非病毒載體負(fù)載增強(qiáng)型綠色熒光蛋白轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞_第1頁
非病毒載體負(fù)載增強(qiáng)型綠色熒光蛋白轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞_第2頁
非病毒載體負(fù)載增強(qiáng)型綠色熒光蛋白轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞_第3頁
非病毒載體負(fù)載增強(qiáng)型綠色熒光蛋白轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞_第4頁
非病毒載體負(fù)載增強(qiáng)型綠色熒光蛋白轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞_第5頁
已閱讀5頁,還剩1頁未讀, 繼續(xù)免費(fèi)閱讀

下載本文檔

版權(quán)說明:本文檔由用戶提供并上傳,收益歸屬內(nèi)容提供方,若內(nèi)容存在侵權(quán),請進(jìn)行舉報(bào)或認(rèn)領(lǐng)

文檔簡介

1、非病毒載體負(fù)載增強(qiáng)型綠色熒光蛋白轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞            非病毒載體負(fù)載增強(qiáng)型綠色熒光蛋白轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞    2008-5-9 12:23:44                      &

2、#160;                                                  

3、                                    作者:桂伶俐,劉志恒,張傳漢,高峰    【關(guān)鍵詞】  綠色熒光蛋白質(zhì)類;,基因表達(dá);,轉(zhuǎn)染;,神經(jīng)前體細(xì)胞 

4、0;  Transfection of enhanced green fluorescent protein into immortalized neural progenitor cells by nonviral vectors    【Abstract】 AIM: To investigate an effective transfection method of nonviral vectors and the expression of enhanced green fluorescent protein (EGFP) in

5、 the transfected immortalized neural progenitor cells (INPC). METHODS: The plasmid EGFPC1 was transfected into INPC by three different nonviral vectors respectively, including Lipofectamine 2000, TRANSfection and Sofast. The expression of EGFP and the transfection efficiency of the 3 vectors were me

6、asured at 24 h after transfection. The transfection efficiency of the vector which was the most efficient, was detected 12, 24, 48 and 72 h after transfection to determine the expression peak of EGFP. The viability of transfected and nontransfected cells was measured by trypan blue rejection test. A

7、fter the plasmid EGFPC1 was transfected into INPC, the stable cell clone designated INPC/EGFP was isolated by G418 selection. The positive rate of EGFP was observed. And the specific molecular marker of neural progenitor cells, nestin, was detected using immunocytochemistry. After INPC/EGFP was indu

8、ced by 50 mL/L fetal bovine serum, the cell morphology and the expression of EGFP were observed in the differentiated cells. RESULTS: The transfection efficiency of Lipofectamine 2000, TRANSfection and Sofast was (25.5±2.9)%, (4.0±1.7)%, (7.9±1.4)% respectively, at 24 h after transfec

9、tion. And Lipofectamine 2000 was the most efficient. Its transfection efficiency at 12, 24, 48 and 72 h after transfection was (17.1±0.7)%, (25.5±2.9)%, (19.4±0.9)%, (15.6±1.4)%, respectively. The expression of EGFP was the highest at 24 h after transfection. The positive rate of

10、 EGFP was 95% in INPC/EGFP. And INPC/EGFP was still nestin positive. The differentiated cells presented as neurons or astrocytes, and EGFP was still found in their somas and processes. CONCLUSION: Extrinsic genes can be effectively transfected into INPC by Lipofectamine 2000. And EGFP is one of the

11、valuable tracking tools for INPC.    【Keywords】 green fluorescent protein; gene expression; transfection; neural progenitor cell    【摘要】 目的: 尋找能高效轉(zhuǎn)染永生化神經(jīng)前體細(xì)胞(INPC)的非病毒載體,觀察轉(zhuǎn)染后增強(qiáng)型綠色熒光蛋白(EGFP)的表達(dá). 方法: 用陽離子脂質(zhì)體Lipofectamine 2000,TRANSfection或陽離子聚合物Sofast分別負(fù)載質(zhì)粒EGFP

