Hieff Canace™ High-Fidelity Long PCR Master Mix

SKU:BHT20800053 PCR & qPCR
Overview
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Hieff Canace™ Long PCR Master Mix (With Dye) is a ready-to-use 2× pre-mixed solution containing Hieff Canace™ High-Fidelity DNA Polymerase, dNTPs, and an optimized buffer system, which contains pre-added electrophoresis indicators. The pre-mix contains pre-added electrophoresis indicator, PCR produc
Mix Type PCR Master Mix
Hot Start No
Grade RUO
Storage -20°C
Shipping Dry Ice
Options selector
Catalog no. Size
10166ES01 250 μL
10166ES03 1 mL
10166ES08 5×1 mL
Available Options

Select the size format that best suits your experiment. Availability and lead time may vary by option.

  • Options: Size (3) — 250 μL, 1 mL, 5×1 mL
  • Lead time: varies by selected option; please contact us for current fulfillment timing.
  • Storage: -20°C
  • Shipping: cold-chain shipment (typically with ice packs).
  • Upon receipt: store at the recommended temperature as soon as possible.
  • Sales terms and conditions: Please review prior to ordering.
Field Specification
Mfr No 10166ES
Product Type
  • PCR Master Mix
Shipping Dry Ice
Storage -20°C

Hieff Canace™ Veritas Long PCR Master Mix (With Dye) is a ready-to-use 2× premix containing Hieff Canace™ High-Fidelity DNA Polymerase, dNTPs, an optimized buffer system, and pre-added electrophoresis indicator dye. PCR products can be loaded directly for gel electrophoresis. Amplification products have blunt ends. A specific protective agent maintains stable enzyme activity through repeated freeze-thaw cycles.

Features

  • Ultra-high fidelity: low mismatch rate in GC-rich and mutation-prone targets
  • Fast extension: as fast as 5 sec/kb
  • Pre-loaded electrophoresis dye: direct gel loading without additional loading buffer
  • Blunt-end products: compatible with blunt-end cloning and Gibson Assembly
  • Wide applicability: high- and low-GC content templates
  • Freeze-thaw stable: protective agent maintains activity through repeated cycles

Recommended PCR Cycling Conditions

Step Temperature Time Cycles
Initial Denaturation 98°C 30 sec 1
Denaturation 98°C 10 sec 30–35
Annealing 60°C 5 sec 30–35
Extension 72°C 5–10 sec/kb 30–35
Final Extension 72°C 2 min 1

Extension: 5 sec/kb recommended; extend to 10 sec/kb for difficult templates.

Selected Citations

[1] Dong W, et al. An SHR-SCR module specifies legume cortical cell fate to enable nodulation. Nature. 2022.

Hieff Canace™ High-Fidelity DNA Polymerase incorporates 3′→5′ proofreading exonuclease activity, delivering significantly lower error rates than standard Taq DNA polymerase. It is validated for amplification of targets with low mismatch tolerance, including mutation-prone GC-rich genes.

No. The With Dye formulation contains pre-added electrophoresis indicator, enabling direct gel loading of PCR products without adding loading buffer. The No Dye version (Cat# 10165ES) is available when direct electrophoresis is not required.

Amplification products have blunt ends, directly compatible with blunt-end cloning, Gibson Assembly, and ligase-independent cloning methods. No additional polishing is required.

This formulation contains a specific protective agent that maintains stable polymerase activity through repeated freeze-thaw cycles, making it suitable for bench use without strict aliquoting requirements.

Recommended extension rate is 5 sec/kb for most templates. For long or complex fragments, extend to 10 sec/kb. Initial denaturation at 98°C for 30 seconds; cycle denaturation at 98°C for 10 seconds; annealing at 60°C for 5 seconds.

Yeasen Biotechnology supports custom formulation and scale-up services for reagent mixes and master mixes. Contact BioHippo to discuss project requirements and initiate an inquiry.

▶ GMP-Grade & Bulk Supply

Select Yeasen reagent mixes are available in GMP grade for IVD assay development. Manufactured in an ISO 13485-certified UCF.ME™ facility with FDA Drug Master File (DMF) support.

