key: cord-0069289-kpgv71p1
authors: Ohno, Tsukasa; Saito, Shunei; Iwata, Eri; Ushida, Sen; Otsuka, Ryohei; Miyahara, Ken; Matsuura, Akio
title: Blood culture–negative endocarditis caused by Bartonella henselae: a case report
date: 2021-11-05
journal: Indian J Thorac Cardiovasc Surg
DOI: 10.1007/s12055-021-01266-2
sha: aca55bc901e1aefabbf5439768292f939ee53df3
doc_id: 69289
cord_uid: kpgv71p1

Bartonella henselae is well known as a causative organism of cat scratch disease. Although this bacterium infrequently involves the heart, the diagnosis is difficult to confirm. A 75-year-old woman who had a pet cat presented with pancytopenia, hepatosplenomegaly, and low-grade fever. Echocardiography depicted sessile nodules on the aortic valve. C-reactive protein concentration was low, and leukocytosis was not seen. Two sets of blood culture turned out negative. However, elevated B. henselae immunoglobulin G titer led us to the diagnosis of infective endocarditis. Minocycline was administered orally in combination with intravenous administration of gentamicin as an antimicrobial treatment. The patient underwent aortic valve replacement 2 months after her initial visit. Warthin–Starry silver staining did not show any bacterial bodies. The culture of the vegetation tissue was negative. Polymerase chain reaction testing of the excised valve tissue detected the deoxyribonucleic acid of the organism. The postoperative course was uneventful, and the patient was discharged home.

Bartonella henselae is well known as a causative organism of cat scratch disease (CSD). Although this bacterium infrequently becomes the etiologic agent of infective endocarditis, it is difficult to confirm the diagnosis. Herein, we describe a case of blood culture-negative endocarditis (BCNE) caused by B. henselae.

A 75-year-old woman was referred to the division of hematology in our institution because of pancytopenia, general fatigue, low-grade fever, and lower leg edema (day 0). The patient had a history of diabetes mellitus as well as hypertension and was keeping a cat, which used to be a stray.

She had not taken any antibiotics before presentation to our institution. Blood analysis at the initial visit was as follows: white blood cell, 4600 /µL (segmented cell, 70%); hemoglobin, 8.2 g/dL; platelet, 70.0 × 10 3 /µL; aspartate aminotransferase, 21 IU/L; alanine transaminase, 9 IU/L; creatinine, 0.71 mg/dL; blood urea nitrogen, 20.2 mg/dL; C-reactive protein (CRP), 3.46 mg/dL; immunoglobulin (Ig) G, 1975 mg/dL; IgA, 90 mg/dL; and IgM, 29 mg/dL. The urine test was positive for protein. On auscultation, slight systolic murmur was audible. Transthoracic echocardiogram revealed sessile nodules on the right coronary cusp (18 × 8 mm) as well as on the left coronary cusp (6 × 6 mm) (Fig. 1a) . The ejection fraction was 55%, and mild to moderate aortic regurgitation was detected. Computed tomography showed moderate hepatosplenomegaly (Fig. 1b) . Although bone marrow aspiration was performed for possible lymphocytic leukemia, no atypical cells were observed. The two sets of blood culture submitted on day 0 came out negative. On day 7, furosemide (20 mg/day) was started as a treatment for lower leg edema. On day 12, in consideration of BCNE, Bartonella antibody test using immunofluorescence assay (IFA) ( Following median sternotomy, extracorporeal circulation was established by ascending aortic return and bicaval drainage. On opening of the aorta, fragile vegetations on the ventricular side of right and left coronary cusps were observed (Fig. 1c) . Neither the annulus nor the mitral valve was involved. The leaflets were excised carefully, and a 21-mm Inspiris Resilia bioprosthesis (Edwards Lifescience, Irvine, CA, USA) was implanted in the supra-annular position.

Histopathology of the valve tissue stained with hematoxylin and eosin revealed infiltration of neutrophils and lymphocytes as well as precipitation of fibrin, which were consistent with infective endocarditis (Fig. 1d) . Warthin-Starry silver staining did not show any bacterial bodies. The culture of the vegetation tissue was negative. However, PCR analysis of the vegetation was positive, detecting deoxyribonucleic acid (DNA) of B. henselae.

On day 75, gentamicin was discontinued. The postoperative course was uneventful, and the patient was discharged on day 87. Blood test results were as follows: white blood cell, 3700 /µL; hemoglobin, 11.1 g/dL; platelet, 153 × 103 /µL; and CRP, 0.17 mg/dL. On day 96, minocycline was stopped to complete the treatment.

