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4. Genetic organization of α-bungarotoxins from Bungarus multicinctus (Taiwan banded krait): evidence showing that the production of α-bungarotoxin isotoxins is not derived from edited mRNAs.

Author

Chang, Long-sen, Shu-kai, Lin, Huang, Hsien-bin, Hsiao, Michael, Endo, T., Yu., C., Basus, V.T., Love, R.A., Kosen, P.A., Scherf, T., Pillet, L., Tremeau, O., Dufton, M.J., Bhaskaran, R., Sivaraman, T., Sun, Y.J., Chang, L.S., Lachumanan, R., Afifuyan, F., and Liu, L.F.

Published
1999
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5. Mimicry between receptors and antibodies. Identification of snake toxin determinants recognized by the acetylcholine receptor and an acetylcholine receptor-mimicking monoclonal antibody.

Author

Ducancel, F, Mérienne, K, Fromen-Romano, C, Trémeau, O, Pillet, L, Drevet, P, Zinn-Justin, S, Boulain, J C, and Ménez, A

Abstract

In several instances, a monoclonal antibody raised against a receptor ligand has been claimed to mimic the ligand receptor. Thus, a specific monoclonal antibody (Malpha2-3) raised against a short-chain toxin from snake was proposed to mimic the nicotinic acetylcholine receptor (AChR) (). Further confirming this mimicry, we show that (i) like AChR, Malpha2-3 elicits anti-AChR antibodies, which in turn elicit anti-toxin antibodies; and (ii) the region 106-122 of the alpha-chain of AChR shares 66% primary structure identity with complementarity-determining regions of Malpha2-3. Also, a mutational analysis of erabutoxin a reveals that the epitope recognized by Malpha2-3 consists of 10 residues, distributed within the three toxin loops. Eight of these residues also belong to the 10-residue epitope recognized by AChR, a result that offers an explanation as to the functional similarities between the receptor and the antibody. Strikingly, however, most of the residues common to the two epitopes contribute differentially to the energetic formation of the antibody-toxin and the receptor-toxin complexes. Together, the data suggest that the mimicry between AChR and Malpha2-3 is partial only.

Published
1996

6. Les huiles essentielles et leurs principaux constituants / par E. Charabot,... J. Dupont,... et L. Pillet,... ; préface de M. E. Grimaux,...

Author

Grimaux, Édouard (1835-1900). Préfacier, Charabot, Eugène (1870-1938). Auteur du texte, Pillet, L.. Auteur du texte, Dupont, Justin (1869-1943). Auteur du texte, Grimaux, Édouard (1835-1900). Préfacier, Charabot, Eugène (1870-1938). Auteur du texte, Pillet, L.. Auteur du texte, and Dupont, Justin (1869-1943). Auteur du texte

Abstract

Avec mode texte

Published
1899

10. Protective effect of the antioxidant and free radical scavenger MCI-186 on chondrocyte viability after injurious compression.

Author

Démarteau, O., Schwitzgu&eacutebel, T., Morel, V., Pillet, L., and Quinn, T. M.

Subjects
ANTIOXIDANTS, FREE radicals, CARTILAGE cells, BONE cells, CELLS
Abstract

Presents a study on the protective effect of the antioxidant and free radical scavenger MCI-186 on chondrocyte viability after injurious compression. Division of explants into groups; Assessment of cell viability within each group; Results of the study.

Published
2004

12. Glycosyl benzoates as novel substrates for glycosynthases.

Author

de Lorenzo S, Pillet L, Lim D, and Paradisi F

Subjects
Glycoside Hydrolases, Glycosylation, Benzoates, Thioglycosides
Abstract

The development of a procedure for the one-pot synthesis of glycosyl benzoates directly from unprotected sugars in aqueous media using 2-chloro-1,3-dimethylimidazolium chloride (DMC), thiobenzoic acid, and triethylamine is reported. These glycosyl donors are excellent substrates for wild-type and mutant glycosidases. β-Glucosyl benzoate was hydrolysed by the GH1 β-glucosidase derived from Halothermothrix orenii ( Hor GH1). Subsequent use of this substrate in thioligase-mediated glycosylation of p -nitrothiophenol demonstrated their superiority as donors compared to their p -nitrophenol counterparts with excellent conversions. Using a series of arene nucleophiles, we also demonstrate good to excellent conversions (up to 94%) of β-glucosyl benzoate to the corresponding p -nitrophenyl- and thioglycosides.

Published
2023
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13. Novel triple mutant of an extremophilic glycosyl hydrolase enables the rapid synthesis of thioglycosides.

