C. Milési-Fluet scite author profile

C. Milési-Fluet

4Publications

36Citation Statements Received

18Citation Statements Given

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127

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Inserm

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Detection of 47, XYY Trophoblast Fetal Cells in Maternal Blood by Fluorescence in situ Hybridization after Using Immunomagnetic Lymphocyte Depletion and Flow Cytometry Sorting

Cacheux

Milési-Fluet²,

Tachdjian

et al. 1992

Fetal Diagn Ther

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Fluorescence in situ hybridization (FISH) allows to diagnose aneuploidy in uncultured interphase nuclei. This rapid method of chromosomal analysis associated with cell-sorting techniques was realized on 47, XYY fetal cells isolated from maternal blood. Trophoblast cells were sorted by combining immunomagnetic removal of maternal lymphocytes and flow cytometry sorting using antitrophoblast monoclonal antibodies. Cells were sorted directly on slides and analyzed by FISH with a Y-centromeric probe. Among 1,387 examinable nuclei, 59 (4.25%) showed one single or two Y-specific domains.

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Identification and characterization of membrane cofactor protein of human spermatozoa.

Cervoni

Oglesby

Adams

et al. 1992

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Membrane cofactor protein (MCP) regulates C activation by serving as a cofactor for the cleavage of C3b and C4b by the serine protease factor I. An MCP-like molecule on the inner acrosomal membrane of human spermatozoa has been characterized. Three mAb and a rabbit polyclonal antibody against MCP recognized the sperm protein. On SDS-PAGE, it migrated as a single band with a molecular mass of 38,000 and 44,000 Da under nonreducing or reducing conditions, respectively. The molecular mass was 10,000 to 20,000 Da less than the two forms of MCP expressed on others cells. The electrophoretic pattern, by one- and two-dimensional gel analysis, and the isoelectric point profile (4.5 to 5.0) of the sperm protein were similar among multiple individuals. In contrast to MCP of other cells, digestion with endoglycosidases did not alter either the m.w. or the pI of the protein, suggesting that it is a poorly or nonglycosylated form of MCP. The solubilized sperm protein bound C3 with broken thioester bond to Sepharose and possessed cofactor activity for factor I-mediated cleavage of C3 with the broken bond. A mAb that blocks the regulatory function of MCP inhibited the cofactor activity of the sperm lysate. Thus, the sperm protein is an antigenic and functional homologue of MCP but has the distinct structural features of a lower m.w. and an apparent lack of glycosylation. MCP may play an essential role in the survival of the acrosome-reacted spermatozoa by modulating C activation in the female genital tract.

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Expression of TLX antigen recognized by GB24 on trophoblast and leukocytes

Hsi¹,

Grivaux²,

Milési-Fluet³

1989

Journal of Reproductive Immunology

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Do human trophoblast, leukocyte and sperm share a common antigen recognized by GB24?

Fénichel¹,

Grivaux²,

Dohr³

et al. 1989

Placenta

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C. Milési-Fluet

Detection of 47, XYY Trophoblast Fetal Cells in Maternal Blood by Fluorescence in situ Hybridization after Using Immunomagnetic Lymphocyte Depletion and Flow Cytometry Sorting

Identification and characterization of membrane cofactor protein of human spermatozoa.

Expression of TLX antigen recognized by GB24 on trophoblast and leukocytes

Do human trophoblast, leukocyte and sperm share a common antigen recognized by GB24?

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