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钾离子通道转基因可能通过翻译后机制降低草履虫中的钾离子电流。

K(+)-channel transgenes reduce K(+) currents in Paramecium, probably by a post-translational mechanism.

作者信息

Ling K Y, Haynes W J, Oesterle L, Kung C, Preston R R, Saimi Y

机构信息

Laboratory of Molecular Biology and Department of Genetics, University of Wisconsin, Madison, Wisconsin 53706, USA.

出版信息

Genetics. 2001 Nov;159(3):987-95. doi: 10.1093/genetics/159.3.987.

Abstract

PAK11 is 1 of more than 15 members in a gene family that encodes K(+)-channel pore-forming subunits in Paramecium tetraurelia. Microinjection of PAK11 DNA into macronuclei of wild-type cells results in clonal transformants that exhibit hyperexcitable swimming behaviors reminiscent of certain loss-of-K(+)-current mutants. PAK2, a distant homolog of PAK11, does not have the same effect. But PAK1, a close homolog of PAK11, induces the same hyperexcitability. Cutting the PAK11 open reading frame (ORF) with restriction enzymes before injection removes this effect entirely. Microinjection of PAK11 ORF flanked by the calmodulin 5' and 3' UTRs also induces the same hyperexcitable phenotype. Direct examination of transformed cells under voltage clamp reveals that two different Ca(2+)-activated K(+)-specific currents are reduced in amplitude. This reduction does not correlate with a deficit of PAK11 message, since RNA is clearly produced from the injected transgenes. Insertion of a single nucleotide at the start of the PAK11 ORF does not affect the RNA level but completely abolishes the phenotypic transformation. Thus, the reduction of K(+) currents by the expression of the K(+)-channel transgenes reported here is likely to be the consequence of a post-translational event. The complexity of behavioral changes, possible mechanisms, and implications in Paramecium biology are discussed.

摘要

PAK11是一个基因家族中15个以上成员之一,该基因家族在四膜虫中编码钾离子通道孔形成亚基。将PAK11 DNA显微注射到野生型细胞的大核中会产生克隆转化体,这些转化体表现出过度兴奋的游泳行为,让人联想到某些钾离子电流缺失突变体。PAK2是PAK11的远亲同源物,没有相同的作用。但PAK1是PAK11的近亲同源物,会诱导相同的过度兴奋。在注射前用限制酶切割PAK11开放阅读框(ORF)可完全消除这种效应。注射两侧带有钙调蛋白5'和3'非翻译区的PAK11 ORF也会诱导相同的过度兴奋表型。在电压钳下直接检查转化细胞发现,两种不同的钙激活钾特异性电流幅度降低。这种降低与PAK11信息的缺乏无关,因为RNA显然是由注射的转基因产生的。在PAK11 ORF起始处插入单个核苷酸不会影响RNA水平,但会完全消除表型转化。因此,此处报道的钾离子通道转基因表达导致的钾离子电流降低可能是翻译后事件的结果。文中讨论了四膜虫行为变化的复杂性、可能的机制及其在生物学中的意义。

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