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eNpHR: a Natronomonas halorhodopsin enhanced for optogenetic applications.

机译:eNpHR:Natronomona的一种卤代视紫红质,可用于光遗传学领域。

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Temporally precise inhibition of distinct cell types in the intact nervous system has been enabled by the microbial halorhodopsin NpHR, a fast light-activated electrogenic Cl(-) pump. While neurons can be optically hyperpolarized and inhibited from firing action potentials at moderate NpHR expression levels, we have encountered challenges with pushing expression to extremely high levels, including apparent intracellular accumulations. We therefore sought to molecularly engineer NpHR to achieve strong expression without these cellular side effects. We found that high expression correlated with endoplasmic reticulum (ER) accumulation, and that under these conditions NpHR colocalized with ER proteins containing the KDEL ER retention sequence. We screened a number of different putative modulators of membrane trafficking and identified a combination of two motifs, an N-terminal signal peptide and a C-terminal ER export sequence, that markedly promoted membrane localization and ER export defined by confocal microscopy and whole-cell patch clamp. The modified NpHR displayed increased peak photocurrent in the absence of aggregations or toxicity, and potent optical inhibition was observed not only in vitro but also in vivo with thalamic single-unit recording. The new enhanced NpHR (eNpHR) allows safe, high-level expression in mammalian neurons, without toxicity and with augmented inhibitory function, in vitro and in vivo.
机译:暂时性的抑制在完整的神经系统中的不同细胞类型已通过微生物的卤代视紫红质NpHR(一种快速光激活的电Cl(-)泵)实现。尽管神经元可以被光学超极化并在中等NpHR表达水平下抑制激发动作电位,但我们在将表达推至极高水平(包括明显的细胞内积累)时遇到了挑战。因此,我们寻求对NpHR进行分子工程改造以实现强表达而又不产生这些细胞副作用。我们发现高表达与内质网(ER)积累相关,并且在这些条件下NpHR与含有KDEL ER保留序列的ER蛋白共定位。我们筛选了许多不同的假定的膜运输调节剂,并鉴定了两个基序的组合:N端信号肽和C端ER出口序列,可显着促进共聚焦显微镜和全细胞所定义的膜定位和ER出口膜片夹。修饰的NpHR在没有聚集或毒性的情况下显示出增加的峰值光电流,并且不仅在体外而且在丘脑单单位记录中在体内均观察到了强光抑制作用。新的增强型NpHR(eNpHR)可以在哺乳动物体内神经元中进行安全,高水平的表达,在体内外均无毒性且具有增强的抑制功能。

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