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[交流] 免疫共沉淀總是出現(xiàn)非特異性條帶

目的蛋白直接用RIPA裂解液裂解（1%NP40），目的蛋白含Biotin.
   Streptavidin-beads做IP.
   WB用的目的蛋白抗體做一抗。

   顯影后，陰性組和陽性組出現(xiàn)類似的條帶，應(yīng)該都是非特異性條帶。目的條帶看不到。

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求助Western Blot實(shí)驗(yàn)條帶沒出現(xiàn)的原因分析及解決辦法已經(jīng)有7人回復(fù)
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【求助/交流】請(qǐng)教Western blot出現(xiàn)非特異性條帶的怎么解決已經(jīng)有8人回復(fù)
【求助/交流】pull down實(shí)驗(yàn)陰性對(duì)照也有帶？已經(jīng)有5人回復(fù)

1樓 2015-02-24 02:39:37

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yyc12596

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最開始用的是Protein A/G beads.
標(biāo)記過目標(biāo)蛋白抗體，也試過標(biāo)記streptavidin抗體，不過效果都不好，總是非特異性條帶。

后來換了Streptavidin-beads，還是出現(xiàn)非特異性條帶。

再找找辦法，看看能不能把這個(gè)問題解決了。

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2樓2015-02-24 03:03:12

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yyc12596

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網(wǎng)上搜到的一些建議：

You may want to start with preclearing your lysates. You incubate your lysates with rabbit IgG (bound to beads) to clear away any binding that nonspecifically occurs with the species antibody. I don't recommend the use of RIPA though. I think it's just too aggressive of a lysis buffer. I use a simple NP40 (1%) buffer to lyse cells for IP. I also prefer to bind the antibody to the bead, wash well and block in 5% BSA before adding the lysate (rather than adding the antibody to the lysate followed by beads). This helps get rid of nonspecific binding to the bead itself. Your washing is definately an issue as well. PBS just isn't going to do the job. Minimally you wash in the buffer you lysed the cells in. You can make more aggressive washes but 1M salt is WAY to high (Urea is very aggressive and will destroy everything). You will disrupt all the interactions. I start by taking the lysis buffer to 250mM and will go up to about 500mM. Additionally you can add a little more detergent but I suggest you do this in small steps to determine the best conditions. It's frustrating to run the gel and see that you washed everything away! The other idea is to use a wash buffer without the salt. Nonspecific interactions can often be through salt bridges. One quick wash in a no salt (or very low) will get rid of this background as well. You can try the washes alone or in combination as well. I had one IP that required a high detergent (high salt did nothing) followed by a no salt wash in order to remove nonspecific bands. You are just going to have to play around with the conditions and see what works best for this situation. I can recommend a book: Using Antibodies by Harlow and Lane. There are many good hint and tips for troubleshooting and this book covers practically all assays involving antibodies.

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3樓2015-02-26 01:46:07

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