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热带利什曼原虫含有不同的胞质和线粒体谷氨酰胺-tRNA合成酶活性。

Leishmania tarentolae contains distinct cytosolic and mitochondrial glutaminyl-tRNA synthetase activities.

作者信息

Nabholz C E, Hauser R, Schneider A

机构信息

Institute of Zoology, University of Fribourg, Pérolles, CH-1700 Fribourg, Switzerland.

出版信息

Proc Natl Acad Sci U S A. 1997 Jul 22;94(15):7903-8. doi: 10.1073/pnas.94.15.7903.

Abstract

The intracellular distribution of glutaminyl-tRNA synthetases and their role in mitochondrial tRNA import were evaluated in the ancient eukaryote Leishmania tarentolae. The following results were obtained: (i) Glutaminyl-tRNA synthetase was detected in leishmanial mitochondria. This was unexpected because it has been postulated that, in organelles, Gln-tRNAGln is not formed by direct acylation of tRNAGln but by enzymatic transamidation of misacylated Glu-tRNAGln. (ii) Whereas the cytosolic extract is able to charge cytosolic and mitochondrial tRNAsGln, the mitochondrial matrix extract does not aminoacylate the cytosol-specific tRNAGln. This indicates that mitochondrial and cytosolic glutaminyl-tRNA synthetases are distinct. (iii) Seven of the 11 nucleotides that differ between the cytosolic and the mitochondrial tRNAGln are sufficient to convert the cytosol-specific tRNAGln into an optimal substrate for the mitochondrial enzyme. These nucleotides are arranged in three groups consisting of the nucleotides flanking the anticodon stem, the 5' nucleotide of the anticodon, and four nucleotides within the acceptor stem. And (iv), it was shown that the identity elements for recognition by the mitochondrial glutaminyl-tRNA synthetase do not overlap with a previously identified sequence segment required for mitochondrial import of the tRNAGln.

摘要

在古老的真核生物大利什曼原虫中,对谷氨酰胺基-tRNA合成酶的细胞内分布及其在线粒体tRNA导入中的作用进行了评估。得到了以下结果:(i) 在利什曼原虫线粒体中检测到谷氨酰胺基-tRNA合成酶。这出乎意料,因为据推测,在细胞器中,Gln-tRNAGln不是通过tRNAGln的直接酰化形成,而是通过错误酰化的Glu-tRNAGln的酶促转酰胺作用形成。(ii) 虽然胞质提取物能够对胞质和线粒体tRNAsGln进行氨酰化,但线粒体基质提取物不能对胞质特异性tRNAGln进行氨酰化。这表明线粒体和胞质谷氨酰胺基-tRNA合成酶是不同的。(iii) 胞质和线粒体tRNAGln之间不同的11个核苷酸中的7个足以将胞质特异性tRNAGln转化为线粒体酶的最佳底物。这些核苷酸分为三组,包括反密码子茎两侧的核苷酸、反密码子的5'核苷酸以及接受茎内的四个核苷酸。并且(iv),结果表明,线粒体谷氨酰胺基-tRNA合成酶识别的识别元件与先前确定的tRNAGln线粒体导入所需的序列片段不重叠。

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