Failure to differentiate Cryptosporidium parvum from C. meleagridis based on PCR amplification of eight DNA sequences.

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RESEARCH PRODUCT

Failure to differentiate Cryptosporidium parvum from C. meleagridis based on PCR amplification of eight DNA sequences.

Roseline Mancassola Dominique Champliaud O. Vagner Alain Bonnin Philippe Gobet J. Lopez Géraldine Harly Muriel Naciri Jean Christophe Buisson István Varga

subject

animal diseases 030231 tropical medicine Genes Protozoan Cryptosporidium Applied Microbiology and Biotechnology Genome Polymerase Chain Reaction Sensitivity and Specificity DNA sequencing 18S ribosomal RNA Microbiology law.invention 03 medical and health sciences 0302 clinical medicine Species Specificity law parasitic diseases TECHNIQUE PCR Animals Humans Gene Polymerase chain reaction ComputingMilieux_MISCELLANEOUS DNA Primers [SDV.EE]Life Sciences [q-bio]/Ecology environment Cryptosporidium parvum 0303 health sciences Ecology biology Base Sequence 030306 microbiology Cryptosporidium DNA Protozoan biology.organism_classification Virology Bacterial Typing Techniques [SDV.EE] Life Sciences [q-bio]/Ecology environment Cryptosporidium parvum Environmental and Public Health Microbiology Primer (molecular biology)Water Microbiology Food Science Biotechnology

description

ABSTRACT In order to determine the specificities of PCR-based assays used for detecting Cryptosporidium parvum DNA, eight pairs of previously described PCR primers targeting six distinct regions of the Cryptosporidium genome were evaluated for the detection of C. parvum , the agent of human cryptosporidiosis, and C. muris , C. baileyi , and C. meleagridis , three Cryptosporidium species that infect birds or mammals but are not considered to be human pathogens. The four Cryptosporidium species were divided into two groups: C. parvum and C. meleagridis , which gave the same-sized fragments with all the reactions, and C. muris and C. baileyi , which gave positive results with primer pairs targeting the 18S rRNA gene only. In addition to being genetically similar at each of the eight loci analyzed by DNA amplification, C. parvum and C. meleagridis couldn’t be differentiated even after restriction enzyme digestion of the PCR products obtained from three of the target genes. This study indicates that caution should be exercised in the interpretation of data from water sample analysis performed by these methods, since a positive result does not necessarily reflect a contamination by the human pathogen C. parvum.

year	journal	country	edition	language
1998-01-01	Applied and environmental microbiology

10.1128/aem.64.4.1454-1458.1998 https://pubmed.ncbi.nlm.nih.gov/9575132