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        枸櫞酸鐵銨和鐵蛋白對原代培養(yǎng)腹側(cè)中腦神經(jīng)元VMAT-2和DAT表達影響
        
                
        2021-04-12 00:00:00肖志新宋立梅謝俊霞徐華敏
        
                
        青島大學學報(醫(yī)學版) 2021年2期 
        
                    
        [摘要]目的 探究枸櫞酸鐵銨(FAC)、含鐵鐵蛋白(Ferritin)和去鐵鐵蛋白(Apoferritin)對原代培養(yǎng)的腹側(cè)中腦神經(jīng)元中單胺囊泡轉(zhuǎn)運蛋白-2(VMAT-2)和多巴胺轉(zhuǎn)運蛋白(DAT)表達的影響。方法 以FAC、Ferritin和Apoferritin處理原代培養(yǎng)的腹側(cè)中腦神經(jīng)元24 h后,應(yīng)用蛋白質(zhì)免疫印跡(Western Blot)方法檢測神經(jīng)元中VMAT-2和DAT的表達情況。結(jié)果 FAC、Ferritin和Apoferritin處理的原代腹側(cè)中腦神經(jīng)元VMAT-2表達較對照組明顯降低,差異具有統(tǒng)計學意義(F=4.295,P<0.05),而DAT的表達沒有明顯變化。結(jié)論 FAC、Ferritin和Apoferritin能夠降低原代培養(yǎng)的腹側(cè)中腦神經(jīng)元的VMAT-2表達,而對DAT表達沒有明顯影響。
        [關(guān)鍵詞]鐵;鐵蛋白質(zhì)類;中腦;神經(jīng)元;囊泡單胺轉(zhuǎn)運蛋白質(zhì)類;多巴胺質(zhì)膜轉(zhuǎn)運蛋白質(zhì)類
        [中圖分類號]R338.2
        [文獻標志碼]A
        [文章編號]2096-5532(2021)02-0194-04
        [ABSTRACT]Objective To investigate the effect of ferric ammonium citrate (FAC), Ferritin, and Apoferritin on the expression of vesicular monoamine transporter 2 (VMAT-2) and dopamine transporter (DAT) in primary cultured ventral midbrain neurons.Methods After primary cultured ventral midbrain neurons were treated with FAC, Ferritin, or Apoferritin for 24 h, Western blot was used to measure the expression of VMAT-2 and DAT in neurons."Results Compared with the control group, the group of primary cultured ventral midbrain neurons treated by FAC, Ferritin, or Apoferritin had a significant reduction in the expression of VMAT-2 (F=4.295,Plt;0.05), while there was no significant change in the expression of DAT."Conclusion FAC, Ferritin, and Apoferritin can reduce the expression of VMAT-2 in primary cultured ventral midbrain neurons, with no significant effect on the expression of DAT.
        [KEY WORDS]iron; ferritins; mesencephalon; neurons; vesicular monoamine transport proteins; dopamine plasma membrane transport proteins
        帕金森病(PD)是第二大常見的神經(jīng)系統(tǒng)退行性疾病,主要臨床表現(xiàn)有運動遲緩、靜止性震顫、姿勢反射障礙等[1-3]。其病理性特征是黑質(zhì)(SN)多巴胺(DA)能神經(jīng)元進行性缺失[4]。迄今為止PD的病因尚未完全闡明,越來越多的證據(jù)表明,SN鐵的過度沉積可能是PD發(fā)病的關(guān)鍵因素之一[5-13]。SN鐵增加會產(chǎn)生活性氧和活性氮物質(zhì),刺激細胞內(nèi)α-突觸核蛋白形成,導致DA能神經(jīng)元變性[14-15]。在腦內(nèi)鐵主要與鐵蛋白結(jié)合,鐵蛋白是一種可儲存多達4 500個鐵原子的蛋白質(zhì)[16-17],有含鐵鐵蛋白(Ferritin)和去鐵鐵蛋白(Apoferritin)兩種形式[18]。有研究表明,鐵蛋白可能不僅是細胞內(nèi)的鐵儲存者,也可能是參與組織和全身鐵調(diào)控的重要因素[19]。但鐵蛋白在DA穩(wěn)態(tài)中起的作用尚不明確。
