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从小牛胸腺中对两种相关的单链核酸结合蛋白UP1和UP2进行高压液相色谱纯化。

High pressure liquid chromatography purification of UP1 and UP2, two related single-stranded nucleic acid-binding proteins from calf thymus.

作者信息

Merrill B M, LoPresti M B, Stone K L, Williams K R

出版信息

J Biol Chem. 1986 Jan 15;261(2):878-83.

PMID:3941105
Abstract

Two single-stranded nucleic acid-binding proteins, UP1 and UP2, that were originally reported by Herrick and Alberts (Herrick, G., and Alberts, B. (1976) J. Biol. Chem. 251, 2124-2132) have been purified to apparent homogeneity from calf thymus by high performance liquid chromatography. The amino acid sequence of UP1 (Williams, K. R., Stone, K. L., LoPresti, M. B., Merrill, B. M., and Planck, S. R. (1985) Proc. Natl. Acad. Sci. U. S. A. 82, 5666-5670) reveals that UP1 contains 195 amino acids, including one dimethylarginine residue near its COOH terminus. Further analysis of this sequence now demonstrates that UP1 contains a 91-residue internal repeat such that when residues 3-93 (the "A" region) are aligned with residues 94-194 (the "B" region), 32% of the amino acids in these two regions are identical and an additional 39% of those changes that are seen could be accomplished by single base changes. The high degree of internal homology between residues 51-61 and 143-152 and in particular the high density of aromatic and positively charged amino acids in these two regions suggest that residues 51-61 and 143-152 may constitute two independent DNA-binding sites. Solid-phase sequencing of three tryptic peptides that together account for 9% of the 39,500-dalton UP2 protein demonstrate that there is a high degree of sequence homology between UP1 and UP2. Of the 34 residues that have been sequenced in UP2, 44% are identical in both UP1 and UP2. The blocked NH2 terminus, amino acid composition, particularly with regard to its high glycine content and the presence of dimethylarginine, and molecular weight of UP2 suggest this protein is related to proteins that have previously been found associated with heterogeneous RNA. Taken together, these data indicate that both UP1 and UP2 belong to a new family of single-stranded nucleic acid-binding proteins that may be closely related to heterogeneous ribonucleoproteins.

摘要

两种单链核酸结合蛋白,UP1和UP2,最初由赫里克和阿尔伯茨报道(赫里克,G.,和阿尔伯茨,B.(1976年)《生物化学杂志》251,2124 - 2132),已通过高效液相色谱法从小牛胸腺中纯化至表观均一。UP1的氨基酸序列(威廉姆斯,K.R.,斯通,K.L.,洛普雷蒂,M.B.,梅里尔,B.M.,和普朗克,S.R.(1985年)《美国国家科学院院刊》82,5666 - 5670)表明UP1含有195个氨基酸,在其COOH末端附近有一个二甲基精氨酸残基。对该序列的进一步分析现在表明,UP1含有一个91个残基的内部重复序列,使得当残基3 - 93(“A”区域)与残基94 - 194(“B”区域)比对时,这两个区域中32%的氨基酸是相同的,并且在这些可见变化中另外39%的变化可以通过单碱基变化实现。残基51 - 61和143 - 152之间高度的内部同源性,特别是这两个区域中芳香族和带正电荷氨基酸的高密度表明,残基51 - 61和143 - 152可能构成两个独立的DNA结合位点。对总共占39,500道尔顿UP2蛋白9%的三个胰蛋白酶肽段的固相测序表明,UP1和UP2之间存在高度的序列同源性。在UP2中已测序的34个残基中,44%在UP1和UP2中是相同的。UP2封闭的NH2末端、氨基酸组成,特别是其高甘氨酸含量和二甲基精氨酸的存在以及分子量表明,这种蛋白质与先前发现与不均一RNA相关的蛋白质有关。综上所述,这些数据表明UP1和UP2都属于一个新的单链核酸结合蛋白家族,可能与不均一核糖核蛋白密切相关。

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