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10. Global impact of mature biofilm lifestyle on Escherichia coli K-12 gene expression

Author

Beloin, C., Valle, J., Latour-Lambert, P., Faure, P., Kzreminski, M., Balestrino, D., Janus Anders Juul Haagensen, Søren Molin, Prensier, G., Arbeille, B., Ghigi, J. M., Génétique des Biofilms, Institut Pasteur [Paris] (IP)-Centre National de la Recherche Scientifique (CNRS), Universidad Pública de Navarra [Espagne] = Public University of Navarra (UPNA), Récepteurs et Cognition (RC), Collège de France (CdF (institution))-Institut Pasteur [Paris] (IP)-Centre National de la Recherche Scientifique (CNRS), Université d'Auvergne - Clermont-Ferrand I (UdA), BioCentrum-DTU (BiC), Danmarks Tekniske Universitet = Technical University of Denmark (DTU), Université Blaise Pascal - Clermont-Ferrand 2 (UBP), Faculté de Médecine, Laboratoire Biologie Cellulaire et Microscopie Electronique, Université Francois Rabelais [Tours], This work was supported by grants from the ‘PRFMMIP – Réseau Infections Nosocomiales’ and the Institut Pasteur., We thank Claude Lebos for preparation of the SEM micrographs. We are grateful to E. Krin for assistance in macroarray procedure. We thank T. Pugsley and C. Dorel for the kind gift of some strains used in this study, and A. Idja, J. Bellalou and R. Longin (PT5, Institut Pasteur) for technical assistance. We thank S. Da Re, B. Lakowski, C. Buchrieser, U. Dobrindt, T. Msadek, I. Lasa, M. Swanson and P. Delepelaire for critical reading of the manuscript. We also thank the referees for their helpful suggestions., Institut Pasteur [Paris]-Centre National de la Recherche Scientifique (CNRS), Collège de France (CdF (institution))-Institut Pasteur [Paris]-Centre National de la Recherche Scientifique (CNRS), and Technical University of Denmark [Lyngby] (DTU)

Subjects
MESH: Gene Expression Regulation, Bacterial, MESH: Mutation, MESH: Escherichia coli, Gene Expression Profiling, [SDV]Life Sciences [q-bio], Statistics as Topic, Gene Expression Regulation, Bacterial, MESH: Biofilms, biochemical phenomena, metabolism, and nutrition, MESH: Phenotype, MESH: Gene Expression Profiling, Phenotype, Biofilms, Mutation, MESH: Oligonucleotide Array Sequence Analysis, Escherichia coli, MESH: Statistics as Topic, Oligonucleotide Array Sequence Analysis
Abstract

International audience; The formation of biofilm results in a major lifestyle switch that is thought to affect the expression of multiple genes and operons. We used DNA arrays to study the global effect of biofilm formation on gene expression in mature Escherichia coli K-12 biofilm. We show that, when biofilm is compared with the exponential growth phase, 1.9% of the genes showed a consistent up- or downregulation by a factor greater than two, and that 10% of the E. coli genome is significantly differentially expressed. The functions of the genes induced in these conditions correspond to stress response as well as energy production, envelope biogenesis and unknown functions. We provide evidence that the expression of stress envelope response genes, such as the psp operon or elements of the cpx and rpoE pathways, is a general feature of E. coli mature biofilms. We also compared biofilm with the stationary growth phase and showed that the biofilm lifestyle, although sharing similarities with the stationary growth phase, triggers the expression of specific sets of genes. Using gene disruption of 54 of the most biofilm-induced genes followed by a detailed phenotypic study, we validated the biological relevance of our analysis and showed that 20 of these genes are required for the formation of mature biofilm. This group includes 11 genes of previously unknown function. These results constitute a comprehensive analysis of the global transcriptional response triggered in mature E. coli biofilms and provide insights into its physiological signature.

Published
2004
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11. Daily Doppler assessment of the fetal hemodynamic response to chronic hypoxia: a five-case report

Author

Salihagić, Aida, Georgescus, M., Perrotin, F., Laurini, R., Arbeille, B., Fignon, A., Zudenigo, Damir, Kurjak, Asim, and Arbeille, P.

Subjects
embryonic structures, Doppler assessment, growth-restricted fetus, chronic hypoxia
Abstract

Objective To determine whether long-term fetal brain vasodilatation and hyperperfusion (duration up to 21 days) with loss of cerebral flow velocity variability is associated with poor fetal outcome and brain damage. Study design The fetal flow redistribution was assessed by using the cerebral/umbilical resistance ratio (VU) in five growth-restricted fetuses, usually every day for 13-21 days. The evolution of the fetal hemodynamics was interpreted according to the fetal clinical, anatomical and histological findings. Results As the C/U ratio was always lower than unity during this period of observation, the fetuses were considered to be in a chronic hypoxic state. All five fetuses had a poor outcome, including death at delivery (n = 2), neonatal intensive assistance (n = 3) followed by death for two of them. The pO(2) was reduced in the two fetuses who survived for some hours and some days. The fetal deterioration was characterized by the progressive development of oligohydramnios ; the disappearance of the cerebral flow velocity, 4-10 days before delivery in all fetuses ; the occurrence of fetal heart rate decelerations in four of them ; and the increase of cerebral vascular resistance for two of them. The anatomical study of the brain in two of them showed a meningeal and periventricular congestion. The histology revealed pathological gliosis and a marked vasodilatation of both anterior and middle cerebral arteries. Conclusion The decrease in the C/U ratio (mean 30-40%) over 11-21 days, which corresponded to sustained hypoxia with increased brain perfusion, and the loss of cerebral flow variability were associated in all cases with severe growth restriction and fetal death (four cases) or very poor fetal outcome (one case). The loss of variability of the cerebral resistance index was probably related to a loss of cerebral flow regulation, or the deterioration of brain tissue. Such a pattern may be considered as a predictor of poor fetal outcome, as it occurred 4-10 days before delivery and 3-7 days before fetal heart rate abnormality or increased cerebral resistance. This hypothesis may have to be confirmed in a larger number of pathological pregnancies.

Published
2000

12. Xenogeneic cellular interaction in an ex vivo model of pig kidney perfused with human lymphocytes

Author

Khalfoun, B., Janin, P., Machet, M.C., Arbeille, B., Lacord, M., Locatelli, Aude, Salmon, Henri, Riess, G., Gruel, Y., Nivet, H., Bardos, P., Lebranchu, Y., Unité de recherche Physiologie de la reproduction des mammifères domestiques, Nouzilly, Institut National de la Recherche Agronomique (INRA), Unité de Pathologie Infectieuse et Immunologie [Nouzilly] (PII), and ProdInra, Migration

Subjects
[SDV] Life Sciences [q-bio], XENOGREFFE, [SDV]Life Sciences [q-bio], [INFO]Computer Science [cs], [INFO] Computer Science [cs], IMMUNOLOGIE, ComputingMilieux_MISCELLANEOUS
Abstract

International audience

Published
1995

15. Abnormal activation of autophagy-induced crinophagy in Paneth cells from patients with Crohn's disease.

Author

Thachil, E., Hugot, J. P., and Arbeille, B.

Subjects
AUTOPHAGY, CROHN'S disease in children, BIOPSY, INFLAMMATORY bowel disease treatment, CONTROL groups, GUANOSINE triphosphatase
Abstract

Thachil et al. have studied the role of autophagy in pediatric Crohn's disease by examining intestinal biopsies of 32 treatment-free pediatric patients with Crohn's disease, and comparing the findings with those of pediatric control subjects (four ulcerative colitis [UC] patients, nine celiac patients, and 20 "healthy controls"). Differences in autophagy were found between Crohn's disease patient samples and control samples, and also independently of genes previously associated with autophagy. The novel autophagy pathway described primarily occurred in Paneth cells, and was associated with the process of crinophagy. [ABSTRACT FROM AUTHOR]

Published
2012

20. The Centriolar Adjunct⁻Appearance and Disassembly in Spermiogenesis and the Potential Impact on Fertility.

Author

Garanina AS, Alieva IB, Bragina EE, Blanchard E, Arbeille B, Guerif F, Uzbekova S, and Uzbekov RE

Subjects
Adult, Animals, Centrioles ultrastructure, Chromatin metabolism, Humans, Infertility, Male pathology, Male, Spermatids metabolism, Spermatids ultrastructure, Swine, Tissue Donors, Centrioles metabolism, Fertility physiology, Spermatogenesis physiology
Abstract

During spermiogenesis, the proximal centriole forms a special microtubular structure: the centriolar adjunct. This structure appears at the spermatid stage, which is characterized by a condensed chromatin nucleus. We showed that the centriolar adjunct disappears completely in mature porcine spermatozoa. In humans, the centriolar adjunct remnants are present in a fraction of mature spermatids. For the first time, the structure of the centriolar adjunct in the cell, and its consequent impact on fertility, were examined. Ultrastructural analysis using transmission electron microscopy was performed on near 2000 spermatozoa per person, in two patients with idiopathic male sterility (IMS) and five healthy fertile donors. We measured the average length of the "proximal centriole + centriolar adjunct" complex in sections, where it had parallel orientation in the section plane, and found that it was significantly longer in the spermatozoa of IMS patients than in the spermatozoa of healthy donors. This difference was independent of chromatin condensation deficiency, which was also observed in the spermatozoa of IMS patients. We suggest that zygote arrest may be related to an incompletely disassembled centriolar adjunct in a mature spermatozoon. Therefore, centriolar adjunct length can be potentially used as a complementary criterion for the immaturity of spermatozoa in the diagnostics of IMS patients., Competing Interests: The authors declare no conflicts of interests.

