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细菌视紫红质中特定氨基酸的取代:用含有改变了的密码子的合成 DNA 片段替换结构基因中的限制酶片段。

Specific amino acid substitutions in bacterioopsin: Replacement of a restriction fragment in the structural gene by synthetic DNA fragments containing altered codons.

机构信息

Department of Biology, Massachusetts Institute of Technology, Cambridge, MA 02139.

出版信息

Proc Natl Acad Sci U S A. 1984 Apr;81(8):2285-9. doi: 10.1073/pnas.81.8.2285.

Abstract

To study the mechanism of light-dependent proton translocation by bacteriorhodopsin, we have introduced single-codon changes in the gene so as to produce the following specific amino acid substitutions in the protein: Tyr-185 to Phe, Pro-186 to Leu, Trp-189 to Phe, Ser-193 to Ala, and Glu-194 to Gln. The strategy involved replacement of a 62-base-pair restriction fragment by synthetic DNA duplexes containing the modified nucleotide sequences. This required a unique restriction site (Xho I) at Ile-203 which was created by oligonucleotide-directed point mutagenesis. The six DNA duplexes corresponding to the modified native and mutant restriction fragments were all prepared by DNA ligase-catalyzed joining of chemically synthesized deoxyribooligonucleotides. The bacterioopsin expression plasmids reconstructed by using the synthetic DNA fragments were characterized by restriction analysis and DNA sequence determination. An extremely rapid, efficient, and general method for purification of the synthetic oligonucleotides and of DNA fragments was developed.

摘要

为了研究细菌视紫红质光依赖质子转移的机制,我们在基因中引入了单密码子变化,从而在蛋白质中产生以下特定的氨基酸取代: Tyr-185 到 Phe,Pro-186 到 Leu,Trp-189 到 Phe,Ser-193 到 Ala,和 Glu-194 到 Gln。该策略涉及用包含修饰核苷酸序列的合成 DNA 双链体替换 62 个碱基对的限制片段。这需要在 Ile-203 处有一个独特的限制位点(Xho I),该位点是通过寡核苷酸定向点突变产生的。与修饰的天然和突变限制片段相对应的六个 DNA 双链体都是通过 DNA 连接酶催化化学合成的脱氧核糖核酸寡核苷酸的连接制备的。使用合成 DNA 片段构建的细菌视紫红质表达质粒通过限制分析和 DNA 序列测定进行了表征。开发了一种极其快速、高效和通用的方法来纯化合成的寡核苷酸和 DNA 片段。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c587/345043/0cd4c6ee39cf/pnas00609-0020-a.jpg

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