NONRADIOISOTOPIC QUANTITATIVE RT-PCR TO DETECT CHANGES IN MESSENGER-RNA LEVELS DURING EARLY MOUSE EMBRYO DEVELOPMENT

被引:97
|
作者
YOKOI, H
NATSUYAMA, S
IWAI, M
NODA, Y
MORI, T
MORI, KJ
FUJITA, K
NAKAYAMA, H
FUJITA, J
机构
[1] KYOTO UNIV,FAC MED,DEPT CLIN MOLEC BIOL,KYOTO 606,JAPAN
[2] KYOTO UNIV,FAC MED,DEPT OBSTET & GYNECOL,KYOTO 606,JAPAN
[3] SHIGA UNIV MED SCI,DEPT OBSTET & GYNECOL,OTSU,SHIGA 52021,JAPAN
[4] NIIGATA UNIV,FAC SCI,DEPT BIOL,NIIGATA 95021,JAPAN
[5] URAWA CITY HOSP,DIV ORTHOPED,URAWA 336,JAPAN
来源
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS | 1993年 / 195卷 / 02期
关键词
D O I
10.1006/bbrc.1993.2112
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
We developed a non-radioisotopic quantitative RT-PCR method with high sensitivity and reproducibility. The results of this RT-PCR were in agreement with those of the Northern blot analysis. We measured the mRNA levels of β-actin, transferrin receptor, and two cell cycle-related genes, cyclin B and cdc25, in early mouse embryos by the RT-PCR. In late two-cell stage embryos, β-actin, transferrin receptor and cyclin B mRNA levels were 10-20% of those in MII stage oocytes. In contrast, the cdc25 mRNA levels were not different between these stages. When we cultured mouse embryos, the presence of an RNA polymerase inhibitor, α-amanitin, in the medium did not affect the mRNA levels at the two-cell stage, indicating that most of the detected mRNAs in two-cell embryos were maternally derived. These results suggest that the rate of mRNA degradation is different between cyclin B and cdc25 during early embryogenesis. © 1993 Academic Press. All rights reserved.
引用
收藏
页码:769 / 775
页数:7
相关论文
共 50 条
  • [1] CHEMOKINE MESSENGER-RNA EXPRESSION PATTERNS IN KERATINOCYTES BY QUANTITATIVE RT-PCR
    BICKEL, M
    NOTHEN, S
    SHIRE, D
    JOURNAL OF DENTAL RESEARCH, 1994, 73 : 184 - 184
  • [2] QUANTITATION OF MESSENGER-RNA SPECIES BY RT-PCR ON TOTAL MESSENGER-RNA POPULATION
    HAMOUI, S
    BENEDETTO, JP
    GARRET, M
    BONNET, J
    PCR-METHODS AND APPLICATIONS, 1994, 4 (03): : 160 - 166
  • [3] APPLICATION OF QUANTITATIVE RT-PCR TO THE ANALYSIS OF DOPAMINE-RECEPTOR MESSENGER-RNA LEVELS IN RAT STRIATUM
    VRANA, SL
    KLUTTZ, BW
    VRANA, KE
    MOLECULAR BRAIN RESEARCH, 1995, 34 (01): : 127 - 134
  • [4] QUANTITATION OF METALLOTHIONEIN MESSENGER-RNA BY RT-PCR AND CHEMILUMINESCENCE
    JESSENELLER, K
    PICOZZA, E
    CRIVELLO, JF
    BIOTECHNIQUES, 1994, 17 (05) : 962 - &
  • [5] RT-PCR WITH AFFINITY-CAPTURED MESSENGER-RNA
    CUDDY, K
    FOLEY, B
    JAFFE, JS
    GILLESPIE, D
    NUCLEIC ACIDS RESEARCH, 1993, 21 (09) : 2281 - 2281
  • [6] MEASUREMENT OF TISSUE FACTOR MESSENGER-RNA LEVELS IN HUMAN ENDOTHELIAL-CELLS BY A QUANTITATIVE RT-PCR ASSAY
    POTGENS, AJG
    LUBSEN, NH
    VANALTENA, G
    SCHOENMAKERS, JGG
    RUITER, DJ
    DEWAAL, RMW
    THROMBOSIS AND HAEMOSTASIS, 1994, 71 (02) : 208 - 213
  • [7] EXON JUNCTION PRIMER IN A RTTH POLYMERASE BASED RT-PCR TO DETECT MESSENGER-RNA OF CYTOKINES
    LEUNG, WC
    LAWRENCE, WF
    HOU, JZ
    LEUNG, MFKL
    JOURNAL OF CELLULAR BIOCHEMISTRY, 1993, : 115 - 115
  • [8] RT-PCR DETECTABLE MESSENGER-RNA LEVELS FOLLOWING MECHANICAL STRAIN APPLICATION TO OSTEOBLASTS
    STANFORD, C
    STEVENS, J
    MIDURA, R
    BRAND, R
    JOURNAL OF DENTAL RESEARCH, 1994, 73 : 242 - 242
  • [9] EXON JUNCTION PRIMERS SPECIFIC FOR MESSENGER-RNA FOR RT-PCR
    LAWRENCE, WF
    HOU, JZ
    LEABER, R
    LEUNG, MFKL
    LEUNG, WC
    FASEB JOURNAL, 1993, 7 (03): : A166 - A166
  • [10] DIRECT RT-PCR AMPLIFICATION OF MESSENGER-RNA SUPPORTED ON MEMBRANES
    RUIZ, A
    BOK, D
    BIOTECHNIQUES, 1993, 15 (05) : 882 - +
12345