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引物設(shè)計(jì)要遵循什么原則?

時(shí)間:2023/11/3閱讀:418
分享:

對(duì)于剛接觸分子生物學(xué)實(shí)驗(yàn)的小伙伴們來說,如果做一些與基因相關(guān)的實(shí)驗(yàn)的話,肯定離不開最基礎(chǔ)的實(shí)驗(yàn)——PCR,目前大家使用PCR技術(shù)做的最多的就是對(duì)基因/物種的鑒定、基因的克隆、基因表達(dá)量測(cè)定等實(shí)驗(yàn)。今天百奧創(chuàng)新將介紹PCR引物設(shè)計(jì)要遵循什么原則。
1、引物長(zhǎng)度一般在15-30bp。常用的為18-27bp,因?yàn)檫^長(zhǎng)會(huì)導(dǎo)致其延伸溫度大于74℃,不適于Taq DNA聚合酶進(jìn)行反應(yīng);

2、引物GC含量一般為40%-60%, 45-55%為宜,GC含量過高或過低都不利于引發(fā)反應(yīng),上下游引物GC含量和Tm值要保持接近,一般Tm值不超過5℃。

3、引物所對(duì)應(yīng)的模板序列的Tm值在55-80℃之間,最好為72℃左右。

4、引物的延伸是從3′端開始的,不能進(jìn)行任何修飾,且 3’端的堿基一般不用A;引物3’端出現(xiàn)3個(gè)以上的連續(xù)堿基,如GGG或CCC,或者引物3’端的互補(bǔ)、二聚體或發(fā)夾結(jié)構(gòu)也可能導(dǎo)致PCR反應(yīng)失敗,

5、堿基要隨機(jī)分布,且引物自身和引物之間不能有連續(xù)4個(gè)堿基的互補(bǔ)。

6、盡量在基因的編碼區(qū)(CDS序列)上設(shè)計(jì)引物,限制基因組DNA擴(kuò)增。

7、使用BLAST檢索,確認(rèn)引物特異性。

以上就是有關(guān)于PCR引物設(shè)計(jì)要遵循什么原則的問題解答,如果你想了解更多請(qǐng)咨詢百奧創(chuàng)新客服哦!


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