12、C1轉(zhuǎn)染INPC,利用熒光顯微鏡檢測轉(zhuǎn)染后24 h的轉(zhuǎn)染效率. 對轉(zhuǎn)染效率最高的一種載體,觀察其轉(zhuǎn)染后12,24,48和72 h轉(zhuǎn)染效率,確定EGFP表達(dá)最高峰. 用臺盼藍(lán)排斥試驗(yàn)檢測轉(zhuǎn)染和未轉(zhuǎn)染細(xì)胞的活力. 質(zhì)粒EGFPC1轉(zhuǎn)染INPC后,經(jīng)G418篩選,挑選細(xì)胞克隆,命名為INPC/EGFP,觀察其EGFP陽性率. 應(yīng)用巢蛋白抗體鑒定INPC/EGFP. 50 mL/L胎牛血清誘導(dǎo)INPC/EGFP分化,觀察分化后細(xì)胞的形態(tài)及EGFP表達(dá). 結(jié)果: Lipofectamine 2000,TRANSfection和Sofast轉(zhuǎn)染INPC后24 h,轉(zhuǎn)染效率分別為(25.5±2.9

13、)%,(4.0±1.7)%,(7.9±1.4)%. Lipofectamine 2000的轉(zhuǎn)染效率最高. 其轉(zhuǎn)染后12,24,48和72 h的轉(zhuǎn)染效率分別為(17.1±0.7)%,(25.5±2.9)%,(19.4±0.9)%,(15.6±1.4)%,EGFP在轉(zhuǎn)染后24 h表達(dá)最高. INPC/EGFP中,EGFP陽性率約為95%. INPC/EGFP巢蛋白表達(dá)陽性,其分化后呈神經(jīng)元或星形膠質(zhì)細(xì)胞樣,且胞體及突起中仍可見綠色熒光.  結(jié)論: Lipofectamine 2000可高效轉(zhuǎn)染INPC. EGFP是INPC理想的

14、示蹤方法之一.    【關(guān)鍵詞】 綠色熒光蛋白質(zhì)類;基因表達(dá);轉(zhuǎn)染;神經(jīng)前體細(xì)胞    0引言    永生化神經(jīng)前體細(xì)胞(immortalized neural progenitor cell, INPC)具有自我更新、無限增殖及多向分化的潛能,且較原代神經(jīng)前體細(xì)胞易行基因操作,成為神經(jīng)系統(tǒng)損傷細(xì)胞替代及基因治療的理想靶細(xì)胞. 而選擇高效的外源基因?qū)胂到y(tǒng)對基因治療的效果至關(guān)重要. 盡管病毒介導(dǎo)的基因轉(zhuǎn)染具有更佳的轉(zhuǎn)染效率,但由于其安全性和技術(shù)方面的原因,探討高效率的非病毒載

15、體基因轉(zhuǎn)染方法更具意義. 本實(shí)驗(yàn)擬以增強(qiáng)型綠色熒光蛋白(enhanced green fluorescent protein, EGFP)為報(bào)告基因, 采用不同種類陽離子脂質(zhì)體或陽離子聚合物轉(zhuǎn)染大鼠INPC, 檢測其轉(zhuǎn)染效率, 并觀察EGFP的表達(dá), 以期尋找轉(zhuǎn)染效率較高的非病毒載體及理想的INPC示蹤方法.    1材料和方法    1.1材料    Neurobasal,B27添加劑,胎牛血清購自美國GIBCO公司;堿性成纖維生長因子(basic fibroblast g

16、rowth factor, bFGF)、表皮生長因子(epidermal growth factor, EGF)購自英國PeproTech公司;多聚鳥氨酸、明膠購自美國SIGMA公司; Lipofectamine 2000購自美國Invitrogen公司;TRANSfection購自北京天為時(shí)代公司;Sofast購自北京天來公司;巢蛋白抗體購自美國NeoMarkers公司;免疫組化試劑盒購自北京中山公司;質(zhì)粒提取試劑盒購自上海華舜公司;攜帶質(zhì)粒EGFPC1(美國BD公司)的菌種由同濟(jì)醫(yī)院麻醉學(xué)教研室保存.    1.2方法  