B. henselae, formerly Rochalimaea, is a bacterium that is the causative agent of CSD. Humans usually get infected through scratches or bites of infected cats. Canine to human transmission is anecdotally reported. The disease is typically characterized by regional lymphadenopathy and fever. Although the heart involvement is known, the diagnosis is often difficult to confirm. Bartonella species account for 9-10% of BCNE [1, 2] . Houpikian et al. [3] reported that among 71 cases of Bartonella endocarditis, B. quintana was responsible for 53 (75%) cases and B. henselae for 17 (24%) cases. The clinical presentations in the B. henselae group were as follows: fever (100%), body weight loss (40%), heart failure (53%), splenomegaly (40%), hepatomegaly (7%), arterial embolism (47%), leukocytosis (38%), anemia (55%), thrombocytopenia (33%), renal failure (50%), and elevated erythrocyte sedimentation rate (83%) [3] .

B. henselae is a Gram-negative rod, which is culturable on chocolate agar or blood agar in 5% CO 2 incubator at 35-37℃ [4] . However, owing to its fastidious nature, 2-3 weeks is required for incubation. Thus, the bacterium cannot be easily isolated from clinical specimens. Blood culture methods have a sensitivity as low as 20% for diagnosing Bartonella endocarditis, while tissue culture of excised valves has a similarly low sensitivity of 30% [3] . Histopathologically, Warthin-Starry silver staining has frequently been employed and reveals black-stained bacteria in the affected valve tissue. The reported sensitivity in Bartonella endocarditis is 46% [5] . However, this staining method also detects Helicobacter pylori, Legionella pneumophila, spirochetes, and Klebsiella species, but does not provide a definitive diagnosis.

For the above reasons, serological as well as PCR testing is essential to confirm B. henselae infection. IgM and IgG antibodies are measured by commercially available IFA. In the kit used, the cutoff indicating acutephase infection was as follows: (1) IgM titers ≥ 1:20 or IgG titers ≥ 1:256, (2) initial specimen IgG titer ≥ 1:64 and < 1:256, and (3) second specimen (drawn 10-21 days after) titer ≥ 1:256 or a fourfold increase. Fournier et al. [6] reported that IgG titer of ≥ 1:800 was highly indicative of current infection in patients with endocarditis. The specificity and sensitivity of serological analysis vary significantly across the literature probably due to crossreactivity and between-kit variability [7] . By contrast, PCR test can identify the DNA of B. henselae. According to Edouard et al. [5] , among patients with endocarditis caused by B. henselae or B. quintana, the sensitivity was 33% and 92% in blood samples and surgically resected valve specimens, respectively. PCR testing of the valve tissue appears to be most useful in confirming the diagnosis, as was in the presented case. Notably, the modified Duke criteria, which mainly rely on blood culture positivity, show a lower accuracy for early diagnosis of endocarditis caused by Bartonella species.

Bartonella species are considered to evade the host immune system because of their intra-erythrocytic propagation and biofilm formation [8] . Thus, the use of at least two antibiotics has been advocated. The Sanford guide [9] recommended 200 mg/day of doxycycline for 6 weeks combined with 3 mg/kg/day of gentamicin for 2 weeks in patients with endocarditis. Since doxycycline was unavailable in our institution, minocycline was employed as an alternative. As regards its intractability to antimicrobial treatment, surgical resection of the infected valve tissue should always be considered.

Delayed diagnosis of endocarditis may cause further destruction of the valve, aggravation of heart failure, and annular abscess, which result in poor surgical outcomes. In our case, CRP before starting antimicrobial treatment remained low between 0.94 and 3.46 mg/dL, and no leukocytosis was detected. Ribeyrolles et al. [10] reported that CRP at admission was < 2 mg/dL in 13 (2.8%) of 469 patients with endocarditis. Not all patients with endocarditis present with elevated CRP or leukocytosis. Moreover, especially in patients with BCNE, the use of transesophageal echocardiography may help identify the progression of valve destruction and aortic regurgitation.

In conclusion, when an echocardiogram shows a mass on the valve leaflet, whereas blood culture is negative, serological as well as PCR testing should be carried out to screen for infection caused by fastidious bacteria, including Bartonella species.

Author contribution All authors contributed to the diagnosis or the treatment of the disease. The first draft of the manuscript was written by Tsukasa Ohno and was critically revised by Shunei Saito. All authors commented on previous versions of the manuscript. All authors read and approved the final manuscript.

Funding None.

Code availability Not applicable.

Ethics approval Ethical approval was waived by the local Ethics Committee of Ichinomiya Municipal Hospital in view of the retrospective nature of the study and all the procedures being performed were part of the routine care.

Informed consent Written informed consent was obtained from the patient for publication of this case report and accompanying images.

The authors declare no competing interests.

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