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Comparative Study of Protein Profile during Development of Mouse Placenta

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  • URLhttps://db.koreascholar.com/Article/Detail/93923
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한국동물번식학회 (The Korean Society of Animal Reproduction)
초록

To examine the differential protein expression pattern in the 11.5 day post-coitus (dpc) and 18.5 dpc placenta of mouse, we have used the global proteomics approach by 2-D gel electrophoresis (2-DE) and MALDI-TOF-MS. The differential protein patterns of 3 placentae at the 11.5 dpc and 18.5 dpc from nature mating mice were analyzed. Proteins within isoelectric point range of 3.0~10.0, separately were analyzed in 2DE with 3 replications of each sample. A total of approximately 1,600 spots were detected in placental 2-D gel stained with Coomassie-blue. In the comparison of 11.5 dpc and 18.5 dpc placentae, a total of 108 spots were identified as differentially expressed proteins, of which 51 spots were up-regulated proteins such as alpha-fetoprotein, mKIAA0635 protein and transferrin, annexin A5, while 48 spots were down-regulated proteins such as Pre-B-cell colony-enhancing factor 1(PBEF), aldolase 1, A isoform, while 4 spots were 11.5 dpc specific proteins such as chaperonin and Acidic ribosomal phosphoprotein P0, while 3 spots were 18.5 dpc specific proteins such as aldo-keto reductase family 1, member B7 and CAST1/ERC2 splicing variant-1. Most identified proteins in this analysis appeared to be related with catabolism, cell growth, metabolism and regulation. Our results revealed composite profiles of key proteins involved in mouse placenta during pregnancy.

목차
ABSTRACT   INTRODUCTION   MATERIALS AND METHODS    Placental Samples    Extraction of Solubilized Proteins from Placenta    2-D Gel Electrophoresis    Staining and Image Analysis of 2-D-Gels    Sample Preparation for MALDI-TOF Mass Spectro-metry Analysis   RESULTS    Analysis of Placenta Proteomes by 2-DE    Identification of Differentially Expressed Spots    DISCUSSION   REFERENCES
저자
  • Rong Xun Han(Division of Animal Science and Resources, Research Center for Transgenic Cloned Pigs, Chungnam National University)
  • Hong Rye Kim(Division of Animal Science and Resources, Research Center for Transgenic Cloned Pigs, Chungnam National University)
  • Kenji Naruse(Division of Animal Science and Resources, Research Center for Transgenic Cloned Pigs, Chungnam National University)
  • Su Min Choi(Division of Animal Science and Resources, Research Center for Transgenic Cloned Pigs, Chungnam National University)
  • Baek-Chul Kim(Division of Animal Science and Resources, Research Center for Transgenic Cloned Pigs, Chungnam National University)
  • Chang Sik Park(Division of Animal Science and Resources, Research Center for Transgenic Cloned Pigs, Chungnam National University)
  • Dong Il Jin(Division of Animal Science and Resources, Research Center for Transgenic Cloned Pigs, Chungnam National University) Corresponding author