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含有12S和9S核糖体RNA的布氏锥虫线粒体核糖核蛋白复合体。

Trypanosoma brucei mitochondrial ribonucleoprotein complexes which contain 12S and 9S ribosomal RNAs.

作者信息

Shu H H, Göringer H U

机构信息

Laboratorium für molekulare Biologie-Genzentrum der LMU München am Max-Planck-Institut für Biochemie, Martinsried, Germany.

出版信息

Parasitology. 1998 Feb;116 ( Pt 2):157-64. doi: 10.1017/s0031182097002023.

Abstract

Antibiotics have been widely used to identify ribosomal activity in Trypanosoma brucei mitochondria. The validity of some of the results has been questioned because the permeability of the trypanosome cell membrane for some antibiotics was not adequately addressed. Here we describe translation inhibition experiments with digitonin-permeabilized trypanosomes to exclude diffusion barriers through the cell membrane. Using this system we were able to confirm, next to the eukaryotic and thus cycloheximide-sensitive translation system, the existence of a prokaryotic-type translational activity being cycloheximide resistant, chloramphenicol sensitive and streptomycin dependent. We interpret this observation analogous to what has been found for other eukarya as the independent protein synthesis activity of the mitochondrial organelle. We further examined the putative translational apparatus by using isokinetic density-gradient analysis of mitochondrial extracts. The 2 mitochondrially encoded rRNAs, the 9S and 12S rRNAs, were found to co-fractionate in a single RNP complex, approximately 80S in size. This complex disassembled at reduced MgCl2 concentrations into 2 unusually small complexes of 17.5S, containing the 9S rRNA, and 20S containing the 12S rRNA. A preliminary stoichiometry determination suggested a multicopy assembly of these putative subunits in a 2:3 ratio (20S:17.5S).

摘要

抗生素已被广泛用于鉴定布氏锥虫线粒体中的核糖体活性。由于某些抗生素对锥虫细胞膜的通透性未得到充分研究,部分结果的有效性受到质疑。在此,我们描述了用洋地黄皂苷通透处理的锥虫进行的翻译抑制实验,以排除细胞膜的扩散屏障。利用该系统,我们能够证实,除了真核生物且对环己酰亚胺敏感的翻译系统外,还存在一种原核生物类型的翻译活性,它对环己酰亚胺具有抗性、对氯霉素敏感且依赖链霉素。我们将这一观察结果解释为与其他真核生物类似,即线粒体细胞器具有独立的蛋白质合成活性。我们还通过对线粒体提取物进行等密度梯度分析,进一步研究了假定的翻译装置。发现线粒体编码的两种rRNA,即9S和12S rRNA,共分离于一个大小约为80S的单一核糖核蛋白复合体中。该复合体在降低的MgCl2浓度下分解为两个异常小的复合体,分别为含有9S rRNA的17.5S复合体和含有12S rRNA的20S复合体。初步的化学计量学测定表明,这些假定的亚基以2:3的比例(20S:17.5S)进行多拷贝组装。

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