Author

Pillet L, Lim D, Almulhim N, Benítez-Mateos AI, and Paradisi F

Subjects
Hydrolases, Fluorides, Glycosylation, Sulfhydryl Compounds, Thioglycosides, Extremophiles
Abstract

In order to expand the toolbox of enzymes available for thioglycoside synthesis, we describe here the first example of an extremophilic glycosyl hydrolase from Halothermothrix orenii ( Hor GH1) engineered towards thioglycosynthase activity with a novel combination of mutations. Using the triple mutant, Hor GH1 M299R/E166A/E354G, a range of thioglycosides from glycosyl fluoride donors and aromatic thiols could be synthesised with exquisite stereoselectivity and good to excellent conversions (61-93%).

Published
2022
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14. Copper-induced Production of Laccases for Lignin Depolymerisation and Micropollutant Degradation by Laccase-mediator Systems.

Author

Pillet L, Dufresne R, and Crelier S

Subjects
Biocatalysis, Copper, Fungi enzymology, Laccase biosynthesis, Lignin
Abstract

Contaminants deriving from human activities represent a constantly growing threat to our environment and have a direct impact on plant and animal health. To alleviate this ecological imbalance, biocatalysis offers a green and sustainable alternative to conventional chemical processes. Due to their broad specificity, laccases are enzymes possessing excellent potential for synthetic biotransformations in various fields as well as for the degradation of organic contaminants. Herein, we produced laccases in submerged cultures of P. ostreatus and T. versicolor in three different media. The fungi/medium combination leading to the highest enzymatic activity was malt extract (2%) + yeast extract (3%) + glucose (0.8%). Laccase production was further increased by supplementing this medium with different concentrations of Cu 2+ , which also provided a better understanding of the induction effect. Additionally, we disclose preliminary results on the interaction of laccases with mediators (ABTS and violuric acid - VA) for two main applications: lignin depolymerisation with guaiacylglycerol-β-guaiacyl ether (GBG) as lignin model and micropollutant degradation with Remazol Brilliant Blue (RBB) as enzymatic bioremediation model. Promising results were achieved using VA to increase depolymerization of GBG dimer and to enhance RBB decolorisation.

Published
2021
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15. Haut les cœurs !

Author

Celeny D, D'Esposito AG, Gueorguiev BR, Haraj M, Laszlo A, Pillet L, and Perrin J

Published
2020

16. Time Calibrated Morpho-molecular Classification of Nassellaria (Radiolaria).

Author

Sandin MM, Pillet L, Biard T, Poirier C, Bigeard E, Romac S, Suzuki N, and Not F

Subjects
DNA, Ribosomal genetics, Microscopy, Electron, Scanning, Rhizaria cytology, Rhizaria genetics, Rhizaria ultrastructure, Time, Phylogeny, Rhizaria classification
Abstract

Nassellaria are marine protists belonging to the Radiolaria lineage (Rhizaria). Their skeleton, made of opaline silica, exhibit an excellent fossil record, extremely valuable in micro-paleontological studies for paleo-environmental reconstruction. Yet, to date very little is known about the extant diversity and ecology of Nassellaria in contemporary oceans, and most of it is inferred from their fossil record. Here we present an integrative classification of Nassellaria based on taxonomical marker genes (18S and 28S ribosomal DNA) and morphological characteristics obtained by optical and scanning electron microscopy imaging. Our phylogenetic analyses distinguished 11 main morpho-molecular clades relying essentially on the overall morphology of the skeleton and not on internal structures as previously considered. Using fossil calibrated molecular clock we estimated the origin of Nassellaria among radiolarians primitive forms in the Devonian (ca. 420 Ma), that gave rise to living nassellarian groups in the Triassic (ca. 250 Ma), during the biggest diversification event over their evolutionary history. This morpho-molecular framework provides both a new morphological classification easier to identify under light microscopy and the basis for future molecular ecology surveys. Altogether, it brings a new standpoint to improve our scarce understanding of the ecology and worldwide distribution of extant nassellarians., (Copyright © 2019 The Authors. Published by Elsevier GmbH.. All rights reserved.)

Published
2019
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17. High-throughput sequencing and morphology perform equally well for benthic monitoring of marine ecosystems.

Author

Lejzerowicz F, Esling P, Pillet L, Wilding TA, Black KD, and Pawlowski J

Subjects
Animals, Computational Biology methods, DNA Barcoding, Taxonomic, Environmental Monitoring, High-Throughput Nucleotide Sequencing, Aquatic Organisms, Biodiversity, Ecosystem
Abstract

Environmental diversity surveys are crucial for the bioassessment of anthropogenic impacts on marine ecosystems. Traditional benthic monitoring relying on morphotaxonomic inventories of macrofaunal communities is expensive, time-consuming and expertise-demanding. High-throughput sequencing of environmental DNA barcodes (metabarcoding) offers an alternative to describe biological communities. However, whether the metabarcoding approach meets the quality standards of benthic monitoring remains to be tested. Here, we compared morphological and eDNA/RNA-based inventories of metazoans from samples collected at 10 stations around a fish farm in Scotland, including near-cage and distant zones. For each of 5 replicate samples per station, we sequenced the V4 region of the 18S rRNA gene using the Illumina technology. After filtering, we obtained 841,766 metazoan sequences clustered in 163 Operational Taxonomic Units (OTUs). We assigned the OTUs by combining local BLAST searches with phylogenetic analyses. We calculated two commonly used indices: the Infaunal Trophic Index and the AZTI Marine Biotic Index. We found that the molecular data faithfully reflect the morphology-based indices and provides an equivalent assessment of the impact associated with fish farms activities. We advocate that future benthic monitoring should integrate metabarcoding as a rapid and accurate tool for the evaluation of the quality of marine benthic ecosystems.