Published
2019
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21. Microvillous atrophy: atypical presentations.

Author

Perry A, Bensallah H, Martinez-Vinson C, Berrebi D, Arbeille B, Salomon J, Goulet O, Marinier E, Drunat S, Samson-Bouma ME, Gérard B, and Hugot JP

Subjects
Atrophy, Biopsy, Diarrhea, Infantile therapy, Female, Follow-Up Studies, Gestational Age, Humans, Infant, Infant, Newborn, Malabsorption Syndromes complications, Malabsorption Syndromes genetics, Male, Microscopy, Electron, Transmission, Microvilli genetics, Mucolipidoses complications, Mucolipidoses genetics, Mutation, Myosin Heavy Chains genetics, Myosin Type V genetics, Parenteral Nutrition, Diarrhea, Infantile pathology, Malabsorption Syndromes pathology, Microvilli pathology, Mucolipidoses pathology
Abstract

Objectives: Microvillous inclusion disease (MVID) is a cause of intractable diarrhea in infancy. In its classic form, the disease is characterized by a severe persistent watery diarrhea starting within the first days of life. Parenteral nutrition and small bowel transplantation are the only known treatments for the affected children. Histologically, periodic acid-Schiff (PAS) staining shows accumulation of periodic acid-Schiff-positive staining material along the apical pole of enterocytes, whereas transmission electron microscopy exhibits microvillus inclusion bodies within the cytoplasm of enterocytes with rarefied and shortened microvilli and secretory granules. The objective of this work was to explore clinical, morphological, and genetic findings in cases of MVID with unusual presentations., Methods: Clinical, histological, and genetic findings are reported for 8 cases of MVID with atypical presentation., Results: The diarrhea started after several months in 3 cases. It was usually less abundant and 3 patients were weaned off parenteral nutrition. None required intestinal transplantation. Three patients experienced malformations, dysmorphy, sensory disabilities, and severe mental retardation. One had a hydrocephaly. Three patients had a cholestasis with low γ-glutamyl transferase levels. Light microscopy showed histological abnormalities consistent with MVID in all of the cases, but the lesions were sometimes focal or delayed. Transmission electron microscopy retrieved some criteria of MVID in 4 patients. Finally, 6 patients were homozygotes or compound heterozygotes for MYO5B mutations., Conclusions: This study extends the spectrum of MVID to less severe clinical presentations.

Published
2014
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22. Compound heterozygous mutations of the TNXB gene cause primary myopathy.

Author

Pénisson-Besnier I, Allamand V, Beurrier P, Martin L, Schalkwijk J, van Vlijmen-Willems I, Gartioux C, Malfait F, Syx D, Macchi L, Marcorelles P, Arbeille B, Croué A, De Paepe A, and Dubas F

Subjects
Adult, DNA Mutational Analysis, Humans, Male, Muscle, Skeletal diagnostic imaging, Muscle, Skeletal pathology, Muscle, Skeletal ultrastructure, Muscular Diseases pathology, Muscular Diseases physiopathology, Tenascin metabolism, Tomography, X-Ray Computed, Muscular Diseases genetics, Mutation genetics, Tenascin genetics
Abstract

Complete deficiency of the extracellular matrix glycoprotein tenascin-X (TNX) leads to recessive forms of Ehlers-Danlos syndrome, clinically characterized by hyperextensible skin, easy bruising and joint hypermobility. Clinical and pathological studies, immunoassay, and molecular analyses were combined to study a patient suffering from progressive muscle weakness. Clinical features included axial and proximal limb muscle weakness, subclinical heart involvement, minimal skin hyperextensibility, no joint abnormalities, and a history of easy bruising. Skeletal muscle biopsy disclosed striking muscle consistency and the abnormal presence of myotendinous junctions in the muscle belly. TNX immunostaining was markedly reduced in muscle and skin, and serum TNX levels were undetectable. Compound heterozygous mutations were identified: a previously reported 30kb deletion and a non-synonymous novel missense mutation in the TNXB gene. This study identifies a TNX-deficient patient presenting with a primary muscle disorder, thus expanding the phenotypic spectrum of TNX-related abnormalities. Biopsy findings provide evidence that TNX deficiency leads to muscle softness and to mislocalization of myotendinous junctions., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published
2013
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23. Cutaneous amyloid elastosis revealing multiple myeloma with systemic amyloidosis.

Author

Marchand A, Levaltier X, Croué A, Arbeille B, Ifrah N, and Martin L

Subjects
Aged, Amyloidosis drug therapy, Amyloidosis immunology, Antineoplastic Combined Chemotherapy Protocols therapeutic use, Biopsy, Boronic Acids administration & dosage, Bortezomib, Dexamethasone administration & dosage, Diagnostic Errors, Fatal Outcome, Female, Humans, Melphalan administration & dosage, Multiple Myeloma complications, Multiple Myeloma drug therapy, Multiple Myeloma immunology, Predictive Value of Tests, Pseudoxanthoma Elasticum diagnosis, Pyrazines administration & dosage, Skin immunology, Treatment Outcome, Amyloidosis pathology, Elastic Tissue pathology, Multiple Myeloma pathology, Skin pathology
Published
2013
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24. The pig as a model for investigating the role of neutrophil serine proteases in human inflammatory lung diseases.

Author

Bréa D, Meurens F, Dubois AV, Gaillard J, Chevaleyre C, Jourdan ML, Winter N, Arbeille B, Si-Tahar M, Gauthier F, and Attucci S

Subjects
Animals, Calcimycin pharmacology, Calcium Ionophores pharmacology, Cell Degranulation, Humans, In Vitro Techniques, Neutrophil Activation, Neutrophils drug effects, Neutrophils microbiology, Pneumonia blood, Pseudomonas aeruginosa physiology, Serine Proteinase Inhibitors pharmacology, Species Specificity, Staphylococcus aureus physiology, Swine, Disease Models, Animal, Neutrophils enzymology, Pneumonia enzymology, Serine Proteases metabolism
Abstract

The serine proteases released by activated polymorphonuclear neutrophils [NSPs (neutrophil serine proteases)] contribute to a variety of inflammatory lung diseases, including CF (cystic fibrosis). They are therefore key targets for the development of efficient inhibitors. Although rodent models have contributed to our understanding of several diseases, we have previously shown that they are not appropriate for testing anti-NSP therapeutic strategies [Kalupov, Brillard-Bourdet, Dade, Serrano, Wartelle, Guyot, Juliano, Moreau, Belaaouaj and Gauthier (2009) J. Biol. Chem. 284, 34084-34091). Thus NSPs must be characterized in an animal model that is much more likely to predict how therapies will act in humans in order to develop protease inhibitors as drugs. The recently developed CFTR-/- (CFTR is CF transmembrane conductance regulator) pig model is a promising alternative to the mouse model of CF [Rogers, Stoltz, Meyerholz, Ostedgaard, Rokhlina, Taft, Rogan, Pezzulo, Karp, Itani et al. (2008) Science 321, 1837-1841]. We have isolated blood neutrophils from healthy pigs and determined their responses to the bacterial pathogens Pseudomonas aeruginosa and Staphylococcus aureus, and the biochemical properties of their NSPs. We used confocal microscopy and antibodies directed against their human homologues to show that the three NSPs (elastase, protease 3 and cathepsin G) are enzymatically active and present on the surface of triggered neutrophils and NETs (neutrophil extracellular traps). All of the porcine NSPs are effectively inhibited by human NSP inhibitors. We conclude that there is a close functional resemblance between porcine and human NSPs. The pig is therefore a suitable animal model for testing new NSP inhibitors as anti-inflammatory agents in neutrophil-associated diseases such as CF.

