PCRPRIMERDESIGNANDREACTIONOPTIMISATION
ContentsFactors Affecting the PCR Nested Primer PCRPrimer LengthDegenerate PrimersElongation Temperature and TimeReaction BufferCycle NumberDenaturing Temperature and TimeAnnealing Temperature and Primer DesignLabelling of PCR products with digoxygenin-11-dUTPHelix Destabilisers / AdditivesUseful Universal cDNA PCR PrimerA simple set of rules for primer sequence designREFERENCESFactors Affecting the P......阅读全文
PCR-PRIMER-DESIGN-AND-REACTION-OPTIMISATION
ContentsFactors Affecting the PCR Nested Primer PCRPrimer LengthDegenerate PrimersElongation Temperature and TimeReaction BufferCycle NumberDenaturin
PCR-Primer-Design(三)
References Albert, J., and Fenyo, E.M. 1990. Simple, sensitive and specific detection of human immunodeficiency virus type 1 in clinical speci
PCR-Primer-Design(二)
Terminal Nucleotides Make a Difference Both the terminals of the primer are of vital importance for a successful amplification. The 3'-end
PCR-Primer-Design(一)
Molecular Biology Today 2001. 2(2): 27-32. Vinay K. Singh and Anil Kumar Bioinformatics Sub-centr
TaqMan-Primer-and-Probe-Design
Adapted from TaqMan® One-Step RT-PCR Master Mix Reagents Kit InstructionDesign of Probes Keep the G-C content in the 20 to 80% range.Avoid runs of an
引物设计(Primer-Design)的原则
首先引物要跟模板紧密结合,其次引物与引物之间不能有稳定的二聚体或发夹结构存在,再次引物不能在别的非目的位点引起DNA聚合反应(即错配)。围绕这几条基本原则,设计引物需要考虑诸多因素,如引物长度(primer length)、产物长度(product length)、序列Tm值(melting t
PCR引物
PCR Primer Design and Reaction Optimization (Molecular Biology Techniques Manual) PCR Primer Design (Newman Lab) PCR Primer Design (Eppendorf)Detail
PCR引物
PCR Primer Design and Reaction Optimization (Molecular Biology Techniques Manual) PCR Primer Design (Newman Lab) PCR Primer Design (Eppendorf)Detail
标准PCR
· What's PCR? (Michael Blaber's Lab)Illustrated introduction to usr/localious aspects of PCR technique. It's very valuable not onl
标准PCR
What's PCR? (Michael Blaber's Lab)Illustrated introduction to usr/localious aspects of PCR technique. It's very valuable not only for thos
Standard-PCR-reaction
Steps for Standard PCR ReactionDesign primers. In general, primers should have the following properties:Tip: Primer3 is an excellent resource for choo
Real-Time-PCR-Primer-Sets
Real Time PCR Primer SetsNOW OVER 300 PRIMER SETS!!!UPDATED: NOVEMBER 10th, 2003Quantitative RT-PCR is an important step for the validation of express
PCR基本实验方法(一)
Recommended Reagent Concentrations:Primers: 0.2 - 1.0 uMNucleotides: 50 - 200 uM EACH dNTPDimethyl sulphoxide (DMSO): 0 - 10% (v/v)Taq polymerase: 0.5
PCR基本实验方法(一)
Recommended Reagent Concentrations:Primers: 0.2 - 1.0 uMNucleotides: 50 - 200 uM EACH dNTPDimethyl sulphoxide (DMSO): 0 - 10% (v/v)Taq polymerase: 0.5
其它PCR方法
· Standard PCR Protocol (Molecular Biology Techniques Manual)The followings are described in detailRecommended Reagent ConcentrationsRecommend
PCR
PCRPolymerase Chain Reaction1) Add the following to a microfuge tube:10 ul reaction buffer1 ul 15 uM forward primer1 ul 15 uM reverse primer1 ul templ
Chemicon-试剂盒的说明
TROUBLESHOOTINGNo products are visible in any lane.1. Potential Problem: PCR amplification is not initiated.Recommendations:a. Confirm that all PCR co
定量PCR(Polymerase-Chain-Reaction)技术
定量PCR(Polymerase Chain Reaction)技术有广义概念和狭义概念。广义概念的定量PCR技术是指以外参或内参为标准,通过对PCR终产物的分析或PCR过程的监测,进行 PCR起始模板量的定量。广义概念下的定量PCR技术可以分为五种类型:(1)外参法+终产物分析。所谓“外参法”是指
Polymerase-Chain-Reaction-(PCR)-cont.
Polymerase Chain Reaction (PCR) cont.Choice of Polymerases for PCROne of the important advances which allowed development of PCR was the availability
sothing-about-Genome-walking
Can anyone recommend a good kit for genome walking? I would like to find out the promoter sequence of a known gene. Is genome walking the way to do it
PCR实验指导与常见问题分析1
CONTENTPCR guide: a discussion of the main parameters influencing the outcome of the PCR and multiplex PCR reaction in 16 pages/sections and using ove
PCR-Primers-For-Gene-Expression-Detection-or-Quantification
Why PrimerBank?PrimerBank is a public resource for PCR primers. These primers are designed for gene expression detection or quantification (real-time
annealing-temp-for-degenerated-primer--PCR-problem
PCR primers should be free of significant complementarily at their 3'-termini as this favours formation of primer-dimer which reduce product yield
Single-Primer-(SemiRandom)-PCR
DescriptionSingle primer PCR allows amplification from known to unknown regions in chromosomes, phage, plasmids, large PCR products and other sources
SuperScript™-III-OneStep-RTPCR-System-with-Platinum®-Taq-High-Fidelity
实验概要The SuperScript™ III One-Step RT-PCR System with Platinum® Taq High Fidelity is designed for sensitive, high-fidelity end-point detection and
Streptomyces:Protocols/PCR
Description Polymerase Chain Reaction (PCR) is a method of amplifying a specific DNA target sequence. The cycle involves denaturing the template doubl
PCR
实验概要protocal for PCR实验步骤PCR 1) Add the following to a microfuge tube: 10 ul reaction buffer 1 ul 15 uM forward primer 1 ul 15 uM
Quantitative-PCR
实验概要Quantitative PCR involves co-amplification of two templates: a constant amount of a preparation containing the desired target sequence and var
Protocol-for-dsRNA-Synthesis
实验概要 We routinely produce dsRNA by in vitro transcription of a PCR generated DNA template containing the T7 promoter sequence on both ends
Methylation-Specific-PCR
Methylation Specific PCRProtocol written by James Herman*Methylation Specific PCR (MSP) is a simple rapid and inexpensive method to determine the meth