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一种组蛋白修饰鉴定出一个控制肌肉中slo BK通道基因表达的DNA元件。

A histone modification identifies a DNA element controlling slo BK channel gene expression in muscle.

作者信息

Li Xiaolei, Ghezzi Alfredo, Krishnan Harish R, Pohl Jascha B, Bohm Arun Y, Atkinson Nigel S

机构信息

a School of Biological Sciences, Nanyang Technological University , Singapore.

b Department of Neuroscience and The Waggoner Center for Alcohol and Addiction Research , The University of Texas at Austin , Austin, Texas , USA.

出版信息

J Neurogenet. 2015;29(2-3):124-34. doi: 10.3109/01677063.2015.1050097. Epub 2015 Jul 13.

Abstract

The slo gene encodes the BK-type Ca(2+)-activated K(+) channels. In Drosophila, expression of slo is induced by organic solvent sedation (benzyl alcohol and ethanol), and this increase in neural slo expression contributes to the production of functional behavioral tolerance (inducible resistance) to these drugs. Within the slo promoter region, we observed that benzyl alcohol sedation produces a localized spike of histone acetylation over a 65-nucleotide (65-n) conserved DNA element called 55b. Changes in histone acetylation are commonly the consequence of transcription factor activity, and previously, a localized histone acetylation spike was used to successfully map a DNA element involved in benzyl alcohol-induced slo expression. To determine whether the 55b element was also involved in benzyl alcohol-induced neural expression of slo, we deleted it from the endogenous slo gene by homologous recombination. Flies lacking the 55b element were normal with respect to basal and benzyl alcohol-induced neural slo expression, the capacity to acquire and maintain functional tolerance, their threshold for electrically-induced seizures, and most slo-related behaviors. Removal of the 55b element did however increase the level of basal expression from the muscle/tracheal cell-specific slo core promoter and produced a slight increase in overall locomotor activity. We conclude that the 55b element is involved in control of slo expression from the muscle and tracheal-cell promoter but is not involved in the production of functional benzyl alcohol tolerance.

摘要

slo基因编码BK型钙激活钾通道。在果蝇中,有机溶剂镇静(苄醇和乙醇)可诱导slo的表达,而神经slo表达的这种增加有助于产生对这些药物的功能性行为耐受性(诱导抗性)。在slo启动子区域内,我们观察到苄醇镇静在一个名为55b的65个核苷酸(65 - n)保守DNA元件上产生了局部组蛋白乙酰化峰值。组蛋白乙酰化的变化通常是转录因子活性的结果,此前,局部组蛋白乙酰化峰值被用于成功定位参与苄醇诱导的slo表达的DNA元件。为了确定55b元件是否也参与苄醇诱导的slo神经表达,我们通过同源重组从内源性slo基因中删除了它。缺乏55b元件的果蝇在基础和苄醇诱导的神经slo表达、获得和维持功能耐受性的能力、电诱导癫痫发作的阈值以及大多数与slo相关的行为方面均正常。然而,去除55b元件确实增加了肌肉/气管细胞特异性slo核心启动子的基础表达水平,并使总体运动活性略有增加。我们得出结论,55b元件参与了肌肉和气管细胞启动子对slo表达的控制,但不参与功能性苄醇耐受性的产生。

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