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IDENTIFICATION OF ACANTHAMOEBA AT THE GENERIC AND SPECIFIC LEVELS USING THE POLYMERASE CHAIN-REACTION

被引:65
作者
VODKIN, MH
HOWE, DK
VISVESVARA, GS
MCLAUGHLIN, GL
机构
[1] PURDUE UNIV,SCH VET MED,DEPT VET PATHOBIOL,W LAFAYETTE,IN 47907
[2] UNIV ILLINOIS,COLL VET MED,DEPT VET PATHOBIOL,URBANA,IL 61801
[3] CTR DIS CONTROL,CTR INFECT DIS,DIV PARASIT DIS,ATLANTA,GA 30333
来源
JOURNAL OF PROTOZOOLOGY | 1992年 / 39卷 / 03期
关键词
AMEBA; NAEGLERIA; HUMAN PATHOGEN; REPETITIVE DNA; RIBOSOMAL DNA;
D O I
10.1111/j.1550-7408.1992.tb01467.x
中图分类号
Q95 [动物学];
学科分类号
071002 ;
摘要
We have adapted the polymerase chain reaction to identify strains of Acanthamoeba. Using computer-assisted analysis, primers were designed from an anonymous repetitive sequence and from published sequences of 18S and 5S ribosomal RNA genes of A. castellanii. Amplification of a short ribosomal DNA target (272 base pairs) at restrictive annealing conditions (> 50-degrees-C) resulted in a single band that was unique for the genus and distinguished Acanthamoeba from Naegleria. This assay functioned with fresh and formalin-fixed cells as starting material. Amplification of longer targets (400-700 base pairs) at less restrictive annealing conditions (< 47-degrees-C) led to more than one band. This multiple banding pattern could reproducibly classify Acanthamoeba at the strain level and was, in certain cases, diagnostic for known pathogenic strains. However, these assays need to be further refined to make them relevant for clinical purposes.
引用
收藏
页码:378 / 385
页数:8
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