| 查看: 2580 | 回复: 7 | |||
[求助]
融合蛋白不挂柱,急!
|
|
大家好,我最近实验遇到了一个问题要请教大家。 我做的是一个膜蛋白的异源表达,载体用的是Bio rad的pPAL7载体,这个载体有一个特色,就是它的tag在我的蛋白质的N端,一旦elution buffer中有氯离子则tag和我的目的蛋白会自动切开。我们通过这个Tag同柱子的亲和层析纯化我的目的蛋白,然后再加入含有氯离子的溶液得到我的目的蛋白。 tag等电点9.0大小8.3kd,目的蛋白等电点11.7大小5.7kd,融合蛋白等电点9.64(软件预测),wash buffer是磷酸钠溶液 pH7.2,融合蛋白在包涵体和可溶性部分均有表达。我每次都摇200ml的菌提取蛋白,可是每次做亲和层析都发现与柱子不结合(可溶性部分和包涵体都试过),望大家指点迷津啊! |
回复此楼» 收录本帖的淘帖专辑推荐
 科研专列 |
» 猜你喜欢
不合理蛙科研实验中的趣事:实验器材的 “乌龙”
已经有0人回复
-
不合理蛙科研实验中的趣事:和实验材料的 “斗智斗勇”
已经有0人回复
-
化学工程及工业化学论文润色/翻译怎么收费?
已经有291人回复
-
蛋白质检测:精准分析,解锁生物分子的密码
已经有0人回复
-
不合理蛙科研实验之小鼠实验:严谨设计,解析生命机制的重要载体
已经有0人回复
-
不合理蛙科研实验之重金属检测:精准筛查,守护健康与环境的防线
已经有0人回复
-
不合理蛙科研实验之“蛙测重金属我背锅三千”
已经有0人回复
-
不合理蛙科研实验之“鼠逃三次我发三篇SCI”
已经有0人回复
-
纳米粒度分析
已经有3人回复
-
林科院林化所招收材料与化工专业硕士,坐标南京
已经有0人回复
» 本主题相关价值贴推荐,对您同样有帮助:
- GST融合蛋白表达纯化
已经有5人回复
- 融合蛋白的linker怎么设计
已经有14人回复
- 融合蛋白在不同细胞系表达
已经有4人回复
- 高等电点(pI8.3)his融合蛋白纯化,选用何种缓冲液?
已经有7人回复
- his标签蛋白纯化,不挂柱
已经有18人回复
- 镍柱纯化蛋白透析出现大量沉淀,请教
已经有18人回复
- GST融合蛋白纯化求助 !!!
已经有19人回复
- 融合蛋白在大肠杆菌中的表达,怎么被我越做越复杂了?
已经有8人回复
- 【求助/交流】重组蛋白融合标签的选择
已经有6人回复
- 【求助/交流】关于GFP融合的蛋白的一些问题
已经有7人回复
- 【求助/交流】MBP融合蛋白的Amylose亲和层析
已经有11人回复
- 【求助/交流】表达蛋白为什么要通过融合蛋白?
已经有4人回复
- 【求助/交流】蛋白不挂柱怎么办
已经有11人回复
2楼2011-09-02 14:45:15
3楼2011-09-02 14:52:31
4楼2011-09-02 15:27:36
labrat
木虫 (著名写手)
- MolEPI: 3
- 应助: 5 (幼儿园)
- 金币: 2250.2
- 帖子: 2297
- 在线: 13.1小时
- 虫号: 100291
- 注册: 2005-11-12
- 性别: GG
- 专业: 生物化学
【答案】应助回帖
★ ★ ★ ★ ★
dhd997(金币+5): good 2011-09-02 18:21:07
甜酒慢品(金币+5): thank you! 2011-09-05 10:09:14
dhd997(金币+5): good 2011-09-02 18:21:07
甜酒慢品(金币+5): thank you! 2011-09-05 10:09:14
hi, i don't really understand chinese  , but this is the technical guide generally used for your application:1. Premature elution of cleaved, target protein is observed: Fusion protein: Insert Thr-Ser spacer between Profinity eXact ™ tag and target protein by cloning into pPAL7’s SpeI site Lysis: For maximum yields, do not use lysis buffers and reagents that contain triggering ions, specifically Cl– or F– *Maintain lysate at 4°C prior to loading *Shorten incubation time *Utilize lysis buffer with pH <7.0 Wash: Pre-chill wash buffer to 4°C prior to use *Do not use lysis buffers and reagents that contain triggering ions, specifically Cl– or F–. When preparing wash buffer, substitute sodium acetate (NaOAc) for NaCl; do not use HCl to adjust pH—phosphoric or acetic acid should be used • Utilize wash buffer with pH <7.0 2. Target protein remains uncleaved and/or does not elute completely: Fusion protein: Verify that first amino acid (P1') downstream of the Profinity eXact cleavage site is not proline • If first amino acid of target protein is undesirable for cleavage, insert amino acid spacer (e.g., Thr-Ser) immediately downstream of cleavage site by site-directed mutagenesis or clone into SpeI site of pPAL7 Elution: • Incubate resin with elution buffer for longer time (try up to 1 hour at room temperature or overnight at 4°C) • If performing elution at 4°C, incubate overnight • Increase fluoride concentration in elution buffer • Substitute 10 mM sodium azide for fluoride in elution buffer • Elute with application of second volume of elution buffer to spin column resin 3. Eluate contains significant contaminants: Load:• Dilute lysate for multimeric proteins • Reduce fusion protein load amount to achieve subsaturating level bound to resin • Incubate lysate with resin for up to an hour at 4°C to increase binding capacity of target fusion protein Wash: • Perform additional wash step • Reduce nonspecific, electrostatic binding by increasing ionic concentration of wash buffer; use up to 0.3 M Sodium phosphate, NaOAc, or (NH4)2SO4 (pH 7.2), or amend wash buffer with any of the aforementioned salts. Do not use NaCl • Reduce hydrophobic interactions by decreasing salt concentration of wash buffer • Supplement wash buffer with suitable detergent 4. Fusion protein binds poorly to the resin: Fusion Protein : Proteins with high N-terminal structure may interfere with binding; adding amino acid spacer (i.e., Thr- Ser) between Profinity eXact tag and target protein will improve tag’s accessibility Lysis : • If using urea to help solubilize proteins, use [urea] <4 M; higher urea concentrations reduce binding capacity Load : • Allow lysate to incubate with resin for up to an hour at 4°C or for 30 minutes at room temperature; lysates with fusion proteins >75 kD often benefit from a longer incubation period • When purifying multimeric proteins, avoid saturating resin; diluting lysate may also improve yields Resin :• Resin previously used must be regenerated to remove cleaved Profinity eXact tag; apply three column volumes of 0.1M H3PO4 to resin |
5楼2011-09-02 16:57:40
charlie2800
木虫 (正式写手)
- 应助: 0 (幼儿园)
- 金币: 4252.8
- 红花: 2
- 帖子: 644
- 在线: 174.7小时
- 虫号: 555732
- 注册: 2008-05-09
- 专业: 生物物理、生物化学与分子
6楼2011-09-03 13:56:14
7楼2011-09-30 00:59:24
8楼2011-09-30 01:14:37
