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通过表达小鼠Na⁺, K⁺-ATP酶α亚基的cDNA所赋予的哇巴因抗性。

Ouabain resistance conferred by expression of the cDNA for a murine Na+, K+-ATPase alpha subunit.

作者信息

Kent R B, Emanuel J R, Ben Neriah Y, Levenson R, Housman D E

出版信息

Science. 1987 Aug 21;237(4817):901-3. doi: 10.1126/science.3039660.

Abstract

The molecular basis for the marked difference between primate and rodent cells in sensitivity to the cardiac glycoside ouabain has been established by genetic techniques. A complementary DNA encoding the entire alpha 1 subunit of the mouse Na+- and K+-dependent adenosine triphosphatase (ATPase) was inserted into the expression vector pSV2. This engineered DNA molecule confers resistance against 10(-4) M ouabain to monkey CV-1 cells. Deletion of sequences encoding the carboxyl terminus of the alpha 1 subunit abolish the activity of the complementary DNA. The ability to assay the biological activity of this ATPase in a transfection protocol permits the application of molecular genetic techniques to the analysis of structure-function relationships for the enzyme that establishes the internal Na+/K+ environment of most animal cells. The full-length alpha 1 subunit complementary DNA will also be useful as a dominant selectable marker for somatic cell genetic studies utilizing ouabain-sensitive cells.

摘要

通过遗传技术已确定了灵长类和啮齿类动物细胞对强心苷哇巴因敏感性存在显著差异的分子基础。将编码小鼠钠钾依赖型三磷酸腺苷酶(ATP酶)整个α1亚基的互补DNA插入表达载体pSV2。这种构建的DNA分子赋予猴CV - 1细胞对10⁻⁴ M哇巴因的抗性。缺失编码α1亚基羧基末端的序列会消除互补DNA的活性。在转染实验中测定这种ATP酶生物活性的能力,使得分子遗传学技术能够应用于分析该酶的结构 - 功能关系,而该酶建立了大多数动物细胞的内部钠/钾环境。全长α1亚基互补DNA也将作为利用对哇巴因敏感细胞进行体细胞遗传学研究的显性选择标记发挥作用。

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