Servillo L, Balestrieri C, Quagliuolo L, Iorio E L, Giovane A
Department of Biochemistry and Biophysics, University of Naples, Italy.
Eur J Biochem. 1993 Apr 1;213(1):583-9. doi: 10.1111/j.1432-1033.1993.tb17797.x.
A fluorescent tRNA derivative labeled at 3'-O position of the ultimate adenosine residue by reaction, under mild conditions, of tRNA with isatoic anhydride [3,1-benzoxazine-2,4(1H)-dione] was obtained. The labeling selectivity was determined by several criteria: digestion with RNase, followed by HPLC of the digest, produces only one labeled nucleoside, identified as 3'-O-anthraniloyladenosine; the ratio of the absorbance at 260 nm to 332 nm also suggests a 1:1 molar ratio between the nucleic acid and the fluorophore; finally, the incapacity of the labeled tRNA to be charged by the specific aminoacyltransferase further demonstrates the engagement of the 3'-O position. Although the 3'-O-anthraniloyl-labeled tRNA does not seem to be functionally active, as far as the aminoacyl charging activity is concerned, surprisingly we found that it is able to form the ternary complex with elongation factor Tu (EF-Tu) and GTP with an affinity consistently higher than uncharged tRNA. From fluorescence anisotropy measurements the ternary complex dissociation constant was estimated as 73 nM for Escherichia coli and 140 nM for yeast anthraniloyl-tRNA(Phe). These results may be interpreted in terms of the particular structure of the anthraniloyl group that makes the labeled tRNA similar to an aminoacyl-tRNA.
通过在温和条件下使tRNA与异吲哚酸酐[3,1-苯并恶嗪-2,4(1H)-二酮]反应,获得了在末端腺苷残基的3'-O位置标记的荧光tRNA衍生物。标记选择性通过几个标准来确定:用核糖核酸酶消化,随后对消化产物进行高效液相色谱分析,仅产生一种标记的核苷,鉴定为3'-O-邻氨基苯甲酰腺苷;260nm与332nm处吸光度的比值也表明核酸与荧光团之间的摩尔比为1:1;最后,标记的tRNA不能被特定的氨酰基转移酶充电,进一步证明了3'-O位置的参与。尽管就氨酰基充电活性而言,3'-O-邻氨基苯甲酰基标记的tRNA似乎没有功能活性,但令人惊讶的是,我们发现它能够与延伸因子Tu(EF-Tu)和GTP形成三元复合物,其亲和力始终高于未充电的tRNA。通过荧光各向异性测量,大肠杆菌的三元复合物解离常数估计为73 nM,酵母邻氨基苯甲酰基-tRNA(Phe)的解离常数估计为140 nM。这些结果可以根据邻氨基苯甲酰基的特殊结构来解释,该结构使标记的tRNA类似于氨酰基-tRNA。