Published
2015
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18. Environmental Monitoring: Inferring the Diatom Index from Next-Generation Sequencing Data.

Author

Visco JA, Apothéloz-Perret-Gentil L, Cordonier A, Esling P, Pillet L, and Pawlowski J

Subjects
Diatoms classification, Ecosystem, Molecular Sequence Data, Phylogeny, Rivers, Switzerland, Diatoms genetics, Environmental Monitoring methods, High-Throughput Nucleotide Sequencing methods, Water Quality
Abstract

Diatoms are widely used as bioindicators for the assessment of water quality in rivers and streams. Classically, the diatom biotic indices are based on the relative abundance of morphologically identified species weighted by their autoecological value. Obtaining such indices is time-consuming, costly, and requires excellent taxonomic expertise, which is not always available. Here we tested the possibility to overcome these limitations using a next-generation sequencing (NGS) approach to identify and quantify diatoms found in environmental DNA and RNA samples. We analyzed 27 river sites in the Geneva area (Switzerland), in order to compare the values of the Swiss Diatom Index (DI-CH) computed either by microscopic quantification of diatom species or directly from NGS data. Despite gaps in the reference database and variations in relative abundance of analyzed species, the diatom index shows a significant correlation between morphological and molecular data indicating similar biological quality status for the majority of sites. This proof-of-concept study demonstrates the potential of the NGS approach for identification and quantification of diatoms in environmental samples, opening new avenues toward the routine application of genetic tools for bioassessment and biomonitoring of aquatic ecosystems.

Published
2015
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19. Towards an Integrative Morpho-molecular Classification of the Collodaria (Polycystinea, Radiolaria).

Author

Biard T, Pillet L, Decelle J, Poirier C, Suzuki N, and Not F

Subjects
Biodiversity, DNA, Ribosomal genetics, Microscopy, Electron, Scanning, Rhizaria genetics, Rhizaria ultrastructure, Phylogeny, Rhizaria classification
Abstract

Collodaria are ubiquitous and abundant marine radiolarian (Rhizaria) protists. They occur as either large colonies or solitary specimens, and, unlike most radiolarians, some taxa lack silicified structures. Collodarians are known to play an important role in oceanic food webs as both active predators and hosts of symbiotic microalgae, yet very little is known about their diversity and evolution. Taxonomic delineation of collodarians is challenging and only a few species have been genetically characterized. Here we investigated collodarian diversity using phylogenetic analyses of both nuclear small (18S) and large (28S) subunits of the ribosomal DNA, including 124 new sequences from 75 collodarians sampled worldwide. The resulting molecular phylogeny was compared to morphology-based classification. Our analyses distinguished the monophyletic clade of skeleton-less and spicule-bearing Sphaerozoidae from the sister clades Collosphaeridae (skeleton-bearing) and Collophidiidae (skeleton-less), while the Thalassicollidae was not retrieved as a monophyletic clade. Detailed morphological examination with electron microscopy combined with molecular analyses revealed many discrepancies, such as a mix between solitary and colonial species, co-existence of skeleton-less and skeleton-bearing specimens within the Collosphaeridae, as well as complex intraspecific variability in silicified structures. Such observations challenge a morphology-based classification and highlight the pertinence of an integrative taxonomic approach to study collodarian diversity., (Copyright © 2015 Elsevier GmbH. All rights reserved.)

Published
2015
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20. The genome of the foraminiferan Reticulomyxa filosa.

Author

Glöckner G, Hülsmann N, Schleicher M, Noegel AA, Eichinger L, Gallinger C, Pawlowski J, Sierra R, Euteneuer U, Pillet L, Moustafa A, Platzer M, Groth M, Szafranski K, and Schliwa M

Subjects
Cytoskeleton genetics, Gene Transfer, Horizontal, Meiosis, Molecular Sequence Data, Rhizaria cytology, Transcription Factors genetics, Genome, Protozoan, Rhizaria genetics
Abstract

