Persing D H, Telford S R, Spielman A, Barthold S W
Department of Laboratory Medicine, Yale University School of Medicine, New Haven, Connecticut 06510.
J Clin Microbiol. 1990 Mar;28(3):566-72. doi: 10.1128/jcm.28.3.566-572.1990.
The polymerase chain reaction (PCR) was used to amplify DNA sequences of the etiologic agent of Lyme disease, Borrelia burgdorferi, and was applied to the detection of the spirochete in its tick vector. The target for PCR amplification was the OSP-A gene of strain B31; analysis of isolates from different geographical areas indicated that this gene could be used to identify most North American isolates. These methods were extended to the analysis of colony-derived and field-collected Ixodes dammini. OSP-A-specific sequences were identified in 15 of 15 colony-derived nymphal ticks that had fed previously on an infected animal; no such amplification products were detected in 8 control ticks. Segregated midgut tissues of field-collected adult and nymphal ticks from Nantucket Island, Mass., and the Crane Reserve, Ipswich, Mass., were examined by both direct fluorescent-antibody (DFA) staining and PCR. The DFA technique identified 16 infected ticks of 30 paired specimens; 15 of these specimens were positive by PCR. One specimen was positive by PCR that was DFA negative. Both live whole ticks and desiccated dead specimens were suitable for this analysis. Because only five ticks are suitable for DFA analysis, the use of PCR may extend the range of specimens that can be analyzed for the presence of the Lyme spirochete.
聚合酶链反应(PCR)用于扩增莱姆病病原体伯氏疏螺旋体的DNA序列,并应用于在其蜱传播媒介中检测该螺旋体。PCR扩增的靶标是B31菌株的OSP-A基因;对来自不同地理区域的分离株进行分析表明,该基因可用于鉴定大多数北美分离株。这些方法被扩展用于分析来自菌落培养的和野外采集的达敏硬蜱。在15只先前吸食过感染动物血液的来自菌落培养的若蜱中,有15只鉴定出了OSP-A特异性序列;在8只对照蜱中未检测到此类扩增产物。对从马萨诸塞州楠塔基特岛和马萨诸塞州伊普斯维奇克兰保护区野外采集的成年蜱和若蜱的中肠组织进行了直接荧光抗体(DFA)染色和PCR检测。DFA技术在30对标本中鉴定出16只感染蜱;其中15个标本通过PCR检测为阳性。有1个标本PCR检测为阳性但DFA检测为阴性。活的整只蜱和干燥的死标本都适用于此分析。由于只有5只蜱适合进行DFA分析,PCR的应用可能会扩大可用于分析是否存在莱姆螺旋体的标本范围。
