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大鼠酪蛋白和α-乳白蛋白cDNA克隆的构建及初步鉴定

Construction and preliminary characterization of the rat casein and alpha-lactalbumin cDNA clones.

作者信息

Richards D A, Rodgers J R, Supowit S C, Rosen J M

出版信息

J Biol Chem. 1981 Jan 10;256(1):526-32.

PMID:7005218
Abstract

We have constructed a double-stranded cDNA library using total poly(A)-containing RNA extracted from 8-day lactating rat mammary gland and have utilized this library to isolate clones for each of the four major milk proteins. These four cDNA clones, representing the three major rat caseins and alpha-lactalbumin, were initially identified by colony hybridization with labeled cDNA probes synthesized from individual mRNA fractions purified by preparative gel electrophoresis. Additional characterization was accomplished by hybridizing individual clones labeled with 32P by nick translation to a Northern gel blot of an enriched fraction of the four major milk protein mRNAs. The individual mRNAs were clearly resolved by electrophoresis on fully denaturing methylmercury hydroxide agarose gels. The identity of each milk protein clone was further established by the location of unique restriction enzyme sites within each clone. Final identification of each clone was performed by hybrid-arrested cell-free translation. The sizes of the milk protein cDNA clones ranged frm 70% for the alpha-lactalbumin gene to essentially full length for the gamma-casein gene, in comparison to their respective mRNAs. This represents the first isolation of a family of peptide hormone-responsive genes.

摘要

我们使用从8日龄泌乳大鼠乳腺中提取的总含聚腺苷酸(poly(A))RNA构建了双链cDNA文库,并利用该文库分离出四种主要乳蛋白各自的克隆。这四个cDNA克隆,分别代表三种主要的大鼠酪蛋白和α-乳白蛋白,最初是通过与由制备性凝胶电泳纯化的各个mRNA组分合成的标记cDNA探针进行菌落杂交来鉴定的。通过将经缺口平移用32P标记的单个克隆与四种主要乳蛋白mRNA富集组分的Northern凝胶印迹杂交,完成了进一步的表征。在完全变性的氢氧化甲基汞琼脂糖凝胶上通过电泳可清晰分辨出各个mRNA。通过每个克隆内独特限制酶位点的定位进一步确定了每个乳蛋白克隆的身份。通过杂交捕获无细胞翻译对每个克隆进行了最终鉴定。与各自的mRNA相比,乳蛋白cDNA克隆的大小从α-乳白蛋白基因的70%到γ-酪蛋白基因的基本全长不等。这代表了一类肽激素反应基因的首次分离。

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