Emerg Infect DisEmerging Infect. DisEIDEmerging Infectious Diseases1080-60401080-6059Centers for Disease Control and Prevention26583204467243415-050110.3201/eid2112.150501ResearchResearchZoonotic Leprosy in the Southeastern United StatesZoonotic Leprosy in the Southeastern United StatesZoonotic Leprosy in the Southeastern United
StatesSharmaRahulSinghPushpendraLoughryW.J.LockhartJ. MitchellInmanW. BarryDuthieMalcolm S.PenaMaria T.MarcosLuis A.ScollardDavid M.ColeStewart T.TrumanRichard W.National Hansen’s Disease Program, Baton Rouge, Louisiana, USA (R.
Sharma, P. Singh, M.T. Pena, D.M. Scollard, R.W. Truman); Louisiana State University School of Veterinary Medicine, Baton Rouge (R.
Sharma, P. Singh, M.T. Pena); Ecole Polytechnique Federale de Lausanne, Lausanne, Switzerland (P.
Singh, S.T. Cole); Valdosta State University, Valdosta, Georgia, USA (W.J. Loughry, J.M.
Lockhart); Florida Department of Health, Merritt Island, Florida, USA (W.B. Inman); Infectious Disease Research Institute, Seattle, Washington, USA (M.S.
Duthie); Hattiesburg Clinic, Hattiesburg, Mississippi, USA (L.A. Marcos)Address for correspondence: Richard W. Truman, National
Hansen’s Disease Program Laboratory Research Branch, LSU-SVM Skip Bertman Dr,
Baton Rouge, LA 70803, USA; email: rtruman@hrsa.gov122015211221272134
The geographic range and complexity of this disease are increasing.
Nine-banded armadillos (Dasypus novemcinctus) are naturally infected
with Mycobacterium leprae and have been implicated in zoonotic
transmission of leprosy. Early studies found this disease mainly in Texas and
Louisiana, but armadillos in the southeastern United States appeared to be free of
infection. We screened 645 armadillos from 8 locations in the southeastern United
States not known to harbor enzootic leprosy for M. leprae DNA and
antibodies. We found M. leprae–infected armadillos at each
location, and 106 (16.4%) animals had serologic/PCR evidence of infection. Using
single-nucleotide polymorphism variable number tandem repeat genotyping/genome
sequencing, we detected M. leprae genotype 3I-2-v1 among 35
armadillos. Seven armadillos harbored a newly identified genotype (3I-2-v15). In
comparison, 52 human patients from the same region were infected with 31 M.
leprae types. However, 42.3% (22/52) of patients were infected with 1 of
the 2 M. leprae genotype strains associated with armadillos. The
geographic range and complexity of zoonotic leprosy is expanding.
Keywords: leprosyzoonotic leprosyHansen’s diseaseHansen diseaseMycobacterium lepraebacteriaarmadillosnine-banded armadilloDasypus novemcinctuszoonosesepidemiologybiomarkersgenotypesoutheastern United States
Leprosy (Hansen disease), a chronic infectious disease caused by Mycobacterium
leprae, primarily affects the peripheral nervous system and involves skin and
other tissues (1). Although this
disease is generally a rare disorder that occurs mainly in tropical and semitropical areas,
the World Health Organization recorded 219,075 new leprosy cases globally in 2011, and
439,670 new cases were reported in the Western Hemisphere over the past decade (2,3). Although leprosy is curable by antimicrobial drug
therapy, the treatment interval for this disease can require >2
years to complete, and underlying nerve damage caused by the infection might be
irreversible. There are no established laboratory screening tests to detect leprosy; the
disease must be diagnosed clinically. Therefore, physician awareness about leprosy and
knowledge of populations potentially at risk for the infection, are paramount for early
detection and treatment (1).
Leprosy was not present in the New World during pre-Columbian times and appears to have
been introduced to the Western Hemisphere after colonization. Early case reports suggest
the disease was well established in most countries surrounding the Gulf of Mexico by the
1750s (4,5). Genomic polymorphisms enable us to trace the spread
of the disease worldwide and confirm the regional origins of most isolates (6). The disease is rare in the United
States; only ≈13,000 cases have been recorded since the 1890s, and ≈200 new
cases are reported each year. Most of these case-patients lived or worked outside the
country in disease-endemic areas and might have acquired their disease abroad (7). However, approximately one third of
all case-patients in the United States report no foreign residence history or known contact
with another person who had leprosy. Therefore, they probably acquired the disease from
local sources (1).