Background: Rhizaria are a major branch of eukaryote evolution with an extensive microfossil record, but only scarce molecular data are available. The rhizarian species Reticulomyxa filosa, belonging to the Foraminifera, is free-living in freshwater environments. In culture, it thrives only as a plasmodium with thousands of haploid nuclei in one cell. The R. filosa genome is the first foraminiferal genome to be deciphered., Results: The genome is extremely repetitive, and the large amounts of identical sequences hint at frequent amplifications and homologous recombination events. Presumably, these mechanisms are employed to provide more gene copies for higher transcriptional activity and to build up a reservoir of gene diversification in certain gene families, such as the kinesin family. The gene repertoire indicates that it is able to switch to a single-celled, flagellated sexual state never observed in culture. Comparison to another rhizarian, the chlorarachniophyte alga Bigelowiella natans, reveals that proteins involved in signaling were likely drivers in establishing the Rhizaria lineage. Compared to some other protists, horizontal gene transfer is limited, but we found evidence of bacterial-to-eukaryote and eukaryote-to-eukaryote transfer events., Conclusions: The R. filosa genome exhibits a unique architecture with extensive repeat homogenization and gene amplification, which highlights its potential for diverse life-cycle stages. The ability of R. filosa to rapidly transport matter from the pseudopodia to the cell body may be supported by the high diversification of actin and kinesin gene family members., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published
2014
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21. Deep relationships of Rhizaria revealed by phylogenomics: a farewell to Haeckel's Radiolaria.

Author

Sierra R, Matz MV, Aglyamova G, Pillet L, Decelle J, Not F, de Vargas C, and Pawlowski J

Subjects
Bayes Theorem, DNA, Protozoan genetics, Expressed Sequence Tags, Gene Library, Genes, Protozoan, Likelihood Functions, Models, Genetic, Rhizaria genetics, Sequence Alignment, Sequence Analysis, DNA, Phylogeny, Rhizaria classification
Abstract

Rhizaria is one of the six supergroups of eukaryotes, which comprise the majority of amoeboid and skeleton-building protists living in freshwater and marine ecosystems. There is an overall lack of molecular data for the group and therefore the deep phylogeny of rhizarians is unresolved. Molecular data are particularly scarce for the clade of Retaria, which include two prominent groups of microfossils: foraminiferans and radiolarians. To fill this gap, we have produced and sequenced EST libraries for 14 rhizarian species including seven foraminiferans, Gromia and six taxa belonging to traditional Haeckel's Radiolaria: Acantharea, Polycystinea, and Phaeodarea. A matrix was constructed for phylogenetic analysis based on 109 genes and a total of 56 species, of which 22 are rhizarians. Our analyses provide the first multigene evidence for branching of Phaeodarea within Cercozoa, confirming the polyphyly of Haeckel's Radiolaria. It confirms the monophyly of Retaria, a clade grouping Foraminifera with other lineages of Radiolaria. However, contrary to what could be expected from morphological observations, Foraminifera do not form a sister group to radiolarians, but branch within them as sister to either Acantharea or Polycystinea depending on the multigene data set. While the monophyly of Foraminifera and Acantharea is well supported, that of Polycystinea, represented in our data by Spumellaria and Collodaria is questionable. In view of our study, Haeckel's Radiolaria appears as both, a polyphyletic and paraphyletic assemblage of independent groups that should be considered as separate lineages in protist classification., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published
2013
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22. The role of horizontal gene transfer in kleptoplastidy and the establishment of photosynthesis in the eukaryotes.

Author

Pillet L

Abstract

Found in different eukaryotic lineages, kleptoplastidy is the ability to sequester chloroplasts from algal preys that are ingested and partially digested. While most of the genetic information required for the activity and maintenance of the kleptoplastids disappeared with the digestion of the algal nuclei, the photosynthetic organelles remain active during extended period of time. Many different hypotheses have been proposed to explain the longevity of the kleptoplastids within their host. The most popular one involves Horizontal Gene Transfer (HGT) from the algal genome to the host nucleus. In order to test this hypothesis, transcriptome-based analyses have been performed on different kleptoplastidic organisms during the past few years. However, the variability of the results obtained does not allow drawing a convincing conclusion regarding the precise role of HGT in kleptoplastidy. Understanding the mechanism that allow persistence of the plastids is crucial, not only for the characterization of kleptoplastidy, but also for important evolutionary questions surrounding endosymbiotic events and the emergence and spread of photosynthesis in the eukaryotes. Here, I discuss alternative theories that could explain the longevity of sequestered plastids in their host, with special focus on the simplest chloroplast stability hypothesis.

Published
2013
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23. Transcriptome analysis of foraminiferan Elphidium margaritaceum questions the role of gene transfer in kleptoplastidy.

