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发育调控且视网膜特异性的核蛋白与大鼠视蛋白基因上游区域一个位点结合的特性分析。

Characterization of developmentally regulated and retina-specific nuclear protein binding to a site in the upstream region of the rat opsin gene.

作者信息

Morabito M A, Yu X, Barnstable C J

机构信息

Department of Ophthalmology and Visual Science, Yale University School of Medicine, New Haven, Connecticut 06510.

出版信息

J Biol Chem. 1991 May 25;266(15):9667-72.

PMID:1827795
Abstract

DNase I protection and gel retardation assays have identified a sequence 5' to the transcription start site of the rat opsin gene that interacts with nuclear proteins from mammalian retinas but not from a variety of other neural and non-neural tissues. Following sodium dodecyl sulfate-polyacrylamide gel electrophoresis and transfer to nitrocellulose the protein(s) responsible for this binding were identified with an oligonucleotide probe and were found to migrate with an apparent molecular size of 40 kilodaltons. The binding complex eluted from fast protein liquid chromatography gel filtration as a peak centered at 100 kilodaltons, suggesting the presence of more than one subunit. Binding activity could be detected in postnatal day 1 retinal extracts and increased over the next 2 weeks of development, a time course coincident with opsin gene expression and maturation of rod photoreceptors. Synthetic oligonucleotides with altered sequences showed that the binding was dependent upon residues in a CTAAT motif and was facilitated by surrounding GGCCCC sequences. The specificity of the binding interaction was measured by inhibition of complex formation in a gel retardation assay. The unaltered sequence was over 2 orders of magnitude more effective at inhibiting complex formation than either an unrelated DNA sequence or a concensus sequence corresponding to a known CCAAT box binding protein NF1.

摘要

DNA酶I保护试验和凝胶阻滞试验已鉴定出大鼠视蛋白基因转录起始位点5'端的一段序列,该序列能与来自哺乳动物视网膜的核蛋白相互作用,但不能与多种其他神经和非神经组织的核蛋白相互作用。在进行十二烷基硫酸钠-聚丙烯酰胺凝胶电泳并转移至硝酸纤维素膜后,用寡核苷酸探针鉴定出负责这种结合的蛋白质,发现其表观分子量为40千道尔顿。从快速蛋白质液相色谱凝胶过滤中洗脱的结合复合物以100千道尔顿为中心的峰形式出现,表明存在不止一个亚基。在出生后第1天的视网膜提取物中可检测到结合活性,并在接下来的2周发育过程中增加,这一时间进程与视蛋白基因表达和视杆光感受器的成熟一致。具有改变序列的合成寡核苷酸表明,这种结合依赖于CTAAT基序中的残基,并受到周围GGCCCC序列的促进。通过凝胶阻滞试验中复合物形成的抑制来测量结合相互作用的特异性。未改变的序列在抑制复合物形成方面比无关DNA序列或对应于已知CCAAT盒结合蛋白NF1的共有序列有效2个数量级以上。

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