Leprosy is believed to be transmitted mainly from person to person through infectious
aerosols or direct contact (1).
However, there is a strong genetic component with regards to susceptibility to infection,
and 95% of all persons appear to be naturally resistant to leprosy (8). M. leprae is an obligate
intracellular parasite that can survive for only short periods unprotected in the natural
environment (9), and few animals
support experimental infection with this bacterium (10). The only known nonhuman reservoir of M.
leprae is the nine-banded armadillo (Dasypus novemcinctus),
and disease prevalence rates among armadillos may exceed 20% in some locales (11).
Armadillos are highly susceptible to M. leprae and can manifest massive
burdens of bacilli in their tissues (1010–11 organisms/g). This sylvatic
infection was first detected in 1975 but is known to have occurred among armadillos for
many decades before that time (12–14). Early surveys in the United States suggested that leprosy
was restricted mainly to armadillos in Texas and Louisiana. No evidence for infection was
found among armadillos in Florida, Georgia, and Alabama (12,14,15).
However, in recent times, the geographic range of the infection seems to be expanding
(16).
We recently showed that armadillos over a 4-state area in the southern United States were
infected with a single predominant M. leprae genotype strain (3I-2-v1),
and we recovered this same strain from a large number of persons with leprosy in these same
states. Leprosy is probably a zoonosis in the southern United States (17). Armadillos are common throughout the southern
United States, and their geographic range extends through Latin America to northern
Argentina (18). To better
understand the geographic range of M. leprae–infected armadillos
and the role that these animals might play in perpetuating leprosy, we surveyed armadillos
for M. leprae and compared genoypes of M. leprae isolated
from these animals with those from biopsy samples obtained from patients with leprosy in
the southeastern United States.
Materials and MethodsStudy Design
In an ecologic cohort study, we surveyed armadillos and patients in the southeastern
United States for M. leprae and genotyped isolated bacilli. Patient
samples were obtained from excess diagnostic materials after a category 4 exemption
was granted by the institutional review board of Louisiana State University (Baton
Rouge, LA, USA). Interviews with some patients were conducted by the Florida
Department of Health, and some patients in Mississippi were interviewed according to
a protocol approved by the institutional review board at Forrest General Hospital
(Hattiesburg, MS, USA). Armadillos were collected according to established protocols
approved by the Institutional Animal Care and Use Committee at the Valdosta State
University (Valdosta, GA, USA) and the University of Georgia (Athens, GA, USA).
Collection of Samples from Wild Armadillos
Blood and reticuloendothelial tissue samples were collected from 645 armadillos at 8
locations in state and federal Wildlife Management Areas, Forests, and Refuges in
Mississippi, Alabama, Georgia, and Florida during 2003–2012 (Figure 1). Armadillo serum or whole blood samples
were dried on filter paper (Nobuto strips; Advantec, Dublin, CA, USA), and tissue
samples were frozen or fixed in 70% ethanol. These specimens were shipped to the
National Hansen’s Disease Program (Baton Rouge, LA, USA) for testing. In
addition, we reexamined 55 frozen serum samples from armadillos collected in Florida
during 1983–1988 (11).
Eight locations in 4 states in the southeastern United States where armadillos
were sampled and tested for infection with Mycobacterium
leprae. Inset (shaded region) indicates location of the 4 states.
DSO, DeSoto National Forest, Mississippi; CON, Conecuh National Forest,
Alabama; PBH, Pebble Hill Plantation, Thomasville, Georgia; PNB, Pinebloom
Plantation, Albany, Georgia; VAL, Valdosta, Georgia; TLT, Tall Timbers Research
Station and Land Conservancy, Tallahassee, Florida; CMB, Camp Blanding,
Florida; MRI, Merritt Island National Wildlife Refuge, Florida.
