Skip directly to site content Skip directly to page options Skip directly to A-Z link Skip directly to A-Z link Skip directly to A-Z link
Volume 12, Number 7—July 2006
Research

Epidemiologic and Molecular Analysis of Human Tularemia, United States, 1964–2004

Tables
Article Metrics
185
citations of this article
EID Journal Metrics on Scopus
Author affiliations: *Centers for Disease Control and Prevention, Fort Collins, Colorado, USA; †Centers for Disease Control and Prevention, Atlanta, Georgia, USA

Cite This Article

Abstract

Tularemia in the United States is caused by 2 subspecies of Francisella tularensis, subspecies tularensis (type A) and subspecies holarctica (type B). We compared clinical and demographic features of human tularemia cases from 1964 to 2004 from 39 states in which an isolate was recovered and subtyped. Our data indicate that type A and type B infections differ with respect to affected populations, anatomic site of isolation, and geographic distribution. Molecular subtyping with pulsed-field gel electrophoresis further defined 2 subpopulations of type A (type A-east and type A-west) that differ with respect to geographic distribution, disease outcome, and transmission. Our data suggest that type A-west infections are less severe than either type B or type A-east infections. Through a combined epidemiologic and molecular approach to human cases of tularemia, we provide new insights into the disease for future investigation.

Tularemia is a zoonotic disease caused by the gram-negative bacterium Francisella tularensis (1). Transmission occurs through arthropod bites (especially ticks and deerflies), ingestion of contaminated food or water, inhalation of contaminated aerosols, and handling of infected animal tissues. Human illness usually takes 1 of several clinical forms. The most common is ulceroglandular tularemia; more serious forms include pneumonic, typhoidal, and meningitic tularemia.

Nearly all human cases of tularemia in the United States are caused by F. tularensis subspecies tularensis (type A) or F. tularensis subspecies holarctica, (type B) (2). Type A and B isolates can be differentiated on the basis of glycerol fermentation, virulence in animal models, and by polymerase chain reaction (35). Recently, molecular assays have been developed to further discriminate within subspecies by using pulsed-field gel electrophoresis (PFGE), multiple-locus variable–number tandem repeat analysis (MLVA), whole-genome microarrays, and single nucleotide variations (69). In nature, the 2 subspecies are thought to be maintained in distinct but incompletely defined cycles (1012).

Although both subspecies of F. tularensis cause human illness (10), the clinical and epidemiologic features of type A and type B infections have not been systematically compared for a substantial number of cases. Furthermore, the implications of other subgroupings, as defined by molecular techniques, are largely unknown. We identified to subspecies level all human F. tularensis isolates that were submitted to the Centers for Disease Control and Prevention (CDC) for a 40-year period and further subtyped a portion by PFGE. Our findings demonstrate distinct subpopulations of F. tularensis that differ in their clinical manifestations, geographic location, and likely modes of transmission.

Methods

We analyzed all available F. tularensis isolates from humans (n = 316) recovered by or submitted to CDC by state and local health departments from 1964 through 2004. All work with F. tularensis cultures was performed in a biosafety level 3 (BSL-3) laboratory using BSL-3 safety precautions. Isolates were confirmed as F. tularensis by characteristic growth on agar and direct fluorescence antibody staining. Type A and type B isolates were differentiated by biochemical subtyping (glycerol fermentation) with the 96-well automated MicroLog MicroStation System with GN2 Microplates (Biolog Inc, Hayward, CA, USA) (13).

Demographic and clinical data on source patients were extracted from submission forms that accompanied the isolates. Extracted information included patient age and sex, date of disease onset, form of clinical disease, anatomic source of isolate, underlying illness, outcome, county where infected, and likely mode of transmission. Isolates received after 1990 (n = 155) were matched with patients reported through the National Electronic Telecommunication Surveillance System to extract county of exposure. Information was verified by contacting the reporting state health department.

