Survey of Borreliae in ticks, canines, and white-tailed deer from Arkansas, USA

被引:16
作者
Fryxell, Rebecca T. Trout [1 ]
Steelman, C. Dayton [2 ]
Szalanski, Allen L. [2 ]
Kvamme, Ken L. [3 ]
Billingsley, Peggy M. [4 ]
Williamson, Philip C. [4 ]
机构
[1] Univ Tennessee, Dept Entomol & Plant Pathol, Knoxville, TN 37901 USA
[2] Univ Arkansas, Dept Entomol, Fayetteville, AR 72701 USA
[3] Univ Arkansas, Dept Anthropol, Fayetteville, AR 72701 USA
[4] Univ N Texas Hlth Sci Ctr, Dept Forens & Invest Genet, Ft Worth, TX USA
关键词
Borrelia; Ticks; Vector borne; Surveillance; Deer; AMBLYOMMA-AMERICANUM ACARI; LYME-DISEASE SPIROCHETE; NORTHEASTERN UNITED-STATES; IXODES-DAMMINI ACARI; LONE-STAR TICKS; DERMACENTOR-VARIABILIS; LONESTARI DNA; HARD-TICK; IXODIDAE; BURGDORFERI;
D O I
10.1186/1756-3305-5-139
中图分类号
R38 [医学寄生虫学]; Q [生物科学];
学科分类号
07 ; 0710 ; 09 ; 100103 ;
摘要
Background: In the Eastern and Upper Midwestern regions of North America, Ixodes scapularis (L.) is the most abundant tick species encountered by humans and the primary vector of B. burgdorferi, whereas in the southeastern region Amblyomma americanum (Say) is the most abundant tick species encountered by humans but cannot transmit B. burgdorferi. Surveys of Borreliae in ticks have been conducted in the southeastern United States and often these surveys identify B. lonestari as the primary Borrelia species, surveys have not included Arkansas ticks, canines, or white-tailed deer and B. lonestari is not considered pathogenic. The objective of this study was to identify Borrelia species within Arkansas by screening ticks (n = 2123), canines (n = 173), and white-tailed deer (n = 228) to determine the identity and locations of Borreliae endemic to Arkansas using PCR amplification of the flagellin (flaB) gene. Methods: Field collected ticks from canines and from hunter-killed white-tailed were identified to species and life stage. After which, ticks and their hosts were screened for the presence of Borrelia using PCR to amplify the flaB gene. A subset of the positive samples was confirmed with bidirectional sequencing. Results: In total 53 (21.2%) white-tailed deer, ten (6%) canines, and 583 (27.5%) Ixodid ticks (252 Ixodes scapularis, 161 A. americanum, 88 Rhipicephalus sanguineus, 50 Amblyomma maculatum, 19 Dermacentor variabilis, and 13 unidentified Amblyomma species) produced a Borrelia flaB amplicon. Of the positive ticks, 324 (22.7%) were collected from canines (151 A. americanum, 78 R. sanguineus, 43 I. scapularis, 26 A. maculatum, 18 D. variabilis, and 8 Amblyomma species) and 259 (37.2%) were collected from white-tailed deer (209 I. scapularis, 24 A. maculatum, 10 A. americanum, 10 R. sanguineus, 1 D. variabilis, and 5 Amblyomma species). None of the larvae were PCR positive. A majority of the flaB amplicons were homologous with B. lonestari sequences: 281 of the 296 sequenced ticks, 3 canines, and 27 deer. Only 22 deer, 7 canines, and 15 tick flaB amplicons (12 I. scapularis, 2 A. maculatum, and 1 Amblyomma species) were homologous with B. burgdorferi sequences. Conclusions: Data from this study identified multiple Borreliae genotypes in Arkansas ticks, canines and deer including B. burgdorferi and B. lonestari; however, B. lonestari was significantly more prevalent in the tick population than B. burgdorferi. Results from this study suggest that the majority of tick-borne diseases in Arkansas are not B. burgdorferi.
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