Biomarkers for <italic>M. leprae</italic> Infection
Serologic and molecular assays were used to identify armadillos infected with
M. leprae. Serum samples were tested for IgM against phenolic
glycolipid-1 (PGL1) antigen of M. leprae (BEI Resources, Manassas,
VA, USA) and for leprosy IDRI diagnostic-1 (LID1) antigen (Infectious Disease
Research Institute, Seattle, WA, USA) by using an ELISA as described (19). Positive results were
determined according to optical density and by using limits described for the PGL1
assay (13,19). Interpretations for the
LID1 ELISA were derived by inspecting the rank-ordered distribution of optical
densities for deflection from linearity, and arbitrarily assigning a value limit. DNA
was extracted from lymph nodes or spleens of animals seropositive by ELISA by using
the DNA Easy Kit (QIAGEN, Valencia, CA, USA) and screened by using a PCR with primers
specific for regions of the M. leprae multicopy repeat sequence and
the heat shock protein gene encoding the 18-kD antigen as described (20). Amplicons were confirmed by
sequencing.
Patient Samples
Skin biopsy specimens collected from patients attending the National Hansen’s
Disease Program outpatient clinic or referred for diagnosis were stored frozen in
optimum cutting-temperature compound or archived as formalin-fixed, paraffin-embedded
blocks and occasionally fixed in 70% ethanol. To assess M. leprae
genotype strains in the region, we used 52 biopsy specimens from cases-patients with
leprosy during 2007–2012. Samples consisted of 47 fixed in formalin and
embedded in paraffin, 4 fixed in ethanol, and 1 frozen.
Genotyping of <italic>M. leprae</italic> from Armadillos and Patients
We genotyped M. leprae isolated from 52 patients and selected
armadillo samples, and assigned their phylogenetic affiliation by using an algorithm
associating 16 major single-nucleotide polymorphisms (SNPs) as described (6,17) (Figure 2).
Because SNP-type 3I predominates in North America, we first sequenced SNP7614 and
insertion/deletion_17915. Samples with a single copy of insertion/deletion_17915 and
a T at SNP7614 were confirmed as 3I and further discriminated as 3I-1 or 3I-2 on the
basis of SNP-1527056. Non-3I isolates were typed for SNPS as described (6,17).
Genotyping scheme for Mycobacterium leprae determined by using
single-nucleotide polymorphisms (SNPs) and variable number tandem repeat (VNTR)
polymorphisms, southeastern United States. Shading indicates the base that
differentiates SNP type and subtype of M. leprae. The
algorithm used for strain typing of M. leprae is based on
specific SNP location and type and VNTR copy number at the various locations
identified along the chromosome. After identification of the major SNP subtype,
M. leprae is further discriminated by using allele numbers
at 10 VNTR loci. INS, insertion; DEL, deletion.
To enhance discrimination of isolates with an identical SNP type, we determined the
copy number of 10 variable number tandem repeats (VNTRs) in a lineage dependent
manner as described (17).
Multiplex nested PCR amplified all 10 VNTR loci, and these loci were used as a
template for individual assessments (Technical
Appendix Table 1). VNTRs <5 bp were sequenced to determine copy number,
and those >5 bp were determined by fragment analysis. A representative number of
amplicons were sequenced to confirm the fragment size (Genelab, Louisiana State
University School of Veterinary Medicine, Baton Rouge, LA, USA). The array of
genotypes determined for patient and armadillo isolates was plotted by using minimum
spanning tree analysis in BioNumerics 7.1 software (Applied Maths NV, Sint-Latem,
Belgium) in a lineage-dependent manner. VNTR further discriminated the SNP lineage
(Figure 3).
Minimum spanning tree constructed by using single-nucleotide polymorphism (SNP)
and variable number tandem repeat (VNTR) polymorphism profiles for
Mycobacterium leprae samples from patients and armadillos
from the southeastern United States. Each circle represents a single strain
genotype of M. leprae. Large circles indicate that >1
sample (number shown) had a common genotype. Values along lines indicate number
of differences between allelic profiles. Human and armadillo samples of common
SNP subtype 3I-2 are indicated by different colors. Only 2 genotypes were
present in >1 sample, and both genotypes were present among armadillos and
patients.
