LEO™ Gold Hotstart Taq DNA Polymerase (5U/µL)

Leo Gold Taq DNA Polymerase is a next-generation enzyme designed to enhance PCR specificity and efficiency through an advanced anti-Taq antibody hot-start mechanism. This technology prevents the enzyme from initiating DNA synthesis at room temperature, significantly reducing non-specific amplification, mispriming, and primer-dimer formation.

The anti-Taq antibody tightly binds to the polymerase, keeping it in an inactive state during reaction setup. Only when the sample undergoes the initial denaturation step at 95°C does the antibody dissociate, releasing the enzyme for precise and controlled amplification. This delayed activation improves reaction specificity, making Leo Gold Taq an excellent choice for complex or low-copy templates, multiplex PCR, and genotyping applications.

In addition to superior specificity, Leo Gold Taq offers high sensitivity and yield, ensuring efficient amplification even in challenging conditions. The optimized buffer system further enhances reaction performance, delivering robust, reproducible results across various PCR applications.

Designed for routine and high-throughput applications, Leo Gold Taq DNA Polymerase is the perfect solution for researchers seeking consistent, high-fidelity PCR performance. Whether you’re working with genotyping, mutation detection, cloning, or qPCR, its hot-start mechanism ensures optimal accuracy and reliability.

With Leo Gold Taq, you can eliminate background noise, enhance target specificity, and achieve cleaner, more reproducible PCR results—making every reaction count.