PFGE subtyping was performed on a subset of isolates with a modified version of the PulseNet 1-day standardized protocol for subtyping foodborne pathogens (14,15). A total of 41 type A and 22 type B isolates were used. DNA-embedded agarose plugs were prepared and lysed under BSL-3 conditions. PFGE plugs were cut (2.0 mm) and digested with 40 U PmeI enzyme (New England Biolabs, Beverly, MA, USA) for 6 hours at 37°C under BSL-2 conditions. Salmonella enterica serotype Braenderup (H9812) was used as a reference standard, and DNA plugs were digested with 50 U XbaI enzyme (Roche Diagnostics, Indianapolis , IN, USA) for 3 hours at 37°C. Seakem agarose gels (1%) were prepared with 0.5× Tris-borate-EDTA buffer (Sigma, Saint Louis, MO, USA), and digested DNA plugs were loaded on the comb. Electrophoresis was performed with a CHEF Mapper (Bio-Rad, Hercules, CA, USA) with switch times of 1.79 to 10.71 s at 6V/cm for 17.5 h at 14°C. Gels were stained with ethidium bromide (1 mg/mL) and gel images captured by using a Gel Doc 1000 imager (Bio-Rad).

Analysis of PFGE gels was performed with BioNumerics software version 3.0 (Applied Maths BVBA, Sint-Martens-Latem, Belgium). Gels were normalized by using the Salmonella reference strain. A dendrogram was constructed with Dice similarity coefficients and unweighted pair group method with averages (UPGMA). Demographic and clinical data were analyzed with EpiInfo 2002 (CDC, Atlanta, GA, USA). To analyze categorical data and nonparametric tests for continuous data, χ2 was used.

Results

Figure 1

Figure 1. Geographic distribution for type A (red circles) and type B (yellow circles) Francisella tularensis isolates from humans, contiguous United States, 1964–2004. Each circle represents 1 isolate. Isolates were plotted randomly within...

A total of 316 F. tularensis isolates from 39 states were available for analysis; 208 (66%) were type A, and 108 (34%) were type B (Table 1). Among the 10 states submitting at least 10 isolates, the distribution of the 2 subspecies was nonrandom (χ2 = 34, p <0.0001). Overall, the 2 subspecies segregated into several geographically distinct clusters (Figure 1). Most isolates on the eastern seaboard, in and around Arkansas and Oklahoma, and in the broad area from the Colorado Rockies west to the Sierra Nevada Mountains were type A. In contrast, most isolates from the northern Pacific Coast and along tributaries of the Mississippi River were type B.

Figure 2

Figure 2. PmeI pulsed-field gel electrophoresis patterns for Francisella tularensis type A and type B. Lanes 1 and 8, Salmonella enterica serotype Braenderup standard; lane 2, Virginia 1997 type B; lane 3, Indiana...

To further understand this geographic clustering, we developed a PFGE subtyping method F. tularensis using PmeI. PFGE differentiated both between type A and B strains and among type A strains (Figure 2). Electrophoresis conditions were optimized to resolve restriction fragments between 25 kb and 125 kb for both F. tularensis and the Salmonella reference strain. Reproducibility testing verified that no differences in PFGE patterns were observed between experiments.

Figure 3

Figure 3. Dendrogram based on PmeI pulsed-field gel electrophoresis patterns of 41 Francisella tularensis type A and 22 type B isolates from humans. A 1.5% optimization and 1.5% tolerance were used to calculate...

Comparison of PFGE patterns for a subset of isolates (41 type A, 22 type B) from distinct locations (Figure 3) showed that all 22 type B isolates yielded the same PFGE pattern, which is consistent with previous data showing that type B strains exhibit little genetic diversity (7). In contrast, the type A isolates yielded PFGE patterns that fell into 2 main clusters (Figure 3; 32 type A-east, 9 type A-west). Isolates from 1 cluster came from states completely west of the 100th meridian (type A-west), while the remainder came from states transecting or east of the 100th meridian (type A-east, Figure 1). Based on the PFGE clustering, subsequent epidemiologic analysis was performed separately for type A isolates from the eastern (n = 133; type A-east) and western (n = 71; type A-west) contiguous United States.

