cluster. Specific PCRs targeting groEL/hsp60, rpoB and gltA genes were performed and led to the identification of B. alsatica. Accordingly, indirect immunofluorescence serological analyses were positive for Bartonella henselae and Bartonella quintana. The patient had a history of regularly hunting wild rabbits. He was treated with 100 mg of doxycycline twice a day for six months and his renal function significantly improved with no sign of persistent infection. This case highlights the contribution of serology assays and molecular-based methods in prosthetic vascular graft infection diagnosis.
Introduction
Bartonella species are fastidious, aerobic or microaerophilic, Gram-negative and facultative intracellular bacteria.Citation1 Bartonella spp. are usually responsible for lymphadenitis and endocarditis. Diagnosis is often difficult and requires the use of serological assays and molecular-based methods.Citation1 Only three cases of B. alsatica infection in humans have been reported so far, one lymphadenitisCitation2 and two endocarditisCitation3 cases. Although two cases of prosthetic vascular graft infection (PVGI) caused by B. henselae were previously reported,Citation4 this is the first case of PVGI associated with B. alsatica and therefore the fourth human case of B. alsatica infection.
Case
A 66-year-old man with an aortobifemoral bypass was admitted to the nephrology department of Périgueux Hospital, France, in November 2016 for acute renal failure (serum creatinine 4.8 mg/dL versus 2.3 mg/dL in October 2016). He had an undiagnosed chronic renal failure evolving since 2013. The patient showed a global cardiac insufficiency and asthenia; he had macroscopic hematuria, lower limb oedema, and one episode of low grade fever during hospitalisation. Biological signs of inflammation were minimal (CRP 18 mg/L (normal value <5 mg/L), neutrophils 5.6 G/L). He had low serum albumin (3.1 g/dL) and glomerular proteinuria (urine protein-creatinine ratio 14 g/g). A renal biopsy showed a membranoproliferative glomerulonephritis, with marked granular subendothelial and mesangial deposits of IgM, C1q, C3 and IgG, and two spots with extracapillary proliferation. Blood cultures, autoimmune assays, cryoglobulinemia, HIV, HBV, and HCV serologies were negative. Trans-thoracic echocardiography showed no sign of endocarditis. Fluorodeoxyglucose positron emission tomography/computed tomography (FDG PET/CT) showed diffuse FDG uptake around the graft with no indication of infection. The left femoral part of the graft was considered to be infected based on white blood cell scan images. Renal function improved slightly after diuretic treatment (serum creatinine 3.2 mg/dL, urine protein-creatinine ratio of 6 g/g).
Subsequently, the patient was admitted to Bordeaux University Hospital, France, in February 2017 with a high suspicion of PVGI, considering the previous episode of low grade fever, the slightly elevated biological signs of inflammation and the signs of infection in the left femoral part of the graft based on white blood cell scan images. In May 2017 he underwent surgery. An abscess around the left iliac part of the graft was found intraoperatively. The graft was replaced by a new graft made of silver-triclosan knitted collagen-coated polyester. The patient was treated postoperatively with meropenem, linezolid, caspofungin and amikacin. All of the intraoperative samples were negative. Only one sample from the right iliac part of the graft was positive for Staphylococcus pasteuri, which was considered to be a contaminant. Coxiella burnetii serology was negative. No multi-drug resistant bacterium was isolated and antimicrobial therapy was changed to piperacillin-tazobactam. Since cultures of graft specimens were negative, a 16S rRNA gene-based PCR with subsequent sequencing was performed.Citation5 The Bioinformatics Bacterial Identification tool (BIBI)Citation6 positioned the primer-less 16S rRNA sequence (GenBank accession number: MH230166) among the Bartonella species cluster. The identification at the species level was then performed using specific PCRs targeting groEL/hsp60, rpoB and gltA genes since these genes have the best discriminating power among the Bartonella species. The BIBI positioned both groEL/hsp60 and rpoB primer-less sequences (GenBank accession numbers: MH230168 and MH230167, respectively) close to B. alsatica. The identification was confirmed by gltA sequence analysis (GenBank accession numbers: MH230169) that presented 100% identity in a 337-nucleotide overlap using the NCBI Blast program. Accordingly, indirect immunofluorescence serological analyses (Bartonella IFA-Focus Diagnostics, Diasorin kit) were positive for B. henselae and B. quintana (IgG titer 1/1280 and 1/640, respectively, thresholds 1/320). Nevertheless, three different specific PCRs identified B. alsatica. We performed Western blotting using Bartonella sp. antigens, and after adsorption, the result was inconclusive, despite a slightly higher reactivity for B. alsatica.Citation7
The antibiotic therapy was switched to 100 mg of doxycycline twice a day, resulting in a rapid drop in the fever and improvement of biological signs of inflammation. PET/CT re-evaluation after a 6-month doxycycline treatment showed a non-specific hypermetabolism of the new graft. Renal function significantly improved with time (serum creatinine 1.7mg/dL, urine protein-creatinine ratio 1g/g in January 2018). Accordingly, the PVGI was considered to be cured and doxycycline treatment was stopped.
