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两种不同调控元件之间的相互作用激活了移植晶状体上皮细胞中的小鼠αA-晶状体蛋白基因启动子。

Interaction between two different regulatory elements activates the murine alpha A-crystallin gene promoter in explanted lens epithelia.

作者信息

Chepelinsky A B, Sommer B, Piatigorsky J

出版信息

Mol Cell Biol. 1987 May;7(5):1807-14. doi: 10.1128/mcb.7.5.1807-1814.1987.

Abstract

Previous experiments have indicated that 5' flanking DNA sequences (nucleotides-366 to +46) are capable of regulating the lens-specific transcription of the murine alpha A-crystallin gene. Here we have analyzed these 5' regulatory sequences by transfecting explanted embryonic chicken lens epithelia with different alpha A-crystallin-CAT (chloramphenicol acetyltransferase) hybrid genes (alpha A-crystallin promoter sequences fused to the bacterial CAT gene in the pSVO-CAT expression vector). The results indicated the presence of a proximal (-88 to +46) and a distal (-111 to -88) domain which must interact for promoter function. Deletion experiments showed that the sequence between -88 and -60 was essential for function of the proximal domain in the explanted epithelia. A synthetic oligonucleotide containing the sequence between -111 and -84 activated the proximal domain when placed in either orientation 57 base pairs upstream from position -88 of the alpha A-crystallin-CAT hybrid gene.

摘要

先前的实验表明,5'侧翼DNA序列(核苷酸-366至+46)能够调节小鼠αA-晶状体蛋白基因的晶状体特异性转录。在此,我们通过用不同的αA-晶状体蛋白-氯霉素乙酰转移酶(CAT)杂交基因(αA-晶状体蛋白启动子序列与pSVO-CAT表达载体中的细菌CAT基因融合)转染外植的胚胎鸡晶状体上皮细胞,分析了这些5'调控序列。结果表明存在一个近端结构域(-88至+46)和一个远端结构域(-111至-88),它们必须相互作用才能实现启动子功能。缺失实验表明,-88至-60之间的序列对于外植上皮细胞中近端结构域的功能至关重要。当一个含有-111至-84之间序列的合成寡核苷酸以任一方向置于αA-晶状体蛋白-CAT杂交基因-88位上游57个碱基对处时,它能激活近端结构域。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a75e/365283/fd5c5c836ae6/molcellb00077-0237-a.jpg

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