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从大豆子叶中纯化亮氨酸同工tRNA:I. 苯甲酰化二乙氨基纤维素分级分离、N-羟基琥珀酰亚胺修饰及产物表征

Purification of Leucine tRNA Isoaccepting Species from Soybean Cotyledons: I. Benzoylated Diethylamino Cellulose Fractionation, N-Hydroxysuccinimide Modification, and Characterization of Product.

作者信息

Lester B R, Cherry J H

机构信息

Department of Horticulture, Purdue University, West Lafayette, Indiana 47907.

出版信息

Plant Physiol. 1979 Jan;63(1):79-86. doi: 10.1104/pp.63.1.79.

Abstract

Transfer RNA from soybean (Glycine max) cotyledons was purified to homogeneity followed by the purification of the family of leucine tRNA via benzoylated diethylaminoethyl cellulose (BDC) chromatography. Nonacylated total purified tRNA was salicylhydroxamate (SHAM) modified by the phenoxyacetyl method and fractionated into three peaks on a BDC column. The first peak containing bulk tRNA with no hydrophobic character amounted to 78% of the added tRNA. The second peak containing 19% of the added tRNA and represents the tRNA with intrinsic hydrophobic properties. The third peak containing 3% of the tRNA represents the SHAM modified tRNA and nonspecifically modified tRNA. Transfer RNA peaks I and II were pooled and subsequently stoichiometrically acylated in two batches, one containing [(14)C]leucine while the other contained unlabeled leucine. The acylated tRNA was loaded on and step-eluted from a BDC column. The purified acylated-tRNA was phenoxyacetyl modified and following ethanol precipitation was fractionated on a BDC column. A double peak eluted from the column in the ethanol gradient contained 5.3% of the starting optical density and 85.3% of the starting counts per minute. Characterization of this leucine tRNA showed typical ultraviolet spectra properties and appeared to be homogeneous on a G-100 Sephadex column. The minimum purity of the tRNA was 32 to 35%. Finally, the acylated tRNA was chromatographed on an RPC-2 column giving six leucine isoaccepting tRNAs. The data indicate that leucine tRNA was highly purified without losing the integrity of the family of isoacceptors.

摘要

大豆(Glycine max)子叶中的转移RNA被纯化至同质,随后通过苯甲酰化二乙氨基乙基纤维素(BDC)色谱法纯化亮氨酸tRNA家族。未酰化的总纯化tRNA通过苯氧乙酰法进行水杨羟肟酸(SHAM)修饰,并在BDC柱上分离成三个峰。第一个峰包含无疏水特性的大量tRNA,占添加tRNA的78%。第二个峰包含19%的添加tRNA,代表具有内在疏水特性的tRNA。第三个峰包含3%的tRNA,代表SHAM修饰的tRNA和非特异性修饰的tRNA。将转移RNA峰I和II合并,随后分两批进行化学计量酰化,一批含有[(14)C]亮氨酸,另一批含有未标记的亮氨酸。将酰化的tRNA加载到BDC柱上并进行分步洗脱。纯化的酰化tRNA进行苯氧乙酰修饰,乙醇沉淀后在BDC柱上分离。在乙醇梯度中从柱上洗脱的双峰包含起始光密度的5.3%和起始每分钟计数的85.3%。这种亮氨酸tRNA的表征显示出典型的紫外光谱特性,并且在G-100 Sephadex柱上似乎是同质的。tRNA的最低纯度为32%至35%。最后,酰化的tRNA在RPC-2柱上进行色谱分离,得到六种亮氨酸同工受体tRNA。数据表明亮氨酸tRNA被高度纯化,同时没有失去同工受体家族的完整性。

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