Author

Pillet L and Pawlowski J

Subjects
Chloroplasts genetics, Diatoms genetics, Evolution, Molecular, Expressed Sequence Tags, Photosynthesis, Phylogeny, Sequence Analysis, Symbiosis, Foraminifera genetics, Gene Expression Profiling methods, Gene Transfer, Horizontal, Plastids genetics
Abstract

Foraminifera from the genus Elphidium are heterotrophic protists that graze on diatoms and sequester chloroplasts from their algal preys, while digesting the rest of the diatom cell. During that process, known as kleptoplastidy, the acquired plastids remain active inside the foraminiferan cell for several months. As most of the genes required to sustain the activity of the chloroplasts are encoded in the diatom nucleus, it is unknown how the host cell can maintain the photosynthetic activity without this information. It has been proposed that maintenance of kleptoplastids could be explained by horizontal gene transfer (HGT). To test this hypothesis we obtained 17,125 EST sequences of Elphidium margaritaceum, and we screened this data set for diatom nuclear-encoded proteins having a function in photosynthetic activity or plastid maintenance. Our analyses show no evidence for the presence of such transcriptionally active genes and suggest that HGT hypothesis alone cannot explain the chloroplast's longevity in Elphidium.

Published
2013
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24. Intra-genomic ribosomal RNA polymorphism and morphological variation in Elphidium macellum suggests inter-specific hybridization in foraminifera.

Author

Pillet L, Fontaine D, and Pawlowski J

Subjects
Cloning, Molecular, DNA, Ribosomal metabolism, Evolution, Molecular, Genomics, Haplotypes, Microscopy, Electron, Scanning methods, Models, Genetic, Nucleic Acid Conformation, Nucleic Acid Hybridization, Phylogeny, Recombination, Genetic, Rhizaria metabolism, Polymorphism, Genetic, RNA, Ribosomal genetics, Rhizaria genetics
Abstract

Elphidium macellum is a benthic foraminifer commonly found in the Patagonian fjords. To test whether its highly variable morphotypes are ecophenotypes or different genotypes, we analysed 70 sequences of the SSU rRNA gene from 25 specimens. Unexpectedly, we identified 11 distinct ribotypes, with up to 5 ribotypes co-occurring within the same specimen. The ribotypes differ by varying blocks of sequence located at the end of stem-loop motifs in the three expansion segments specific to foraminifera. These changes, distinct from typical SNPs and indels, directly affect the structure of the expansion segments. Their mosaic distribution suggests that ribotypes originated by recombination of two or more clusters of ribosomal genes. We propose that this expansion segment polymorphism (ESP) could originate from hybridization of morphologically different populations of Patagonian Elphidium. We speculate that the complex geological history of Patagonia enhanced divergence of coastal foraminiferal species and contributed to increasing genetic and morphological variation.

Published
2012
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25. Molecular identification of sequestered diatom chloroplasts and kleptoplastidy in foraminifera.

Author

Pillet L, de Vargas C, and Pawlowski J

Subjects
Base Sequence, Chloroplasts genetics, DNA, Chloroplast chemistry, DNA, Chloroplast genetics, DNA, Protozoan chemistry, DNA, Protozoan genetics, DNA, Ribosomal chemistry, DNA, Ribosomal genetics, Diatoms classification, Evolution, Molecular, Foraminifera genetics, Heterotrophic Processes, Molecular Sequence Data, Photosynthesis, Phylogeny, RNA, Ribosomal, 16S genetics, Sequence Analysis, DNA, Chloroplasts classification, Diatoms genetics, Foraminifera classification, Foraminifera microbiology
Abstract

Kleptoplastidy is the ability of heterotrophic organisms to preserve chloroplasts of algal preys they eat and partially digest. As the sequestered chloroplasts stay functional for months, the "host" becomes photosynthetically active. Although remaining a marginal process, kleptoplastidy was observed in different protist lineages, including foraminifera. Previous studies showed at least eight species of the foraminiferal genera Haynesina and Elphidium grazing on diatoms and husbanding their chloroplasts. In order to characterize more precisely the origin of kleptochloroplasts in these genera, we obtained 1027 chloroplastic 16S rDNA sequences from 13 specimens of two Haynesina and five Elphidium species. We identified the foraminiferal kleptochloroplasts using a reference phylogeny made of 87 chloroplastic sequences of known species of diatoms and brown algae. All the analyzed specimens were performing kleptoplastidy and according to our phylogenetic analyses they seem to retain exclusively chloroplasts of diatom origin. There is no apparent specificity for the type of diatom from which chloroplasts originated, however some foraminiferal species seem to accept a wider range of diatoms than others. Possibly the diversity of kleptochloroplasts depends on the type of diatoms the foraminiferans feed on., (Copyright © 2010 Elsevier GmbH. All rights reserved.)

Published
2011
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26. Improvement of monitoring of melanocytic skin lesions with the use of a computerized acquisition and surveillance unit with a skin surface microscopic television camera.