  • GMP release testing and CoA documentation
  • Scalable from milliliter to liter-scale quantities
  • Consistent lot-to-lot performance specifications

▶ Glycerol-Free & Lyophilization-Ready Formats

Glycerol-free and lyophilization-ready formats are available for reagents intended for cartridge-based point-of-care devices, liquid handling automation, or ambient-temperature distribution.

  • Glycerol-free liquid formulation
  • Lyophilization-compatible format with cryoprotectant
  • Custom reaction buffer optimization

▶ Molecular IVD RDC Service

Yeasen's Research and Development Contracting team provides end-to-end support for molecular diagnostic product development using Yeasen reagent mixes as a foundation.

  • Master mix selection and performance matching for target assay
  • Primer/probe design and assay buffer optimization
  • Sensitivity, specificity, and LOD validation
  • Instrument compatibility assessment

▶ Custom Formulation

Custom formulation services are available for researchers requiring modifications to standard reagent mix compositions, including ROX level adjustment, dye substitution, stabilizer optimization, and buffer modification.

  • ROX concentration customization (No / Low / High ROX)
  • Reference dye and indicator dye options
  • Buffer composition and pH optimization
  • Scale-up to commercial quantities on confirmation

ⓘ Customization services fulfilled by Yeasen Biotechnology. Contact BioHippo for project scoping and pricing.

