Human infection caused by leptospira fainei. (Dispatches).We report a human case of leptospirosis leptospirosis (lĕp'təspīrō`sĭs), febrile disease caused by bacteria of the genus Leptospirae. The disease occurs in dogs, cattle, pigs, sheep, goats, and horses and is transmissible to humans. in which the spirochete spirochete Any of an order (Spirochaetales) of spiral-shaped bacteria. Some are serious pathogens for humans, causing such diseases as syphilis, yaws, and relapsing fever. Spirochetes are gram-negative (see gram stain) and motile. was detected by dark-field microscopy examination of cerebrospinal fluid (CSF Cerebrospinal Fluid (CSF) Analysis Definition Cerebrospinal fluid (CSF) analysis is a laboratory test to examine a sample of the fluid surrounding the brain and spinal cord. ) and isolated from both CSF and blood. Leptospira fainei was identified by sequencing the 16S rDNA gene, which had been amplified by polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is . This case confirms the role of L. fainei as a human pathogen and extends its distribution to southern Europe. ********** Leptospirosis is a worldwide zoonosis Zoonosis Definition Zoonosis, also called zoonotic disease refers to diseases that can be passed from animals, whether wild or domesticated, to humans. , usually transmitted to humans through contaminated water or direct exposure to the urine of infected animals. The clinical spectrum of the disease ranges from an influenza-like syndrome to Weil's disease and multiple organ dysfunction syndrome Multiple organ dysfunction syndrome MODS, previously known as multiple organ failure (MOF), is altered organ function in an acutely ill patient requiring medical intervention to perform homeostasis. (1). The causative agents of human leptospirosis belong to the genus Leptospira, which contains both saprophytic saprophytic pertaining to saprophyte. and pathogenic species (1). L. fainei was first isolated from pigs in Australia (2). Subsequently, several reports based on serologic testing suggested that L. fainei might be pathogenic for humans as well (3,4). This potential has been recently confirmed by isolating L. fainei from the urine of two patients and the blood of one patient in Denmark (5). We report a typical case of leptospirosis in which L. fainei was directly observed in the cerebral spinal fluid (CSF) and was isolated from both CSF and blood. Case Report In February 2001, a 39-year-old man was hospitalized in Marseilles, France, with fever and disorientation. This truck driver lived in Portugal and had been driving in Spain for 2 weeks before entering France. He arrived in France 3 days before admission. The day of admission, his co-workers found him confused and febrile after sleeping in his truck. He had no previous relevant medical history. On admission, his temperature was 40[degrees]C with tachycardia, and his blood pressure was 120/80 mm Hg. Clinical examination showed a drowsy, confused man with a bilateral headache, provoked myalgia of the legs, hepatalgia, and conjunctivitis conjunctivitis (kənjəngtəvī`təs), inflammation or infection of the mucosal membrane that covers the eyeball and lines the eyelid, usually acute, caused by a virus or, less often, by a bacillus, an allergic reaction, or an . Neurologic examination showed signs of meningeal me·nin·ge·al adj. Of, relating to, or affecting the meninges. meningeal pertaining to the meninges. meningeal hemorrhage irritation, including cervical rigidity, Brudzinski's sign, hyperesthesia hyperesthesia /hy·per·es·the·sia/ (-es-the´zhah) increased sensitivity to stimulation, particularly to touch.hyperesthet´ic acoustic hyperesthesia , auditory hyperesthesia hyperacusis. , and photophobia photophobia /pho·to·pho·bia/ (-fo´be-ah) abnormal visual intolerance to light.photopho´bic pho·to·pho·bi·a n. 1. . There was no rash, and the rest of the physical examination was normal. Results of biochemical investigation included increased alanine aminotransferase (61 IU/L), aspartate aminotransferase (78 IU/L), lactate dehydrogenase (781 IU/L), fibrinogen Fibrinogen The major clot-forming substrate in the blood plasma of vertebrates. Though fibrinogen represents a small fraction of plasma proteins (normal human plasma has a fibrinogen content of 2–4 mg/ml of a total of 70 mg protein/ml), its conversion level (6.44 g/L), and C-reactive protein (273 mg/L), associated with hypoglycemia hypoglycemia: see diabetes. hypoglycemia Below-normal levels of blood glucose, quickly reversed by administration of oral or intravenous glucose. Even brief episodes can produce severe brain dysfunction. (2.9 mmol/L), hypoalbuminemia (26 g/L), hypoproteinemia (54 g/L), and hypocholesterolemia (2.3 mmol/L). The leukocyte