Louise Coutu scite author profile

Louise Coutu

5Publications

14Citation Statements Received

17Citation Statements Given

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Affiliations

Université du Québec à Rimouski, Université de Montréal

Publications

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Purification of P26h: a hamster sperm protein

Coutu¹,

P²,

Sullivan³

1996

Biochem. Cell Biol.

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P26h is a 26 kDa glycoprotein, located on the acrosome cap of hamster spermatozoa, involved in the species specificity of gamete interaction. We have purified this protein from hamster spermatozoa collected from the distal cauda region of the epididymis. Its purification was realized following a three-step procedure: detergent extraction, ion-exchange chromatography, and chromatofocusing. Protein partitioning using Triton X-114 (the first step) showed a ratio of 5:1 between the resulting aqueous and detergent phase. P26h was found almost exclusively in the aqueous phase where it represented about 10-12% of the total protein content. When the desalted aqueous phase was loaded on a carboxymethyl column for cation-exchange chromatography, about 80% of the proteins did not bind to the matrix and were eliminated. P26h was eluted from the column with a linear gradient of salt. At this point, P26h had a rate of purification estimated at 45-55%; three other major proteins of <21, 45, and 63 kDa remained in the sample. These undesired proteins were eliminated by submitting these samples to chromatofocusing using a PBE 94 polybuffer exchanger column. Indeed, P26h was collected almost in the dead volume of the column while the other proteins were eluted much later. Two-dimensional gel electrophoresis and Western blotting were performed to determine the purity of P26h. Only one major spot was detected, confirming the purity of P26h. Usefulness of this purified sperm antigen in the understanding of the physiology of mammalian fertilization is discussed.

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The Elimination of Keratin Artifacts in Immunoblots Probed with Polyclonal Antibodies

Bherer¹,

Coutu²,

Lefièvre³

et al. 1994

Analytical Biochemistry

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Influence of ACTH on anaphylactic shock in guinea pigs

et al. 1952

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Protein phosphorylation during activation of surf clam oocytes

Dubé

Dufresne

Coutu

et al. 1991

Developmental Biology

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Partial activation of surf clam oocytes by hypertonic treatment.

Coutu

Larochelle

Dubé

1993

Cell Biology International

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In prophase I‐arrested surf clam oocytes, fertilization is the normal trigger for resumption of meiosis, first evidenced by germinal vesicle breakdown (GVBD). Various artificial agents are able to induce GVBD and most of them require the presence of external Ca2+ to be efficient. One exception to this rule is the reported possibility of inducing GVBD by an hypertonic treatment, using high concentrations of glycerol, in the complete absence of external Ca2+. We have investigated the processes underling glycerol‐induced activation and found that, under this condition, GVBD shows very slow kinetics and is not followed by any normal subsequent steps of meiosis, such as formation of metaphase chromosomes or polar body extrusion. Glycerol‐activated oocytes do not show the normal response in protein synthesis but they undergo increased protein phosphorylation which is inhibited by 6‐dimethylaminopurine (6‐DMAP), which also inhibits GVBD. We conclude that the hypertonic treatment by glycerol, in the complete absence of external Ca2+, induces a partial program of activation through increased protein phosphorylation but that the normal full response requires an increased Ca2+ influx as triggered by other well‐known artificial activating agents.

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Louise Coutu

Purification of P26h: a hamster sperm protein

The Elimination of Keratin Artifacts in Immunoblots Probed with Polyclonal Antibodies

Influence of ACTH on anaphylactic shock in guinea pigs

Protein phosphorylation during activation of surf clam oocytes

Partial activation of surf clam oocytes by hypertonic treatment.

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