Detection of Giardia in environmental waters by immuno-PCR amplification methods

Detection of Giardia in environmental waters by immuno-PCR amplification methods

Genomic DNA was extracted either directly from Giardia muris cysts seeded into environmental surface waters or from cysts isolated by immunomagnetic beads (IMB). A 0.171-kbp segment of the giardin gene was PCR-amplified following "direct extraction" of Giardia DNA from seeded Cahaba river...

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Bibliographic Details
Published in:Current microbiology Vol. 36; no. 2; pp. 107 - 113
Main Authors: MAHBUBANI, M. H, SCHAEFER, F. W, JONES, D. D, BEJ, A. K
Format: Journal Article
Language:English
Published: New York, NY Springer 01-02-1998
Springer Nature B.V
Subjects:
Animals
Biological and medical sciences
Biotechnology
Cysts
Deoxyribonucleic acid
DNA
DNA, Protozoan - analysis
DNA, Protozoan - genetics
Formaldehyde - pharmacology
Fresh Water - parasitology
Fundamental and applied biological sciences. Psychology
General aspects and techniques
Giardia - drug effects
Giardia - genetics
Giardia - isolation & purification
Immunoassay
Immunomagnetic Separation
Methods
Microbiology
Nephelometry and Turbidimetry
Polymerase Chain Reaction - methods
Protozoa
Rivers
Sensitivity and Specificity
Spores - drug effects
Spores - genetics
Surface water
Turbidity
Water - parasitology
Water
Performance evaluation
Polymerase chain reaction
Protozoa
Gene amplification
Coupled method
Parasite
Environment
Diplomonadida
Method
Detection
Immunological method
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Summary:Genomic DNA was extracted either directly from Giardia muris cysts seeded into environmental surface waters or from cysts isolated by immunomagnetic beads (IMB). A 0.171-kbp segment of the giardin gene was PCR-amplified following "direct extraction" of Giardia DNA from seeded Cahaba river water concentrate with moderate turbidity (780 JTU's), but DNA purified from seeded Colorado river water concentrates with high turbidity (2 x 10(5) JTUs) failed to amplify. However, if the cysts were first separated by the IMB approach from seeded Cahaba or Colorado river waters, and the DNA released by a freeze-boil Chelex(R)100 treatment, detection of G. muris by PCR amplification could be achieved at a sensitivity of 3 x 10(0) or 3 x 10(1) cysts/ml, respectively. If, however, the G. muris cysts used to seed even moderately turbid river waters (780 JTUs) were formalin treated (which is conventionally used for microscopic examination), neither direct extraction nor IMB purification methods yielded amplifiable DNA. Use of immunomagnetic beads to separate Giardia cysts from complex matrices of environmental surface waters followed by DNA release and PCR amplification of the target giardin gene improved the reliability of detection of this pathogen with the required sensitivity.
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ISSN:0343-8651
1432-0991
DOI:10.1007/s002849900288