Published
2012
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25. Ultrastructural scoring of skin biopsies for diagnosis of vascular Ehlers-Danlos syndrome.

Author

Ong KT, Plauchu H, Peyrol S, Roux E, Errazuriz E, Khau Van Kien P, Arbeille B, Gaulier A, Georgescou G, Collignon P, Germain DP, Gaveau MN, Perdu J, Laurent S, Bruneval P, and Boutouyrie P

Subjects
Biopsy, Collagen Type III ultrastructure, Ehlers-Danlos Syndrome genetics, Ehlers-Danlos Syndrome pathology, Humans, Collagen Type III genetics, Ehlers-Danlos Syndrome diagnosis, Skin ultrastructure
Abstract

Vascular Ehlers-Danlos syndrome (vEDS) results from a mutation in the gene encoding alpha-1, type III pro-collagen (COL3A1) and confers fragility to skin, ligament and vascular tissue. We tested the value of skin biopsy for diagnosis of vEDS through an ultrastructure scoring procedure. Study design was a multicentric, case-control, blinded trial consisting of two phases: phase 1 was to identify an ultra-structure score providing the best discriminative value for vEDS and phase 2 was to replicate this result in a different population. We enrolled 103 patients, 66 cases defined through the revised nosology for Ehlers-Danlos syndromes and 37 control subjects selected from patients referred for other pathologies. Ultrastructure of extracellular matrix was read by three to five experienced pathologists blinded for diagnosis. We used the receiver operating curves and logistic regression analysis for ranking ultrastructure scores. We created a detailed description of lesions observed in vEDS patients with 27 items (coded 0 or 1). In the phase 1 (17 cases and 20 controls), abnormal fibroblast shape, presence of lysosomes in the fibroblast and abnormal basal lamina were found to be independent discriminative items. Addition of these three items (defining an ultrastructure score) had the best diagnosis value (area under the curve (AUC) = 0.96). In the phase 2 (49 cases, 17 controls), ultrastructure score provided odds ratio of 9.76 (95 % CI 2.91-32.78), and AUC of 0.90. The ultrastructure score of skin biopsy has predictive value for the diagnosis of vEDS. Presence of two or more signs (either abnormal fibroblast, presence of lysosomes in the fibroblast or abnormal basal lamina) is very evocative of vEDS.

Published
2012
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26. Abnormal activation of autophagy-induced crinophagy in Paneth cells from patients with Crohn's disease.

Author

Thachil E, Hugot JP, Arbeille B, Paris R, Grodet A, Peuchmaur M, Codogno P, Barreau F, Ogier-Denis E, Berrebi D, and Viala J

Subjects
Autophagy-Related Proteins, Carrier Proteins genetics, Child, Female, GTP-Binding Proteins genetics, Humans, Infant, Male, Microtubule-Associated Proteins analysis, Nod2 Signaling Adaptor Protein genetics, Polymorphism, Single Nucleotide, Autophagy physiology, Crohn Disease pathology, Paneth Cells ultrastructure, Secretory Vesicles physiology
Abstract

Autophagy-related 16 like-1 (ATG16L-1), immunity-related GTPase-M (IRGM), and nucleotide-binding oligomerization domain-containing 2 (NOD2) regulate autophagy, and variants in these genes have been associated with predisposition to Crohn's disease (CD). However, little is known about the role of autophagy in CD. Intestinal biopsies from untreated pediatric patients with CD, celiac disease, or ulcerative colitis were analyzed by immunohistochemistry and electron microscopy. We observed that autophagy was specifically activated in Paneth cells from patients with CD, independently of mucosal inflammation or disease-associated variants of ATG16L1 or IRGM. In these cells, activation of autophagy was associated with a significant decrease in number of secretory granules and features of crinophagy. These observations might account for the disorganization of secretory granules previously reported in Paneth cells from patients with CD., (Copyright © 2012 AGA Institute. Published by Elsevier Inc. All rights reserved.)

Published
2012
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27. Platelet type III collagen binding protein (TIIICBP) presents high biochemical and functional similarities with kindlin-3.

Author

Djaafri I, Maurice P, Labas V, Vinh J, Lemesle M, Arbeille B, Legrand C, Mourah S, and Fauvel-Lafeve F

Subjects
Adenosine Diphosphate pharmacology, Amino Acid Sequence, Antibodies metabolism, Blood Platelets drug effects, Crotalid Venoms pharmacology, Humans, Immunoprecipitation, Lectins, C-Type, Membrane Proteins chemistry, Molecular Sequence Data, Neoplasm Proteins chemistry, Platelet Activation drug effects, Platelet Adhesiveness drug effects, Platelet Aggregation drug effects, Platelet Membrane Glycoproteins metabolism, Receptors, Collagen chemistry, Sequence Homology, Amino Acid, Thrombin pharmacology, Blood Platelets metabolism, Collagen Type III metabolism, Membrane Proteins metabolism, Neoplasm Proteins metabolism, Receptors, Collagen metabolism
Abstract

Type III collagen binding protein (TIIICBP) was previously described as a platelet membrane protein that recognizes the KOGEOGPK peptide sequence within type III collagen. In order to better characterize this protein, we performed different approaches including mass spectrometry sequencing and functional experiments. This study leads to identify high biochemical and functional similarities between TIIICBP and kindlin-3, a member of a family of focal adhesion proteins. Indeed, mass spectrometry surveys indicated that TIIICBP contains several peptides identical to kindlin-3, covering 41% of the amino acid sequence. Polyclonal antibodies raised against a kindlin-3 specific N-terminal sequence, recognized and immunoprecipitated TIIICBP from platelet lysates. Electron microscopy and flow cytometry experiments showed that kindlin-3, as well as TIIICBP, were present associated to platelet membrane and a translocation of cytosolic kindlin-3 to the platelet membrane was observed after platelet activation. Similarly to anti-TIIICBP antibodies and the KOGEOGPK peptide, anti-kindlin-3 antibodies inhibited platelet interactions with type III collagen under flow conditions and slowed down platelet aggregation induced by glycoprotein VI agonists; e.g. collagen-related peptides and convulxin. In addition, the anti-kindlin-3 antibody inhibited platelet aggregation induced by low - but not high - doses of ADP or thrombin which depends on α(IIb)β(3) integrin function. In conclusion, our results show that the peptides identified by mass spectrometry from purified TIIICBP correspond to the kindlin-3 protein and demonstrate biochemical and functional similarities between TIIICBP and kindlin-3, strengthening a key role for TIIICBP/kindlin-3 in platelet interactions with collagen by cooperating with glycoprotein VI activation and integrin clustering in focal adhesion complexes., (Copyright © 2011 Elsevier Masson SAS. All rights reserved.)

Published
2012
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28. Stimulation of kainate toxicity by zinc in cultured cerebellar granule neurons and the role of mitochondria in this process.

Author

Lozier ER, Stelmashook EV, Uzbekov RE, Novikova SV, Zorov SD, Alieva IB, Arbeille B, Zorov DB, and Isaev NK

Subjects
Animals, Calcium metabolism, Cells, Cultured, Cerebellum cytology, Drug Synergism, Rats, Rats, Wistar, Zinc metabolism, Cerebellum drug effects, Chlorides toxicity, Excitatory Amino Acid Agonists toxicity, Kainic Acid toxicity, Mitochondria drug effects, Neurons drug effects, Zinc toxicity, Zinc Compounds toxicity
Abstract

Zinc chloride (0.01 mM kept for 3h) is not toxic to cultured cerebellar granule neurons (CGNs) while kainate (0.1mM kept for 3h) demonstrates some but very low toxicity towards these cells. Measurements of the relative intraneuronal zinc ion concentration showed that increase in [Zn(2+)](i) under the simultaneous action of ZnCl(2) and kainate was significantly stronger compared to their separate action. Simultaneous treatment of CGNs with kainate and zinc chloride caused the swelling of neuronal mitochondria and consequent intensive neuronal death, which was totally prevented by NBQX (an AMPA/kainate-receptors blocker) or ruthenium red (a mitochondrial Ca(2+) uniporter blocker). These data imply that Zn(2+) synergistically to kainate increase their separate toxic effects on mitochondria leading to rapid neuronal death., (Copyright © 2011 Elsevier Ireland Ltd. All rights reserved.)

Published
2012
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29. Ultrasound and microbubble-assisted gene delivery in Achilles tendons: long lasting gene expression and restoration of fibromodulin KO phenotype.

