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克隆的tRNA基因片段和亚片段转录后注入非洲爪蟾卵母细胞核内。

Transcription of cloned tRNA gene fragments and subfragments injected into the oocyte nucleus of Xenopus laevis.

作者信息

Kressmann A, Clarkson S G, Pirrotta V, Birnstiel M L

出版信息

Proc Natl Acad Sci U S A. 1978 Mar;75(3):1176-80. doi: 10.1073/pnas.75.3.1176.

Abstract

Cloned 3.18 kilobase fragments of Xenopus laevis DNA containing genes for tRNAMet1 and for at least one other 4S RNA species are transcribed rapidly after their injection into the nucleus of X. laevis oocytes. The newly synthesized RNA can be resolved by gel electrophoresis into a few predominant 4S RNA species and a series of slower migrating components. One of the 4S RNA species appears to be identical, by fingerprint analysis, to the tRNAMet1 isolated by hybridization of somatic cell RNA to this cloned tRNA gene fragment (tDNA). Thus, the tRNAMet1 produced after injection can be both fully processed and modified. Its rate of synthesis is estimated to be about 6 x 10(9) molecules/hr in each oocyte injected with 2 ng of tDNA. When the tDNA fragment is cleaved into two halves with restriction endonuclease Sst I, each injected half gives rise to a subset of the RNAs produced after injection of the intact fragment. This experiment thus suggests the presence of at least two transcriptional units on this cloned tDNA. This simple way of biologically testing defined restriction fragments may be of value for analyzing the functional organization of other cloned eukaryotic DNA units.

摘要

含有甲硫氨酸转运RNA基因(tRNAMet1)和至少一种其他4S RNA种类基因的非洲爪蟾DNA的3.18千碱基克隆片段,在注入非洲爪蟾卵母细胞核后能迅速被转录。新合成的RNA通过凝胶电泳可分离为几种主要的4S RNA种类和一系列迁移较慢的组分。通过指纹分析,其中一种4S RNA种类似乎与通过体细胞RNA与该克隆的tRNA基因片段(tDNA)杂交分离得到的tRNAMet1相同。因此,注射后产生的tRNAMet1能够被完全加工和修饰。在每个注射了2纳克tDNA的卵母细胞中,其合成速率估计约为6×10⁹个分子/小时。当用限制性内切酶Sst I将tDNA片段切成两半时,每个注射的半片段产生的RNA是完整片段注射后产生的RNA的一个子集。因此,该实验表明在这个克隆的tDNA上至少存在两个转录单位。这种对特定限制性片段进行生物学测试的简单方法,对于分析其他克隆的真核DNA单位的功能组织可能具有价值。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6bdf/411432/73f70b63c4cf/pnas00015-0139-a.jpg

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