Genome Sequencing
The M. leprae genome sequences from 4 armadillos harboring the
3I-2-v15 genotype were obtained by fragment library sequencing by using the Ion
Proton System Libraries Kit (Life Technologies, Grand Island, NY, USA). DNA quality
and integrity were validated by using the Agilent 2000 Bioanalyzer (Agilent
Technologies, Santa Clara, CA, USA) and sequenced with an Ion PI Chip Kit v2 (Life
Technologies). The sequence data were compared with the published genome of the
M. leprae TN reference standard (21), and variant calls were generated by using Partek
4.0 software (Partek, St. Louis, MO, USA). Variants with frequency >90%, and a
minimum 10× coverage were compared with 3I-specific variants of the
armadillo-associated M. leprae genotype strain 3I-2-v1 (Technical Appendix Table 2) (17). The 13 unique variants that
differentiated 3I-2-v15 from 3I-2-v1 were confirmed by direct sequencing of
additional human (n = 10) and armadillo (n = 15) isolates of both strain types
(primer sequences Technical Appendix
Table 3).
ResultsExpanded Geographic Range of <italic>M. leprae</italic> Infection among
Armadillos
We screened blood and tissue samples to determine the prevalence of M.
leprae infection among 645 armadillos obtained at 8 locations in the
southeastern United States (Mississippi, Alabama, Georgia, and Florida) (Figure 1). We detected antibodies to M.
leprae−specific antigens at each location and in 16.4% (106/645)
of all the samples screened: 10.1% (65/645) had antibodies to PGL1, and 9.9% (64/645)
had antibodies to LID1. Only 23 samples showed positive results in both assays. These
samples included LID1 antigen−enhanced serologic detection of infection versus
screening with PGL1 alone (Table 1).
Serologic and molecular detection of <italic>Mycobacterium leprae</italic>
infections among armadillos from various locations in the southeastern United
States*
Location
No. blood or serum
samples
Serologic screening,
no. samples positive for M. leprae antigen
No. lymph node samples
tested
PCR, no. samples
positive for M. leprae DNA
LID1
PGL1
LID1 or PGL1
LID1 and PGL1
RLEP locus
hsp 18 locus
1 site
2 sites
CMB
31
2
2
2
2
2
2
0
2
0
VAL
8
1
0
1
0
0
0
0
0
0
MRI
65
9
16
18
7
17
16
14
17
13
CON
38
5
2
7
0
5
5
2
5
2
DSO
23
7
0
7
0
7
6
3
7
3
PNB
117
11
13
20
4
19
19
19
19
19
PBH
23
5
1
6
0
3
3
2
3
2
TLT
340
24
31
45
10
42
41
36
42
36
Total
645
64
65
106
23
95
92
76
95
75
*LID, leprosy IDRI diagnostic 1 antigen; PGL, phenolic glycolipid 1 antigen;
RLEP, mutlicopy repeat sequence; hsp, heat shock protein; CMB,
Camp Blanding, FL; VLD: Valdosta, GA; MRI, Merritt Island National Wildlife
Refuge, FL; CON, Conecuh National Forest, AL; DSO, DeSoto National Forest, MS;
PNB, Pinebloom Plantation, Albany, GA; PBH, Pebble Hill Plantation, Thomasville
GA; TLT, Tall Timbers Research Station and Land Conservancy, Tallahassee,
FL.
M. leprae was not found among armadillos in this region before 2009
(11,16). Two of the areas surveyed (Tall Timbers
Research Station and Land Conservancy, Tallahassee, Florida, and Pinebloom
Plantation, Albany, Georgia) also had been sampled in earlier studies (14). In addition, we examined 55
serum samples collected from armadillos in nearby regions of Florida. These samples
had been stored frozen since 1983–1988 (11). Rescreening these samples by using the current
PGL1 and LID1 ELISAs, we again found no serologic reactivity, which confirmed the
earlier findings.
Lymph node tissues were available from 95 of the 106 animals considered serologically
positive by either ELISA. DNA was extracted from tissues and tested by PCR for
M. leprae−specific multicopy repeat sequence and heat
shock protein 18 gene fragments. All 95 samples amplified in
>1 M. leprae−specific PCR, and
75/95 (80%) amplified with both PCRs (Table
1). Amplicon sequencing confirmed specificity for M.
leprae.