Information on age and sex was known for 290 (92%) and 312 (99%) source patients, respectively. Males accounted for 75% (157/208) of type A and 72% (75/104) of type B infections. Patients with type A infections were significantly younger than patients with type B infections (median age 38 years vs. 50 years, p<0.01), and patients with type A-west infections were significantly younger than those with type A-east infections (median age 33 years vs. 44 years, p <0.02). An immunocompromising condition (e.g., malignancy, organ transplant, and HIV infection) was reported for 11 (10%) of 108 type B–infected patients, 6 (5%) of 133 type A-east–infected patients, and none (0%) of 68 type A-west–infected patients (p<0.01). For the 235 (74%) source patients for whom outcome was known, the overall case-fatality rate was 9% (20/235), with similar rates for infections caused by type A (9%, [15/161]) and type B (7%, 5/74) isolates. However, among type A infections, case-fatality rates differed markedly between type A-east (14% [15/106]) and type A-west (0% [0/55]) (p<0.002).

Information on anatomic source was available for 280 (89%) isolates. Overall, more than half of the isolates were recovered from lymph nodes and a quarter from blood (Table 2). While type A and type B isolates did not differ significantly with respect to anatomic source, significant differences were observed between type A-west and both type A-east (p<0.001) and type B (p<0.002) isolates. Type A-east and type B isolates were more likely than type A-west isolates to be recovered from blood and lung (Table 2), whereas type A-west isolates were more likely to be recovered from lymph nodes.

The clinical form of the disease was known for only 104 (33%) source patients. Ulceroglandular and glandular were the most commonly reported clinical forms of tularemia, accounting for 68 (65%) of 104 cases with information available. Other clinical syndromes included pneumonic (17%, 18/104), typhoidal (12%, 12/104), oculoglandular (4%, 4/104), meningitic (1%, 1/104) and pharyngeal (1%, 1/104) forms. Patients with typhoidal or pneumonic disease were generally older (median age 48 years and 53 years, respectively) than those with either glandular or ulceroglandular disease (median age 11 years and 37 years, respectively). Among the subset of patients for whom a clinical form of infection was reported, glandular or ulceroglandular disease was diagnosed more frequently in patients with type A infections (71% vs. 52% for type B) and pneumonic disease was diagnosed less frequently (12% vs. 30% for type B).

Figure 4

Figure 4. Seasonal distribution of type A and type B Francisella tularensis isolates from humans, United States, 1964–2004.

Among 292 source patients whose date of disease onset was known, 210 (72%) were infected in May through September; no difference in onset between type A and B infections was noted (Figure 4). A possible source of infections was reported for 133 (42%) of 316 patients. Direct animal contact accounted for 47 (47%) of 99 type A and 18 (53%) of 34 type B infections. Most type A infections were associated with exposure to either lagomorphs (53%, 25/47) or cats (30%, 14/47). Type B infections were most often associated with exposure to rodents (33%, 6/18) or cats (22%, 4/18); none were linked to lagomorph exposure. Arthropod bites accounted for 44 (44%) type A infections and 10 (29%) type B infections. Although the arthropod involved was not always identified, ticks were reported as the source for 21 (100%) of 21 type A-east, 9 (100%) of 9 type B, and 4 (44%) of 9 type A-west infections. Biting flies were only linked to type A-west infections and accounted for 5 (55%) of 9 type A-west infections attributed to a known arthropod bite. The remaining 8 (8%) type A and 6 (18%) type B infections were in patients with both animal and arthropod exposure or were attributed to environmental exposures such as landscaping.

Discussion

Categorization of F. tularensis type A and type B was first proposed by Olsufiev et al. in 1959 (16). These 2 subspecies have been suggested to differ in their ecology and possibly their virulence for humans (17). Our study, which includes isolates obtained during a 40-year period, further refines these views. By combining PFGE subtyping of isolates with geographic data, we found evidence that human type A infections can be further divided into at least 2 distinct subgroups (type A-east and type A-west). In addition, our data suggest that type A-west infections are less severe than type B or type A-east infections.

