Knockout or Knock-in? A Truncated D2 Receptor Protein Is Expressed in the Brain of Functional D2 Receptor Knockout Mice

IF 1.6 Q3 CLINICAL NEUROLOGY
NeuroSci Pub Date : 2021-06-01 DOI:10.3390/NEUROSCI2020014
Natalia Sánchez, Montserrat Olivares-Costa, Marcela P. González, R. Munita, Angelica P. Escobar, Rodrigo C. Meza, Mauricio Herrera-Rojas, Jessica Albornoz, Gianluca Merello, M. Andrés
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引用次数: 1

Abstract

Null mice for the dopamine D2 receptor (D2R) have been instrumental in understanding the function of this protein. For our research, we obtained the functional D2R knockout mouse strain described initially in 1997. Surprisingly, our biochemical characterization showed that this mouse strain is not a true knockout. We determined by sequence analysis of the rapid 3′ amplification of cDNA ends that functional D2R knockout mice express transcripts that lack only the eighth exon. Furthermore, immunofluorescence assays showed a D2R-like protein in the brain of functional D2R knockout mice. We verified by immunofluorescence that the recombinant truncated D2R is expressed in HEK293T cells, showing intracellular localization, colocalizing in the Golgi apparatus and the endoplasmic reticulum, but with less presence in the Golgi apparatus compared to the native D2R. As previously reported, functional D2R knockout mice are hypoactive and insensitive to the D2R agonist quinpirole. Concordantly, microdialysis studies confirmed that functional D2R knockout mice have lower extracellular dopamine levels in the striatum than the native mice. In conclusion, functional D2R knockout mice express transcripts that lead to a truncated D2R protein lacking from the sixth transmembrane domain to the C-terminus. We share these findings to avoid future confusion and the community considers this mouse strain in D2R traffic and protein–protein interaction studies.
淘汰赛还是淘汰赛?D2受体敲除小鼠脑内表达一种截断的D2受体蛋白
多巴胺D2受体(D2R)缺失的小鼠有助于理解该蛋白的功能。在我们的研究中,我们获得了1997年最初描述的功能性D2R敲除小鼠品系。令人惊讶的是,我们的生化表征表明,这种小鼠品系并不是真正的基因敲除。我们通过对cDNA末端快速3 '扩增的序列分析确定,功能性D2R敲除小鼠表达的转录本仅缺少第8个外显子。此外,免疫荧光分析显示,功能性D2R基因敲除小鼠的大脑中存在D2R样蛋白。我们通过免疫荧光证实,重组截断的D2R在HEK293T细胞中表达,表现出细胞内定位,在高尔基体和内质网中共定位,但与天然D2R相比,在高尔基体中的存在较少。正如先前报道的那样,功能性D2R基因敲除小鼠对D2R激动剂喹匹罗缺乏活性和不敏感。与此同时,微透析研究证实,功能性D2R基因敲除小鼠的纹状体细胞外多巴胺水平低于正常小鼠。综上所述,功能性D2R基因敲除小鼠表达的转录本导致D2R蛋白从第6跨膜结构域到c端缺失。我们分享这些发现以避免未来的混淆,并且社区在D2R流量和蛋白质-蛋白质相互作用研究中考虑了该小鼠品系。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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