Fabienne Brulé
Centre national de la recherche scientifique
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Featured researches published by Fabienne Brulé.
Current Microbiology | 1997
Sabine Herbin; Florence Mathieu; Fabienne Brulé; Christiane Branlant; Gérard Lefebvre; Ahmed Lebrihi
Abstract.Carnobacterium piscicola CP5, isolated from a French mold-ripened soft cheese, produced a bacteriocin activity named carnocin CP5, which inhibited Carnobacterium, Enterococcus and Listeria spp. strains, and among the Lactobacillus spp. only Lactobacillus delbrueckii spp. [24]. The activity was purified by ammonium sulfate precipitation, anion exchange, and hydrophobic interaction chromatography followed by reverse-phase high-performance liquid chromatography (RP-HPLC). This latter step separated two peaks with anti-listerial activity (CP51 and CP52). Carnocin CP51 was partially sequenced, and the N-terminal part revealed the presence of the “pediocin-like consensus” sequence-Tyr-Gly-Asn-Gly-Val-. Then, a degenerated 24-mer oligonucleotide probe was constructed from the N-terminal sequence and used to detect the structural gene. It was localized on a plasmid of about 40 kb. Cloning of restriction fragments of this one, followed by DNA sequencing, revealed the presence of the second anti-Listeria bacteriocin gene (CP52). By comparing sequences in data banks and confirming results with PCR reactions, carnocin CP51 shared homologies with carnobacteriocin BM1, and carnocin CP52 was similar to carnobacteriocin B2, both produced by C. piscicola LV17 [2]. However, carnobacteriocin A from C. piscicola LV17 gene was lacking in C. piscicola CP5, and the two microorganisms have been isolated from different ecological environments: C. piscicola CP5 and C. piscicola LV17 were isolated from soft cheese and vacuum-packed meat respectively. This fact could allow different application perspectives for C. piscicola CP5.
Nucleic Acids Research | 2006
Fabien Kieken; Françoise Paquet; Fabienne Brulé; Jacques Paoletti; Gérard Lancelot
Dimerization of genomic RNA is directly related with the event of encapsidation and maturation of the virion. The initiating sequence of the dimerization is a short autocomplementary region in the hairpin loop SL1. We describe here a new solution structure of the RNA dimerization initiation site (DIS) of HIV-1Lai. NMR pulsed field-gradient spin-echo techniques and multidimensional heteronuclear NMR spectroscopy indicate that this structure is formed by two hairpins linked by six Watson–Crick GC base pairs. Hinges between the stems and the loops are stabilized by intra and intermolecular interactions involving the A8, A9 and A16 adenines. The coaxial alignment of the three A-type helices present in the structure is supported by previous crystallography analysis but the A8 and A9 adenines are found in a bulged in position. These data suggest the existence of an equilibrium between bulged in and bulged out conformations in solution.
RNA | 2002
Fabienne Brulé; Roland Marquet; Liwei Rong; Mark A. Wainberg; Bernard P. Roques; Stuart F. J. Le Grice; Bernard Ehresmann; Chantal Ehresmann
RNA | 1996
Annie Mougin; A Grégoire; J Banroques; Véronique Ségault; Régis Fournier; Fabienne Brulé; M Chevrier-Miller; Christiane Branlant
Nucleic Acids Research | 2000
Fabienne Brulé; Guillaume Bec; Gérard Keith; Stuart F. J. Le Grice; Bernard P. Roques; Bernard Ehresmann; Chantal Ehresmann; Roland Marquet
RNA | 1996
Fabienne Brulé; J Venema; Véronique Ségault; D Tollervey; Christiane Branlant
Archive | 2009
Roland Benoit; Marie-Louise Saboungi; Fabienne Brulé
Nucleic Acids Research | 2003
Mickaël Rigourd; Valérie Goldschmidt; Fabienne Brulé; Casey D. Morrow; Bernard Ehresmann; Chantal Ehresmann; Roland Marquet
RNA | 1998
Régis Fournier; Fabienne Brulé; Véronique Ségault; Annie Mougin; Christiane Branlant
Archive | 2004
Fabienne Brulé; Catherine Isel; Roland Marquet; Mickaeel Rigourd