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Protein databases for compacted eight‐cell and blastocyst‐stage mouse embryos
Author(s) -
Shi C. Z.,
Collins H. W.,
Garside W. T.,
Buettger C. W.,
Matschinsky F. M.,
Heyner S.
Publication year - 1994
Publication title -
molecular reproduction and development
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.745
H-Index - 105
eISSN - 1098-2795
pISSN - 1040-452X
DOI - 10.1002/mrd.1080370106
Subject(s) - biology , blastocyst , embryo , andrology , stage (stratigraphy) , developmental stage , microbiology and biotechnology , database , embryogenesis , genetics , medicine , paleontology , developmental psychology , psychology , computer science
Abstract High‐resolution two‐dimensional sodium dodecyl sulfate‐polyacrylamide (2D‐SDS) gel electrophoresis combined with computerized analysis of gel images was used to construct and analyze protein databases for two stages of preimplantation mouse embryogenesis, the compacted eight‐cell stage and the fully expanded blastocyst stage. These stages were chosen for their ease in identification of multiple synchronous embryos. Synchronous cohorts of 30–50 embryos were labelled with L‐[ 35 S]methionine for 2 hr. The embryos were then lysed in 30 μl hot SDS sample buffer, and the lysates were stored at −80°C until the gels were run. Five replicates were run for eight‐cell embryos, and four for blastocyst‐stage embryos. The samples were processed for 2D gel electrophoresis and fluorography; multiple exposures were made. Gel images were analyzed using the PDQUEST system, and databases were constructed. Analysis of the databases for both developmental stages showed high reproducibility of protein spots in multiple gel images. Of 1,674 total spots in eight‐cell embryo standards, >79% of spots had a percentage error (S.E.M./average) <50%, and >45% had a percentage error <30%. Similarly, of 1,653 total spots in blastocyst‐stage embryo standards, 74% of spots had a percentage error <50%, and approximately 47% of spots had a percentage error <30%. Forty‐three spots (approximately 3% of the total spots) were found to be detected only in the eight‐cell stage, while 75 spots were detected solely in the blastocyst stage. Sixty‐nine proteins showed a greater than threefold increase in isotope incorporation from the eight‐cell to the blastocyst stage, with a percentage error <50% in both the eight‐cell and the blastocyst stages. In contrast, 41 of the proteins showed a decrease during this period. Analysis of the protein databases described in this study has allowed us to document the overall quantitative changes in proteins from the compacted eight‐cell stage to the blastocyst stage of mouse preimplantation development. These databases provide a valuable tool for further detailed quantitative analysis of specific proteins associated with developmental events. In addition they will permit analysis of the effects of environmental factors, such as growth factors, on early embryo development. © 1994 Wiley‐Liss, Inc.