count was 11,000/[mm.sup.3] with 69% polymorphonuclear polymorphonuclear /poly·mor·pho·nu·cle·ar/ (-noo´kle-er) having a nucleus so deeply lobed or so divided as to appear to be multiple. pol·y·mor·pho·nu·cle·ar adj. Having a lobed nucleus. forms. Thrombocytopenia Thrombocytopenia Definition Thrombocytopenia is an abnormal drop in the number of blood cells involved in forming blood clots. These cells are called platelets. (110 G/L) was also observed. The kaolin cephalin ceph·a·lin or keph·a·lin n. Any of a group of phospholipids having hemostatic properties and found especially in the nervous tissue of the brain and spinal cord. time was 58 s (control 34 s), and the prothrombin prothrombin Carbohydrate-protein compound in plasma essential to coagulation. In response to bleeding, a complex series of clotting-factor interactions leads to its conversion by thromboplastin to thrombin, which transforms fibrinogen in plasma into fibrin. rate was 42%. Blood smears showed no parasites. Cerebral scanning was normal. Analysis of the CSF on day 1 showed 4 leukocytes/[mm.sup.3], 50,000 erythrocytes/ [mm.sup.3], and elevated protein levels (1.48 g/L). On day 2, another CSF analysis showed 75 leukocytes/[mm.sup.3], with 70% polymorphonuclear forms, 5,500 erythrocytes/[mm.sup.3], and increased protein (0.64 g/L). Direct examination by dark-field microscopy of the CSF from day 2 was performed and controlled by two experimental investigators, who observed many spirochetes (6). The patient received a 10-day treatment with 12 g/day intravenous amoxicillin. The fever decreased to 38[degrees]C on day 4 and resolved on day 7. The patient was discharged from the hospital and remained well. No occupational or recreational risks for leptospirosis could be established. The patient had been traveling recently in Spain and Portugal but had no apparent exposure to sources of leptospires. The Study Specific diagnostic tools were used to identify the spirochete responsible for this infection. Single 0.1 mL- and 0.01 mL-aliquots of lithium-heparin anticoagulated whole blood were spread onto 10 mL of Leptospira medium, a polysorbate polysorbate /poly·sor·bate/ (pol?e-sor´bat) any of various oleate esters of sorbitol and its anhydrides condensed with polymers of ethylene oxide, numbered to indicate chemical composition and used as surfactant agents. medium similar to Ellinghausen and McCullough modified Johnson and Harris medium (EMJH) (Bio-Rad Laboratories, Inc., Aulnay/Bois, France), and was incubated at 30[degrees]C. The same procedure was carried out for CSF. For urine samples, the specimens were first filtered on 0.45- and then 0.22-[micro]m filters before inoculation. Once a week, 10 [micro]L of culture medium was examined by dark-field microscopy. Cultures from both blood and CSF were positive and yielded Leptospira after 1 week of incubation. Urine cultures remained negative. No agglutination agglutination, in biochemistry agglutination, in biochemistry: see immunity. agglutination, in linguistics agglutination, in linguistics: see inflection. of the isolated strain was obtained with any reference sera, except a weak agglutination (titer 400) with serovar hurstbridge antiserum antiserum /an·ti·se·rum/ (an´ti-se?rum) a serum containing antibody(ies), obtained from an animal immunized either by injection of antigen or by infection with microorganisms containing antigen. . The genomic DNA of the spirochete was extracted from the blood culture by the Qiamp blood kit procedure (QIAGEN GmbH, Hilden, Germany). For polymerase chain reaction (PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) ), universal 16S rDNA primers fD1 and rP2 (7) were used, and sequences of the PCR products were obtained as previously described (8). The 16S rDNA sequence of the isolate had 100% identity with the prototype strain sequence of L. fainei (GenBank accession no. 60594) (Figure 1). Pulsed-field gel electrophoresis of NotI macrorestriction fragments of Leptospira DNAs was performed as previously described (9). However, the NotI macrorestriction pattern was quite different from all patterns previously recorded for a large collection of Leptospira strains belonging to different species and serovars (Figure 2). Sera collected on days 4, 8, 10, and 45 were tested by a microimmunofluorescent antibody assay (MIFA MIFA Member of the Institute of Field Archaeologists MIFA Materials and Information Flow Analysis ) with L. biflexa serovar patoc, L. fainei, L. interrogans, and own strain as antigens (cut-off titer _200); Western immuiloblot with L. biflexa patoc and L. fainei as antigens; and a microagglutination test (MAT) (10,11). For MAT, sera were incubated with suspensions of live leptospires belonging to 17 distinct