Discussion
The Bartonella genus was first described during World War I, since B. quintana was responsible for the trench fever which killed more than one million troops.Citation1 The bacterium Rickettsia quintana was isolated in the 1920s, cultured in the 1960s and reclassified as B. quintana. Thirty-five species have been identified so far but only 13 have been implicated in human infections.Citation1 Besides trench fever, B. quintana can be responsible for bacteremia, blood-culture-negative endocarditis, bacillary angiomatosis, bacillary peliosis, splenitis, osteomyelitis or orthopedic prosthesis infections, and chronic lymphadenopathy. B. henselae is also frequently involved in human infections and can be responsible for all the infections mentioned above, especially subacute lymphadenopathy and blood-culture-negative endocarditis.Citation1 Membranoproliferative glomerulonephritis has already been described in B. henselae infections,Citation8 however, it has never been associated with B. alsatica infection.
Bartonella spp. live in the gut of bloodsucking arthropod vectors (fleas, lice, ticks, and sandflies) and in the bloodstream of their mammalian hosts. The most well-known animal reservoirs are cats, rodents, and humans. However, new hosts have been identified such as marine mammals, camels, lions, bears, rabbits and foxes.Citation1
B. alsatica was first isolated from the blood of wild rabbits in Alsace, France, in 1999.Citation2 It is recognized as a wild rabbit pathogen causing bacteremia. Humans may be infected when they come into contact with wild rabbits while hunting, especially during evisceration with bare hands. They could also be infected by flea or tick bites.Citation2
The present patient used to hunt wild rabbits regularly until 2015 and may have been infected at least two years before presentation of any symptoms. However, he never butchered the rabbits. Since 2015, he had only been hunting large wild game such as boars. He would still occasionally eat rabbit meat and had no recollection of ever being bitten by a tick. His wife, who butchered the rabbits, was not infected, suggesting that B. alsatica may present a tropism for patients with cardiovascular abnormalities including prosthetic grafts. This is in agreement with one of the two previously described B. alsatica endocarditis cases in which a bioprosthetic aortic valve was also infected.Citation4
Laboratory diagnosis of Bartonella infections is difficult.Citation1 As Bartonella spp. are fastidious bacteria, blood and tissue culture have a low sensitivity (20–30%). Serological assays are widely used, especially indirect fluorescent antibody assays. However, the diagnosis at the species level is not reliable as there are a lot of cross-reactivities between B. henselae, B. quintana and other Bartonella species. Enzyme-linked-immunosorbent-assay, cross-adsorption and Western blot may also be used. Furthermore, diagnosis can be made by histopathology. Warthin-Starry silver staining can reveal dark-stained rods in various tissues, but immunohistochemical staining seems to be more specific. Molecular-based methods are now widely used, especially on various tissues (ie valvular, liver, etc) or grafts (ie valvular, vascular or orthopedic), as well as on whole blood, plasma or serum. Real-time PCR sensitivity is much higher than culture and more than specific than serology, especially for the diagnosis of Bartonella species. The most common molecular targets are the citrate synthase gene (gltA) and the RNA polymerase b-subunit gene (rpoB). However, the 16S rRNA gene-based PCR can also be useful and enables the microbiological diagnosis. Specific B. alsatica PCRs targeting rpoB, gltA and groEL/hsp60 genes were also positive on samples of the patient’s vascular graft.Citation1
Bartonella spp. are difficult-to-treat bacteria due to their capacity to evade the host immune system, in particular by living within the erythrocytes, and their capacity to form biofilm. Therefore, infection relapses are frequent after antibiotic withdrawal. Bartonella spp. are susceptible to most beta-lactams (apart from oxacillin and cephalothin), aminoglycosides, macrolides, doxycycline, quinolones and rifampin. However, only gentamicin and, perhaps to a lesser extent, rifampin are bactericidal against Bartonella spp. Bartonella infection therapy depends on the type of infection. For instance, lymphadenitis can be treated by macrolides, eg azithromycin for 5 days only, but for endocarditis a combination of two antibiotic treatments are recommended, doxycycline for four weeks and gentamicin for two weeks.Citation1,Citation9 Because there is no clear therapeutic recommendation for PVGI due to Bartonella spp., we successfully treated the patient with a long-course of doxycycline only. Gentamicin was not used due to the patient’s acute renal failure.
In conclusion, the possibility of a Bartonella species infection should be considered in culture-negative cases of PVGI, as is currently done in blood culture-negative endocarditis. This case highlights the contribution of serology assays for PVGI diagnosis, especially targeting fastidious bacteria including Coxiella burnetii, Bartonella and Brucella species. However, molecular-based methods are helpful to elucidate and confirm diagnosis of these severe infections at the species level.
Consent
Written informed consent was obtained from the patient for publication of this case report.
Acknowledgment
Charles Cazanave and Sabine Pereyre equally contributed to this study.
Disclosure
The authors report no conflicts of interest in this work.
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