Author

Delalande A, Bouakaz A, Renault G, Tabareau F, Kotopoulis S, Midoux P, Arbeille B, Uzbekov R, Chakravarti S, Postema M, and Pichon C

Subjects
Achilles Tendon pathology, Animals, DNA administration & dosage, DNA genetics, Fibromodulin, Gene Expression Regulation, Luciferases genetics, Mice, Mice, Knockout, Phenotype, Plasmids genetics, Transgenes, Achilles Tendon metabolism, Extracellular Matrix Proteins genetics, Microbubbles, Plasmids administration & dosage, Proteoglycans genetics, Transfection, Ultrasonics
Abstract

The aim of this study is to deliver genes in Achilles tendons using ultrasound and microbubbles. The rationale is to combine ultrasound-assisted delivery and the stimulation of protein expression induced by US. We found that mice tendons injected with 10 μg of plasmid encoding luciferase gene in the presence of 5×10⁵ BR14 microbubbles, exposed to US at 1 MHz, 200 kPa, 40% duty cycle for 10 min were efficiently transfected without toxicity. The rate of luciferase expression was 100-fold higher than that obtained when plasmid alone was injected. Remarkably, the luciferase transgene was stably expressed for up to 108 days. DNA extracted from these sonoporated tendons was efficient in transforming competent E. coli bacteria, indicating that persistent intact pDNA was responsible for this long lasting gene expression. We used this approach to restore expression of the fibromodulin gene in fibromodulin KO mice. A significant fibromodulin expression was detected by quantitative PCR one week post-injection. Interestingly, ultrastructural analysis of these tendons revealed that collagen fibrils diameter distribution and circularity were similar to that of wild type mice. Our results suggest that this gene delivery method is promising for clinical applications aimed at modulating healing or restoring a degenerative tendon while offering great promise for gene therapy due its safety compared to viral methods., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published
2011
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30. Changes in the Daphnia magna midgut upon ingestion of copper oxide nanoparticles: a transmission electron microscopy study.

Author

Heinlaan M, Kahru A, Kasemets K, Arbeille B, Prensier G, and Dubourguier HC

Subjects
Animals, Eating, Daphnia ultrastructure, Gastrointestinal Tract ultrastructure, Metal Nanoparticles chemistry, Microscopy, Electron, Transmission methods, Zinc Oxide chemistry
Abstract

This work is a follow-up of our previous paper (Heinlaan et al., 2008. Chemosphere 71, 1308-1316) where we showed about 50-fold higher acute toxicity of CuO nanoparticles (NPs) compared to bulk CuO to water flea Daphnia magna. In the current work transmission electron microscopy (TEM) was used to determine potential time-dependent changes in D. magna midgut epithelium ultrastructure upon exposure to CuO NPs compared to bulk CuO at their 48 h EC(50) levels: 4.0 and 175 mg CuO/L, respectively. Special attention was on potential internalization of CuO NPs by midgut epithelial cells. Ingestion of both CuO formulations by daphnids was evident already after 10 min of exposure. In the midgut lumen CuO NPs were dispersed whereas bulk CuO was clumped. By the 48th hour of exposure to CuO NPs (but not to equitoxic concentrations of bulk CuO) the following ultrastructural changes in midgut epithelium of daphnids were observed: protrusion of epithelial cells into the midgut lumen, presence of CuO NPs in circular structures analogous to membrane vesicles from holocrine secretion in the midgut lumen. Implicit internalization of CuO NPs via D. magna midgut epithelial cells was not evident however CuO NPs were no longer contained within the peritrophic membrane but located between the midgut epithelium microvilli. Interestingly, upon exposure to CuO NPs bacterial colonization of the midgut occurred. Ultrastructural changes in the midgut of D. magna upon exposure to CuO NPs but not to bulk CuO refer to its nanosize-related adverse effects. Time-dependent solubilisation of CuO NPs and bulk CuO in the test medium was quantified by recombinant Cu-sensor bacteria: by the 48th hour of exposure to bulk CuO, the concentration of solubilised copper ions was 0.05 ± 0.01 mg Cu/L that was comparable to the acute EC(50) value of Cu-ions to D. magna (48 h CuSO(4) EC(50) = 0.07 ± 0.01 mg Cu/L). However, in case of CuO NPs, the solubilised Cu-ions 0.01 ± 0.001 mg Cu/L, explained only part of the toxicity., (Copyright © 2010 Elsevier Ltd. All rights reserved.)

Published
2011
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31. The interperiosteo-dural concept applied to the perisellar compartment: a microanatomical and electron microscopic study.

Author

François P, Travers N, Lescanne E, Arbeille B, Jan M, and Velut S

Subjects
Adult, Humans, Microscopy, Electron, Scanning, Cranial Sinuses anatomy & histology, Dura Mater anatomy & histology, Skull Base anatomy & histology
Abstract

Object: The dura mater has 2 dural layers: the endosteal layer (outer layer), which is firmly attached to the bone, and the meningeal layer (inner layer), which directly covers the brain. These 2 dural layers join together in the middle temporal fossa or the convexity and separate into the orbital, lateral sellar compartment (LSC), or spinal epidural space to form the extradural neural axis compartment (EDNAC). The aim of this work was to anatomically verify the concept of the EDNAC by using electron microscopy., Methods: The authors studied the cadaveric heads obtained from 13 adults. Ten of the specimens (or 20 perisellar areas) were injected with colored latex and fixed in formalin. They carefully removed each brain to allow a superior approach to the perisellar area. The 3 other specimens were studied by microscopic and ultrastructural methods to describe the EDNAC in the perisellar area. Special attention was paid to the dural layers surrounding the perisellar area. The authors studied the anatomy of the meningeal architecture of the LSC, the petroclival venous confluence, the orbit, and the trigeminal cave. After dissection, the authors took photographs of the dural layers with the aid of optical magnification. The 3 remaining heads, obtained from fresh cadavers, were prepared for electron microscopic study., Results: The EDNAC is limited by the endosteal layer and the meningeal layer and contains fat and/or venous blood. The endosteal layer and meningeal layer were not identical on electron microscopy; this finding can be readily related to the histology of the meninges., Conclusions: In this study, the authors demonstrated the existence of the EDNAC concept in the perisellar area by using dissected cadaveric heads and verified the reality of the concept of the meningeal layer with electron microscopy. These findings clearly demonstrated the existence of the EDNAC, a notion that has generally been accepted but never demonstrated microscopically.

Published
2010
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32. Ultrastructural demonstration of a relationship between acquired cutis laxa and monoclonal gammopathy.

Author

Maruani A, Arbeille B, Machet MC, Barbet C, Laure B, Martin L, and Machet L

Subjects
Adult, Autoantibodies analysis, Collagen ultrastructure, Cutis Laxa immunology, Dermis immunology, Elastic Tissue ultrastructure, Humans, Immunoglobulin lambda-Chains immunology, Immunohistochemistry, Male, Microscopy, Electron, Paraproteinemias immunology, Cutis Laxa pathology, Dermis ultrastructure, Paraproteinemias pathology
Abstract

Acquired cutis laxa is an uncommon disorder sometimes associated with monoclonal gammopathy and multiple myeloma, although the mechanism of this link is unclear. We report here a case of a 34-year-old man with generalized acquired cutis laxa and monoclonal light chain disease with renal and neurological involvement. Electron microscopy examination of a skin sample revealed shortened and fragmented elastic fibres in the reticular dermis and normal collagen bundles. Immunogold labelling revealed anti-lambda antibodies closely bound to the microfibrillar component of elastic fibres, thus supporting a causal relationship between monoclonal gammopathy and the changes in skin elasticity.

Published
2010
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33. Effect of transitory glucose deprivation on mitochondrial structure and functions in cultured cerebellar granule neurons.

Author

Stelmashook EV, Isaev NK, Plotnikov EY, Uzbekov RE, Alieva IB, Arbeille B, and Zorov DB

Subjects
Animals, Calcium metabolism, Cells, Cultured, Membrane Potential, Mitochondrial, Mitochondria ultrastructure, Neurons ultrastructure, Rats, Rats, Wistar, Cerebellum cytology, Glucose deficiency, Mitochondria physiology, Neurons physiology
Abstract

We found that 60-min glucose deprivation leads to progressive decrease in the mitochondrial membrane potential and increase in [Ca(2+)](i) in cultured cerebellar granule neurons. The latter effect was fully reversible, returning to the basal level 60 min after restoration of normal glucose level in the incubation medium, whereas mitochondrial membrane potential remained at 10.0+/-1.8% below the initial value. Electron microscopy indicated that glucose deprivation induced appearance of mitochondria with local lightening of the matrix and destruction of cristae. This mitochondrial conformation was preserved during the restoration phase after glucose level in the cultivation medium returned to the normal level. Neuronal death within a 24-h period after 60-min glucose deprivation was relatively small, being 14.0+/-4.4%.

Published
2009
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34. Breast tumor cells transendothelial migration induces endothelial cell anoikis through extracellular matrix degradation.

