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胍丁胺,古细菌 tRNA(Ile)反密码子中的一种修饰胞嘧啶,与腺嘌呤配对而不与鸟嘌呤配对。

Agmatidine, a modified cytidine in the anticodon of archaeal tRNA(Ile), base pairs with adenosine but not with guanosine.

机构信息

Department of Biology, Massachusetts Institute of Technology, Cambridge, MA 02139, USA.

出版信息

Proc Natl Acad Sci U S A. 2010 Feb 16;107(7):2872-7. doi: 10.1073/pnas.0914869107. Epub 2010 Jan 26.

Abstract

Modification of the cytidine in the first anticodon position of the AUA decoding tRNA(Ile) (tRNA2(Ile)) of bacteria and archaea is essential for this tRNA to read the isoleucine codon AUA and to differentiate between AUA and the methionine codon AUG. To identify the modified cytidine in archaea, we have purified this tRNA species from Haloarcula marismortui, established its codon reading properties, used liquid chromatography-mass spectrometry (LC-MS) to map RNase A and T1 digestion products onto the tRNA, and used LC-MS/MS to sequence the oligonucleotides in RNase A digests. These analyses revealed that the modification of cytidine in the anticodon of tRNA2(Ile) adds 112 mass units to its molecular mass and makes the glycosidic bond unusually labile during mass spectral analyses. Accurate mass LC-MS and LC-MS/MS analysis of total nucleoside digests of the tRNA2(Ile) demonstrated the absence in the modified cytidine of the C2-oxo group and its replacement by agmatine (decarboxy-arginine) through a secondary amine linkage. We propose the name agmatidine, abbreviation C(+), for this modified cytidine. Agmatidine is also present in Methanococcus maripaludis tRNA2(Ile) and in Sulfolobus solfataricus total tRNA, indicating its probable occurrence in the AUA decoding tRNA(Ile) of euryarchaea and crenarchaea. The identification of agmatidine shows that bacteria and archaea have developed very similar strategies for reading the isoleucine codon AUA while discriminating against the methionine codon AUG.

摘要

对细菌和古菌的 AUA 解码 tRNA(Ile)(tRNA2(Ile))的反密码子第一位的胞嘧啶进行修饰对于该 tRNA 读取异亮氨酸密码子 AUA 并区分 AUA 和甲硫氨酸密码子 AUG 至关重要。为了鉴定古菌中的修饰胞嘧啶,我们从盐沼盐杆菌中纯化了这种 tRNA 种类,确定了其密码子阅读特性,使用液相色谱-质谱联用 (LC-MS) 将 RNase A 和 T1 消化产物映射到 tRNA 上,并使用 LC-MS/MS 对 RNase A 消化物中的寡核苷酸进行测序。这些分析表明,tRNA2(Ile)反密码子中胞嘧啶的修饰为其分子量增加了 112 个质量单位,并使其糖苷键在质谱分析中异常不稳定。对 tRNA2(Ile)的总核苷消化物进行精确质量 LC-MS 和 LC-MS/MS 分析表明,修饰胞嘧啶中不存在 C2-氧代基团,而是通过仲胺键被胍基丁氨酸(脱羧精氨酸)取代。我们提议将这种修饰的胞嘧啶命名为胍丁啶,缩写为 C(+)。胍丁啶也存在于 Methanococcus maripaludis tRNA2(Ile)和 Sulfolobus solfataricus 总 tRNA 中,表明其可能存在于真细菌和古细菌的 AUA 解码 tRNA(Ile)中。胍丁啶的鉴定表明,细菌和古菌在读取异亮氨酸密码子 AUA 的同时,发展出了非常相似的策略,从而区分了甲硫氨酸密码子 AUG。

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