        單胺囊泡轉(zhuǎn)運蛋白-2(VMAT-2)是位于DA能神經(jīng)元突觸囊泡的一種膜蛋白,可以將胞漿內(nèi)游離的DA轉(zhuǎn)運到囊泡內(nèi),并調(diào)節(jié)隨后的釋放。它通過向單胺能神經(jīng)元傳遞DA小泡來保護DA能神經(jīng)元[20]。多巴胺轉(zhuǎn)運蛋白(DAT)在SN神經(jīng)元胞體和樹突中大量表達[21-23],可將DA從細胞外迅速轉(zhuǎn)運到突觸前神經(jīng)元胞質(zhì)內(nèi),以維持細胞內(nèi)外DA穩(wěn)態(tài)。但是在高鐵以及存在外源性鐵蛋白的狀態(tài)下,原代培養(yǎng)腹側(cè)中腦神經(jīng)元中VMAT-2和DAT的表達是否改變尚不清楚。本實驗旨在探究高鐵、Ferritin和Apoferritin對原代培養(yǎng)的腹側(cè)中腦神經(jīng)元VMAT-2和DAT表達的影響?,F(xiàn)將實驗結(jié)果報告如下。
        1 材料與方法
        1.1 實驗材料
        原代培養(yǎng)的腹側(cè)中腦神經(jīng)元細胞(取自孕14 d的Wistar大鼠的胎鼠腹側(cè)中腦),DMEM/F12培養(yǎng)液、2.5 g/L的胰酶(美國Hyclone公司),B27營養(yǎng)因子、胎牛血清(美國Gibco公司),青霉素-鏈霉素溶液(100×,中國索萊寶科技有限公司),D-多聚賴氨酸、枸櫞酸鐵銨(FAC)、Ferritin、Apoferritin(美國Sigma公司),VMAT-2抗體和DAT抗體(中國上海Abcam公司),ECL發(fā)光液(Millipore公司)。
        1.2 原代腹側(cè)中腦神經(jīng)元的培養(yǎng)
        實驗前將實驗器械進行高壓處理,提前3 h用D-多聚賴氨酸鋪培養(yǎng)板,以高壓滅菌水清洗3次放置超凈臺內(nèi)備用。將孕14 d的Wistar大鼠以聯(lián)合麻醉藥深度麻醉后,用體積分數(shù)0.75的乙醇進行腹部消毒,沿中線剪開,取出串珠樣胚胎,放置在預(yù)冷的DMEM/F12培養(yǎng)液中。將胚胎移至超凈臺中顯微鏡下,在冰上操作,剖開胚胎外膜取出胎鼠置于另一裝有DMEM/F12培養(yǎng)液的玻璃皿中。使用眼科鑷、眼科剪將中腦部分取出,去除端腦及血管膜,修剪組織留出蝴蝶狀的腹側(cè)中腦,將其轉(zhuǎn)移至含預(yù)冷DMEM/F12培養(yǎng)液的玻璃皿中。去除DMEM/F12培養(yǎng)液,加入37 ℃預(yù)溫的2.5 g/L胰酶,在培養(yǎng)箱中消化5 min。加入含有胎牛血清的終止液終止消化。用移液器將組織吹打成單細胞懸液,用藍槍頭吹打約10次,收集單細胞懸液至50 mL離心管中,后套用黃槍頭和白槍頭重復(fù)上述操作。將裝有單細胞懸液的離心管以1 000 r/min離心5 min。棄上清,加入含有B27和雙抗的DMEM/F12培養(yǎng)液,用吸管吹打成細胞懸液,以2×108/L的密度種板。此后每隔2 d換1次液,第6天細胞成熟可用于實驗。
        1.3 實驗分組及處理
        實驗分為對照組、FAC處理組、Ferritin處理組和Apoferritin處理組,將原代培養(yǎng)的腹側(cè)中腦神經(jīng)元培養(yǎng)液換成DMEM/F12基礎(chǔ)培養(yǎng)液,對照組細胞只用DMEM/F12基礎(chǔ)培養(yǎng)液孵育,F(xiàn)AC處理組細胞加入100 μmol/L的FAC,F(xiàn)erritin處理組細胞加入80 μmol/L的Ferritin,Apoferritin處理組細胞加入50 μmol/L的Apoferritin。將各組細胞置于37 ℃、含體積分數(shù)0.05 CO2的培養(yǎng)箱中孵育24 h。
        1.4 VMAT-2和DAT的蛋白免疫印跡(Western Blot)檢測
        在6孔板中加入100 μL蛋白裂解液,冰上裂解30 min,用刮板將板底的細胞刮下,用移液器轉(zhuǎn)移至1.5 mL的EP管中,在4 ℃下以12 000 r/min離心20 min。用移液器吸取80 μL上清至另一EP管中,使用BCA試劑盒檢測上清中蛋白質(zhì)濃度,加入5×Loading Buffer,95 ℃煮5 min。按照BCA試劑盒檢測的蛋白濃度計算SDS-PAGE凝膠電泳的上樣量。加入樣品后,調(diào)節(jié)電壓至80 V,待樣品進入分離膠后,將電壓調(diào)至120 V,電泳之后將蛋白轉(zhuǎn)至PVDF膜上,以300 mA濕轉(zhuǎn)90 min,切下所需分子量的條帶,用含50 g/L脫脂奶粉的TBST室溫封閉2 h后,再加入用含50 g/L脫脂奶粉的TBST稀釋的VMAT-2抗體(稀釋度為1∶1 000)、DAT抗體(稀釋度為1∶1 000)和β-actin抗體(稀釋度為1∶10 000)孵育相應(yīng)的條帶,4 ℃搖床過夜。用TBST洗條帶3次,每次10 min,加入HRP偶聯(lián)的山羊抗兔二抗(稀釋度為1∶10 000),室溫孵育1 h,孵育完成后以TBST洗3次,每次10 min。加ECL發(fā)光液避光孵育1 min顯影。利用Image J軟件對條帶進行分析,以目的條帶與內(nèi)參照條帶的比值作為目的蛋白的相對含量。
