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不均一核RNA二级结构:与聚腺苷酸碱基配对的寡聚(U)序列及其作为不均一核RNA特异性蛋白质结合位点的可能作用。

Heterogeneous nuclear RNA secondary structure: oligo (U) sequences base-paired with poly (A) and their possible role as binding sites for heterogeneous nuclear RNA-specific proteins.

作者信息

Kish V M, Pederson T

出版信息

Proc Natl Acad Sci U S A. 1977 Apr;74(4):1426-30. doi: 10.1073/pnas.74.4.1426.

Abstract

HeLa cell heterogeneous nuclear RNA derived from high-molecular-weight nuclear ribonucleoprotein (RNP) particles contains oligo(U) sequences of 15-50 nucleotides base-paired with poly(A). These duplexes are resistant to pancreatic RNase at 0.5 M NaCl in native RNP, remain so after chemical deproteinization of the RNP digests, and then copurify with poly(A) on oligo(dT)-cellulose chromatography. Oligo(dT)-cellulose binding capacity of the oligo(U)-poly(A) duplexes is abolished by prior titration of the nonduplex poly(A) regions with excess poly(U). The oligo(dT)-purified fraction is 97.5 mole % A + U and the [3H]uridine-labeled component is resistant to redigestion by pancreatic RNase at 0.5 M NaCl but not at 0.01 M NaCl. After thermal denaturation, the [3H]uridine-labeled chains become RNase-sensitive at 0.5 M NaCl. Electrophoresis of [3H]adenosine- or [3H]uridine-labeled material in polyacrylamide gels containing 99% formamide confirms that the oligo(U) sequences are not covalently linked to poly(A). Controls establish that the A-U duplexes are not formed artifactually during isolation of heterogeneous nuclear RNP or subsequent fractionation. The oligo(U)-poly(A) duplexes appear to be associated with protein in native heterogeneous nuclear RNP, as reflected by the differential pancreatic RNase sensitivity of the duplexed oligo(U) in RNP (resistant) and RNA (sensitive), measured at physiological ionic strength.

摘要

源自高分子量核糖核蛋白(RNP)颗粒的海拉细胞不均一核RNA含有15 - 50个核苷酸的寡聚(U)序列,这些序列与多聚(A)碱基配对。在天然RNP中,这些双链体在0.5M NaCl条件下对胰核糖核酸酶有抗性,在RNP消化物化学脱蛋白后仍保持这种抗性,然后在寡聚(dT)-纤维素色谱上与多聚(A)共纯化。通过用过量的聚(U)预先滴定非双链多聚(A)区域,寡聚(U)-多聚(A)双链体的寡聚(dT)-纤维素结合能力被消除。寡聚(dT)纯化的部分为97.5摩尔%的A + U,并且[3H]尿苷标记的组分在0.5M NaCl但不在0.01M NaCl条件下对胰核糖核酸酶的再消化有抗性。热变性后,[3H]尿苷标记的链在0.5M NaCl条件下对核糖核酸酶敏感。在含有99%甲酰胺的聚丙烯酰胺凝胶中对[3H]腺苷或[3H]尿苷标记的物质进行电泳,证实寡聚(U)序列不与多聚(A)共价连接。对照表明,在不均一核RNP的分离或随后的分级分离过程中,A - U双链体不是人为形成的。寡聚(U)-多聚(A)双链体似乎在天然不均一核RNP中与蛋白质相关,这通过在生理离子强度下测量的RNP(抗性)和RNA(敏感)中双链寡聚(U)对胰核糖核酸酶的不同敏感性来反映。

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