产品说明
Direct PCR [3G]Amplify directly from whole blood, animal and plantsSkip DNA purificationVarious genotypingPrevention of carryover contaminationProductsCat.No.ProductSizeDPR200HelixAmp™ Direct PCR [3G]200 rxnsDPRU200HelixAmp™ Direct PCR [3G] [Containing UDG/dUTP]200 rxnsDPRH200HelixAmp™ Direct PCR [3G] (Hot-start)200 rxnsDPRHU200HelixAmp™ Direct PCR [3G] (Hot-start) [Containing UDG/dUTP]200 rxnsDescriptionDataDetailsDocumentsHelixAmp™ Direct PCR [3G] is designed for the PCR amplification directly from animal tissues, whole blood, and plant tissues without any DNA purification processes. This kit contains a 2x reaction mix including Taq DNA polymerase, dNTPs, MgCl2, and unique buffer system to resist various PCR inhibitors of tissue samples. HelixAmp™ Direct PCR [3G] (Hot-start) is including hot-start Taq DNA polymerase that is inactive at lower temperature by an inhibitory antibody and using this enzyme avoids the polymerization from non-specifically bound primers during the setting of PCR mix and at the start of PCR cycles. At high temperature of the initial denaturation step of PCR, the inhibitory antibody is released by denaturation and the free Taq DNA polymerase becomes active. NanoHelix’s Direct PCR [3G] is based on Taq polymerase. Due to this enzyme’s robust amplification and 3’ to 5’ exo-negative properties, this kit could be used for allele specific PCR which is routinely used for various genotyping. Moreover the Uracil-DNA glycosylase with dUTP system for the prevention of carryover contamination can be applied to this Taq polymerase-based kit. dUTP could not be used with the Pfu DNA polymerase and its derivatives. A Uracil-DNA glycosylase and dUTP applied version is also available. Figure 1. Direct PCR from various mouse tissues. Lysates directly extracted from each tissue without any DNA purification were used as template. 1: Heart, 2: Liver, 3: Large intestine, 4: Small intestine, 5: Kidney, 6: Stomach, 7: Ear, 8: Brain, 9: spleen, NTC: No template control. Figure 2. Direct PCR from whole blood and saliva. Human whole blood or saliva were use as template for direct PCR without any pre-treatment. Lane 1~10 : Amount of whole blood or saliva as template(μl), PTC: Purified genomic DNA, 10 ng was used as template, NTC: No template control. Figure 3. Direct PCR from various plant tissues. Lysate directly extracted from each Plant tissues without any DNA purification were used as templates. Direct PCRs were performed with a primer set specific for Chloroplast. NTC : No template control. Figure 4. Direct genotyping for selection of knock-out mice. WT: Wild type mouse(339 bp), HZ: Heterozygotic mouse, KO: Knock-out mouse(589 bp), NTC: No template control. Figure 5. Direct PCR for selection of transgenic plants. Lysates directly extracted from each plant leaves were used as template for PCR detection of transgenic plants. Figure 6. Direct PCR and RFLP analysis for Zebrafish genotyping. Target DNA were amplified directly from zerafish’s fin without DNA purification. RFLP analysis were done using a restriction enzyme (Rsa I). Application Allele-specific PCRPCR for genotypingPCR for selection of genetically modified organisms (GMO)Direct PCR amplification of target DNA without any DNA purification from various sample types such as whole blood, saliva, mouse tissues (tail, heart, liver, large intestine, small intestine, kidney, stomach, ear, brain, spleen), zebrafish’s fin, pork, beef, plant tissues (leaf and seed). Contents 2x Direct PCR premix (with UDG or without UDG)10x Dilution Buffer6x Loading Dye Quality controlHelixAmp™ Direct PCR [3G] is evaluated by amplification of PCR product corresponding to each sample type-specific DNA region directly using whole blood, leaf tissue, or animal tissue according to protocol.ManualMSDSBrochure
NanoHelix热逆转录酶是M-MLV逆转录酶(RTase)的一种热稳定且RNase H阴性的变体,是一种可在42℃〜55℃的温度下从RNA模板合成cDNA的酶,在50℃时显示最高的活性。热逆转录酶的高生产力和生产力可以扩增产物的高产率,并且可以从RNA模板合成高达12 kb的靶基因cDNA。
应用
生成长达12 kb的第一链cDNA用于文库或克隆
两步或一步RT-PCR应用
常规或实时RT-PCR
RT-PCR检测病毒RNA
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