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酵母tRNA连接酶功能结构域的遗传与生化分析

Genetic and biochemical analysis of the functional domains of yeast tRNA ligase.

作者信息

Sawaya Rana, Schwer Beate, Shuman Stewart

机构信息

Molecular Biology Program, Sloan-Kettering Institute, New York, New York 10021, USA.

出版信息

J Biol Chem. 2003 Nov 7;278(45):43928-38. doi: 10.1074/jbc.M307839200. Epub 2003 Aug 21.

DOI:10.1074/jbc.M307839200
PMID:12933796
Abstract

Yeast tRNA ligase (Trl1) converts cleaved tRNA half-molecules into spliced tRNAs containing a 2'-PO4, 3'-5' phosphodiester at the splice junction. Trl1 performs three reactions: (i) the 2',3'-cyclic phosphate of the proximal fragment is hydrolyzed to a 3'-OH, 2'-PO4 by a cyclic phosphodiesterase (CPD); (ii) the 5'-OH of the distal fragment is phosphorylated by an NTP-dependent polynucleotide kinase; and (iii) the 3'-OH, 2'-PO4, and 5'-PO4 ends are sealed by an ATP-dependent RNA ligase. Trl1 consists of an N-terminal adenylyltransferase domain that resembles T4 RNA ligase 1, a central domain that resembles T4 polynucleotide kinase, and a C-terminal CPD domain that resembles the 2H phosphotransferase enzyme superfamily. Here we show that all three domains are essential in vivo, although they need not be linked in the same polypeptide. We identify five amino acids in the adenylyltransferase domain (Lys114, Glu266, Gly267, Lys284, and Lys286) that are essential for Trl1 activity and are located within motifs I (114KANG117), IV (266EGFVI270), and V (282FFKIK286) that comprise the active sites of DNA ligases, RNA capping enzymes, and T4 RNA ligases 1 and 2. Mutations K404A and T405A in the P-loop (401GXGKT405) of the central kinase-like domain had no effect on Trl1 function in vivo. The K404A and T405A mutations eliminated ATP-dependent kinase activity but preserved GTP-dependent kinase activity. A double alanine mutant in the P-loop was lethal in vivo and abolished GTP-dependent kinase activity. These results suggest that GTP is the physiological substrate and that the Trl1 kinase has a single NTP binding site of which the P-loop is a component. Two other mutations in the central domain were lethal in vivo and either abolished (D425A) or severely reduced (R511A) GTP-dependent RNA kinase activity in vitro. Mutations of the signature histidines of the CPD domain were either lethal (H777A) or conferred a ts growth phenotype (H673A).

摘要

酵母tRNA连接酶(Trl1)将切割后的tRNA半分子转化为在剪接连接处含有2'-磷酸、3'-5'磷酸二酯的剪接tRNA。Trl1执行三个反应:(i)近端片段的2',3'-环磷酸通过环磷酸二酯酶(CPD)水解为3'-羟基、2'-磷酸;(ii)远端片段的5'-羟基由依赖NTP的多核苷酸激酶磷酸化;(iii)3'-羟基、2'-磷酸和5'-磷酸末端由依赖ATP的RNA连接酶封闭。Trl1由一个类似于T4 RNA连接酶1的N端腺苷酸转移酶结构域、一个类似于T4多核苷酸激酶的中央结构域和一个类似于2H磷酸转移酶超家族的C端CPD结构域组成。在这里我们表明,所有这三个结构域在体内都是必需的,尽管它们不必连接在同一多肽中。我们在腺苷酸转移酶结构域中鉴定出五个对Trl1活性至关重要的氨基酸(Lys114、Glu266、Gly267、Lys284和Lys286),它们位于基序I(114KANG117)、IV(266EGFVI270)和V(282FFKIK286)内,这些基序构成了DNA连接酶、RNA封端酶以及T4 RNA连接酶1和2的活性位点。中央类激酶结构域的P环(401GXGKT405)中的K404A和T405A突变在体内对Trl1功能没有影响。K404A和T405A突变消除了依赖ATP的激酶活性,但保留了依赖GTP的激酶活性。P环中的双丙氨酸突变体在体内是致死的,并消除了依赖GTP的激酶活性。这些结果表明GTP是生理底物,并且Trl1激酶具有一个单一的NTP结合位点,其中P环是其组成部分。中央结构域中的另外两个突变在体内是致死的,并且在体外要么消除了(D425A)要么严重降低了(R511A)依赖GTP的RNA激酶活性。CPD结构域的标志性组氨酸突变要么是致死的(H777A)要么赋予温度敏感生长表型(H673A)。

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