- Poissy, Île-de-France, France
Research Interests:
Research Interests:
Research Interests: Biology, Medicine, DNA, Single cell analysis, Humans, and 15 moreSperm, Male, Three Dimensional Imaging, Male Infertility, Chromatin, Cell nucleus, Adult, Spermatozoon, Acrosome, Spermatozoa, Sperm Motility, Acrosome Reaction, Severity of Illness Index, Asthenozoospermia, and Paediatrics and reproductive medicine
Research Interests:
Research Interests: Biology, Medicine, Multidisciplinary, Multivariate Analysis, Humans, and 15 moreIn Vitro Fertilisation, Female, Intracytoplasmic Sperm Injection, Polymerase Chain Reaction, PLoS one, Genotype, Single Nucleotide Polymorphism, Age Factors, European Continental Ancestry Group, Fertilization in Vitro, Ovary, Oocytes, Follicle stimulating hormone, Gene frequency, and Estrogen Receptor beta
Research Interests:
Research Interests:
Background The bacterial elongation factor P (EF-P) is strictly conserved in bacteria and essential for protein synthesis. It is homologous to the eukaryotic translation initiation factor 5A (eIF5A). A highly conserved eIF5A lysine is... more
Background The bacterial elongation factor P (EF-P) is strictly conserved in bacteria and essential for protein synthesis. It is homologous to the eukaryotic translation initiation factor 5A (eIF5A). A highly conserved eIF5A lysine is modified into an unusual amino acid derived from spermidine, hypusine. Hypusine is absolutely required for eIF5A's role in translation in Saccharomyces cerevisiae. The homologous lysine of EF-P is also modified to a spermidine derivative in Escherichia coli. However, the biosynthesis pathway of this modification in the bacterial EF-P is yet to be elucidated. Presentation of the Hypothesis Here we propose a potential mechanism for the post-translational modification of EF-P. By using comparative genomic methods based on physical clustering and phylogenetic pattern analysis, we identified two protein families of unknown function, encoded by yjeA and yjeK genes in E. coli, as candidates for this missing pathway. Based on the analysis of the structural and biochemical properties of both protein families, we propose two potential mechanisms for the modification of EF-P. Testing the hypothesis This hypothesis could be tested genetically by constructing a bacterial strain with a tagged efp gene. The tag would allow the purification of EF-P by affinity chromatography and the analysis of the purified protein by mass spectrometry. yjeA or yjeK could then be deleted in the efp tagged strain and the EF-P protein purified from each mutant analyzed by mass spectrometry for the presence or the absence of the modification. This hypothesis can also be tested by purifying the different components (YjeK, YjeA and EF-P) and reconstituting the pathway in vitro. Implication of the hypothesis The requirement for a fully modified EF-P for protein synthesis in certain bacteria implies the presence of specific post-translational modification mechanism in these organisms. All of the 725 bacterial genomes analyzed, possess an efp gene but only 200 (28%) possess both yjeA and yjeK genes. In the other organisms, EF-P may be modified by another pathway or the translation machinery must have adapted to the lack of EF-P modification. Our hypotheses, if confirmed, will lead to the discovery of a new post-translational modification pathway. Reviewers This article was reviewed by Céline Brochier-Armanet, Igor B. Zhulin and Mikhail Gelfand. For the full reviews, please go to the Reviewers' reports section.