Author

Stolz W, Schiffner R, Pillet L, Vogt T, Harms H, Schindewolf T, Landthaler M, and Abmayr W

Subjects
Carcinoma, Basal Cell pathology, Dermatology instrumentation, Follow-Up Studies, Hemangioma pathology, Humans, Keratosis, Seborrheic pathology, Medical Records Systems, Computerized instrumentation, Melanoma pathology, Melanosis pathology, Nevus, Epithelioid and Spindle Cell pathology, Photography instrumentation, Software, Computers, Information Systems instrumentation, Microscopy instrumentation, Nevus, Pigmented pathology, Skin Neoplasms pathology, Television
Abstract

Background: Photographic documentation of melanocytic skin lesions is important. Storage and retrieval of slides, however, take much time and space., Objective: Our purpose was to develop and clinically test a computerized acquisition and surveillance (CAS) unit with a television camera for monitoring including measurements of lesional areas., Methods: A CAS unit connected with a skin surface microscopic television camera was used for monitoring of melanocytic nevi (MN). The lesional area and the skin surface microscopic appearance (SMA) were analyzed after 10 to 21 months in 54 of 1355 MN., Results: In 19 MN (35.2%), changes were found. In eight cases, changes in size of more or less than 15% were detected; in five cases only the SMA changed. In six cases both characteristics changed., Conclusion: In approximately 25% of MN, changes were only detectable in the SMA but not with area measurements. This favors the use of systems such as CAS because only they allow a time-saving comparison of actual and previous images.

Published
1996
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27. Engineering of protein epitopes: a single deletion in a snake toxin generates full binding capacity to a previously unrecognized antibody.

Author

Zinn-Justin S, Pillet L, Ducancel F, Thomas A, Smith JC, Boulain JC, and Ménez A

Subjects
Amino Acid Sequence, Antigen-Antibody Reactions, Cholinergic Antagonists, Cobra Neurotoxin Proteins chemistry, Cobra Neurotoxin Proteins genetics, Computer Simulation, Cross Reactions, Erabutoxins chemistry, Erabutoxins genetics, Models, Molecular, Molecular Sequence Data, Mutagenesis, Site-Directed, Protein Conformation, Recombinant Fusion Proteins chemistry, Sequence Deletion, Antibodies, Monoclonal immunology, Cobra Neurotoxin Proteins immunology, Epitopes chemistry, Erabutoxins immunology, Protein Engineering
Abstract

Structural features associated with the ability of a monoclonal antibody (mAb) to discriminate between protein variants are identified and engineered. The variants are the curaremimetic toxin alpha from Naja nigricollis and erabutoxin a or b from Laticauda semifasciata, which differ from each other by 16 substitutions and one insertion. The neutralizing mAb M alpha 1 recognizes with high affinity a topographical epitope on the surface of toxin alpha, but fails to recognize the erabutoxins although they possess most of the residues forming the presumed epitope. Examinations of the toxin alpha and erabutoxin 3-D structures and molecular dynamics simulations reveal several differences between the variants. In particular, the region involving the beta-turn 17-24 is organized differently. Analysis of the differences found in this region suggest that the insertion (or deletion) at position 18 of the variant amino acid sequences is particularly important in determining the differential cross-reactivity. To test this proposal, residue 18 was deleted in one erabutoxin using site-directed mutagenesis, and the biological properties of the resulting mutant were examined. We found that full antigenicity was restored in the previously unrecognized variant. The implications of this finding are discussed.

Published
1994
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28. Genetic engineering of snake toxins. Role of invariant residues in the structural and functional properties of a curaremimetic toxin, as probed by site-directed mutagenesis.

Author

Pillet L, Trémeau O, Ducancel F, Drevet P, Zinn-Justin S, Pinkasfeld S, Boulain JC, and Ménez A

Subjects
Amino Acid Sequence, Animals, Base Sequence, Binding Sites, Binding, Competitive, Chromatography, High Pressure Liquid, Circular Dichroism, Cloning, Molecular methods, Erabutoxins metabolism, Escherichia coli genetics, Kinetics, Molecular Sequence Data, Oligodeoxyribonucleotides, Protein Conformation, Protein Structure, Secondary, Receptors, Cholinergic metabolism, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins metabolism, Erabutoxins chemistry, Erabutoxins genetics, Genetic Engineering methods, Mutagenesis, Site-Directed, Neuromuscular Nondepolarizing Agents chemistry, Neuromuscular Nondepolarizing Agents metabolism
Abstract