The most notable finding of this investigation concerns fatality rates. The case-fatality rate for type A-east infections was 14%, compared with 7% for type B infections and 0% for type A-west infections. Type A-east and type B isolates were more likely to have been recovered from patients' lungs or blood, whereas type A-west isolates were more often isolated from lymph nodes. The apparent reduced invasiveness of type A-west strains may be explained by the younger age of the patients infected. However, a review of the literature shows that few, if any, tularemia deaths have been reported in the Rocky Mountain region (1821), regardless of patient age. We hypothesize that the milder form of clinical disease associated with type A-west may be due to differences in virulence factors or perhaps infectious doses associated with differing modes of transmission.

Infections caused by type A-west, type A-east, and type B appear to occur in distinct geographic foci, suggestive of different ecologic niches. Type B infections cluster along major waterways, such as the upper Mississippi River, and in areas with high rainfall, such as coastal areas of the Pacific Northwest. Type A-west infections predominate in the arid region from the Rocky Mountains west to the Sierra Nevada Mountains. Type A-east infections occur in 2 main areas: 1) the central southeast states of Arkansas, Missouri, and Oklahoma and 2) along the Atlantic Coast, east of the Appalachians. The central southeast region is a major focus of human tularemia, accounting for 50% of all reported cases in the United States (22). The type A-east infections along the Atlantic Coast may be linked to the importation of rabbits from Arkansas, Oklahoma, Missouri, and Kansas to hunting clubs in Massachusetts, Pennsylvania, New Jersey, and Maryland in the 1920s and 1930s (17,23). Whether the geographic demarcation of type A-west and type A-east adheres strictly with the 100th meridian will require further PFGE analysis of more type A strains.

Animal studies have indicated that type A isolates are often associated with lagomorphs (rabbits and hares), while type B isolates are more often obtained from rodents (12,17). Consistent with these findings, our results show that human type A-east and type A-west infections were associated with exposure to lagomorphs, whereas human type B infections were associated with exposure to rodents. Both type A and type B infections were associated with exposure to cats. Ticks were implicated in transmission of both type A-east and type B infections to humans, whereas biting flies were only implicated in transmission of type A-west infections. The restriction of deerflies (Chrysops spp.) and associated human cases to western states was previously noted by Jellison (24).

This study is subject to several limitations, including record completeness, ascertainment bias, and number of F. tularensis isolates PFGE subtyped. Subspecies differentiation for F. tularensis has historically been dependent on the recovery of an isolate, and subtype information is not captured in the national disease reporting system. The overall case-fatality rate in this study was 9%, which is severalfold higher than the <2% previously reported (25). The higher rate suggests enhanced ascertainment of fatal cases. In addition, 36% of type A-east and 25% of type B isolates were recovered from blood, a much higher rate than previously reported. By analyzing only patients with culture-confirmed infections, we may have selected for patients with more fulminant disease.

Our results demonstrate that PmeI PFGE subtyping is useful for dividing type A isolates into geographically and clinically meaningful subgroups. Nineteen type A isolates analyzed by PFGE in this study (12 type A-east, 7 type A-west) were previously analyzed by MLVA and divided into 2 subpopulations, A.I and A.II (26). Subpopulations independently identified by the 2 methods are in complete agreement, which suggests that type A-west is analogous to A.II and type A-east is analogous to A.I. With training and interlaboratory validation, the PFGE method described here could be adopted by PulseNet laboratories throughout the country that use the standardized PulseNet PFGE protocol for foodborne pathogens (27). The PulseNet network is an existing laboratory infrastructure with all of the necessary equipment and software to perform, normalize, and compare PFGE patterns. PFGE subtyping of F. tularensis isolates would allow states to determine the potential geographic origins of tularemia cases and also share and compare their PFGE patterns within the PulseNet network.

Although type A is often referred to as the more virulent subspecies of F. tularensis and of greatest concern with respect to bioterrorism, our comparative analysis suggests that this view should be reevaluated. We found that human type A-west infections are markedly less severe than type B infections. Further studies are warranted to determine the basis of the clinical, geographic, and ecologic differences between infections caused by type B, type A-west, and type A-east.

