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利用分子杂交技术从大鼠肝脏中纯化和分析白蛋白信使核糖核酸。

Use of molecular hybridization to purify and analyze albumin messenger RNA from rat liver.

作者信息

Strair R K, Yap S H, Shafritz D A

出版信息

Proc Natl Acad Sci U S A. 1977 Oct;74(10):4346-50. doi: 10.1073/pnas.74.10.4346.

Abstract

A new procedure is described for purification of rat liver albumin mRNA. First a population of RNA molecules is enriched for albumin mRNA by immunoprecipitation of polysomes containing albumin nascent chains. Polyadenylylated RNA is prepared from immunoprecipitates, transcribed into complementary DNA, and shown to be enriched severalfold for a particular RNA frequency component. This enriched RNA component is then purified by molecular hybridization to a limited R(0)t value (product of RNA concentration and incubation time), under conditions in which only the most abundant sequence component is annealed. Potentially, this procedure can be employed for the purification of a wide variety of mRNAs present in lesser amounts in the cell. The isolated RNA appears to be a single frequency component by hybridization to complementary DNA transcribed from itself. This RNA is a 17S species and represents 5-8% of total cytoplasmic polyadenylylated RNA. In vitro translation of the purified RNA has shown that it codes for a single polypeptide that can be identified immunologically as albumin and migrates with rat serum albumin on sodium dodecyl sulfate/polyacrylamide gels. This albumin mRNA was determined to be essentially pure by comparing its kinetics of hybridization to those obtained with rabbit alpha + beta globin mRNA and its DNA complement. The sequence complexity of purified rat albumin mRNA corresponds to 5.9 x 10(5) daltons.

摘要

本文描述了一种纯化大鼠肝脏白蛋白mRNA的新方法。首先,通过免疫沉淀含有白蛋白新生链的多核糖体,富集RNA分子群体中的白蛋白mRNA。从免疫沉淀产物中制备聚腺苷酸化RNA,转录成互补DNA,并显示出特定RNA频率成分富集了几倍。然后,在仅使最丰富的序列成分退火的条件下,通过与有限的R(0)t值(RNA浓度与孵育时间的乘积)进行分子杂交,纯化这种富集的RNA成分。该方法有可能用于纯化细胞中含量较少的多种mRNA。通过与自身转录的互补DNA杂交,分离得到的RNA似乎是单一频率成分。这种RNA是17S种类,占细胞质聚腺苷酸化RNA总量的5 - 8%。纯化RNA的体外翻译表明,它编码一种单一多肽,经免疫鉴定为白蛋白,并且在十二烷基硫酸钠/聚丙烯酰胺凝胶上与大鼠血清白蛋白迁移情况相同。通过比较其杂交动力学与兔α + β珠蛋白mRNA及其DNA互补物的杂交动力学,确定这种白蛋白mRNA基本纯净。纯化的大鼠白蛋白mRNA的序列复杂度相当于5.9×10(5)道尔顿。

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