Molecular, clinical, and pathologic comparison of two distinct strains of Haemobartonella felis in domestic cats

Janet E. Foley From the Center for Companion Animal Health (Foley, Harrus, Poland, Pedersen) and Departments of Population Health and Reproduction (Chomel), School of Veterinary Medicine, University of California, Davis, CA 95616.

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Shimon Harrus From the Center for Companion Animal Health (Foley, Harrus, Poland, Pedersen) and Departments of Population Health and Reproduction (Chomel), School of Veterinary Medicine, University of California, Davis, CA 95616.

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Amy Poland From the Center for Companion Animal Health (Foley, Harrus, Poland, Pedersen) and Departments of Population Health and Reproduction (Chomel), School of Veterinary Medicine, University of California, Davis, CA 95616.

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Bruno Chomel From the Center for Companion Animal Health (Foley, Harrus, Poland, Pedersen) and Departments of Population Health and Reproduction (Chomel), School of Veterinary Medicine, University of California, Davis, CA 95616.

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Niels C. Pedersen From the Center for Companion Animal Health (Foley, Harrus, Poland, Pedersen) and Departments of Population Health and Reproduction (Chomel), School of Veterinary Medicine, University of California, Davis, CA 95616.

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Abstract

Objective

To characterize 2 strains of Haemobartonella felis by use of molecular techniques.

Animals

35 specific-pathogen-free cats, 6 months to 4 years old.

Procedure

Intraperitoneal or IV inoculation with blood containing H felis small form (Hfsm, 18 cats) or H felis large form (Hflg, 11 cats); 6 cats were uninfected controls. Hfsm was evaluated for capability to cross-protect against the more virulent Hflg. Morphology of both strains was compared by light microscopy of Wright-Giemsa-stained blood smears, and the 16S rRNA genes were sequenced.

Results

Infection with Hflg induced signs of depression, fever, and severe macrocytic normochromic anemia with nucleated erythrocytes. More than 95% of erythrocytes were parasitized. Inoculation with Hfsm and uninfected control blood induced mild or no clinical signs and no hematologic abnormalities. Anti-Hfelis lgG was first detected on postinoculation day (PID) 21, and increased to maximal titer of 400 by PID 28. Reactivated infection was observed in 8 of 29 cats (4 Hfsm and 4 Hflg), with 5% parasitized erythrocytes during the later attack. On PID 8, Hflg-inoculated cats had positive results of polymerase chain reaction analysis (PCR) that persisted until cats were treated with doxycycline or oxytetracycline; Hfsm-inoculated cats had positive PCR results that persisted for duration of observation (3 months).

Conclusions

Genetically and morphologically distinct strains of H felis infect cats in the field. The level of genetic difference suggested that these strains may be different species or genera.

Clinical Relevance

PCR is a critical diagnostic aid to detect occult Haemobartonella spp infection, as well as response to treatment and clearance of the organism. (Am J Vet Res 1998;59:1581-1588)

Abstract

Objective

To characterize 2 strains of Haemobartonella felis by use of molecular techniques.

Animals

35 specific-pathogen-free cats, 6 months to 4 years old.

Procedure

Intraperitoneal or IV inoculation with blood containing H felis small form (Hfsm, 18 cats) or H felis large form (Hflg, 11 cats); 6 cats were uninfected controls. Hfsm was evaluated for capability to cross-protect against the more virulent Hflg. Morphology of both strains was compared by light microscopy of Wright-Giemsa-stained blood smears, and the 16S rRNA genes were sequenced.

Results

Infection with Hflg induced signs of depression, fever, and severe macrocytic normochromic anemia with nucleated erythrocytes. More than 95% of erythrocytes were parasitized. Inoculation with Hfsm and uninfected control blood induced mild or no clinical signs and no hematologic abnormalities. Anti-Hfelis lgG was first detected on postinoculation day (PID) 21, and increased to maximal titer of 400 by PID 28. Reactivated infection was observed in 8 of 29 cats (4 Hfsm and 4 Hflg), with 5% parasitized erythrocytes during the later attack. On PID 8, Hflg-inoculated cats had positive results of polymerase chain reaction analysis (PCR) that persisted until cats were treated with doxycycline or oxytetracycline; Hfsm-inoculated cats had positive PCR results that persisted for duration of observation (3 months).

Conclusions

Genetically and morphologically distinct strains of H felis infect cats in the field. The level of genetic difference suggested that these strains may be different species or genera.

Clinical Relevance

PCR is a critical diagnostic aid to detect occult Haemobartonella spp infection, as well as response to treatment and clearance of the organism. (Am J Vet Res 1998;59:1581-1588)

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