        1.5 統(tǒng)計學處理
        應(yīng)用GraphPad Prism 5.0軟件進行統(tǒng)計學處理,計量資料結(jié)果以x2±s的形式表示,多組比較采用單因素方差分析(One way ANOVA檢驗),并繼以Tukey法進行組間兩兩比較,以P<0.05為差異有統(tǒng)計學意義。
        2 結(jié) 果
        2.1 FAC、Ferritin和Apoferritin對原代培養(yǎng)的腹側(cè)中腦神經(jīng)元VMAT-2表達的影響
        對照組、FAC處理組、Ferritin處理組和Apoferritin處理組細胞內(nèi)的VMAT-2蛋白表達水平分別為1.175±0.075、0.938±0.044、0.945±0.046和0.921±0.062(n=17)。與對照組相比,F(xiàn)AC處理組、Ferritin處理組和Apoferritin處理組VMAT-2蛋白表達水平明顯降低,差異具有統(tǒng)計學意義(F=4.295,q=3.952~4.370,P<0.05),而Ferritin處理組與Apoferritin處理組相比差異無顯著意義(q=0.417,P>0.05)。
        2.2 FAC、Ferritin和Apoferritin對原代培養(yǎng)的腹側(cè)中腦神經(jīng)元DAT表達的影響
        對照組、FAC處理組、Ferritin處理組和Apoferritin處理組細胞內(nèi)DAT蛋白表達水平分別為0.910±0.055、0.931±0.679、0.937±0.056、0.958±0.088(n=12),各組間比較,差異均無顯著性(F=0.084,q=0.297~0.706,P>0.05)。
        3 討 論
        PD是全球第二大神經(jīng)退行性疾病,其發(fā)病與年齡老化、氧化應(yīng)激、炎癥反應(yīng)、環(huán)境因素、遺傳因素等有關(guān)。越來越多的證據(jù)表明,SN鐵過度沉積參與了PD的發(fā)病,過多的鐵激活的小膠質(zhì)細胞會釋放大量的神經(jīng)炎性因子,增加了DA能神經(jīng)元的變性[24]。在腦內(nèi),鐵主要與鐵蛋白結(jié)合,鐵蛋白兩種亞型以互補的方式儲存細胞內(nèi)的鐵[25]。
        有研究提出DA作用的區(qū)域概念,VMAT-2和DAT在調(diào)節(jié)這些區(qū)域之間DA轉(zhuǎn)移中起著核心作用[26-27]。VMAT-2將突觸前神經(jīng)元合成的DA攝取到突觸囊泡中,釋放到突觸間隙,從而作用到相應(yīng)的受體。而DAT可以將突觸間隙的DA重新攝取到突觸前神經(jīng)元。它們共同調(diào)節(jié)DA活性,從而改變DA的含量[28]。本文研究結(jié)果顯示,給予高鐵會導致原代培養(yǎng)的腹側(cè)中腦神經(jīng)元的VMAT-2表達降低。有實驗研究表明,當VMAT-2水平降低約95%時,小鼠表現(xiàn)為DA穩(wěn)態(tài)失調(diào),而且神經(jīng)元對多種有毒化合物的敏感性增強[29-34]。這提示高鐵導致的VMAT-2表達降低可能影響了DA的釋放,從而引起DA穩(wěn)態(tài)失調(diào)。本文結(jié)果還顯示,給予鐵蛋白后,細胞VMAT-2的表達也會下降,說明腹側(cè)中腦神經(jīng)元VMAT-2的表達變化不是鐵依賴性的,鐵蛋白和鐵均可通過影響VMAT-2的表達參與DA穩(wěn)態(tài)調(diào)控。Western Blot結(jié)果顯示,經(jīng)高鐵及鐵蛋白處理的腹側(cè)中腦神經(jīng)元DAT的表達沒有發(fā)生明顯變化,提示高鐵及鐵蛋白并不影響DA重新攝取到突觸前神經(jīng)元。以上結(jié)果提示,高鐵及鐵蛋白能夠減少突觸前神經(jīng)元的DA釋放,但并不影響DAT介導的DA重新攝取,這就導致了DA的穩(wěn)態(tài)失調(diào),可能增加了神經(jīng)元對有毒物質(zhì)的敏感性。本實驗以原代細胞為模型,更好地探究了高鐵誘導的DA代謝和轉(zhuǎn)運情況,為開發(fā)影響DA穩(wěn)態(tài)的鐵螯合劑提供了新的依據(jù),也為PD的治療提供了新的思路。
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        (本文編輯 馬偉平)
        

        
            
        
        
        
        
        
        
    
        

        









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