Dr Staples served as an Epidemic Intelligence Service officer in the Bacterial Zoonoses Branch, Division of Vector-Borne Infectious Diseases, National Center for Infectious Diseases, CDC, Fort Collins , Colorado, from 2003 to 2005. She is currently a pediatric infectious disease fellow at Duke University Medical Center in Durham, North Carolina.

Top

Acknowledgment

We thank all the persons at state and local health departments who aided in obtaining isolates and clarifying information related to the isolates. We also thank Leon Carter, Kiersten Kugeler, Sandy Urich, and Brook Yockey for their assistance in growing F. tularensis isolates and data extraction and the Special Bacteriology Reference Laboratory, Meningitis and Special Pathogens Branch, CDC, for sharing their archived F. tularensis isolates.

Top

References

  1. Ellis  J, Oyston  CF, Green  M, Titball  RW. Tularemia. Clin Microbiol Rev. 2002;15:63146. DOIPubMedGoogle Scholar
  2. Petersen  JM, Schriefer  ME. Tularemia: emergence/re-emergence. Vet Res. 2005;36:45567. DOIPubMedGoogle Scholar
  3. Olsufiev  NG, Meshcheryakova  IS. Infraspecific taxonomy of tularemia agent Francisella tularensis McCoy et Chapin. J Hyg Epidemiol Microbiol Immunol. 1982;26:2919.PubMedGoogle Scholar
  4. Jellison  WL, Owen  C, Bell  JF, Kohls  GM. Tularemia and animal populations: ecology and epizootiology. Wildl Dis. 1961;17:122.
  5. Johansson  A, Ibrahim  A, Goransson  I, Eriksson  U, Gurycova  D, Clarridge  JE III, Evaluation of PCR-based methods for discrimination of Francisella species and subspecies and development of a specific PCR that distinguishes the two major subspecies of Francisella tularensis. J Clin Microbiol. 2000;38:41805.PubMedGoogle Scholar
  6. Garcia Del Blanco  N, Dobson  ME, Vela  AI, De La Puente  VA, Gutierrez  CB, Hadfield  TL, Genotyping of Francisella tularensis strains by pulsed-field gel electrophoresis, amplified fragment length polymorphism fingerprinting, and 16S rRNA gene sequencing. J Clin Microbiol. 2002;40:296472. DOIPubMedGoogle Scholar
  7. Johansson  A, Farlow  J, Larsson  P, Dukerich  M, Chambers  E, Bystrom  M, Worldwide genetic relationships among Francisella tularensis isolates determined by multiple-locus variable-number tandem repeat analysis. J Bacteriol. 2004;186:580818. DOIPubMedGoogle Scholar
  8. Samrakandi  MM, Zhang  C, Zhang  M, Nietfeldt  J, Kim  J, Iwen  PC. Genome diversity among regional populations of Francisella tularensis subspecies tularensis and Francisella tularensis subspecies holarctica isolated from the US. FEMS Microbiol Lett. 2004;237:917. DOIPubMedGoogle Scholar
  9. Svensson  K, Larsson  P, Johansson  D, Bystrom  M, Forsman  M, Johansson  A. Evolution of subpecies of Francisella tularensis. J Bacteriol. 2005;187:39038. DOIPubMedGoogle Scholar
  10. Jellison  WL. Tularemia in Montana. Mont Wildl. 1971;:524.PubMedGoogle Scholar
  11. Bell  JF. Tularemia—a review. CRC handbook series in zoonoses. Boca Raton (FL): CRC Press; 1977. Section A, p. 161.
  12. Hopla  CE, Hopla  AK. Tularemia. In: Beran GW, Steele JH, editors. Handbook of zoonoses. 2nd ed. Boca Raton (FL): CRC Press, Inc.; 1994. p. 113–26.
  13. Petersen  JM, Schriefer  M, Carter  LG, Zhou  Y, Sealy  T, Bawiec  D, Laboratory analysis of tularemia in wild trapped, commercially distributed prairie dogs, Texas, 2002. Emerg Infect Dis. 2004;10:41925.PubMedGoogle Scholar
  14. Ribot  EM, Fair  M, Gautom  R, Cameron  DN, Hunter  SB, Swaminathan  B, Standardization of pulsed-field gel electrophoresis protocols for the subtyping of Escherichia coli O157:H7, Salmonella, and Shigella for PulseNet. Foodborne Pathog Dis. 2006;3:5967. DOIPubMedGoogle Scholar