To study the site by which erabutoxin a (Ea) from Laticauda semifasciata binds to the nicotinic acetylcholine receptor, we mutated most residues that are shared with other curaremimetic toxins and studied the structural and biological consequences of introduced mutations. By site-directed mutagenesis, we changed Ser-8 into Gly (EaS8G), Lys-27 into Glu (EaK27E), Trp-29 into Phe (EaW29F) and His (EaW29H), Asp-31 into His (EaD31H), Phe-32 into Leu (EaF32L), Arg-33 into Lys (EaR33K) and Glu (EaR33E), Gly-34 into Ser (EaG34S), Glu-38 into Gln (EaE38Q) and Lys (EaE38K), Gly-49 into Val (EaG49V), and Leu-52 into Ala (EaL52A). All mutants were homogeneous as judged by various analytical procedures. EaE38Q, EaG49V, and EaL52A bound the nicotinic acetylcholine receptor with apparent Kd values close to 10(-10) M, virtually identical to wild Ea. Therefore, Glu-38, Gly-49, and Leu-52 are not important elements in the expression of curaremimetic function in Ea. Mutations of Phe-32 and Gly-34 provoked a 7-fold affinity decrease, suggesting that these residues moderately contribute to function. The 176-fold affinity decrease due to mutation of Ser-8 may reflect some structural change that operates in the polypeptide chain of the mutant, as detected by circular dichroism. Decreases in affinity by a factor of 175, 67, 46, and 318 were seen upon mutations of Lys-27 into Glu, Trp-29 into Phe, Asp-31 into His, and Arg-33 into Glu, with no concomitant change in secondary structure. These residues appear to be important elements of the curaremimetic function of Ea. Thus, a picture of the contribution of conserved residues to the function of a curaremimetic toxin is proposed on the basis of experimental evidence.

Published
1993

29. Role and environment of the conserved Lys27 of snake curaremimetic toxins as probed by chemical modifications, site-directed mutagenesis and photolabelling experiments.

Author

Hervé M, Pillet L, Humbert P, Trémeau O, Ducancel F, Hirth C, and Ménez A

Subjects
Amino Acid Sequence, Animals, Binding Sites, Binding, Competitive, Cell Membrane metabolism, Cobra Neurotoxin Proteins genetics, Cross-Linking Reagents, Erabutoxins genetics, Neurotoxins metabolism, Recombinant Proteins metabolism, Structure-Activity Relationship, Cobra Neurotoxin Proteins metabolism, Erabutoxins metabolism, Lysine, Mutagenesis, Site-Directed, Receptors, Nicotinic metabolism
Abstract

The positive charge of Lys27 was suppressed by chemical means in two short-chain curaremimetic toxins, namely erabutoxin a (Ea) from Laticauda semifasciata and toxin alpha from Naja nigricollis. This modification leads to a decrease in the binding affinity of the toxins for the nicotinic acetylcholine receptor, which range 6-15-fold, as judged from both the data reported here and those previously described in the literature. A negatively charged glutamate residue has been introduced at position 27 of erabutoxin a by site-directed mutagenesis. This change provokes a 120-fold decrease in the affinity, which reflects a major alteration of toxin-receptor cognate events. Using toxin-alpha derivative harbouring a photoactive group at Lys27, we probed the toxin local environment in a receptor-bound state by photocoupling experiments. The delta chain was the predominant coupling target, in contrast to previous observations indicating that a photoactive probe on Lys47 predominantly labelled the alpha chain. The toxin derivative weakly labelled the alpha and gamma chains but not the beta chain. The toxin may therefore interact with subunits other than the alpha chain, at least in the vicinity of Lys27.

Published
1992
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30. Anti-idiotypic and anti-anti-idiotypic responses to a monoclonal antibody directed to the acetylcholine receptor binding site of curaremimetic toxins.

Author

Pillet L, Charpentier I, Léonetti M, and Ménez A

Subjects
Animals, Antibodies, Anti-Idiotypic isolation & purification, Antibodies, Monoclonal isolation & purification, Autoimmune Diseases immunology, Binding Sites, Immunization, Myasthenia Gravis immunology, Nicotine immunology, Protein Conformation, Rabbits, Antibodies, Anti-Idiotypic immunology, Antibodies, Monoclonal immunology, Cobra Neurotoxin Proteins immunology, Neuromuscular Nondepolarizing Agents immunology, Receptors, Cholinergic immunology
Abstract

Serotherapy, an approach currently used to protect humans against animal bites or stings, is often too specific. To broaden antiserum paraspecificity, use of antibodies directed against areas shared by all members of a toxin family was previously proposed. MST2 is a mAb that recognizes all long-chain curaremimetic toxins (Charpentier et al. (1990) J. Mol. Recog. 3, 74-81). It binds to toxin residues that make contact with the toxin's target, e.g., the nicotinic acetylcholine receptor (AcChoR). We now show that MST2 also recognizes (-) nicotine, an agonist of AcChoR. Binding properties of MST2 therefore mimick, at least partially, binding properties of AcChoR. Injection in rabbits of MST2 mixed with adjuvant, elicited anti-idiotypic (anti-Id) antibodies that inhibited binding of the toxin to AcChoR. A proportion of these anti-Id antibodies specifically bound AcChoR and thereby mimicked the toxin. Furthermore, rabbits immunized with MST2 elicited auto-anti-anti-Id antibodies capable of binding the toxin. Our data provide a molecular explanation for the previously reported signs of myasthenia gravis as triggered by antibodies raised against cholinergic antagonists. Implications in the design of antisera to toxic proteins are discussed.

