Mycoplasma DNA amplification

Mycoplasma DNA amplification

High-efficiency Mycoplasma DNA amplification plays a crucial role in confirming sample authenticity and eliminating contamination risks in biological research and product testing. This process utilizes real-time PCR (qPCR) technology, which amplifies a specific region of the Mycoplasma genome. The amplification is tracked in real time through fluorescent probes that bind specifically to the target DNA sequence. As the PCR product accumulates, the fluorescent signal increases proportionally, allowing for immediate detection and precise quantification of Mycoplasma DNA. This method ensures accurate identification of contamination at the earliest stages, preserving the integrity of valuable samples.

The Tribioscience Mycoplasma qPCR Kit exemplifies this high-efficiency amplification technology. It includes comprehensive components such as Mycoplasma positive and negative controls, an internal control labeled with Hex, a qPCR super mix, and a primer-probe mix featuring a FAM-labeled probe for the target gene. These reagents create an optimized system that enhances amplification performance and simplifies result interpretation. The kit’s high sensitivity and specificity ensure that even small amounts of Mycoplasma DNA are reliably detected, while its no cross-reactivity with other species minimizes false positives, which is critical for ensuring confidence in test outcomes.

Through its optimized amplification conditions, the system delivers both high efficiency and reproducibility, streamlining laboratory workflows. The simple “just add DNA template and water” protocol enables rapid setup and consistent results across different sample types. Applications extend beyond traditional cell culture testing to include diverse materials such as FBS medium, plants, cannabis, grains, food, herbs, and animal feed. By ensuring robust Mycoplasma DNA amplification and accurate detection, this approach safeguards experimental validity, product purity, and overall biosafety.