Literature DB >> 3794601

Quantification of the transition from oocyte-coded to embryo-coded glucose phosphate isomerase in mouse embryos.

J D West, R Leask, J F Green.   

Abstract

A quantitative electrophoretic analysis of glucose phosphate isomerase (GPI-1) allozymes produced by heterozygous Gpi-1sa/Gpi-1sb mouse embryos has enabled us to estimate separately the contributions of GPI-1 enzyme that were oocyte coded, encoded by the embryonic, maternally derived Gpi-1sa allele and encoded by the embryonic, paternally derived Gpi-1sb allele. The oocyte-coded GPI-1 activity is stable until 2 1/2 days and then declines and is exhausted by 5 1/2 to 6 1/2 days post coitum (p.c.). The maternally and paternally derived Gpi-1s alleles are probably usually activated synchronously but several possible exceptions were observed. This activation was first detected in 2 1/2-day embryos. Total GPI-1 activity falls to a minimum around 3 1/2 to 4 1/2 days, even though embryonic gene expression has already begun. The profile of oocyte-coded GPI-1 activity is consistent with the suggestion (Harper & Monk, 1983) that there is a mechanism for the removal of oocyte-coded gene products at around 2 1/2 days p.c. The method of analysis described is applicable to other dimeric enzymes with electrophoretic variants.

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Year:  1986        PMID: 3794601

Source DB:  PubMed          Journal:  J Embryol Exp Morphol        ISSN: 0022-0752


  6 in total

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4.  Quantitative analysis of mid-gestation mouse aggregation chimaeras: non-random composition of the placenta.

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5.  Maternal enzyme masks the phenotype of mouse embryos lacking dihydrolipoamide dehydrogenase.

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6.  High activity of an unstable form of glucose phosphate isomerase in the mouse.

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  6 in total

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