Gene probe-based detection of type E botulinum neurotoxin binding protein using polymerase chain reaction

Gene probe-based detection of type E botulinum neurotoxin binding protein using polymerase chain reaction

Using primers based on the nucleotide sequence of a neurotoxin binding protein from Type E Clostridium botulinum cultures, an amplified DNA product was obtained through polymerase chain reaction. The 400 base pair amplified DNA fragment was detectable with as low as 0.1 pg template DNA from Type E C...

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Veröffentlicht in:Toxicon (Oxford) 1996-07, Vol.34 (7), p.737-742
Hauptverfasser: Singh, Bal Ram, Barcomb-Caddle, Linda A., Fu, Fen-Ni, Li, Bilian
Format: Artikel
Sprache:eng
Schlagworte:
Bacteriology
binding proteins
Biological and medical sciences
Botulinum Toxins - analysis
Botulinum Toxins - metabolism
Carrier Proteins
Clostridium botulinum
Clostridium botulinum - metabolism
Clostridium tetani
Culture Media
DNA - chemistry
DNA - genetics
DNA - metabolism
DNA Primers
foodborne illness
Fundamental and applied biological sciences. Psychology
Microbiology
neurotoxins
Neurotoxins - analysis
Neurotoxins - metabolism
Oligonucleotide Probes
Pathogenicity, virulence, toxins, bacteriocins, pyrogens, host-bacteria relations, miscellaneous strains
Polymerase Chain Reaction
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Zusammenfassung:Using primers based on the nucleotide sequence of a neurotoxin binding protein from Type E Clostridium botulinum cultures, an amplified DNA product was obtained through polymerase chain reaction. The 400 base pair amplified DNA fragment was detectable with as low as 0.1 pg template DNA from Type E C. botulinum, and its fidelity was confirmed by Southern blotting using a DNA probe designed to detect the expected amplified DNA fragment. On the other hand, no DNA amplification was observed with as high as 10 ng template DNA from related Types A and B C. botulinum or from C. tetani, indicating the specificity of the probe.
ISSN:0041-0101
1879-3150
DOI:10.1016/0041-0101(95)00166-2