Author

Peyri N, Berard M, Fauvel-Lafeve F, Trochon V, Arbeille B, Lu H, Legrand C, and Crepin M

Subjects
Blotting, Western, Cells, Cultured, Coculture Techniques, Female, Humans, Immunoenzyme Techniques, Matrix Metalloproteinase 14 metabolism, Matrix Metalloproteinases metabolism, Umbilical Veins cytology, Anoikis, Breast Neoplasms pathology, Cell Movement, Endothelium, Vascular pathology, Extracellular Matrix metabolism
Abstract

Mutual interactions between human breast cancer cells and endothelial cells were studied in a model mimicking tumor cell intravasation. MDA-MB-231 tumor cells and human umbilical vein endothelial cells (HUVEC) were cocultured on opposite sides of a Transwell filter allowing tumor cell contacts with the basement membrane of the HUVEC forming endothelium and tumor cell transendothelial migration. Confocal microscopy analysis showed that transmigrating MDA-MB-231 cells lay under the HUVEC, thereby inducing HUVEC detachment and tumor cell-HUVEC contact-dependent apoptosis. GM6001 a matrix metalloproteinase (MMP) inhibitor inhibited almost completely, the MDA-MB-231 cell transendothelial migration and the anoikis process. In this intravasation model, a tumor cell invasive mechanism was demonstrated (i) induction of extensive endothelial anoikis induced by degradation of the extracellular matrix (ECM) components, (ii) activation of pro-matrix metalloproteinase (MMP)-2 into MMP-2 by the MT1-MMP-TIMP (tissue inhibitor metalloproteinase) 2-pro-MMP-2 membrane complex and (iii) attraction and migration of metastatic cell through apoptotic endothelium. These interactions could partly explain the necrosis-angiogenesis relationship in tumor angiogenesis.

Published
2009

35. Very-high-frequency ultrasound corneal imaging as a new tool for early diagnosis of ocular surface toxicity in rabbits treated with a preserved glaucoma drug.

Author

Denoyer A, Ossant F, Arbeille B, Fetissof F, Patat F, Pourcelot L, and Pisella PJ

Subjects
Animals, Conjunctival Diseases chemically induced, Cornea drug effects, Epithelium, Corneal diagnostic imaging, Epithelium, Corneal drug effects, Keratitis chemically induced, Male, Microscopy, Electron, Scanning, Prospective Studies, Rabbits, Radio Waves, Timolol toxicity, Ulcer chemically induced, Ultrasonography, Antihypertensive Agents toxicity, Benzalkonium Compounds toxicity, Conjunctival Diseases diagnostic imaging, Cornea diagnostic imaging, Keratitis diagnostic imaging, Preservatives, Pharmaceutical toxicity, Ulcer diagnostic imaging
Abstract

Aim: To evaluate very-high-frequency (VHF) ultrasound imaging as a new method to detect and quantify early corneal epithelium changes induced by chronic exposure to a benzalkonium-chloride-containing antiglaucoma drug., Methods: Timolol preserved with 0.01% benzalkonium chloride solution was applied b.i.d. in 1 eye of 10 rabbits for 56 days. Unpreserved timolol solution was used as control. Ocular surface changes were assessed weekly combining clinical examinations, in vivo 60-MHz ultrasound imaging and ex vivo histological analysis., Results: VHF ultrasound imaging allowed quantitative measurement of corneal epithelium thickness and qualitative imaging of toxic epithelial damage. It revealed significantly decreased epithelial thickness in vivo as early as the 21st day of treatment (40.75 +/- 1.72 microm at D0 vs. 39 +/- 2 at D21, vs. 31.9 +/- 2.98 at D56; p = 0.017 and p = 0.005, respectively). The first clinical changes appeared from the 42nd day of treatment (conjunctival redness, conjunctival staining and corneal staining; D56 compared to D0: p = 0.005, 0.01 and 0.004, respectively) and then correlated with VHF ultrasound data. Epithelial thickness measured with VHF ultrasound was correlated with histological epithelial pachymetry (p < 0.001) and with the corneal damage score assessed with scanning electron microscopy (p = 0.038)., Conclusion: VHF ultrasound imaging provided an early in vivo diagnosis of corneal epithelium pathology induced by chronic exposure to a preserved glaucoma drug, before the first clinical evidence of ocular toxicity. It could be a new reproducible method to detect the toxicity of glaucoma medication so that therapy can then be adapted., (Copyright 2008 S. Karger AG, Basel.)

Published
2008
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36. Contractile and relaxant properties of rat-isolated pulmonary veins related to localization and histology.

Author

Bronquard C, Maupoil V, Arbeille B, Fetissof F, Findlay I, Cosnay P, and Freslon JL

Subjects
15-Hydroxy-11 alpha,9 alpha-(epoxymethano)prosta-5,13-dienoic Acid pharmacology, Acetylcholine pharmacology, Adrenergic beta-2 Receptor Agonists, Adrenergic beta-2 Receptor Antagonists, Adrenergic beta-Agonists pharmacology, Adrenergic beta-Antagonists pharmacology, Albuterol pharmacology, Angiotensin II pharmacology, Animals, Bradykinin pharmacology, Bronchi, Endothelium, Vascular drug effects, Endothelium, Vascular physiology, Heart Atria, In Vitro Techniques, Isoproterenol pharmacology, Male, Nitroprusside pharmacology, Phenylephrine pharmacology, Propanolamines pharmacology, Pulmonary Veins anatomy & histology, Pulmonary Veins drug effects, Rats, Rats, Wistar, Receptors, Adrenergic, beta-2 physiology, Vasoconstriction drug effects, Vasoconstrictor Agents pharmacology, Vasodilation drug effects, Vasodilator Agents pharmacology, Pulmonary Veins physiology, Vasoconstriction physiology, Vasodilation physiology
Abstract

The aim of this study was to investigate the in vitro vasomotor properties of rat extra-and intralobar pulmonary veins (PVs) related to their localization and to assess the modulatory role of endothelium on these properties. Segments from PVs were mounted in small vessel myograph and stretched at various diameters (D(10), D(20), D(30)) corresponding to intraluminal pressures of 10, 20 or 30 mmHg. At D(10) or D(20), contractile responses to phenylephrine, U46619 and angiotensin II of distal intralobar part of PVs were smaller compared with those of proximal extralobar part, but no longer different when distal part was stretched at D(30). When submitted to an NO donor, sodium nitroprusside, distal part of PV relaxed more strongly when stretched at D(30) compared with D(10). Acetylcholine and bradykinin were devoid of relaxing effect on distal parts stretched at D(10), but in contrast to acetylcholine, bradykinin slightly relaxed preparations stretched at D(30). Isoprenaline strongly relaxed PVs ( approximately 80% of initial precontraction), with the distal part exhibiting a higher sensitivity to the agonist compared with the proximal part. This relaxation was also observed with salbutamol and suppressed with ICI 118551, which is in favour of the involvement of beta(2)-adrenoceptors in this effect. Preincubation of the preparations with N(G)-nitro-l-arginine methyl ester (10(-4) m) and indomethacin (10(-5) m) did not modify the contractile responses to U46619, nor the relaxing response to isoprenaline, which support that endothelium does not appear to play a significant modulatory role in these responses. Histological and electron microscopical examinations of proximal and distal sections of the same vein show that the layers of smooth muscle cells and cardiomyocytes were thicker in the proximal compared with the distal part. This study shows that, because of morphological heterogeneity of the PVs, the site of dissection and the initial condition of tension can play a significant role upon the sensitivity and the magnitude of the responses to both contractile and relaxing agonists.

Published
2007
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37. The platelet receptor for type III collagen (TIIICBP) is present in platelet membrane lipid microdomains (rafts).

Author

Maurice P, Waeckel L, Pires V, Sonnet P, Lemesle M, Arbeille B, Vassy J, Rochette J, Legrand C, and Fauvel-Lafève F

Subjects
Blood Platelets ultrastructure, Cell Membrane metabolism, Cell Membrane ultrastructure, Cholesterol metabolism, Cytoskeleton metabolism, Cytoskeleton ultrastructure, Humans, Integrin alpha2beta1 metabolism, Membrane Microdomains ultrastructure, Peptide Fragments metabolism, Platelet Membrane Glycoproteins metabolism, Blood Platelets metabolism, Collagen Type III metabolism, Membrane Microdomains metabolism, Receptors, Collagen metabolism
Abstract

Platelet interactions with collagen are orchestrated by the presence or the migration of platelet receptor(s) for collagen into lipid rafts, which are specialized lipid microdomains from the platelet plasma membrane enriched in signalling proteins. Electron microscopy shows that in resting platelets, TIIICBP, a receptor specific for type III collagen, is present on the platelet membrane and associated with the open canalicular system, and redistributes to the platelet membrane upon platelet activation. After platelet lysis by 1% Triton X-100 and the separation of lipid rafts on a discontinuous sucrose gradient, TIIICBP is recovered in lipid raft-containing fractions and Triton X-100 insoluble fractions enriched in cytoskeleton proteins. Platelet aggregation, induced by type III collagen, was inhibited after disruption of the lipid rafts by cholesterol depletion, whereas platelet adhesion under static conditions did not require lipid raft integrity. These results indicate that TIIICBP, a platelet receptor involved in platelet interaction with type III collagen, is localized within platelet lipid rafts where it could interact with other platelet receptors for collagen (GP VI and alpha2beta1 integrin) for efficient platelet activation.

