Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract

Using a chemiluminescence (CL) test, it had been previously demonstrated that Vibrio pectenicida, which is pathogenic to Pecten maximus larvae, was able to inhibit completely the CL activity of P. maximus hemocytes and partially inhibit those of Crassostrea gigas. Conversely, a Vibrio sp. strain, S3...

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Main Authors: Christophe Lamberta, Jean-louis Nicolasa, Valérie Bultelb
Other Authors: The Pennsylvania State University CiteSeerX Archives
Format: Text
Language:English
Published: 2001
Subjects:
IJPA2000-0042
C. LAMBERT
Crassostrea gigas
Online Access:http://citeseerx.ist.psu.edu/viewdoc/summary?doi=10.1.1.614.71
http://archimer.ifremer.fr/doc/2001/publication-466.pdf
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spelling ftciteseerx:oai:CiteSeerX.psu:10.1.1.614.71 2023-05-15T15:58:41+02:00 Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract Christophe Lamberta Jean-louis Nicolasa Valérie Bultelb The Pennsylvania State University CiteSeerX Archives 2001 application/pdf http://citeseerx.ist.psu.edu/viewdoc/summary?doi=10.1.1.614.71 http://archimer.ifremer.fr/doc/2001/publication-466.pdf en eng http://citeseerx.ist.psu.edu/viewdoc/summary?doi=10.1.1.614.71 http://archimer.ifremer.fr/doc/2001/publication-466.pdf Metadata may be used without restrictions as long as the oai identifier remains attached to it. http://archimer.ifremer.fr/doc/2001/publication-466.pdf IJPA2000-0042 C. LAMBERT text 2001 ftciteseerx 2016-01-08T14:41:25Z Using a chemiluminescence (CL) test, it had been previously demonstrated that Vibrio pectenicida, which is pathogenic to Pecten maximus larvae, was able to inhibit completely the CL activity of P. maximus hemocytes and partially inhibit those of Crassostrea gigas. Conversely, a Vibrio sp. strain, S322, pathogenic to C. gigas larvae was more active in reducing the CL activity of oyster hemocytes than of scallop hemocytes. Using this same CL biotest, V. pectenicida and S322 cytoplasmic extracts were shown to reproduce CL inhibition while the cytoplasmic extract of a nonpathogenic strain (U1, Pseudoalteromonas) was without effect. Moreover, cytoplasmic extract as well as live V. pectenicida cells provoked, within a few hours, death of P. maximus hemocytes adhering to a glass slide. After partial purification, it was shown that toxic activities of V. pectenicida cytoplasmic extract was due to a toxin, named VHKT (for vibrio hemocyte-killer toxin), which is heat stable, acid and protease resistant, and less than 3 kDa in molecular weight. Attempts to purify VHKT by reverse-phase (C18) HPLC separated activity into the fraction eluted by water at a retention time of 4.02 min. Text Crassostrea gigas Unknown
institution Open Polar
collection Unknown
op_collection_id ftciteseerx
language English
topic IJPA2000-0042
C. LAMBERT
spellingShingle IJPA2000-0042
C. LAMBERT
Christophe Lamberta
Jean-louis Nicolasa
Valérie Bultelb
Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract
topic_facet IJPA2000-0042
C. LAMBERT
description Using a chemiluminescence (CL) test, it had been previously demonstrated that Vibrio pectenicida, which is pathogenic to Pecten maximus larvae, was able to inhibit completely the CL activity of P. maximus hemocytes and partially inhibit those of Crassostrea gigas. Conversely, a Vibrio sp. strain, S322, pathogenic to C. gigas larvae was more active in reducing the CL activity of oyster hemocytes than of scallop hemocytes. Using this same CL biotest, V. pectenicida and S322 cytoplasmic extracts were shown to reproduce CL inhibition while the cytoplasmic extract of a nonpathogenic strain (U1, Pseudoalteromonas) was without effect. Moreover, cytoplasmic extract as well as live V. pectenicida cells provoked, within a few hours, death of P. maximus hemocytes adhering to a glass slide. After partial purification, it was shown that toxic activities of V. pectenicida cytoplasmic extract was due to a toxin, named VHKT (for vibrio hemocyte-killer toxin), which is heat stable, acid and protease resistant, and less than 3 kDa in molecular weight. Attempts to purify VHKT by reverse-phase (C18) HPLC separated activity into the fraction eluted by water at a retention time of 4.02 min.
author2 The Pennsylvania State University CiteSeerX Archives
format Text
author Christophe Lamberta
Jean-louis Nicolasa
Valérie Bultelb
author_facet Christophe Lamberta
Jean-louis Nicolasa
Valérie Bultelb
author_sort Christophe Lamberta
title Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract
title_short Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract
title_full Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract
title_fullStr Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract
title_full_unstemmed Archive Institutionnelle de l’Ifremer Toxicity to Bivalve Hemocytes of Pathogenic Vibrio Cytoplasmic Extract
title_sort archive institutionnelle de l’ifremer toxicity to bivalve hemocytes of pathogenic vibrio cytoplasmic extract
publishDate 2001
url http://citeseerx.ist.psu.edu/viewdoc/summary?doi=10.1.1.614.71
http://archimer.ifremer.fr/doc/2001/publication-466.pdf
genre Crassostrea gigas
genre_facet Crassostrea gigas
op_source http://archimer.ifremer.fr/doc/2001/publication-466.pdf
op_relation http://citeseerx.ist.psu.edu/viewdoc/summary?doi=10.1.1.614.71
http://archimer.ifremer.fr/doc/2001/publication-466.pdf
op_rights Metadata may be used without restrictions as long as the oai identifier remains attached to it.
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