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黑腹果蝇胚胎发育过程中多巴脱羧酶表达的分析。

An analysis of dopa decarboxylase expression during embryogenesis in Drosophila melanogaster.

作者信息

Gietz R D, Hodgetts R B

出版信息

Dev Biol. 1985 Jan;107(1):142-55. doi: 10.1016/0012-1606(85)90383-5.

Abstract

Dopa decarboxylase (DDC) activity appears near the end of embryogenesis in Drosophila. High titers of 20-OH-ecdysone on the other hand are found at midembryogenesis. Several explanations for this lag were investigated, since this hormone has been shown to induce a rapid increase in DDC activity at pupariation (G. P. Kraminsky, W. C. Clark, M. A. Estelle, R. D. Gietz, B. A. Sage, J. D. O'Connor, and R. B. Hodgetts, 1980, Proc. Natl. Acad. Sci. USA 77, 4175-4179). Using immunological and genetical criteria, it was shown that the same structural gene encodes DDC in embryos, mature larvae, and young adults. This rules out the existence of a distinct embryonic DDC gene unresponsive to 20-OH-ecdysone. Second, no evidence was found to support the hypothesis that a delay in the translation of DDC transcripts, produced in response to the elevated titer of 20-OH-ecdysone at midembryogenesis, caused the lag. Northern analysis of the RNA molecules homologous to cloned genomic sequences revealed that DDC transcripts were present at two different times during embryogenesis. A transcript was found in both ovaries and 0- to 2-hr embryos. However, this species disappeared by 4 hr and DDC transcript levels remained low until late in embryogenesis, when a significant increase occurred. This increase was presumably responsible for the appearance of the enzyme at this time. The northern blotting revealed nine DDC transcript species were present during embryogenesis and hybridization to intron-specific probes indicated that five of these contained at least part of one (or both) of the two introns. Three putative mature mRNA species were identified by their small size, relative abundance, apparent lack of intron sequence, and their presence on polysomes. The two mature species found during the late stages were postulated to differ in the length of their poly(A)+ tails. The third mature species was found only in ovaries and very young embryos and may well be of maternal origin. Data are examined in light of the possibility that this species is derived from a precursor initiated at a novel promotor.

摘要

多巴脱羧酶(DDC)活性在果蝇胚胎发育后期出现。另一方面,在胚胎发育中期可发现高滴度的20-羟基蜕皮激素。由于已证明这种激素在化蛹时能诱导DDC活性迅速增加(G.P.克拉明斯基、W.C.克拉克、M.A.埃斯特尔、R.D.吉茨、B.A.塞奇、J.D.奥康纳和R.B.霍奇茨,1980年,《美国国家科学院院刊》77卷,4175 - 4179页),因此对这种延迟现象进行了几种解释的研究。利用免疫学和遗传学标准表明,在胚胎、成熟幼虫和年轻成虫中,同一个结构基因编码DDC。这排除了存在一个对20-羟基蜕皮激素无反应的独特胚胎DDC基因的可能性。其次,没有发现证据支持这样的假说,即胚胎发育中期20-羟基蜕皮激素滴度升高所产生的DDC转录本翻译延迟导致了这种延迟。对与克隆基因组序列同源的RNA分子进行的Northern分析表明,DDC转录本在胚胎发育过程中出现在两个不同的时间。在卵巢和0至2小时的胚胎中都发现了一种转录本。然而,这种转录本在4小时时消失,并且DDC转录本水平在胚胎发育后期之前一直保持较低,直到后期才出现显著增加。这种增加可能是此时该酶出现的原因。Northern印迹分析表明,胚胎发育过程中存在9种DDC转录本,与内含子特异性探针杂交表明其中5种至少包含两个内含子中的一个(或两个)的一部分。通过它们的小尺寸、相对丰度、明显缺乏内含子序列以及它们在多核糖体上的存在,鉴定出了三种假定的成熟mRNA物种。后期发现的两种成熟物种被推测在其聚腺苷酸(poly(A)+)尾巴的长度上有所不同。第三种成熟物种仅在卵巢和非常年轻的胚胎中发现,很可能是母源的。根据这种物种可能源自一个由新启动子起始的前体的可能性对数据进行了研究。

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