Published
2006
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38. Global impact of mature biofilm lifestyle on Escherichia coli K-12 gene expression.

Author

Beloin C, Valle J, Latour-Lambert P, Faure P, Kzreminski M, Balestrino D, Haagensen JA, Molin S, Prensier G, Arbeille B, and Ghigo JM

Subjects
Gene Expression Profiling, Mutation, Oligonucleotide Array Sequence Analysis, Phenotype, Statistics as Topic, Biofilms, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression Regulation, Bacterial
Abstract

The formation of biofilm results in a major lifestyle switch that is thought to affect the expression of multiple genes and operons. We used DNA arrays to study the global effect of biofilm formation on gene expression in mature Escherichia coli K-12 biofilm. We show that, when biofilm is compared with the exponential growth phase, 1.9% of the genes showed a consistent up- or downregulation by a factor greater than two, and that 10% of the E. coli genome is significantly differentially expressed. The functions of the genes induced in these conditions correspond to stress response as well as energy production, envelope biogenesis and unknown functions. We provide evidence that the expression of stress envelope response genes, such as the psp operon or elements of the cpx and rpoE pathways, is a general feature of E. coli mature biofilms. We also compared biofilm with the stationary growth phase and showed that the biofilm lifestyle, although sharing similarities with the stationary growth phase, triggers the expression of specific sets of genes. Using gene disruption of 54 of the most biofilm-induced genes followed by a detailed phenotypic study, we validated the biological relevance of our analysis and showed that 20 of these genes are required for the formation of mature biofilm. This group includes 11 genes of previously unknown function. These results constitute a comprehensive analysis of the global transcriptional response triggered in mature E. coli biofilms and provide insights into its physiological signature.

Published
2004
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39. Breast adenocarcinoma cell adhesion to the vascular subendothelium in whole blood and under flow conditions: effects of alphavbeta3 and alphaIIbbeta3 antagonists.

Author

Gomes N, Vassy J, Lebos C, Arbeille B, Legrand C, and Fauvel-Lafeve F

Subjects
Abciximab, Acetates pharmacology, Adenocarcinoma pathology, Antibodies, Monoclonal pharmacology, Blood Platelets metabolism, Blood Vessels, Breast Neoplasms pathology, Endothelium, Vascular pathology, Extracellular Matrix metabolism, Female, Humans, Immunoglobulin Fab Fragments pharmacology, Platelet Adhesiveness, Platelet Aggregation Inhibitors pharmacology, Pyridines pharmacology, Receptors, Vitronectin antagonists & inhibitors, Regional Blood Flow, Tumor Cells, Cultured, Tyrosine pharmacology, Adenocarcinoma metabolism, Breast Neoplasms metabolism, Cell Adhesion, Endothelium, Vascular metabolism, Integrin alphaVbeta3 antagonists & inhibitors, Platelet Glycoprotein GPIIb-IIIa Complex antagonists & inhibitors, Tyrosine analogs & derivatives
Abstract

Tumour cell adhesion to vascular extracellular matrix (ECM), an important step of metastatic progression, is promoted by platelets. The aim of our study was to investigate, in whole blood under venous and arterial shear conditions, the respective role of tumour cell alphavbeta3 and platelet alphaIIbbeta3 integrins in MDA-MB-231 breast adenocarcinoma cell adhesion to human umbilical vein endothelial cell ECM. For that purpose, blood containing MDA-MB-231 cells was incubated with non-peptide antagonists specific for platelet alphaIIbbeta3 (lamifiban) or tumour cell alphavbeta3 (SB-273005). At 300 s(-1), each antagonist used alone did not modify tumour cell adhesion, whereas, at 1500 s(-1), tumour cell adhesion was decreased by 25% in presence of lamifiban indicating a role of platelet alphaIIbbeta3 at higher shear rate. However, a combination of SB-273005 and lamifiban, or c7E3 Fab (a potent inhibitor of both alphaIIbbeta3 and alphavbeta3) inhibited tumour cell adhesion by 40-45%, at either shear rate applied, indicating a cooperation between these two integrins in MDA-MB-231 cell adhesion to ECM, as well as the participation of other adhesive receptors on tumour cells and/or platelets. Thus, efficient anti-metastatic therapy should target multiple receptors on tumour cells and platelets.

Published
2004
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40. In vitro study of low-frequency ultrasound-enhanced transdermal transport of fentanyl and caffeine across human and hairless rat skin.

Author

Boucaud A, Machet L, Arbeille B, Machet MC, Sournac M, Mavon A, Patat F, and Vaillant L

Subjects
Administration, Cutaneous, Analgesics, Opioid administration & dosage, Animals, Area Under Curve, Caffeine administration & dosage, Central Nervous System Stimulants administration & dosage, Diffusion, Fentanyl administration & dosage, Humans, In Vitro Techniques, Male, Membranes drug effects, Membranes ultrastructure, Rats, Skin ultrastructure, Ultrasonics, Analgesics, Opioid pharmacokinetics, Caffeine pharmacokinetics, Central Nervous System Stimulants pharmacokinetics, Fentanyl pharmacokinetics, Skin Absorption radiation effects
Abstract

The effect of low-frequency sonophoresis on fentanyl and caffeine permeation through human and hairless rat skin was studied in vitro. Experiments were performed using 20 kHz ultrasound applied at either continuous or discontinuous mode and with an average intensity of 2.5 W/cm(2). The results showed that low-frequency ultrasound enhanced the transdermal transport of both fentanyl and caffeine across human and hairless rat skin. This was explained by both increasing flux during sonication and shortening the lag time. Discontinuous mode was found to be more effective in increasing transdermal penetration of fentanyl while transdermal transport of caffeine was enhanced by both continuous and pulsed mode. Histological and electron microscopy studies showed that human and hairless rat skin was unaffected by ultrasound exposure. Further studies will be necessary to determine the relative contribution of ultrasound parameters in low-frequency ultrasound-induced percutaneous enhancement of drug transport.

Published
2001
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41. Clinical, histologic, and electron microscopy study of skin exposed to low-frequency ultrasound.

Author

Boucaud A, Montharu J, Machet L, Arbeille B, Machet MC, Patat F, and Vaillant L

Subjects
Animals, Humans, In Vitro Techniques, Male, Microscopy, Electron, Optics and Photonics, Rats, Skin physiopathology, Skin pathology, Skin radiation effects, Skin Temperature radiation effects, Ultrasonics
Abstract

The use of low-frequency ultrasound has been proposed to enhance the transdermal transport of various drugs, a technique referred to as sonophoresis. The aim of the present study was to determine the safety of low-frequency sonophoresis on human and rat skin by evaluating their structural modifications after ultrasound exposure. Human skin samples and hairless rats were exposed to 20 kHz ultrasound in vitro and in vivo, respectively. Ultrasound was used with average intensities ranging from 0.25 to 7 W/cm(2) in pulsed or continuous mode. Hairless rats were also exposed to a heat source mimicking the temperature versus time profile during sonication. Skin samples were observed under optical and electron microscopy to detect any structural changes. Human skin samples exposed to intensities lower than 2.5 W/cm(2) showed no modification. For hairless rats, slight and transient erythema was observed after 2.5 W/cm(2) exposure, whereas deep lesions (dermal and muscle necrosis) were observed 24 hr later. These lesions were also observed when a plastic film was placed between the coupling medium and the animals' skin during sonication. In contrast, no histologic lesion could be seen when a heat source was applied to animal skin. Low-frequency ultrasound induces delayed and deep lesions in hairless rat skin at 2.5 W/cm(2) which are not only attributable to the increase in temperature at the skin surface during ultrasound exposure. By using the same ultrasound conditions, human skin seems to be less sensitive in vitro., (Copyright 2001 Wiley-Liss, Inc.)

Published
2001
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42. MMP-2 colocalizes with caveolae on the surface of endothelial cells.

