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當(dāng)前位置 > 首頁(yè) > 技術(shù)文章 > 單個(gè)神經(jīng)元O2消耗量、細(xì)胞內(nèi)Ca2+濃度和線粒體膜電位的同時(shí)記錄

單個(gè)神經(jīng)元O2消耗量、細(xì)胞內(nèi)Ca2+濃度和線粒體膜電位的同時(shí)記錄

瀏覽次數(shù):3170 發(fā)布日期:2009-6-17  來(lái)源:本站 僅供參考,謝絕轉(zhuǎn)載,否則責(zé)任自負(fù)
    非損傷微測(cè)技術(shù)用于神經(jīng)毒性機(jī)制的研究
    谷氨酸毒性研究:?jiǎn)蝹(gè)神經(jīng)元O2消耗量、細(xì)胞內(nèi)Ca2+濃度和線粒體膜電位的同時(shí)記錄
    點(diǎn)擊查看大圖

    神經(jīng)元是可興奮性細(xì)胞,在突觸活動(dòng)及產(chǎn)生動(dòng)作電位后,神經(jīng)元要產(chǎn)生大量的ATP驅(qū)動(dòng)離子泵以提高胞內(nèi)的Na+和Ca2+水平。谷氨酸(Glu)是重要的神經(jīng)遞質(zhì),負(fù)責(zé)快速突觸傳遞及突觸傳遞強(qiáng)度的長(zhǎng)期變化,并參與認(rèn)知和記憶等過(guò)程;但如果過(guò)度激活谷氨酸受體,谷氨酸會(huì)導(dǎo)致離子平衡破壞、細(xì)胞死亡等毒性反應(yīng)。

    本文為明確谷氨酸神經(jīng)毒性的機(jī)制,將非損傷微測(cè)技術(shù)與激光共聚焦技術(shù)結(jié)合,以大鼠幼崽大腦皮層的神經(jīng)元為被測(cè)樣品,用非損傷微測(cè)技術(shù)(a self-referencing O2 electrode)檢測(cè)單個(gè)神經(jīng)元O2消耗量(即O2內(nèi)流),而用激光共聚焦技術(shù)檢測(cè)其胞內(nèi)Ca2+濃度和線粒體膜電位。


    點(diǎn)擊查看大圖
    單個(gè)神經(jīng)元細(xì)胞在Glu作用下O2消耗量、胞內(nèi)Ca2+濃度
    和線粒體膜電位的變化過(guò)程

    研究發(fā)現(xiàn),在谷氨酸作用下,細(xì)胞內(nèi)Ca2+濃度上升,隨后O2消耗量增加,這期間線粒體膜電位也發(fā)生相應(yīng)改變。該結(jié)論直接證實(shí)了下述谷氨酸毒性機(jī)理模型:谷氨酸受體被激活后能引起Ca2+內(nèi)流,導(dǎo)致細(xì)胞內(nèi)ATP損耗。

    將非損傷微測(cè)技術(shù)與激光共聚焦等技術(shù)相結(jié)合,檢測(cè)生物樣品內(nèi)部和外部離子分子或其他信息的變化情況,已經(jīng)成為揭示生命過(guò)程機(jī)理機(jī)制的重要手段。

    關(guān)鍵詞:非損傷微測(cè)技術(shù)(a self-referencing O2 electrode), 氧氣消耗量(oxygen consumption), 谷氨酸(glutamate);
    參考文獻(xiàn):Gleichmann M, et al. J Neurochem, 2009,109: 644-655
    全文下載:http://www.xuyue.net/xylt/viewthread.php?tid=535&extra=page%3D1

    Abstract:
    In order to determine the sequence of cellular processes in glutamate toxicity, we simultaneously recorded O2 consumption,cytosolic Ca2+ concentration ([Ca2+]i), and mitochondrial membrane potential (mDw) in single cortical neurons. Oxygen consumption was measured using an amperometric selfreferencing platinum electrode adjacent to neurons in which [Ca2+]i and mDw were monitored with Fluo-4 and TMRE+,respectively, using a spinning disk laser confocal microscope.Excitotoxic doses of glutamate caused an elevation of [Ca2+]i followed seconds afterwards by an increase in O2 consumption which reached a maximum level within 1–5 min. A modest increase in mDw occurred during this time period, and then, shortly before maximalO2 consumption was reached, themDw, as indicated by TMRE+ fluorescence, dissipated. Maximal O2 consumption lasted up to 5 min and then declined together with mDw and ATP levels, while [Ca2+]i further increased. mDw and [Ca2+]i returned to baseline levels when neurons were treated
    with an NMDA receptor antagonist shortly after the [Ca2+]i increased. Our unprecedented spatial and time resolution revealed that this sequence of events is identical in all neurons, albeit with considerable variability in magnitude and kinetics of changes in O2 consumption, [Ca2+]i, and mDw. The data obtained using this new method are consistent with a model where Ca2+ influx causes ATP depletion, despite maximal mitochondrial respiration, minutes after glutamate receptor activation.
    Keywords: excitotoxicity, glutamate, oxygen consumption.

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