  15. Kubota  K, Barrett  TJ, Ackers  ML, Brachman  PS, Mintz  ED. Analysis of Salmonella serotype Typhi pulsed-field gel electrophoresis patterns associated with international travel. J Clin Microbiol. 2005;43:12059. DOIPubMedGoogle Scholar
  16. Olsufiev  NG, Emelyanova  OS, Dunaeva  TN. Comparative study of strains of B. tularense in the Old and New World and their taxonomy. J Hyg Epidemiol Microbiol Immunol. 1959;3:13849.PubMedGoogle Scholar
  17. Jellison  W. Tularemia in North America, 1930–1974. Missoula (MT): University of Montana; 1974.
  18. Geiger  JC, Meyer  KF. Tularemia in Nevada. California and Western Medicine. 1929;31:14.PubMedGoogle Scholar
  19. Lane  R. Ecological and epidemiological studies of tularemia in California. California Vector Views. 1977;24:3949.
  20. Hillman  CC, Morgan  MT. Tularemia: report of a fulminant epidemic transmitted by the deer fly. JAMA. 1937;108:53840. DOIGoogle Scholar
  21. Klock  LE, Olsen  PF, Fukushima  T. Tularemia epidemic associated with the deerfly. JAMA. 1973;226:14952. DOIPubMedGoogle Scholar
  22. Centers for Disease Control and Prevention. Tularemia—United States, 1990–2000. MMWR Morb Mortal Wkly Rep. 2002;51:1824.
  23. Belding  DL, Merrill  B. Tularemia in imported rabbits in Massachusetts. N Engl J Med. 1941;224:10857. DOIGoogle Scholar
  24. Jellison  W. Tularemia: geographic distribution of "deerfly fever" and the biting fly, Chrysops discalis Williston. Public Health Rep. 1950;65:14952. DOIGoogle Scholar
  25. Dennis  DT, Inglesby  TV, Henderson  DA, Bartlett  JG, Ascher  MS, Eitzen  E, Tularemia as a biological weapon: medical and public health management. JAMA. 2001;285:276373. DOIPubMedGoogle Scholar
  26. Farlow  J, Wagner  DM, Dukerich  M, Stanley  M, Chu  M, Kubota  K, Francisella tularensis in the United States. Emerg Infect Dis. 2005;11:183541.PubMedGoogle Scholar
  27. Swaminathan  B, Barrett  TJ, Hunter  SB, Tauxe  RV. CDC PulseNet Task Force. PulseNet: The molecular subtyping network for foodborne bacterial disease surveillance, United States. Emerg Infect Dis. 2001;7:3829.PubMedGoogle Scholar

Top

Figures
Tables

Top

Cite This Article

DOI: 10.3201/eid1207.051504

1These authors contributed equally to this article.

Table of Contents – Volume 12, Number 7—July 2006

EID Search Options
presentation_01 Advanced Article Search – Search articles by author and/or keyword.
presentation_01 Articles by Country Search – Search articles by the topic country.
presentation_01 Article Type Search – Search articles by article type and issue.

Top

Comments

Please use the form below to submit correspondence to the authors or contact them at the following address:

Jeannine M. Petersen, Centers for Disease Control and Prevention, Division of Vector-borne Infectious Diseases, Bacterial Zoonoses Branch, PO Box 2087, Fort Collins, CO 80522, USA

Send To

10000 character(s) remaining.

Top

Page created: December 16, 2011
Page updated: December 16, 2011
Page reviewed: December 16, 2011
The conclusions, findings, and opinions expressed by authors contributing to this journal do not necessarily reflect the official position of the U.S. Department of Health and Human Services, the Public Health Service, the Centers for Disease Control and Prevention, or the authors' affiliated institutions. Use of trade names is for identification only and does not imply endorsement by any of the groups named above.
file_external