Author

Puyraimond A, Fridman R, Lemesle M, Arbeille B, and Menashi S

Subjects
Adult, Caveolin 1, Cells, Cultured, Endothelium, Vascular cytology, Humans, Matrix Metalloproteinases, Membrane-Associated, Metalloendopeptidases analysis, Receptors, Vitronectin analysis, Caveolae chemistry, Caveolins analysis, Endothelium, Vascular chemistry, Matrix Metalloproteinase 2 analysis
Abstract

We examined the spatial distribution of MMP-2 on the surface of human endothelial cells using immunofluorescence and confocal microscopy. Staining endothelial cells with MMP-2-specific antibodies revealed a punctate labeling at the basolateral side of the cell periphery, which colocalized with patches of caveolin-1, a major constituent of the caveolae. This colocalization was confirmed by immunogold electron microscopy. MT1-MMP, TIMP-2, and the alphavbeta3 integrin exhibited a similar pattern of staining, with pericellular patches that colocalized with either MMP-2 or caveolin-1. The presence of MT1-MMP and TIMP-2 in caveolae patches could be seen only after treatment with concanavalin A, which induced MMP-2 activation but had no noticeable effect on the pattern or intensity of MMP-2 immunostaining. In contrast, MMP-9 and TIMP-1 staining showed a pattern completely different from that of MMP-2 and TIMP-2, with positive spots uniformly distributed throughout the cell body. Our data show that MMP-2, its activator the MT1-MMP, and its proposed receptor, the alphavbeta3 integrin, are all targeted to the same membrane microdomains on the endothelial cell, thereby restricting matrix proteolysis to a limited microenvironment at the cell surface., (Copyright 2001 Academic Press.)

Published
2001
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43. Different role of platelet glycoprotein GP Ia/IIa in platelet contact and activation induced by type I and type III collagens.

Author

Monnet E, Sizaret P, Arbeille B, and Fauvel-Lafève F

Subjects
Antibodies, Monoclonal pharmacology, Blood Platelets cytology, Collagen metabolism, Endothelium, Vascular ultrastructure, Extracellular Matrix metabolism, Humans, Integrins immunology, Kinetics, Microscopy, Electron, Scanning, Phosphorylation, Platelet Adhesiveness, Platelet Aggregation drug effects, Receptors, Collagen, Tyrosine metabolism, Blood Platelets chemistry, Collagen pharmacology, Integrins physiology, Platelet Activation drug effects
Abstract

The role of glycoprotein Ia/IIa was studied during platelet contact and aggregation induced by type I and type III collagen. The anti-glycoprotein Ia/IIa (6F1) antibody inhibited type I collagen-induced aggregation but did not inhibit the first contact between platelets and collagen. In contrast, it was without effect either on type III collagen-induced contact or platelet interaction with the subendothelium in a static assay. Platelet aggregation induced by type III collagen was only slightly slowed down by 6F1 but pp72 spleen tyrosine kinase phosphorylation was not modified even at concentrations of 6F1 that completely blocked platelet activation induced by type I collagen. Our results indicate that glycoprotein Ia/IIa is not a primary binding site for type I or type III collagen on the platelet membrane. This receptor is more specifically involved in type I collagen-induced platelet spreading and aggregation.

Published
2000
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44. Cerebral MRI on fetuses submitted to repeated cocaine administration during the gestation: an ovine model.

Author

Akoka S, Descamps P, Genberg C, Franconi F, Arbeille B, Laurini R, Locatelli A, Platt LD, and Arbeille P

Subjects
Animals, Brain pathology, Brain Edema chemically induced, Cerebral Hemorrhage chemically induced, Cocaine administration & dosage, Female, Gestational Age, Maternal-Fetal Exchange, Microscopy, Electron, Neurons pathology, Pregnancy, Sheep, Brain embryology, Cocaine adverse effects, Magnetic Resonance Imaging
Abstract

The aim of this study was to determine the role of Magnetic Resonance Imaging (MRI) in investigating fetal cerebral lesions induced by long term exposure to cocaine during sheep pregnancy. Cerebral Magnetic Resonance Imaging was performed on two groups of fetuses at 125 days of gestation (normal gestation: 145 days). The control group consisted of eight fetuses of four pregnant ewes. The study group consisted of eight fetuses of four pregnant ewes receiving daily 140 mg/kg injection of cocaine from day 60 until delivery. The following MR sequences were applied: T1-weighted FLASH, and T2-weighted Fast-Spin-Echo. Cerebral images were evaluated semi quantitatively using the following criteria: Heterogenicity, contrast between grey and white matter, contours irregularity, hyposignal, lateral ventricle sizes. The brightness distribution and homogenicity of the images were analysed by means of edge pair distributions using a new computerized method originally designed for ultrasound images analysis developed by Ultrasight inc (USA). (1) Flash T1: Heterogenic areas and irregular contours were more frequent in cocaine exposed fetuses. The contrast between grey and white matter was more important in the cocaine group. Hyposignal was found only in the cocaine group. Enlarged lateral ventricle occurred more frequently in the cocaine group. (2) Spin echo T2: The contrast between grey and white matter was higher and the contours of the brain more irregular in the cocaine group. Heterogenicity and hyposignal were also more frequent in this group but the difference with the control group was not significant. The computerized analysis of the contrast density on the cerebral images showed that 88% of the areas exceeding the reference level concerned the cocaine group, while only 14% of the areas exceeding the reference level concerned the control group. Long term exposure to cocaine induces cerebral tissue modifications, in favor of an advanced maturation and the development of hypoxic lesions. The histology of the brains confirmed in the cocaine group, the existence of hypoxic lesions with gliosis, perivascular edema and hemorrhages, and neuronal death.

Published
1999
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45. Evaluation of clinical criteria for diagnosis of bullous pemphigoid. French Bullous Study Group.

Author

Vaillant L, Bernard P, Joly P, Prost C, Labeille B, Bedane C, Arbeille B, Thomine E, Bertrand P, Lok C, and Roujeau JC

Subjects
Aged, Female, Humans, Male, Multivariate Analysis, Predictive Value of Tests, Prospective Studies, Sensitivity and Specificity, Pemphigoid, Bullous pathology
Abstract

Objective: To check the potential usefulness of clinical criteria for the diagnosis of bullous pemphigoid when state-of-the-art techniques such as Western immunoblotting, immunoprecipitation, and indirect immunofluorescence on salt-split skin or direct immunoelectron microscopy are not available., Design: Comparison of the clinical criteria between 2 groups (with and without bullous pemphigoid) as defined by immunoelectron microscopy used as standard criterion, in a prospective study. Multivariate logistic regression analysis was carried out by including all items that were statistically significant (at P < .05 level) in univariate analysis., Setting: Five dermatology departments in teaching hospitals., Patients: The 231 patients studied had subepidermal autoimmune bullous diseases with linear IgG or C3 deposits in the basement membrane zone (157 with bullous pemphigoid, 33 with cicatricial pemphigoid, 30 with epidermolysis bullous acquisita, 5 with lupus erythematosus, and 6 others). A second set of patients was used to calculate predictive values., Results: The multivariate logistic stepwise analysis resulted in a final set of predictors that included only 4 items: absence of atrophic scars, absence of head and neck involvement, absence of mucosal involvement, and age greater than 70 years. No additional variables met the .05 significance level to enter into the model. If 3 of these 4 characteristics were present, a diagnosis of bullous pemphigoid could be made with a sensitivity of 90% and a specificity of 83%; these predictive values were calculated on a sample of 70 new cases., Conclusions: With and estimated incidence of bullous pemphigoid among subepidermal autoimmune bullous diseases of 80%, the presence of 3 of the 4 significant criteria allows the diagnosis of bullous pemphigoid, with a positive predictive value of 95%. Our set of clinical criteria thus allows the diagnosis of bullous pemphigoid with good validity for both clinical practice and therapeutic trials.

Published
1998
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46. Evidence for an alpha-granular pool of the cytoskeletal protein alpha-actinin in human platelets that redistributes with the adhesive glycoprotein thrombospondin-1 during the exocytotic process.

