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在转基因小鼠中研究的睾丸血管紧张素转换酶启动子的物种差异。

Species variation in the testicular angiotensin converting enzyme promoter studied in transgenic mice.

作者信息

Erickson R P, Kessler S, Kremling H, Sen G C

机构信息

Angel Charity for Children-Wings for Genetic Research, Steele Memorial Children's Research Center, Department of Pediatrics, University of Arizona, College of Medicine, Tucson 85724, USA.

出版信息

Mol Reprod Dev. 1996 Jul;44(3):324-31. doi: 10.1002/(SICI)1098-2795(199607)44:3<324::AID-MRD6>3.0.CO;2-O.

Abstract

We have studied the control of transcription of the testicular angiotensin converting enzyme (ACEt) in normal and transgenic mice. Northern analyses, including a developmental curve and separated germ cells, for ACEt mRNA suggest predominantly post-meiotic expression. Mice transgenic for a construct containing the proximal 298 bp of the rabbit ACEt promoter, with chloramphenicol acetyl transferase (CAT) as a recorder, showed correct tissue regulation while a 86 bp fragment of the promoter led to no expression. Many candidate transacting factor binding elements, previously identified as candidate regulators of transcription driving spermatogenesis, are scattered across this 298 bp in the rabbit (but not the mouse) promoter and may lead to tissue specificity. The recent finding that the proximal 91 bp of the mouse ACEt promoter leads to tissue specific expression of a recorder gene (Howard et al., 1993) emphasizes the difference between the two species and the importance of a cAMP response element (CRE) within this fragment for tissue specific expression. This CRE is conserved in the rabbit promoters we used.

摘要

我们研究了正常小鼠和转基因小鼠中睾丸血管紧张素转换酶(ACEt)的转录调控。对ACEt mRNA进行的Northern分析,包括发育曲线分析和分离的生殖细胞分析,表明其主要在减数分裂后表达。以氯霉素乙酰转移酶(CAT)作为报告基因,对含有兔ACEt启动子近端298 bp的构建体进行转基因的小鼠显示出正确的组织调控,而启动子的86 bp片段则未导致表达。许多先前被鉴定为驱动精子发生的转录候选调节因子的结合元件,分散在兔(而非小鼠)启动子的这298 bp区域内,可能导致组织特异性。最近的研究发现,小鼠ACEt启动子近端91 bp可导致报告基因的组织特异性表达(Howard等人,1993年),这强调了两个物种之间的差异以及该片段内的环磷酸腺苷反应元件(CRE)对组织特异性表达的重要性。我们使用的兔启动子中的这个CRE是保守的。

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