<italic>M. leprae</italic> Isolated from Armadillos and Patients
Sufficient DNA was available to genotype the M. leprae recovered
from 42/95 armadillos and from the biopsy samples of 52 patients who had leprosy in
the same geographic region. Among armadillos, only 2 M. leprae
genotype strains were recovered. We found 35/42 (83%) of the animals harbored
M. leprae SNP-VNTR type 3I-2-v1, which we had identified as
infecting patients and armadillos in Texas, Louisiana, Mississippi, and Arkansas
(17). Therefore, type
3I-2-v1 can be found among armadillos in Mississippi, Alabama, Georgia, and northern
Florida. However, in southern Florida, we found 7 armadillos infected with an
M. leprae genotype strain not previously observed among
armadillos. Designated 3I-2-v15, this new armadillo-associated genotype strain
differed from 3I-2-v1 by having multiple allele changes at 3 VNTR loci. The 3I-2-v15
allele profile was unique and had not been previously identified in a global database
of M. leprae VNTR strain types (22). According to allele frequencies derived from that
database, the 3I-2-v15 genotype had only a 1:3,700 probability for random
recombination within any of these 7 samples. Subsequent deep sequencing of 3I-2-v15
isolates from 4 armadillos showed that this genotype was uniform and consistent among
all animals examined and had multiple SNP differences between 3I-2-v15 and 3I-2-v1
M. leprae. Four SNPs common among 3I-2-v1 isolates were not
present in 3I-2-v15, and 9 additional common SNPs were unique to 3I-2-v15 (Table 2). These same 13 polymorphisms were
confirmed by direct PCR of M. leprae from an additional 10 human and
15 armadillo isolates. 3I-2-v15 is the most diverse representative of the 3I-2
lineage sequenced to date.
Next-generation whole-genome sequencing of <italic>Mycobacterium
leprae</italic> strain 3I-2-v15 derived from wild armadillos from the
southeastern United States compared with that for armadillo-associated strain
3I-2-v1
Sample no.
Average coverage (%
genome covered)*
No. variants partially
shared†
No. variants only in
3I-2-v15‡
No. 3I-2 variants
absent in 3I-2-v15‡
No. variants in both
strains
No. TN strain variants
in both strains
US-36
19.8 (88.72)
7
9
4
20
37
US-95
97.99 (98.36)
1
9
4
14
37
FL-26
119.32 (99.00)
0
9
4
13
37
MRI-9
25.3 (92.08)
6
9
4
19
37
*Average no. of consensus sequence reads obtained from the particular specimen
covering the entire genome. †No. variants reported to be specific
for single-nucleotide polymorphism (SNP) type 3I-2 that are present in all
samples of the 3I-2-v1 genotype and that were found in some, but not all,
samples of the 3I-2-v15 genotype. ‡Resequencing referenced the M.
leprae TN standard genomic sequence, identified 13 variants present only in
3I-2-v1 (2 SNP, 2 insertion/deletions) or 3I-2-v15 (9 SNP), and differentiated
the strains.
Patient Samples
In contrast to SNP-VNTR analysis of M. leprae from armadillos,
analysis of M. leprae from patient biopsy specimens discriminated
multiple M. leprae genotypes. The 3I-2 lineage, which predominates
in North America (17), was
most common and found in 41 samples. The other samples had genotypes found more
commonly in other parts of the world; 9 were 3K, and 1 each were 3J or 3M lineages
(6). SNP-VNTR genotyping
showed that 30 patients were infected with entirely unique M. leprae
genotypes. However, 22 patients, as well as armadillos, had identical M.
leprae genotypes: 12 patient biopsy samples harbored M.
leprae type 3I-2-v1, and 10 samples harbored newly identified type
3I-2-v15. In this study, only the 2 M. leprae genotype strain types
recovered from armadillos were present in >1 patient. Overall, 42% (22/52) of the
patients were infected with M. leprae genotypes that were found
associated with armadillos (Figure 3). All
patients harboring type 3I-2-v1 had residence histories in areas of the southern
United States where they may have been exposed to M. leprae through
armadillos. All 10 patients infected with 3I-2-v15 resided and consulted physicians
in southern Florida, the only region where armadillos with this same M.
leprae genotype strain type also had been found.
None of the patients in this study reported any previous contact with another person
who had leprosy. In separate studies, small groups of patients in Florida and
Mississippi were interviewed about their medical history and exposure to armadillos.