Author

Dubernard V, Arbeille BB, Lemesle MB, and Legrand C

Subjects
Blotting, Western, Cytoskeleton chemistry, Fluorescent Antibody Technique, Indirect, Humans, Microscopy, Immunoelectron, Precipitin Tests, Thrombin pharmacology, Actinin metabolism, Blood Platelets metabolism, Cytoplasmic Granules chemistry, Exocytosis, Thrombospondins metabolism
Abstract

In a previous study, we have demonstrated that the platelet adhesive glycoprotein thrombospondin-1 (TSP-1) interacts specifically with the cytoskeletal protein alpha-actinin in a solid-phase binding assay. Stored in the alpha-granules of platelets, TSP-1 is secreted during cell activation and binds to the plasma membrane promoting the platelet macroaggregate formation. However, the molecular mechanism by which TSP-1 reaches and binds to the platelet surface is to date unelucidated. alpha-Actinin is an actin-binding and actinin-cross-linking protein that is present in most cells and may act as a link between the bundles of F-actin and the plasma membrane. In this study, we have investigated a possible interaction of alpha-actinin with TSP-1 in platelets by examining their respective subcellular location during the platelet activation process. By indirect immunofluorescence. alpha-actinin was found to display a granular staining in resting platelets similar to that of TSP-1. Performing postembedding immunogold labeling for electron microscopy, we detected the presence of alpha-actinin throughout the cytoplasm, but the strongest gold staining was found in organelles identified as alpha-granules on the basis of their ultrastructure and TSP-1 content. With the use of double immunogold labeling on platelets at different stages of activation by thrombin, both alpha-actinin and TSP-1 were seen redistributing from the alpha-granules to the platelet surface via the open canalicular system (OCS). At the same time, the cytoplasmic alpha-actinin concentrated toward the plasma membrane, but no colocalization with the F-actin bundles was evidenced. Finally, preembedding immunogold labeling and immunoprecipitation of 125I-surface-labeled, thrombin-activated platelets further demonstrated that alpha-actinin was expressed on the plasma membrane in the absence of any detectable expression of actin and that it could from molecular complexes with TSP-1 on activated platelets. These results suggest that alpha-actinin found to be present on the platelet surface together with TSP-1 originates in the alpha-granules by fusion of the alpha-granules with the plasma membrane during platelet exocytosis.

Published
1997
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47. A new concept in Dorello's canal microanatomy: the petroclival venous confluence.

Author

Destrieux C, Velut S, Kakou MK, Lefrancq T, Arbeille B, and Santini JJ

Subjects
Abducens Nerve anatomy & histology, Cadaver, Cranial Fossa, Posterior innervation, Humans, Petrous Bone innervation, Veins anatomy & histology, Cranial Fossa, Posterior anatomy & histology, Cranial Fossa, Posterior blood supply, Petrous Bone anatomy & histology, Petrous Bone blood supply
Abstract

The so-called Dorello's canal was studied in 32 specimens (16 human cadaver heads) injected with colored latex and fixed in formalin (28 specimens) or studied with microscopic and ultrastructural methods (four specimens). To avoid the differences usually encountered in the description of this area, the authors preferred to consider a larger space that they have named the petroclival venous confluence (PVC). It was located between two dural layers: inner (or cerebral) and outer (or osteoperiosteal). The PVC was quadrangular on transverse section. The posterior petroclinoid fold and the axial plane below the dural foramen of the abducent nerve (sixth cranial nerve) limited the PVC at the top and bottom, respectively. Its anteroinferior limit was the posterosuperior aspect of the upper clivus and outer layer of the dura mater. Its anterior limit was the vertical plane containing the posterior petroclinoid fold, and its posterior limit was the inner layer of the dura. The PVC was limited laterally by the medial aspect of the petrous bone apex and medially by the virtual sagittal plane extending the medial limit of the inferior petrosal sinus upward. The PVC was a venous space bordered by endothelium and continuous with the cavernous sinus, the basal sinus of the clivus, and the inferior petrosal sinus. There were trabeculations between the two dural layers. The petrosphenoidal ligament of Gruber may be regarded as a larger trabeculation, and it divided the PVC into a superior and an inferior compartment. The abducent nerve generally ran through the inferior compartment, where it was fixed to the surrounding dura mater. This nerve was only separated from venous blood by a meningeal sheath of varying thinness lined with endothelium. The clinical implications of these findings are discussed.

Published
1997
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48. Heterogeneity of microfibrils: role of thrombospondin-microfibrils in the thrombogenicity of the subendothelium.

Author

Fauvel-Lafève F, Arbeille B, de Romeuf C, Lemesle M, and Legrand YJ

Subjects
Collagen immunology, Extracellular Matrix Proteins, Fibrillins, Humans, In Vitro Techniques, Microfilament Proteins immunology, Microscopy, Immunoelectron, Platelet Aggregation, Thrombospondins, von Willebrand Factor immunology, Endothelium, Vascular immunology, Membrane Glycoproteins immunology, Microfilament Proteins metabolism
Abstract

We report the results of an immunogold electron microscopical analysis on microfibrils from the arterial subendothelium showing that thrombospondin (TSP) is present on 40 nm-diameter structures joining 8-10 nm-diameter microfibrils containing fibrillin. They differ from type VI collagen which forms 3-5 nm-diameter microfibrils. TSP containing microfibrils (TSP-MF) extracted from human umbilical arteries did not contain fibrillin or type VI collagen. Blood platelet interactions with TSP-MF were not modified by anti-fibrillin or anti-type VI collagen antibodies. In situ, vWF was bound to cross-linked microfibrils, at the level of their 40 nm junction, and a double-labeling with the anti-thrombospondin and anti-vWF antibodies was observed. In vitro, vWF binding to TSP-MF was not inhibited by anti-fibrillin or anti-type VI collagen antibodies. These results suggest a structural and functional heterogeneity of microfibrils and emphasize the role of TSP-MF in the thrombogenicity of the subendothelium.

Published
1996

49. Optimal antagonism of GPIIb/IIIa favors platelet adhesion by inhibiting thrombus growth. An ex vivo capillary perfusion chamber study in the guinea pig.

Author

André P, Arbeille B, Drouet V, Hainaud P, Bal dit Sollier C, Caen JP, and Drouet LO

Subjects
Animals, Capillary Action, Collagen, Fibrin metabolism, Guinea Pigs, Humans, In Vitro Techniques, Male, Microscopy, Electron, Scanning, Perfusion, Platelet Aggregation drug effects, Platelet Aggregation Inhibitors pharmacology, Thrombosis pathology, Tyrosine pharmacology, Acetates pharmacology, Anticoagulants pharmacology, Platelet Adhesiveness drug effects, Platelet Glycoprotein GPIIb-IIIa Complex antagonists & inhibitors, Thrombosis prevention & control, Tyrosine analogs & derivatives
Abstract

To evaluate the involvement of the glycoprotein (GP) IIb/IIIa-dependent process in platelet deposition and thrombus growth on capillaries coated with human type III collagen, the effects of incremental doses of Lamifiban, a potent specific synthetic GPIIb/IIIa antagonist, were studied in ex vivo capillary perfusion chambers using guinea pig blood. In this model, nonanticoagulated blood was perfused for 4.5 minutes at three shear rates: 100, 650, and 1600 s-1. Platelet deposition was quantified by computer-assisted morphometry and expressed as platelet adhesion (percentage of capillary surface covered with spread and contact platelets and platelets implicated in thrombus), mean thrombus height, and total thrombus cross-sectional area. In control untreated guinea pigs, platelet adhesion and thrombus height were 63% and 2.5 microns at 100 s-1, 60.5% and 13.8 microns at 650 s-1, and 45% and 28.1 microns at 1600 s-1, respectively. At 100 s-1, Lamifiban had no effect on platelet deposition at any of the three doses administered to the guinea pigs (0.3, 1, and 3 mg/kg). At 0.3 mg/kg and shear rates of 650 and 1600 s-1, Lamifiban had no effect on platelet adhesion or thrombus size, but at 1 and 3 mg/kg and shear rates of 650 and 1600 s-1, it significantly reduced thrombus size. At 1600 s-1, 1 mg/kg Lamifiban significantly increased platelet adhesion from 45% to 62.5%, whereas at 3 mg/kg it induced a significant overall decrease from 45% to 25% and qualitatively increased the ratio of contact to spread platelets. These data suggest that at high shear rates, GPIIb/IIIa participates in platelet spreading and that there is a balance between platelet involvement in adhesion to the thrombogenic surface and the growth of the already formed thrombus. This indicates that important clinical implications of an optimal therapeutic degree of GPIIb/IIIa antagonism could be expected.

Published
1996
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50. Xenogeneic cellular interaction in an ex vivo model of pig kidney perfused with human lymphocytes.

Author

Khalfoun B, Janin P, Machet MC, Arbeille B, Lacord M, Locatelli A, Salmon H, Riess G, Gruel Y, and Nivet H

Subjects
Animals, Cells, Cultured, Diuresis, Haplotypes immunology, Humans, In Vitro Techniques, Kidney immunology, Perfusion, Renal Circulation, Swine, Vascular Resistance, Kidney physiology, Lymphocytes immunology, Transplantation, Heterologous immunology
Published
1995

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