Login
欢迎浏览恩派尔生物资料网
我要投稿 请登录 免费注册 安全退出

您现在的位置是: 首页 > 实验方法 > PCR

PCR

反转录生产cDNA链以及PCR扩增

2024-11-19 PCR 加入收藏
The usual precautions for avoiding degradation of RNA should be taken until the

The usual precautions for avoiding degradation of RNA should be taken until the reverse transcription reaction is complete.

1. Make solution of 1 µg poly(A)+ RNA or 10 µg total RNA in 9 µl of 1X annealing buffer. This may require ethanol precipitating the RNA, washing with 70% EtOH, drying the pellet, and adding 9 µl 1X buffer. Or, if your starting solution of RNA in water is concentrated enough, you can simply mix the RNA, some 2X buffer, and water in the correct proportions.

2. Add 1 µl of the oligodeoxynucleotide primer:

100 pmol/µl for a specific 3' primer, 1000 pmol/µl for random hexamers

3. Heat 3 minutes at 65° and allow to cool to room temperature.

4. Make up some cDNA synthesis mix, and add 15 µl to each 10 µl annealed RNA sample.

5. Allow the reverse transcriptase reaction to go for 1 hour at 37° C.

When random hexamers are used, start the reaction at room temperature for 10 minutes.

6. Heat inactive for 10 minutes at 75°.

7. Use 2 µl of this cDNA mixture as a template for each 50 µl PCR amplification reaction, following standard procedures.

1X Annealing buffer:

250 mM KCl

10 mM Tris pH 8.3

1 mM EDTA

2X cDNA buffer:

48 mM Tris pH8.3

32 mM MgCl2

cDNA synthesis mix:

for each 15 µl reaction:

2X cDNA buffer 7.5 µl

100 mM DTT 1.25 µl

RNAse Block (Stratagene) 1 µl =40 U or other RNAsin

1.25 mM dNTPs 5 µl

M-MuLV reverse transcriptase 0.25 µl = 6 U (Biolabs)

 

上一篇:RT-PCR Analysis--详细的RT-PCR方法   下一篇:Long-PCR Reagents and Guidelines


文章底部广告位

文章评论

加载中~