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发现并鉴定一种参与古菌 tRNA 修饰的氨甲酰转移酶。

Discovery and characterization of an amidinotransferase involved in the modification of archaeal tRNA.

机构信息

Department of Microbiology, University of Florida, Gainesville, Florida 32611-0700, USA.

出版信息

J Biol Chem. 2010 Apr 23;285(17):12706-13. doi: 10.1074/jbc.M110.102236. Epub 2010 Feb 3.

Abstract

The presence of the 7-deazaguanosine derivative archaeosine (G(+)) at position 15 in tRNA is one of the diagnostic molecular characteristics of the Archaea. The biosynthesis of this modified nucleoside is especially complex, involving the initial production of 7-cyano-7-deazaguanine (preQ(0)), an advanced precursor that is produced in a tRNA-independent portion of the biosynthesis, followed by its insertion into the tRNA by the enzyme tRNA-guanine transglycosylase (arcTGT), which replaces the target guanine base yielding preQ(0)-tRNA. The enzymes responsible for the biosynthesis of preQ(0) were recently identified, but the enzyme(s) catalyzing the conversion of preQ(0)-tRNA to G(+)-tRNA have remained elusive. Using a comparative genomics approach, we identified a protein family implicated in the late stages of archaeosine biosynthesis. Notably, this family is a paralog of arcTGT and is generally annotated as TgtA2. Structure-based alignments comparing arcTGT and TgtA2 reveal that TgtA2 lacks key arcTGT catalytic residues and contains an additional module. We constructed a Haloferax volcanii DeltatgtA2 derivative and demonstrated that tRNA from this strain lacks G(+) and instead accumulates preQ(0). We also cloned the corresponding gene from Methanocaldococcus jannaschii (mj1022) and characterized the purified recombinant enzyme. Recombinant MjTgtA2 was shown to convert preQ(0)-tRNA to G(+)-tRNA using several nitrogen sources and to do so in an ATP-independent process. This is the only example of the conversion of a nitrile to a formamidine known in biology and represents a new class of amidinotransferase chemistry.

摘要

在 tRNA 中,位于 15 位的 7-脱氮鸟苷衍生物(archaeosine,G(+))是古菌的特征性分子标志物之一。该修饰核苷的生物合成过程尤其复杂,涉及到初始产物 7-氰基-7-脱氮鸟苷(preQ(0))的生成,preQ(0)是生物合成中非 tRNA 依赖部分的一个高级前体,然后由 tRNA-鸟嘌呤转糖苷酶(arcTGT)将其插入 tRNA 中,取代靶标鸟嘌呤碱基生成 preQ(0)-tRNA。负责 preQ(0)生物合成的酶最近已经被鉴定出来,但催化 preQ(0)-tRNA 转化为 G(+)-tRNA 的酶仍然难以捉摸。我们使用比较基因组学方法,鉴定出一个参与 archaeosine 生物合成晚期阶段的蛋白质家族。值得注意的是,这个家族是 arcTGT 的旁系同源物,通常被注释为 TgtA2。基于结构的比对分析表明,TgtA2 缺乏关键的 arcTGT 催化残基,并包含一个额外的模块。我们构建了一个 Haloferax volcanii DeltatgtA2 衍生物,并证明该菌株的 tRNA 缺乏 G(+),而是积累了 preQ(0)。我们还从 Methanocaldococcus jannaschii (mj1022) 中克隆了相应的基因,并对纯化的重组酶进行了表征。结果表明,重组 MjTgtA2 可以利用多种氮源将 preQ(0)-tRNA 转化为 G(+)-tRNA,并且该反应是在 ATP 非依赖的过程中进行的。这是生物学中唯一已知的将腈转化为脒的例子,代表了一类新的酰胺转移酶化学。

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