中国动物传染病学报
中國動物傳染病學報
중국동물전염병학보
CHINESE JOURNAL OF VETERINARY PARASITOLOGY
2014年
6期
38-45
,共8页
李树清%李雯雯%张鸿满%陈韶红%李健%陈志飞%王巧全%张永年%黄维义
李樹清%李雯雯%張鴻滿%陳韶紅%李健%陳誌飛%王巧全%張永年%黃維義
리수청%리문문%장홍만%진소홍%리건%진지비%왕교전%장영년%황유의
棘颚口线虫%日本颚口线虫%杜氏颚口线虫%多重PCR%虫种鉴定
棘顎口線蟲%日本顎口線蟲%杜氏顎口線蟲%多重PCR%蟲種鑒定
극악구선충%일본악구선충%두씨악구선충%다중PCR%충충감정
G.spinigerum%G.nipponicum%G.doloresi%multiplex PCR%identification
为了建立快速、灵敏、可靠的鉴别颚口线虫虫种的方法,根据GenBank中发表的棘颚口线虫、日本颚口线虫和杜氏颚口线虫ITS-2序列,设计了3对特异引物,建立了这3种颚口线虫的单一PCR和多重PCR检测方法,并分别对单一PCR和多重PCR方法的特异性和敏感性进行了鉴定。结果显示单一PCR和多重PCR均能特异扩增出棘颚口线虫、日本颚口线虫和杜氏颚口线虫,其片段大小分别为282、358、183 bp,单一PCR对棘颚口线虫、日本颚口线虫和杜氏颚口线虫虫体DNA最小检出量分别为0.2、0.01、0.01 ng/μL。对宫脂线虫、异尖线虫、棘口吸虫以及迭宫绦虫均不能进行扩增。用建立的多重PCR方法对菲律宾、印度尼西亚、黑龙江颚口线虫等12条颚口线虫DNA模板进行扩增,经鉴定菲律宾与印度尼西亚的颚口线虫为棘颚口线虫,黑龙江的颚口线虫为日本颚口线虫。鉴定结果与原虫体样本的形态鉴定和测序分析结果一致。研究显示建立的多重PCR方法具有很强的特异性和较高的敏感性,可用于棘颚口线虫、日本颚口线虫和杜氏颚口线虫虫种的鉴定和流行病学调查。
為瞭建立快速、靈敏、可靠的鑒彆顎口線蟲蟲種的方法,根據GenBank中髮錶的棘顎口線蟲、日本顎口線蟲和杜氏顎口線蟲ITS-2序列,設計瞭3對特異引物,建立瞭這3種顎口線蟲的單一PCR和多重PCR檢測方法,併分彆對單一PCR和多重PCR方法的特異性和敏感性進行瞭鑒定。結果顯示單一PCR和多重PCR均能特異擴增齣棘顎口線蟲、日本顎口線蟲和杜氏顎口線蟲,其片段大小分彆為282、358、183 bp,單一PCR對棘顎口線蟲、日本顎口線蟲和杜氏顎口線蟲蟲體DNA最小檢齣量分彆為0.2、0.01、0.01 ng/μL。對宮脂線蟲、異尖線蟲、棘口吸蟲以及迭宮縚蟲均不能進行擴增。用建立的多重PCR方法對菲律賓、印度尼西亞、黑龍江顎口線蟲等12條顎口線蟲DNA模闆進行擴增,經鑒定菲律賓與印度尼西亞的顎口線蟲為棘顎口線蟲,黑龍江的顎口線蟲為日本顎口線蟲。鑒定結果與原蟲體樣本的形態鑒定和測序分析結果一緻。研究顯示建立的多重PCR方法具有很彊的特異性和較高的敏感性,可用于棘顎口線蟲、日本顎口線蟲和杜氏顎口線蟲蟲種的鑒定和流行病學調查。
위료건립쾌속、령민、가고적감별악구선충충충적방법,근거GenBank중발표적극악구선충、일본악구선충화두씨악구선충ITS-2서렬,설계료3대특이인물,건립료저3충악구선충적단일PCR화다중PCR검측방법,병분별대단일PCR화다중PCR방법적특이성화민감성진행료감정。결과현시단일PCR화다중PCR균능특이확증출극악구선충、일본악구선충화두씨악구선충,기편단대소분별위282、358、183 bp,단일PCR대극악구선충、일본악구선충화두씨악구선충충체DNA최소검출량분별위0.2、0.01、0.01 ng/μL。대궁지선충、이첨선충、극구흡충이급질궁조충균불능진행확증。용건립적다중PCR방법대비률빈、인도니서아、흑룡강악구선충등12조악구선충DNA모판진행확증,경감정비률빈여인도니서아적악구선충위극악구선충,흑룡강적악구선충위일본악구선충。감정결과여원충체양본적형태감정화측서분석결과일치。연구현시건립적다중PCR방법구유흔강적특이성화교고적민감성,가용우극악구선충、일본악구선충화두씨악구선충충충적감정화류행병학조사。
Three pairs of primers specific for G.spinigerum (JN408326), G.nipponicum (JN408315) and G.doloresi (JN408329) were designed based on their ITS-2 sequences. Accordingly, single and multiplex PCR methods were developed to identify Gnathostoma species. The amplified products in both single and multiplex PCR methods were 282 bp for G.spinigerum, 358 bp for G.nipponicum and 183 bp for G.doloresi. The DNA detection limits were 0.2 ng for G.spinigerum, 0.01 ng for G.nipponicum and also 0.01 ng for G.doloresi.No PCR products were amplified from genomes of Hysterothylacium, Anisakis, Echinostoma and Spirometra erinaceieuropaei. In addition, 12 species of Gnathostoma isolated from Philippines, Indonesia and Heilongjiang were identified in multiplex PCR and the results were in agreement with morphology and sequence analysis. The isolates from Philippines and Indonesia were G.spinigerum and isolates from Heilongjiang were G. nipponicum. These data suggested that multiplex PCR methods could be used for identifying G. spinigerum, G.nipponicum and G.doloresi.
