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

PCR基本实验方法

2024-11-19 PCR 加入收藏
Reagent Concentrations:Primers: 0.2 - 1.0 uMNucleotides: 50 - 200 uM EACH dNTPDi

Reagent Concentrations:

  • Primers: 0.2 - 1.0 uM
  • Nucleotides: 50 - 200 uM EACH dNTP
  • Dimethyl sulphoxide (DMSO): 0 - 10% (v/v)
  • Taq polymerase: 0.5 - 1.0 Units/50ul rxn

Target DNA : 1 ng - 1 ug (NB: higher concn for total genomic DNA ; lower for plasmid / purified DNA / virus DNA target)

Buffer : use proprietary or home-made 10x rxn mix; eg: Cetus, Promega. This should contain: minimum of 1.5mM Mg2+, usually some detergent, perhaps some gelatin or BSA. Promega now supply 25mM MgCl2, to allow user-specified [Mg2+] for reaction optimisation with different combinations of primers and targets.

MAKE POOLED MASTER MIX OF REAGENTS IN ABSENCE OF DNA using DNA -free pipette, then dispense to individual tubes (using DNA -free pipette), and add DNA to individual reactions USING PLUGGED TIPS.

OVERLAY REACTIONS WITH 50UL OF HIGH-QUALITY LIQUID PARAFFIN OR MINERAL OIL to ensure no evaporation occurs: this changes reactant concentrations. NOTE : latest wisdom has it one can use VASELINE - this also allows "HOT START" PCR.

 

NOTE:


USE PLUGGED PIPETTE TIPS: prevents aerosol contamination of pipettes.

Use of detergents is recommended only for Taq from Promega (up to 0.1% v/v, Triton X-100 or Tween-20). DMSO apparently allows better denaturation of longer target sequences (>1kb) and more product.

DO NOT USE SAME PIPETTE FOR DISPENSING NUCLEIC ACIDS AS YOU USE FOR DISPENSING REAGENTS

Remember sample volume should not exceed 1/10th reaction volume, and sample DNA /NTP/primer concentrations should not be too high as otherwise all available Mg2+ is chelated out of solution and enzyme reactivity is adversely affected. Any increase in dNTPs over 200uM means [Mg2+] should be re-optimised.

AVOID USING EDTA-CONTAINING BUFFERS AS EDTA CHELATES Mg2+

Low primer, target, Taq, and nucleotide concentrations are to be favoured as these generally ensure cleaner product and lower background, perhaps at the cost of detection sensitivity.


 

上一篇:PCR基本实验方法(二)   下一篇:PCR产物的克隆


文章底部广告位

文章评论

加载中~