J. Gilchrist scite author profile

Genetic studies have shown that mutations within the mahogany locus suppress the pleiotropic phenotypes, including obesity, of the agouti-lethal-yellow mutant. Here we identify the mahogany gene and its product; this study, to our knowledge, represents the first positional cloning of a suppressor gene in the mouse. Expression of the mahogany gene is broad; however, in situ hybridization analysis emphasizes the importance of its expression in the ventromedial hypothalamic nucleus, a region that is intimately involved in the regulation of body weight and feeding. We present new genetic studies that indicate that the mahogany locus does not suppress the obese phenotype of the melanocortin-4-receptor null allele or those of the monogenic obese models (Lep(db), tub and Cpe(fat)). However, mahogany can suppress diet-induced obesity, the mechanism of which is likely to have implications for therapeutic intervention in common human obesity. The amino-acid sequence of the mahogany protein suggests that it is a large, single-transmembrane-domain receptor-like molecule, with a short cytoplasmic tail containing a site that is conserved between Caenorhabditis elegans and mammals. We propose two potential, alternative modes of action for mahogany: one draws parallels with the mechanism of action of low-affinity proteoglycan receptors such as fibroblast growth factor and transforming growth factor-beta, and the other suggests that mahogany itself is a signalling receptor.

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The effects of different laser pulse lengths on the embryo biopsy procedure and embryo development to the blastocyst stage

Taylor

Gilchrist

Hallowell

et al. 2010

J Assist Reprod Genet

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Purpose A laser is commonly used to remove a blastomere from an embryo for genetic testing. The laser uses intense heat which could possibly disrupt embryo development. It is the goal of this study to test the effects of different laser pulse lengths (and consequently heat) on the embryo biopsy procedure and embryo development. Methods Each embryo biopsy was performed randomly utilizing laser pulse lengths of 0.604mS (group I), 0.708mS (group II), and 1.010mS (group III). Results For groups I, II, and III, 83, 86, and 71 embryos were biopsied, respectively. There was no difference in day 5 embryo quality or lysed blastomeres between groups. Average number of blastomeres biopsied between group I (1.0±0.0), II (1.0±0.2), and III (1.1±0.2) was significant (0.0001). Conclusion Our data demonstrates that laser pulse length does not influence the embryo biopsy procedure or embryo development.

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The utility of embryo banking in order to increase the number of embryos available for preimplantation genetic screening in advanced maternal age patients

Orris

Taylor

Gilchrist

et al. 2010

J Assist Reprod Genet

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Flux flow resistivity by surface resistance measurements

Gilchrist¹,

Monçeau²

1970

J. Phys. C: Solid State Phys.

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Non-inferiority study of the effect of oocyte vitrification on fertilization rate and embryo development using a sibling oocyte model

Anderson

Gilchrist

Jones

et al. 2013

Fertility and Sterility

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J. Gilchrist

The mahogany protein is a receptor involved in suppression of obesity

The effects of different laser pulse lengths on the embryo biopsy procedure and embryo development to the blastocyst stage

The utility of embryo banking in order to increase the number of embryos available for preimplantation genetic screening in advanced maternal age patients

Flux flow resistivity by surface resistance measurements

Non-inferiority study of the effect of oocyte vitrification on fertilization rate and embryo development using a sibling oocyte model

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