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Identification of the neuromuscular junction transcriptome of extraocular muscle by laser capture microdissection.

机译:激光捕获显微切割鉴定眼外肌神经肌肉连接转录组。

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PURPOSE: To examine and characterize the profile of genes expressed at the synapses or neuromuscular junctions (NMJs) of extraocular muscles (EOMs) compared with those expressed at the tibialis anterior (TA). METHODS: Adult rat eyeballs with rectus EOMs attached and TAs were dissected, snap frozen, serially sectioned, and stained for acetylcholinesterase (AChE) to identify the NMJs. Approximately 6000 NMJs for rectus EOM (EOMsyn), 6000 NMJs for TA (TAsyn), equal amounts of NMJ-free fiber regions (EOMfib, TAfib), and underlying myonuclei and RNAs were captured by laser capture microdissection (LCM). RNA was processed for microarray-based expression profiling. Expression profiles and interaction lists were generated for genes differentially expressed at synaptic and nonsynaptic regions of EOM (EOMsyn versus EOMfib) and TA (TAsyn versus TAfib). Profiles were validated by using real-time quantitative polymerase chain reaction (qPCR). RESULTS: The regional transcriptomes associated with NMJs of EOMs and TAs were identified. Two hundred seventy-five genes were preferentially expressed in EOMsyn (compared with EOMfib), 230 in TAsyn (compared with TAfib), and 288 additional transcripts expressed in both synapses. Identified genes included novel genes as well as well-known, evolutionarily conserved synaptic markers (e.g., nicotinic acetylcholine receptor (AChR) alpha (Chrna) and epsilon (Chrne) subunits and nestin (Nes). CONCLUSIONS: Transcriptome level differences exist between EOM synaptic regions and TA synaptic regions. The definition of the synaptic transcriptome provides insight into the mechanism of formation and functioning of the unique synapses of EOM and their differential involvement in diseases noted in the EOM allotype.
机译:目的:检查并鉴定与眼前肌(TA)表达的基因相比,眼外肌(EOMs)的突触或神经肌肉接头(NMJ)表达的基因的特征。方法:解剖附有直肌EOM和TA的成年大鼠眼球,速冻,连续切片,并用乙酰胆碱酯酶(AChE)染色以鉴定NMJ。通过激光捕获显微切割术(LCM)捕获了约6000 NMJ的直肌EOM(EOMsyn),6000 NMJ的TA(TAsyn),等量的无NMJ的纤维区域(EOMfib,TAfib)以及潜在的肌核和RNA。 RNA进行了基于微阵列的表达谱分析。产生了在EOM(EOMsyn与EOMfib)和TA(TAsyn与TAfib)的突触和非突触区域差异表达的基因的表达谱和相互作用列表。通过使用实时定量聚合酶链反应(qPCR)验证配置文件。结果:确定了与EOM和TA的NMJ相关的区域转录组。在EOMsyn(与EOMfib相比)中优先表达了275个基因,在TAsyn(与TAfib相比)中优先表达了230个基因,在两个突触中均表达了288个其他转录物。鉴定出的基因包括新基因以及众所周知的,进化上保守的突触标记(例如,烟碱型乙酰胆碱受体(AChR)α(Chrna),ε(Chrne)亚基和巢蛋白(Nes)。结论:EOM突触之间存在转录组水平差异。突触转录组的定义为了解EOM独特突触的形成和功能机制以及它们在EOM同种异型中所涉及的疾病的不同参与提供了见识。

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