serogroups, including a strain of L. fainei serovar hurstbridge. The titer was defined as the highest dilution giving 50% agglutination. The presence of immunoglobulin (Ig) M was investigated by an enzymelinked immunosorbent assay (ELISA ELISA (e-li´sah) Enzyme-Linked Immuno-Sorbent Assay; any enzyme immunoassay using an enzyme-labeled immunoreactant and an immunosorbent. ELISA n. ) developed at the Institut Pasteur, with serovar patoc as an antigen (12). All sera were negative by MIFA, MAT, and IgM ELISA, even when L. fainei was used as an antigen. For Western blot, the spirochetes were grown on Leptospira medium centrifuged and used at a concentration of 2 mg/mL. After blocking, the nitrocellulose nitrocellulose, nitric acid ester of cellulose (a glucose polymer). It is usually formed by the action of a mixture of nitric and sulfuric acids on purified cotton or wood pulp. was incubated overnight at 4[degrees]C with patient sera diIuted 1:50. Seroconversion was demonstrated by Western blot analysis West·ern blot analysis n. An electrophoretic procedure for separating proteins. . The first two sera were negative by Western blot, but a reaction with L. fainei was observed in IgG and IgM at days 10 and 45. Sera reacted with protein bands of 28, 25, 24, and 19 kDa from L. fainei, while no reaction was obtained with serovar patoc (Figure 3). [FIGURES 1-3 OMITTED] Conclusions This clinical picture was highly suggestive of leptospirosis, with the association of meningeal syndrome, provoked leg myalgias, and conjunctivitis; nonspecific laboratory findings included hepatic enzyme elevation, hyperleukocytosis, thrombocytopenia, and low prothrombin rate (1). In fact, the case was considered clinically to be leptospirosis. The isolated Leptospira was identified as closely related to L. fainei on the basis of 16rRNA amplification and sequencing. The strain has been isolated in our laboratory in Marseille, where this species had never been cultivated. Thus, laboratory contamination is unlikely, and the isolated strain of L. fainei, which is close to the serovar hurstbridge, can be considered the causative agent of the patient's meningitis. Moreover, a spirochete resembling a leptospire was seen by well-trained investigators at the darkfield microscope. L. fainei has been only recently been considered an emerging pathogen. In Australia, a sample of 723 human sera from patients from a dairy and pig-producing area of Victoria, all of whom had symptoms consistent with leptospirosis, was submitted for leptospirosis serologic testing. The sera were also tested for antibodies to L. fainei serovar hurstbridge. MAT titers [greater than or equal to] 128 were detected in 13.4% (3). Furthermore, a leptospirosis surveillance program was conducted for 12 months on the entire population of the Seychelles; the incidence of leptospirosis was 10/100,000, with a 20 % seroprevalence seroprevalence Immunology The proportion of a population that is seropositive–ie, has been exposed to a particular pathogen or immunogen; the seropositivity of a population is calculated as the number of individuals who produce a particular antibody divided of L. fainei. This organism was suspected to be involved in severe forms such as acute renal failure acute renal failure Acute kidney failure Nephrology An abrupt decline in renal function, triggered by various processes–eg, sepsis, shock, trauma, kidney stones, drug toxicity-aspirin, lithium, substances of abuse, toxins, iodinated radiocontrast. , pulmonary hemorrhage, and possibly death (4). The first human isolation ofL. fainei occurred in Denmark, from two patients (5). The first patient had chronic disease with increasing jaundice for 6 months before admission to the hospital, and test results showed elevated hepatic enzymes. The second patient had abdominal and lower back pain for 5 months and severe headaches and dizziness for 2 months before admission. Thus, both patients had atypical chronic disease, unlike the typical case of leptospirosis that we describe. In our case, we tested sera 4, 8, 10, and 45 days after onset of illness. No reactivity was detected by MIF (1) (Maker Interchange Format) An alternate file format for a FrameMaker document. A MIF file is ASCII text, which can be created in another program and imported into FrameMaker. and MAT tests, although a reaction in IgG and IgM at day 10 and 45 was detected by Western blot. Early antibiotic treatment may have affected the serologic responses. The two Danish patients from whom L. fainei was isolated were tested by MAT and showed no substantial serologic reaction (5). However, published serologic studies have shown that an immunologic response may be observed, in some cases at a high level (4). As reported here, Western