Published
1992
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31. Immunization with a peptide having both T cell and conformationally restricted B cell epitopes elicits neutralizing antisera against a snake neurotoxin.

Author

Léonetti M, Pillet L, Maillère B, Lamthanh H, Frachon P, Couderc J, and Ménez A

Subjects
Amino Acid Sequence, Animals, Antibody Formation, Circular Dichroism, Epitopes, Lymphocyte Activation, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Peptides, Cyclic immunology, Protein Conformation, Structure-Activity Relationship, Vaccines, Synthetic, B-Lymphocytes immunology, Cobra Neurotoxin Proteins immunology, Peptides immunology, T-Lymphocytes immunology
Abstract

We have synthesized a free peptide capable of eliciting antibodies that neutralize toxin alpha from Naja nigricollis, a protein that binds specifically to the acetylcholine nicotinic receptor. Of the five tested fragments that encompassed the whole toxin sequence, only fragment 24-41 stimulated T cells from BALB/c mice primed with the whole toxin and conversely, only T cells from mice primed with fragment 24-41 could be stimulated by both the toxin and priming peptide. No other peptides had such properties, indicating that only fragment 24-41 possessed T determinant(s) in BALB/c mice (H-2d haplotype). In agreement with the current view that B cell proliferation requires specific T cell stimulation, only fragment 24-41 elicited an antibody response. However, the antipeptide antisera failed to bind to the native toxin and thereby to neutralize it. Instead, it recognized an unfolded form of the toxin. The peptide 24-41 was then made cyclic. A circular dichroism analysis revealed that, in organic solvent, this peptide had a tendency to adopt a beta-sheet structure, as in the folded toxin, whereas the linear peptide adopted an helical structure. The cyclic peptide not only remained T stimulating but elicited antisera that recognized and neutralized the native toxin. Furthermore, the antisera cross-reacted with several toxin variants. Our data show, therefore, that it is possible to give an appropriate B cell specificity directly to a T cell-stimulating peptide, an approach that may be of value for the design of synthetic vaccines.

Published
1990

32. A recombinant snake neurotoxin generated by chemical cleavage of a hybrid protein recovers full biological properties.

Author

Boyot P, Pillet L, Ducancel F, Boulain JC, Tremeau O, and Ménez A

Subjects
Amino Acid Sequence, Amino Acids analysis, Antibodies, Monoclonal immunology, Chromatography, High Pressure Liquid, Circular Dichroism, Cyanogen Bromide, Elapid Venoms immunology, Molecular Sequence Data, Neurotoxins immunology, Protein Conformation, Recombinant Fusion Proteins, Staphylococcal Protein A, Elapid Venoms genetics, Neurotoxins genetics
Abstract

We previously reported the production of a fused snake neurotoxin composed of protein A and erabutoxin a in E. coli. The hybrid had much lower toxicity and affinity for the acetylcholine nicotinic receptor than natural erabutoxin. By treating the hybrid with cyanogen bromide we generated a toxin which was purified in a single step by RP-HPLC. This compound, produced in a good yield, recovered all properties of native erabutoxin a, implying that the lower toxic activities of the hybrid were due to the bulky protein A and not to an incorrect folding of the toxin. This work serves as a basis for future studies of toxin-receptor interactions using engineered toxin mutants.

Published
1990
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33. Recognition of the acetylcholine receptor binding site of a long-chain neurotoxin by toxin-specific monoclonal antibodies.

Author

Charpentier I, Pillet L, Karlsson E, Couderc J, and Ménez A

Subjects
Amino Acid Sequence, Animals, Antibodies, Monoclonal, Binding Sites, Binding, Competitive, Cobra Neurotoxin Proteins immunology, Epitopes, In Vitro Techniques, Molecular Sequence Data, Molecular Structure, Protein Conformation, Cobra Neurotoxin Proteins metabolism, Elapid Venoms metabolism, Receptors, Nicotinic metabolism
Abstract

The present paper reports the preparation and characterization of two neutralizing monoclonal antibodies (Mabs), called MST1 and MST2, which bind at the central loop of a long-chain neurotoxin from cobra venom. The central loop is a critical region for the binding of the toxin to the nicotinic acetylcholine receptor. Some of the residues incorporated in the epitopes recognized by MST1 and MST2 have been identified on the basis of competition experiments using a set of 'chemical mutants' of the toxin. We show that MST1 and MST2 bind at the base and at the tip of the central loop of the toxin, respectively, however, only MST2 actually overlaps the acetylcholine receptor binding site. Accordingly, only MST2 is capable of recognizing all homologous toxins so far examined. MST2, therefore, mimicks, at least partially, the site by which the nicotinic acetylcholine receptor recognizes a long-chain neurotoxin.

Published
1990
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