首页> 外文期刊>The Journal of Comparative Neurology >Calretinin expression in the chick brainstem auditory nuclei develops and is maintained independently of cochlear nerve input.
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Calretinin expression in the chick brainstem auditory nuclei develops and is maintained independently of cochlear nerve input.

机译:鸡脑干听觉核中的钙调蛋白表达独立于耳蜗神经输入而发展并维持。

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摘要

The expression of the calcium-binding protein calretinin (CR) in the chick brainstem auditory nuclei angularis (NA), laminaris (NL), and magnocelularis (NM) was studied during normal development and after deafening by surgical removal of the otocyst (embryonic precursor of the inner ear) or columella (middle ear ossicle). CR mRNA was localized by in situ hybridization by using a radiolabeled oligonucleotide chick CR probe. CR immunoreactivity (CR-IR) was localized on adjacent tissue sections. CR mRNA signal in the auditory nuclei was expressed at comparable levels at embryonic day (E)9 and E11 and increased thereafter to reach the highest levels in posthatch chicks. CR-IR neurons were apparent in NM and NA at E11 and in NL by E13, and CR-IR increased in all three auditory nuclei thereafter. Neither unilateral nor bilateral otocyst removal caused detectable changes in the intensity of CR mRNA expression or CR-IR in the auditory nuclei at any of the several ages examined. Similarly, columella removal at posthatching day 2 or 3 failed to significantly affect CR mRNA or CR-IR levels at 3 hours, 1 day, or 3-4 days survival times. We conclude that cochlear nerve input is not necessary for expression of either calretinin mRNA or protein and that the profound decrease in sound-evoked activity caused by columella removal does not affect the maintenance of CR expression after hatching.
机译:研究了正常发育过程中以及耳聋手术切除耳囊(胚前体)后钙的结合蛋白降钙素(CR)在鸡脑干听觉角核(NA),椎板(NL)和木突肌(NM)中的表达。内耳)或小肠(中耳小骨)。通过使用放射性标记的寡核苷酸小鸡CR探针通过原位杂交来定位CR mRNA。 CR免疫反应性(CR-IR)位于相邻组织切片上。听觉核中的CR mRNA信号在胚胎第(E)9天和E11天以可比较的水平表达,此后增加,达到孵化后雏鸡的最高水平。到E11时,NM和NA中的CR-IR神经元很明显;到E13时,NL-NL中的CR-IR神经元很明显,此后所有三个听核中的CR-IR都增加了。在所检查的多个年龄中的任何一个年龄段,单侧或双侧耳囊切除均未引起听核中CR mRNA表达或CR-IR强度的可检测变化。类似地,在孵化后第2天或第3天去除小柱不能在3小时,1天或3-4天生存时间显着影响CR mRNA或CR-IR水平。我们得出的结论是,耳蜗神经输入对于钙网蛋白mRNA或蛋白质的表达不是必需的,并且由于去除小柱引起的声音诱发活动的显着降低并不影响孵化后CR表达的维持。

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