[1] Dong W, Zhu Y, Chang H, et al. An SHR-SCR module specifies legume cortical cell fate to enable nodulation. Nature. 2021;589(7843):586-590. doi:10.1038/s41586-020-3016-z (IF:42.779) [2] Sun L, Yan Y, Lv H, et al. Rapamycin targets STAT3 and impacts c-Myc to suppress tumor growth. Cell Chem Biol. 2022;29(3):373-385.e6. doi:10.1016/j.chembiol.2021.10.006 (IF:8.116) [3] Ye M, Xiong L, Dong Y, et al. The Potential Role of the Methionine Aminopeptidase Gene PxMetAP1 in a Cosmopolitan Pest for Bacillus thuringiensis Toxin Tolerance. Int J Mol Sci. 2022;23(21):13005. Published 2022 Oct 27. doi:10.3390/ijms232113005 (IF:6.208) [4] He Y, Zhou J, Fu R, et al. The application of DNA-HRP functionalized AuNP probes in colorimetric detection of citrus-associated Alternaria genes. Talanta. 2022;237:122917. doi:10.1016/j.talanta.2021.122917 (IF:6.057) [5] Guo L, Yang W, Huang Q, et al. Selenocysteine-Specific Mass Spectrometry Reveals Tissue-Distinct Selenoproteomes and Candidate Selenoproteins. Cell Chem Biol. 2018;25(11):1380-1388.e4. doi:10.1016/j.chembiol.2018.08.006 (IF:5.592) [6] Dou W, Zhu Q, Zhang M, Jia Z, Guan W. Screening and evaluation of the strong endogenous promoters in Pichia pastoris. Microb Cell Fact. 2021;20(1):156. Published 2021 Aug 9. doi:10.1186/s12934-021-01648-6 (IF:5.328) [7] Xiong Y, Yi Y, Wang Y, Yang N, Rudd CE, Liu H. Ubc9 Interacts with and SUMOylates the TCR Adaptor SLP-76 for NFAT Transcription in T Cells. J Immunol. 2019;203(11):3023-3036. doi:10.4049/jimmunol.1900556 (IF:4.718) [8] Huang L, Xiang M, Ye P, Zhou W, Chen M. Beta-catenin promotes macrophage-mediated acute inflammatory response after myocardial infarction. Immunol Cell Biol. 2018;96(1):100-113. doi:10.1111/imcb.1019 (IF:4.557) [9] Wang X, Du A, Yu G, Deng Z, He X. Guanidine N-methylation by BlsL Is Dependent on Acylation of Beta-amine Arginine in the Biosynthesis of Blasticidin S. Front Microbiol. 2017;8:1565. Published 2017 Aug 22. doi:10.3389/fmicb.2017.01565 (IF:4.076) [10] Yu P, Zhou L, Yang WT, et al. Comparative mitogenome analyses uncover mitogenome features and phylogenetic implications of the subfamily Cobitinae. BMC Genomics. 2021;22(1):50. Published 2021 Jan 14. doi:10.1186/s12864-020-07360-w (IF:3.969) [11] Liu G, Liu Y, Niu B, et al. Genetic mutation of TRPV2 induces anxiety by decreasing GABA-B R2 expression in hippocampus. Biochem Biophys Res Commun. 2022;620:135-142. doi:10.1016/j.bbrc.2022.06.079 (IF:3.575) [12] Tan KS, Zhang Y, Liu L, et al. Molecular cloning and characterization of an atypical butyrylcholinesterase-like protein in zebrafish. Comp Biochem Physiol B Biochem Mol Biol. 2021;255:110590. doi:10.1016/j.cbpb.2021.110590 (IF:2.231) FAQ Q: When performing long fragment amplification (over 10kb) with this product, does it still follow the reaction procedure for reactions under 10kb? A: When dealing with fragments larger than 10 kb, it is advisable to combine 68℃ with 10 sec/kb to enhance the amplification success rate. For fragments smaller than 10 kb, an amplification speed of 5 sec/kb can be used. Q: Can the 10166ES product be used for the amplification of long cDNA fragments? What suggestions do you have for the experiment? A: (1) This 10166ES product can accommodate cDNA amplification ranging from 1 kb to 14 kb. If you need to perform long fragment amplification, it is recommended to use the validated 11149ES reverse transcription kit from Yeasen Biotechnology to reverse transcribe the target RNA. The resulting cDNA template can then be used in conjunction with 10166ES for long fragment amplification. (2) If the RNA sample is small or if you need to obtain a very long target fragment, it is recommended not to perform digestion during reverse transcription. The longer the target fragment, the more RNA needs to be input, and accordingly, more cDNA will be required. Q: What should we do if there are mutations in the amplified product? A: 10166ES is a high-fidelity PCR product. High fidelity means a lower error rate and more accurate sequences. However, different experimental methods may result in variations. Product mutations are low-probability events. It is recommended to perform multiple repeated sets of new amplifications to obtain unmutated amplification products. Q: Can the 10166ES be used to amplify fragments with high GC content? A: Yes, after testing, the 10166ES can cover fragments with GC content ranging from 20% to 80%. When expanding fragments with a high GC content, it is recommended to adjust the temperature to 68℃, which will significantly increase the success rate. Q: My sample is a bacterial culture solution. Can I directly use 10166ES to amplify the bacterial culture solution? A: The 10166ES can tolerate a certain amount of bacterial solution. After testing, it has been found that this product can tolerate bacterial solution at a proportion of 12.5% in the reaction system, and it has good specificity. If you need to directly expand the bacterial solution, please keep the proportion below 12.5%. Q: Can Hieff Canace®Veritas Long PCR Master Mix (with Dye) be used for amplifying cDNA templates containing uracil? A: The 10166ES product can tolerate a certain amount of cDNA stock solution, which contains residual RNA and degraded RNA. Therefore, cDNA containing uracil can be used as the template. However, there is a certain range. After product performance testing, 10166ES can meet the requirement of a cDNA input volume accounting for 15% of the reaction system. Q: How much sample can the Hieff Canace®Veritas Long PCR Master Mix (with Dye) detect? A: (1) For plant genomes, after product performance testing, it can detect as low as 100pg of plant genome. (2) For animal genomes, after product performance testing, the minimum detectable amount is 100pg of animal genome. (3) For plasmids, since they are relatively pure, after product performance testing, the minimum detectable amount is 1pg of plasmid. Q: Why did I have no problem using 10166ES several times before, but this time when expanding the long fragment, there was no band? A: Possible causes and solutions: The thawing requirements for 10166ES stipulate that it should be thawed slowly on ice, and it cannot be thawed at room temperature or through heating. (2) When performing the amplification process, it is recommended to set the temperature at 68℃ and the amplification speed at 10 seconds per kilobase. (3) The longer the target fragment to be amplified is, the more template should be used. (4) In the PCR system, the concentration of primers is too low or the number of cycles is insufficient: appropriately increase the amount of primers, or increase the number of amplification cycles;

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Experience the power of Celltrypse™, c-LEcta's innovative enzyme solution for gentle and efficient cell dissociation. Request your free sample and discover a superior alternative for your cell culture workflows.

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Experience the power of Celltrypse™, c-LEcta's innovative enzyme solution for gentle and efficient cell dissociation. Request your free sample and discover a superior alternative for your cell culture workflows.

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