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Melody an ENU mutation in Caspase 3 alters the catalytic cysteine residue and causes sensorineural hearing loss in mice

机译:旋律Caspase 3中的ENU突变改变了催化的半胱氨酸残基并导致小鼠的感音神经性听力减退

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摘要

Progeny from the Harwell N-ethyl-N-nitrosourea (ENU) recessive mutagenesis screen were assessed for auditory defects. A pedigree was identified with multiple progeny lacking response to a clickbox test. Auditory brainstem response (ABR) analysis showed that homozygous mutant mice were profoundly deaf and the line was named melody. We subsequently mapped this mutation to a 6-Mb region on chromosome 8 and identified a point mutation in melody that results in a C163S substitution in the catalytic site of Caspase 3, a cysteine protease involved in apoptosis. Melody fails to complement a null Caspase-3 mutant. Scanning electron microscopy (SEM) has revealed disorganised sensory hair cells and hair cell loss. Histological analysis of melody has shown degeneration of spiral ganglion cells in homozygote mice, with a gradient of severity from apical to basal turns. Melody heterozygotes also show evidence of loss of spiral ganglion neurons, suggesting that the C163S mutation may show dominant negative effects by binding and sequestering proteins at the active site. The melody line provides a new model for studying the role of Caspase 3 in deafness and a number of other pathways and systems.
机译:对来自Harwell N-乙基-N-亚硝基脲(ENU)隐性诱变筛选的后代进行听觉缺陷评估。谱系被确定为多个子代对点击框测试没有反应。听性脑干反应(ABR)分析表明,纯合突变小鼠严重失聪,该品系被称为旋律。随后,我们将该突变定位到8号染色体上的6-Mb区,并确定了旋律中的点突变,该突变导致Caspase 3(参与凋亡的半胱氨酸蛋白酶)的催化位点发生C163S取代。旋律无法补充无效的Caspase-3突变体。扫描电子显微镜(SEM)显示感觉毛细胞紊乱和毛细胞丢失。旋律的组织学分析显示纯合子小鼠中螺旋神经节细胞变性,其严重程度从顶转到基转。旋律杂合子还显示出螺旋神经节神经元丢失的证据,表明C163S突变可能通过在活性位点结合和隔离蛋白质而表现出显性的负作用。旋律谱系为研究Caspase 3在耳聋以及许多其他途径和系统中的作用提供了新模型。

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