Only 4 of the patients in Florida interviewed could be fully typed: 3 had M.
leprae 3I-2-v15 and 1 had 3I-2-v1. In Mississippi, all 4 patients were
infected with 3I-2-v1. None of the patients interviewed in Mississippi or Florida
recalled direct contact with armadillos. All patients were familiar with armadillos
in their environment, and many reported gardening and other outdoor activities that
might have provided some exposure to environments possibly contaminated by M.
leprae from armadillos.
In this study, patients with no foreign residence history had 16 times greater odds
of being infected with 1 of the 2 armadillo-associated M. leprae
genotype strain types than with any other type of M. leprae (odds
ratio 16.8, 95% CI 3.881–73.374, p<0.0001). Patients with residence
histories in areas where they may have been exposed to M. leprae
from armadillos also had 41 times greater odds of being infected with 1 of the 2
armadillo-associated types than with any other M. leprae genotype
(odds ratio 41.3, 95% CI 2.297–742.68, p<0.0001). Although leprosy
has not previously been recognized among armadillos in Florida, 16% of the animals
that we studied in the region harbored M. leprae, and 22/52 patients
that we examined also were found to be infected with 1 of the same 2 M.
leprae genotype strain types that we recovered from armadillos in the
region.
Discussion
Leprosy appears to be an emerging infection of armadillos throughout the southeastern
United States. Most armadillos are infected with a single predominant M.
leprae strain type (3I-2-v1), which has been associated with probable
zoonotic transmission of leprosy to humans (17). However, armadillos in southern Florida, as well as
several patients from that region, are infected with a distinctly different M.
leprae genotype strain (3I-2-v15). Armadillos must have acquired M.
leprae from humans within the past 400 years, after the disease was
introduced into the Western Hemisphere. The 3I-2-v15 strain type was not used for in
vivo propagation of M. leprae in armadillos. With its multiple genomic
polymorphisms, this train type does not appear to have evolved recently from the 3I-2-v1
strain type. Armadillos must have acquired these infections from humans who originally
harbored the strains in the region, and M. leprae appears to have been
naturally transferred to armadillos on >1 occasion and in >1 location.
Interspecies transfer of M. leprae between humans and armadillos
appears to be rare and inefficient. However, emergence of the infection among armadillos
in southeastern states, which were previously believed to be free of M.
leprae, suggests that the disease will eventually be detected among animals
throughout North America, and additional M. leprae genotype strains
might also be acquired by animals in other locations over time.
Three epidemiologic case studies in the United States (23–25) and 1 in Brazil (26) have implicated contact with armadillos as a risk
factor for leprosy infection. Leprosy is not highly communicable, and knowledge about
potential transmission of the infection through armadillos can help reduce the overall
risk for disease among persons who come in contact with these animals or environments
contaminated by them. M. leprae may be spread through direct or
indirect routes, but long-term direct contact with an infectious source is believed to
be the most effective means to transmit the infection (1). None of the patients interviewed in this study
recalled any direct contact with armadillos, although they may have had indirect
exposure to M. leprae through gardening or other outdoor activities.
Because leprosy is a rare disease, any risk for infection attributable to indirect
exposure to armadillos would have to be extremely low overall. Nevertheless, persons
concerned about exposure to M. leprae from armadillos in their
environment might be advised to wear gloves while gardening or use similar general
hygienic practices commonly recommended for avoiding exposure to other pathogens in the
environment (27). Physicians
caring for patients with possible exposure to M. leprae through
armadillos should retain leprosy in their differential diagnoses for cutaneous lesions,
especially for patients who do not respond well to most common therapies.
The range of armadillos in the Western Hemisphere is the southern United States, Central
America, and northern Argentina. Biomarkers of M. leprae have been
reported among armadillos in Argentina, Brazil, and Colombia (28–30). However, reports of detection of the infection have
been inconsistent in different locales (14,31). Disease prevalence rates among animal populations might
be influenced by the season and local variations in animal density or population
structure that can affect detectability of disease (32). Among armadillos, typically only small numbers of
animals can be screened from any given location, and relatively high prevalence rates
are required to reliably detect the infection. The role that armadillos might play in
helping to perpetuate leprosy throughout the Western Hemisphere merits
consideration.