blot may prove to be a good tool for diagnosis. Antibiotic treatment by amoxicillin (12 g/day for 10 days) was effective. In the Seychelles, for 8 patients among 75 with confirmed leptospirosis, a 5-day treatment with penicillin was insufficient to eradicate the bacteria, as indicated by positive PCR results (4). Treatment for longer than 1 week may be necessary, because L. fainei could be still isolated from Danish patients after a 1-week treatment with intravenous penicillin, but not after 4 weeks of amoxicillin treatment (3). This case confirms the pathogenic role of L. fainei in humans and extends its geographic distribution to southern Europe. The clinical finding of our case did not differ from that of other Leptospira infections, but the route of exposure remains unknown. Although the usual procedures of direct detection, isolation, and identification of leptospires are effective for L. fainei, we did not observe substantial serologic reactivity. Further studies, including Western blot, are needed to explain the weak immune response and to evaluate the prevalence of infection by this newly discovered Leptospira species. Acknowledgments We thank Odessa Deffenbaugh for linguistic assistance. References (1.) Levett PN. Leptospirosis. Clin Microbiol Rev 2001;14:296-326. (2.) Perolat P, Chappel RJ, Adler B, Baranton G, Bulach DM, Billinghurst ML, et al. Leptospira fainei sp.nov., isolated from pigs in Australia. Int J Syst Bacteriol 1998;48:851-8. (3.) Chappel RJ, Khalik DA, Adler B, Bulach DM, Faine S, Perolat P. Serological serological pertaining to or emanating from serology. serological test one involving examination of blood serum usually for antibody. titres to Leptospira fainei serovar hurstbridge in human sera in Australia. Epidemiol Infect 1998;121:473-5. (4.) Yersin C, Bovet P, Merien F, Wong T, Panowsky J, Perolat P. Human leptospirosis in the Seychelles (Indian Ocean): a population-based study. Am J Trop Med Hyg 1998;59:933-40. (5.) Petersen AM, Boyde K, Blom J, Schliting P, Krogfelt KA. First isolation of Leptospira fainei serovar hurstbridge from two human patients with Weil's syndrome. J Med Microbiol 2001;50:96-100. (6.) Arzouni JP, Laveran M, Beytout J, Ramousse O, Raoult D. Comparison of western blot and microimmunofluorescence as tools for Lyme disease seroepidemiology. Eur J Epidemiol 1993;9:269-73. (7.) Weisburg WG, Barns SM, Pelletier DA, Lane DJ. 16S ribosomal DNA amplification for phylogenetic study. J Bacteriol 1991;173:697-703. (8.) Drancourt M, Bollet C, Carlioz A, Martelin R, Gayral JP, Raoult D. 16S ribosomal DNA sequence analysis of a large collection of environmental and clinical unidentifiable bacterial isolates. J Clin Microbiol 2000;38:3623-30. (9.) Herrmann JL, Bellenger E, Perolat P, Baranton G, Saint Girons I. Pulsedfield gel electrophoresis of NotI digests of leptospiral DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. : a new rapid method of serovar identification. J Clin Microbiol 1992;30:1696-702. (10.) Raoult D, Bres P, Baranton G. Serologic diagnosis of leptospirosis: comparison of line blot and immunofluorescence techniques with the genus-specific microscopic agglutination test. J Infect Dis 1989;160:734-5. (11.) La Scola B, Rydkina L, Ndihokubwayo JB, Vene S, Raoult D. Serological differentiation of murine typhus and epidemic typhus using cross-adsorption and western blotting. Clin Diagn Lab Immunol 2000;7:612-6. (12.) Postic D, Merien F, Perolat P, Baranton G. Biological diagnosis. Leptospirosis-Lyme borreliosis. 2nd ed. Paris: Collection des Laboratoires de Reference et d'Expertise; 2000. Dr. Arzouni is a physician in the Clinical Microbiology Laboratory of the University Hospital Timone, Marseilles, France. He is especially interested in spirochete infections and has developed techniques for molecular detection and cultivation of spirochetes in human specimens. Address for correspondence: Didier Raoult, Unite des Rickettsies, Faculte de Medecine, Universite de la Mediterranee, CNRS CNRS Centre National de la Recherche Scientifique (National Center for Scientific Research, France) CNRS Centro Nacional de Referencia Para El Sida (Argentinean National Reference Center for Aids) UMR 6020, 27 Bd Jean Moulin, 13385 Marseille Cedex 5, France; fax: 33 4 91 83 03 90; e-mail: Didier.Raoult@medecine.univ-mrs.fr Jean-Pierre Arzouni, * Philippe Parola, * ([dagger]) Bernard La Scola, * Daniele Postic, ([double dagger]) Philippe Brouqui, * ([dagger]) and Didier Raoult * Unite de Rickettsies, Universite de la Mediterranee, Marseille, France; ([dagger]) Service de Maladies Infectieuses et Tropicales, Marseille, France; and ([double dagger]) Institut Pasteur, Paris, France |
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