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Western Blotting|實驗技術(shù)服務(wù)

時間:2015/7/1閱讀:202
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關(guān)鍵詞:Western Blotting|實驗技術(shù)服務(wù)
簡介:世界*品牌Western Blotting|實驗技術(shù)服務(wù)原裝,質(zhì)量保證,*。
Western Blotting|實驗技術(shù)服務(wù)——pCzn1質(zhì)粒+Arctic Express宿主菌低溫表達(dá)體系,。
我們具備豐富的蛋白表達(dá)設(shè)計經(jīng)驗及實驗操作技巧,承諾客戶不成功不收費,。在獲得重組蛋白產(chǎn)品的同時,,我們也會提供相應(yīng)的原始數(shù)據(jù)和原始圖片,不需要再額外花費精力重復(fù)實驗。另一方面,,我們所有的實驗數(shù)據(jù)真實可信,,我們提供原始的表達(dá)菌株和克隆質(zhì)粒,客戶可以依據(jù)我們的實驗報告重復(fù)我們的實驗結(jié)果,。
產(chǎn)品品牌:   http://www.,。。com/goodsid/fenleiyi/2868603/1.html    
測序?qū)嶒灹鞒蹋?br>對于Western Blotting實驗而言,,樣品處理是關(guān)鍵步驟之一,,獲得的蛋白樣品必須均質(zhì)、可溶,,并解離成單個多肽亞基,,且盡量減少相互間的聚集,使其zui終僅依賴本身的分子量大小進(jìn)行分離,。當(dāng)目標(biāo)蛋白的含量很低時,,需要選取目標(biāo)蛋白含量較高的組織或細(xì)胞器(如核抽提物),或者通過免疫沉淀等方式進(jìn)行富集,。通常樣品有重組蛋白,、細(xì)胞和組織等,。
1.樣品收集
1)培養(yǎng)的細(xì)胞
貼壁和懸浮細(xì)胞收集方式不同,細(xì)胞裂解液種類各異,,推薦含SDS的凝膠加樣緩沖液裂解,,煮沸即可。
2)動物組織
與細(xì)胞不同,,組織塊由于體積較大,,須預(yù)先經(jīng)破碎勻漿處理。
2.樣品定量
樣品電泳前需測定蛋白濃度,,以便保證上樣量一致,,有利于后續(xù)定量或半定量分析。常用的蛋白質(zhì)濃度測定方法有好多種,,其靈敏度和所需時間不同,,且不同的方法會受不同干擾物質(zhì)的影響,實驗者可根據(jù)樣品制備方法(裂解液成分,、去垢劑和還原劑種類等)自行選擇,。
注意事項:
a. 應(yīng)盡量避免引入影響后續(xù)定量的雜蛋白(如細(xì)胞培養(yǎng)液、蛋白酶抑制劑等)及其他干擾物質(zhì),;
b. 樣品濃度應(yīng)適中,,1×SDS凝膠加樣緩沖液建議用量:貼壁細(xì)胞按10cm2培養(yǎng)皿/0.1ml,懸浮細(xì)胞按5×106細(xì)胞/0.1ml比例加入,;
c. SDS對蛋白質(zhì)變性和電泳分離至關(guān)重要,,濃度應(yīng)控制在2-10%之間,并根據(jù)具體需要調(diào)整,;
d. 制備好的樣品可以在-20℃保存,,但時間不宜過長,并避免反復(fù)凍融,,否則蛋白會發(fā)生降解,;
e. 內(nèi)參對實驗結(jié)果至關(guān)重要,應(yīng)選擇合適的內(nèi)參,。
Western印跡含一系列步驟,,包括:
?? 用聚丙烯酰胺凝膠分離蛋白樣品。
?? 將膠上的蛋白轉(zhuǎn)移到膜上,。
?? 鑒定膜上特定蛋白,。
下面將從理論和實踐方面討論Western印跡方法。
用1-D或2-D凝膠分離復(fù)雜蛋白質(zhì)混合物
印跡前分離復(fù)雜蛋白質(zhì)混合物的zui常見方法是一維(1-D)SDS-PAGE電泳,,它根據(jù)蛋白質(zhì)的分子量進(jìn)行分離,。有時用非變性電泳分離天然蛋白質(zhì)。盡管這種方法通常缺乏變性電泳的分辨率,,但當(dāng)?shù)鞍醉毐A羯锘钚詴r非常有用,。
二維(2-D)凝膠電泳用于分析細(xì)胞,、組織、和體液蛋白質(zhì)的組成,,是現(xiàn)代蛋白質(zhì)組學(xué)的關(guān)鍵技術(shù),。2-D免疫印跡可提供分子量和等電點信息,并可用于區(qū)分翻譯后修飾產(chǎn)生的不同蛋白質(zhì)形式,。有些情況下只進(jìn)行1-D電泳分離也可用免疫印跡對蛋白分型,。

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