There are currently no established laboratory tests to aid in the diagnosis of leprosy,
and the disease can only be detected once persons have clinical disease. Serologic
screening for PGL1 antibodies has shown only limited utility, and effective tools to aid
diagnosis or monitor progress of individual infections are needed (33). Wild armadillos showed considerable diversity
in their response to LID1 and PGL1 antigens. Use of the antigens in combination markedly
enhanced serologic detection of M. leprae infection among armadillos,
and PCR analysis of matching tissue samples showed those reactions were highly specific
for M. leprae. For infection of armadillos initiated by intravenous
administration of 1 × 109M. leprae, antibodies against LID1 and PGL1 become detectable only
after a delay of several months, and it appears that relatively well-established
infections are required before either antibody is produced (19). Naturally transmitted infections would involve
much lower initiating doses, and the amount of bacilli required to elicit T
cell−dependent IgM responses against PGL1 might be higher that needed to initiate
T cell−dependent IgG responses to LID1. Trials are underway to discern the
efficacy of using these antigen combinations in screening human populations, and in 1
leprosy-endemic region, LID1 antibodies appeared to be more prevalent than PGL1
antibodies (33−35).
Elimination of an infectious mycobacterium from a wildlife species is extremely
difficult and costly. Authorities have struggled for decades with bovine tuberculosis in
the United Kingdom and Ireland, where the badger (Meles meles) plays a
role in spread of the disease (36); in New Zealand, where the opossum (Trichosurus
vulpecula) is responsible (37); and, more recently, in the northern United States,
where white-tailed deer (Odocoileus virginianus) and other cervids are
involved (38). It is unlikely
that any effort to remove armadillos from large areas would be effective, and the
removal process might provide even greater risks to humans for exposure to M.
leprae from animals. Public education about the risk for exposure to
infectious agents through animals can be highly effective. The greatest potential for
exposure to M. leprae through armadillos would probably be direct
contact with the flesh of animals hunted or prepared as food. However, armadillos can
also shed leprosy bacilli into the environment in bodily secretions, and bacilli might
survive extracellularly in the environment for short periods, or may even be sustained
within encysted amoeba or other reservoirs for 8 months (39). In addition, potential involvement of insects in
leprosy transmission has never been fully discounted, and the role that biting insects
might play in mechanically transmitting M. leprae between hosts also
merits attention (9). A better
understanding of the specific risk factors that might be involved in transmission of
M. leprae between armadillos and humans is needed.
Current leprosy control efforts focus on use of multiple antimicrobial drugs to treat
clinically active human cases. The decreases in global leprosy prevalence reported over
the past decade seem to validate this approach because millions of persons have been
cured of leprosy. However, as 1 source of infection is brought under control, other
major sources might arise. Evidence is now accumulating that leprosy is a zoonosis in
North America, and the infection could extend throughout the range of the armadillo. New
strategies to detect leprosy and prevent its spread will be needed. Molecular genotyping
of M. leprae enables application of modern public health principles of
infectious disease control to identify sources of infection and related clusters of new
cases (40). Insight into the
dynamics of leprosy transmission in different populations will help clarify the
proportional risk related to nonhuman reservoirs and could facilitate objective
development of new methods to ultimately eliminate leprosy.
Technical Appendix. Analysis of zoonotic leprosy in the southeastern
United States by multiplex nested PCR.
Suggested citation for this article: Sharma R, Singh P, Loughry WJ,
Lockhart JM, Inman WB, Duthie MS, et al. Zoonotic leprosy in the southeastern United
States. Emerg Infect Dis. 2015 Dec [date cited]. http://dx.doi.org/10.3201/eid2112.150501
We thank the participants in this study and Anne Burdick, T.P. Gillis, Barbara
Stryjewska, and Ramesh Subramanian, for providing advice and support; and P. Andrews, M.
Kearney, S. Keas, G. McCormick, N. Robbins, R. Stevenson, and H. Zhang for providing
expert assistance.
Acknowledgments
Dr. Sharma is a research fellow at the National Hansen’s Disease Program, Baton
Rouge, Louisiana. His research interests are molecular biology applications in
mycobacterial diseases, including leprosy and tuberculosis, and advancing the armadillo
model for pathogenesis of nerve injury in leprosy.
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