17、0;     原代大鼠神經(jīng)前體細(xì)胞后建立的INPC,由同濟(jì)醫(yī)院麻醉學(xué)教研室構(gòu)建并保存. INPC應(yīng)用含20 mL/L B27,20 g/L bFGF,20 g/L EGF的無血清Neurobasal培養(yǎng)基,在預(yù)先采用10 mg/L多聚鳥氨酸和2 g/L明膠包被的六孔板中貼壁培養(yǎng).        將攜帶EGFPC1質(zhì)粒的菌種接種于含氨芐青霉素的LB培養(yǎng)基中,振搖12 h,按試劑盒操作說明提取質(zhì)粒,采用瓊脂糖凝膠電泳及紫外分光光度法確定質(zhì)粒的純度與濃度. 分別參照陽離子

18、脂質(zhì)體Lipofectamine 2000,TRANSfection及陽離子聚合物Sofast的說明書進(jìn)行轉(zhuǎn)染(轉(zhuǎn)染試劑與質(zhì)粒按說明書推薦量). 將兩者混合物輕輕滴加于匯合率為80%90%的INPC中,繼續(xù)培養(yǎng)5 h后換液. 每組設(shè)3 個(gè)復(fù)孔. 轉(zhuǎn)染后24 h,倒置熒光顯微鏡觀察EGFP的表達(dá). 分別記錄每個(gè)轉(zhuǎn)染細(xì)胞培養(yǎng)孔隨機(jī)5個(gè)視野內(nèi)明視野和暗視野所觀察到的細(xì)胞數(shù). 轉(zhuǎn)染效率(%)暗視野發(fā)綠色熒光細(xì)胞數(shù)/明視野細(xì)胞數(shù)×100%. 對轉(zhuǎn)染效率最高的一種載體,在轉(zhuǎn)染后12,24,48和72 h觀察轉(zhuǎn)染效率.        細(xì)胞活力取出同期培養(yǎng)的未轉(zhuǎn)染和轉(zhuǎn)染剛結(jié)束的細(xì)胞培養(yǎng)板,室溫下用0.4 g/L臺盼藍(lán)溶

溫馨提示

  • 1. 本站所有資源如無特殊說明,都需要本地電腦安裝OFFICE2007和PDF閱讀器。圖紙軟件為CAD,CAXA,PROE,UG,SolidWorks等.壓縮文件請下載最新的WinRAR軟件解壓。
  • 2. 本站的文檔不包含任何第三方提供的附件圖紙等,如果需要附件,請聯(lián)系上傳者。文件的所有權(quán)益歸上傳用戶所有。
  • 3. 本站RAR壓縮包中若帶圖紙,網(wǎng)頁內(nèi)容里面會有圖紙預(yù)覽,若沒有圖紙預(yù)覽就沒有圖紙。
  • 4. 未經(jīng)權(quán)益所有人同意不得將文件中的內(nèi)容挪作商業(yè)或盈利用途。
  • 5. 人人文庫網(wǎng)僅提供信息存儲空間,僅對用戶上傳內(nèi)容的表現(xiàn)方式做保護(hù)處理,對用戶上傳分享的文檔內(nèi)容本身不做任何修改或編輯,并不能對任何下載內(nèi)容負(fù)責(zé)。
  • 6. 下載文件中如有侵權(quán)或不適當(dāng)內(nèi)容,請與我們聯(lián)系,我們立即糾正。
  • 7. 本站不保證下載資源的準(zhǔn)確性、安全性和完整性, 同時(shí)也不承擔(dān)用戶因使用這些下載資源對自己和他人造成任何形式的傷害或損失。

評論

0/150

提交評論