斑马鱼的腺苷脱氨酶作用于RNA的蛋白2(Adar2)对α-氨基-3-羟基-5-甲基-4-异恶唑丙酸(AMPA)受体亚基谷氨酸受体离子型AMPA 2α(gria2α)转录本的Q/R位点进行编辑,以确保神经系统和颅神经嵴细胞的正常发育。
Zebrafish Adar2 Edits the Q/R site of AMPA receptor Subunit gria2α transcript to ensure normal development of nervous system and cranial neural crest cells.
作者信息
Li I-Chen, Chen Yu-Chia, Wang Yi-Yun, Tzeng Bo-Wei, Ou Chun-Wen, Lau Yi-Yan, Wu Kan-Mai, Chan Tzu-Min, Lin Wei-Hsiang, Hwang Sheng-Ping L, Chow Wei-Yuan
机构信息
Institute of Molecular and Cellular Biology, National Tsing Hua University, Hsinchu, Taiwan.
Institute of Systems Neuroscience, National Tsing Hua University, Hsinchu, Taiwan.
出版信息
PLoS One. 2014 May 12;9(5):e97133. doi: 10.1371/journal.pone.0097133. eCollection 2014.
BACKGROUND
Adar2 deaminates selective adenosines to inosines (A-to-I RNA editing) in the double-stranded region of nuclear transcripts. Although the functions of mouse Adar2 and its biologically most important substrate gria2, encoding the GluA2 subunit of AMPA (α-amino-3-hydroxy-5-methyl-4-isoxazole propionic acid) receptor, have been extensively studied, the substrates and functions of zebrafish Adar2 remain elusive.
METHODS/PRINCIPAL FINDINGS: Expression of Adar2 was perturbed in the adar2 morphant (adar2MO), generated by antisense morpholio oligonucleotides. The Q/R editing of gria2α was reduced in the adar2MO and was enhanced by overexpression of Adar2, demonstrating an evolutionarily conserved activity between zebrafish and mammalian Adar2 in editing the Q/R site of gria2. To delineate the role of Q/R editing of gria2α in the developmental defects observed in the adar2MO, the Q/R editing of gria2α was specifically perturbed in the gria2αQRMO, generated by a morpholio oligonucleotide complementary to the exon complementary sequence (ECS) required for the Q/R editing. Analogous to the adar2-deficient and Q/R-editing deficient mice displaying identical neurological defects, the gria2αQRMO and adar2MO displayed identical developmental defects in the nervous system and cranial cartilages. Knockdown p53 abolished apoptosis and partially suppressed the loss of spinal cord motor neurons in these morphants. However, reducing p53 activity neither replenished the brain neuronal populations nor rescued the developmental defects. The expressions of crestin and sox9b in the neural crest cells were reduced in the adar2MO and gria2αQRMO. Overexpressing the edited GluA2αR in the adar2MO restored normal expressions of cresting and sox9b. Moreover, overexpressing the unedited GluA2αQ in the wild type embryos resulted in reduction of crestin and sox9b expressions. These results argue that an elevated GluA2αQ level is sufficient for generating the cranial neural crest defects observed in the adar2MO. Our results present a link between dysfunction of AMPA receptors and defective development of the nervous system and cranial neural crest in the zebrafish.
背景
Adar2可将核转录本双链区域中的选择性腺苷脱氨基转化为肌苷(A-to-I RNA编辑)。尽管小鼠Adar2及其生物学上最重要的底物gria2(编码AMPA(α-氨基-3-羟基-5-甲基-4-异恶唑丙酸)受体的GluA2亚基)的功能已得到广泛研究,但斑马鱼Adar2的底物和功能仍不清楚。
方法/主要发现:通过反义吗啉代寡核苷酸产生的adar2 morphant(adar2MO)中,Adar2的表达受到干扰。adar2MO中gria2α的Q/R编辑减少,而Adar2的过表达则增强了这种编辑,这表明斑马鱼和哺乳动物的Adar2在编辑gria2的Q/R位点方面具有进化上保守的活性。为了阐明gria2α的Q/R编辑在adar2MO中观察到的发育缺陷中的作用,通过与Q/R编辑所需的外显子互补序列(ECS)互补的吗啉代寡核苷酸在gria2αQRMO中特异性干扰gria2α的Q/R编辑。类似于缺乏Adar2和缺乏Q/R编辑的小鼠表现出相同的神经缺陷,gria2αQRMO和adar2MO在神经系统和颅软骨中表现出相同的发育缺陷。敲低p53可消除凋亡并部分抑制这些morphant中脊髓运动神经元的丧失。然而,降低p53活性既不能补充脑神经元群体,也不能挽救发育缺陷。在adar2MO和gria2αQRMO中,神经嵴细胞中crestin和sox9b的表达降低。在adar2MO中过表达编辑后的GluA2αR可恢复cresting和sox9b的正常表达。此外,在野生型胚胎中过表达未编辑的GluA2αQ会导致crestin和sox9b表达降低。这些结果表明,升高的GluA2αQ水平足以产生在adar2MO中观察到的颅神经嵴缺陷。我们的结果揭示了斑马鱼中AMPA受体功能障碍与神经系统和颅神经嵴发育缺陷之间的联系。
Zotero 插件